CA1175740A - Immunolabelled liposomes - Google Patents
Immunolabelled liposomesInfo
- Publication number
- CA1175740A CA1175740A CA000369832A CA369832A CA1175740A CA 1175740 A CA1175740 A CA 1175740A CA 000369832 A CA000369832 A CA 000369832A CA 369832 A CA369832 A CA 369832A CA 1175740 A CA1175740 A CA 1175740A
- Authority
- CA
- Canada
- Prior art keywords
- enzyme
- antigen
- accordance
- liposome
- antibody
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Expired
Links
- 239000002502 liposome Substances 0.000 title claims abstract description 140
- 102000004190 Enzymes Human genes 0.000 claims abstract description 112
- 108090000790 Enzymes Proteins 0.000 claims abstract description 112
- 239000000427 antigen Substances 0.000 claims abstract description 103
- 108091007433 antigens Proteins 0.000 claims abstract description 103
- 102000036639 antigens Human genes 0.000 claims abstract description 103
- 230000000295 complement effect Effects 0.000 claims abstract description 45
- 238000003018 immunoassay Methods 0.000 claims abstract description 24
- 238000012360 testing method Methods 0.000 claims description 60
- 239000000758 substrate Substances 0.000 claims description 55
- 239000000203 mixture Substances 0.000 claims description 44
- 238000000034 method Methods 0.000 claims description 41
- 150000002632 lipids Chemical class 0.000 claims description 35
- 239000000463 material Substances 0.000 claims description 29
- 230000000694 effects Effects 0.000 claims description 19
- 238000010998 test method Methods 0.000 claims description 16
- 230000002255 enzymatic effect Effects 0.000 claims description 15
- 229910001868 water Inorganic materials 0.000 claims description 13
- XLYOFNOQVPJJNP-UHFFFAOYSA-N water Substances O XLYOFNOQVPJJNP-UHFFFAOYSA-N 0.000 claims description 12
- 238000000926 separation method Methods 0.000 claims description 9
- 229910019142 PO4 Inorganic materials 0.000 claims description 5
- 239000003795 chemical substances by application Substances 0.000 claims description 5
- OGQYPPBGSLZBEG-UHFFFAOYSA-N dimethyl(dioctadecyl)azanium Chemical compound CCCCCCCCCCCCCCCCCC[N+](C)(C)CCCCCCCCCCCCCCCCCC OGQYPPBGSLZBEG-UHFFFAOYSA-N 0.000 claims description 5
- 230000008105 immune reaction Effects 0.000 claims description 5
- 102000004157 Hydrolases Human genes 0.000 claims description 4
- 108090000604 Hydrolases Proteins 0.000 claims description 4
- 102000003992 Peroxidases Human genes 0.000 claims description 4
- 229930182558 Sterol Natural products 0.000 claims description 4
- 108040007629 peroxidase activity proteins Proteins 0.000 claims description 4
- 235000021317 phosphate Nutrition 0.000 claims description 4
- 235000003702 sterols Nutrition 0.000 claims description 4
- 108010026217 Malate Dehydrogenase Proteins 0.000 claims description 3
- 102000013460 Malate Dehydrogenase Human genes 0.000 claims description 3
- 150000003432 sterols Chemical class 0.000 claims description 3
- 230000008961 swelling Effects 0.000 claims description 3
- 102000004316 Oxidoreductases Human genes 0.000 claims description 2
- 108090000854 Oxidoreductases Proteins 0.000 claims description 2
- 238000000746 purification Methods 0.000 claims description 2
- 230000014759 maintenance of location Effects 0.000 claims 4
- 150000003013 phosphoric acid derivatives Chemical class 0.000 claims 1
- 238000006243 chemical reaction Methods 0.000 abstract description 28
- 229940088598 enzyme Drugs 0.000 description 95
- 230000009089 cytolysis Effects 0.000 description 20
- 102000002260 Alkaline Phosphatase Human genes 0.000 description 18
- 108020004774 Alkaline Phosphatase Proteins 0.000 description 18
- HEDRZPFGACZZDS-UHFFFAOYSA-N Chloroform Chemical compound ClC(Cl)Cl HEDRZPFGACZZDS-UHFFFAOYSA-N 0.000 description 16
- 229960005156 digoxin Drugs 0.000 description 16
- 239000000523 sample Substances 0.000 description 16
- LFQSCWFLJHTTHZ-UHFFFAOYSA-N Ethanol Chemical compound CCO LFQSCWFLJHTTHZ-UHFFFAOYSA-N 0.000 description 15
- 238000003556 assay Methods 0.000 description 15
- LTMHDMANZUZIPE-AMTYYWEZSA-N Digoxin Natural products O([C@H]1[C@H](C)O[C@H](O[C@@H]2C[C@@H]3[C@@](C)([C@@H]4[C@H]([C@]5(O)[C@](C)([C@H](O)C4)[C@H](C4=CC(=O)OC4)CC5)CC3)CC2)C[C@@H]1O)[C@H]1O[C@H](C)[C@@H](O[C@H]2O[C@@H](C)[C@H](O)[C@@H](O)C2)[C@@H](O)C1 LTMHDMANZUZIPE-AMTYYWEZSA-N 0.000 description 14
- HVYWMOMLDIMFJA-DPAQBDIFSA-N cholesterol Chemical compound C1C=C2C[C@@H](O)CC[C@]2(C)[C@@H]2[C@@H]1[C@@H]1CC[C@H]([C@H](C)CCCC(C)C)[C@@]1(C)CC2 HVYWMOMLDIMFJA-DPAQBDIFSA-N 0.000 description 14
- 239000003599 detergent Substances 0.000 description 14
- LTMHDMANZUZIPE-PUGKRICDSA-N digoxin Chemical compound C1[C@H](O)[C@H](O)[C@@H](C)O[C@H]1O[C@@H]1[C@@H](C)O[C@@H](O[C@@H]2[C@H](O[C@@H](O[C@@H]3C[C@@H]4[C@]([C@@H]5[C@H]([C@]6(CC[C@@H]([C@@]6(C)[C@H](O)C5)C=5COC(=O)C=5)O)CC4)(C)CC3)C[C@@H]2O)C)C[C@@H]1O LTMHDMANZUZIPE-PUGKRICDSA-N 0.000 description 14
- LTMHDMANZUZIPE-UHFFFAOYSA-N digoxine Natural products C1C(O)C(O)C(C)OC1OC1C(C)OC(OC2C(OC(OC3CC4C(C5C(C6(CCC(C6(C)C(O)C5)C=5COC(=O)C=5)O)CC4)(C)CC3)CC2O)C)CC1O LTMHDMANZUZIPE-UHFFFAOYSA-N 0.000 description 14
- 239000012528 membrane Substances 0.000 description 14
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- HEMHJVSKTPXQMS-UHFFFAOYSA-M Sodium hydroxide Chemical compound [OH-].[Na+] HEMHJVSKTPXQMS-UHFFFAOYSA-M 0.000 description 12
- 210000002966 serum Anatomy 0.000 description 12
- 239000000243 solution Substances 0.000 description 12
- 239000002904 solvent Substances 0.000 description 12
- 230000008859 change Effects 0.000 description 11
- XZKIHKMTEMTJQX-UHFFFAOYSA-N 4-Nitrophenyl Phosphate Chemical compound OP(O)(=O)OC1=CC=C([N+]([O-])=O)C=C1 XZKIHKMTEMTJQX-UHFFFAOYSA-N 0.000 description 10
- FAPWRFPIFSIZLT-UHFFFAOYSA-M Sodium chloride Chemical compound [Na+].[Cl-] FAPWRFPIFSIZLT-UHFFFAOYSA-M 0.000 description 10
- 238000002835 absorbance Methods 0.000 description 10
- 239000010408 film Substances 0.000 description 10
- 102000004169 proteins and genes Human genes 0.000 description 10
- 108090000623 proteins and genes Proteins 0.000 description 10
- -1 sterol esters Chemical class 0.000 description 10
- 239000007864 aqueous solution Substances 0.000 description 9
- 238000012216 screening Methods 0.000 description 9
- RTZKZFJDLAIYFH-UHFFFAOYSA-N Diethyl ether Chemical compound CCOCC RTZKZFJDLAIYFH-UHFFFAOYSA-N 0.000 description 8
- JZNWSCPGTDBMEW-UHFFFAOYSA-N Glycerophosphorylethanolamin Natural products NCCOP(O)(=O)OCC(O)CO JZNWSCPGTDBMEW-UHFFFAOYSA-N 0.000 description 8
- 241000283973 Oryctolagus cuniculus Species 0.000 description 8
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- 239000004472 Lysine Substances 0.000 description 7
- 239000000370 acceptor Substances 0.000 description 7
- 235000012000 cholesterol Nutrition 0.000 description 7
- 230000008878 coupling Effects 0.000 description 7
- 238000010168 coupling process Methods 0.000 description 7
- 239000007788 liquid Substances 0.000 description 7
- 239000008363 phosphate buffer Substances 0.000 description 7
- 238000002360 preparation method Methods 0.000 description 7
- 239000000126 substance Substances 0.000 description 7
- 108091003079 Bovine Serum Albumin Proteins 0.000 description 6
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- 229940098773 bovine serum albumin Drugs 0.000 description 6
- 239000003153 chemical reaction reagent Substances 0.000 description 6
- 238000006911 enzymatic reaction Methods 0.000 description 6
- 235000013305 food Nutrition 0.000 description 6
- 229920002521 macromolecule Polymers 0.000 description 6
- BTBUEUYNUDRHOZ-UHFFFAOYSA-N Borate Chemical compound [O-]B([O-])[O-] BTBUEUYNUDRHOZ-UHFFFAOYSA-N 0.000 description 5
- 241000700199 Cavia porcellus Species 0.000 description 5
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- 239000002609 medium Substances 0.000 description 5
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- 239000012071 phase Substances 0.000 description 5
- 150000008104 phosphatidylethanolamines Chemical class 0.000 description 5
- 150000003384 small molecules Chemical class 0.000 description 5
- TZCPCKNHXULUIY-RGULYWFUSA-N 1,2-distearoyl-sn-glycero-3-phosphoserine Chemical compound CCCCCCCCCCCCCCCCCC(=O)OC[C@H](COP(O)(=O)OC[C@H](N)C(O)=O)OC(=O)CCCCCCCCCCCCCCCCC TZCPCKNHXULUIY-RGULYWFUSA-N 0.000 description 4
- BTJIUGUIPKRLHP-UHFFFAOYSA-N 4-nitrophenol Chemical compound OC1=CC=C([N+]([O-])=O)C=C1 BTJIUGUIPKRLHP-UHFFFAOYSA-N 0.000 description 4
- XKRFYHLGVUSROY-UHFFFAOYSA-N Argon Chemical compound [Ar] XKRFYHLGVUSROY-UHFFFAOYSA-N 0.000 description 4
- ZWZWYGMENQVNFU-UHFFFAOYSA-N Glycerophosphorylserin Natural products OC(=O)C(N)COP(O)(=O)OCC(O)CO ZWZWYGMENQVNFU-UHFFFAOYSA-N 0.000 description 4
- 239000000232 Lipid Bilayer Substances 0.000 description 4
- 230000001413 cellular effect Effects 0.000 description 4
- 229940093541 dicetylphosphate Drugs 0.000 description 4
- 238000001704 evaporation Methods 0.000 description 4
- 230000008020 evaporation Effects 0.000 description 4
- 230000002163 immunogen Effects 0.000 description 4
- 238000010348 incorporation Methods 0.000 description 4
- 230000001404 mediated effect Effects 0.000 description 4
- 239000010452 phosphate Substances 0.000 description 4
- 239000011780 sodium chloride Substances 0.000 description 4
- 239000000725 suspension Substances 0.000 description 4
- LENZDBCJOHFCAS-UHFFFAOYSA-N tris Chemical compound OCC(N)(CO)CO LENZDBCJOHFCAS-UHFFFAOYSA-N 0.000 description 4
- UHOVQNZJYSORNB-UHFFFAOYSA-N Benzene Chemical compound C1=CC=CC=C1 UHOVQNZJYSORNB-UHFFFAOYSA-N 0.000 description 3
- 101100080807 Drosophila melanogaster mt:ND2 gene Proteins 0.000 description 3
- LYCAIKOWRPUZTN-UHFFFAOYSA-N Ethylene glycol Chemical compound OCCO LYCAIKOWRPUZTN-UHFFFAOYSA-N 0.000 description 3
- VEXZGXHMUGYJMC-UHFFFAOYSA-N Hydrochloric acid Chemical compound Cl VEXZGXHMUGYJMC-UHFFFAOYSA-N 0.000 description 3
- MHAJPDPJQMAIIY-UHFFFAOYSA-N Hydrogen peroxide Chemical compound OO MHAJPDPJQMAIIY-UHFFFAOYSA-N 0.000 description 3
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- 241001465754 Metazoa Species 0.000 description 3
- OKKJLVBELUTLKV-UHFFFAOYSA-N Methanol Chemical compound OC OKKJLVBELUTLKV-UHFFFAOYSA-N 0.000 description 3
- 102100028488 NADH-ubiquinone oxidoreductase chain 2 Human genes 0.000 description 3
- 101150102231 ND2 gene Proteins 0.000 description 3
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- 239000004098 Tetracycline Substances 0.000 description 3
- ZMANZCXQSJIPKH-UHFFFAOYSA-N Triethylamine Chemical compound CCN(CC)CC ZMANZCXQSJIPKH-UHFFFAOYSA-N 0.000 description 3
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- KXGVEGMKQFWNSR-LLQZFEROSA-N deoxycholic acid Chemical compound C([C@H]1CC2)[C@H](O)CC[C@]1(C)[C@@H]1[C@@H]2[C@@H]2CC[C@H]([C@@H](CCC(O)=O)C)[C@@]2(C)[C@@H](O)C1 KXGVEGMKQFWNSR-LLQZFEROSA-N 0.000 description 3
- RNPXCFINMKSQPQ-UHFFFAOYSA-N dicetyl hydrogen phosphate Chemical compound CCCCCCCCCCCCCCCCOP(O)(=O)OCCCCCCCCCCCCCCCC RNPXCFINMKSQPQ-UHFFFAOYSA-N 0.000 description 3
- LOKCTEFSRHRXRJ-UHFFFAOYSA-I dipotassium trisodium dihydrogen phosphate hydrogen phosphate dichloride Chemical compound P(=O)(O)(O)[O-].[K+].P(=O)(O)([O-])[O-].[Na+].[Na+].[Cl-].[K+].[Cl-].[Na+] LOKCTEFSRHRXRJ-UHFFFAOYSA-I 0.000 description 3
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- 239000000787 lecithin Substances 0.000 description 3
- 230000002934 lysing effect Effects 0.000 description 3
- BOPGDPNILDQYTO-NNYOXOHSSA-N nicotinamide-adenine dinucleotide Chemical compound C1=CCC(C(=O)N)=CN1[C@H]1[C@H](O)[C@H](O)[C@@H](COP(O)(=O)OP(O)(=O)OC[C@@H]2[C@H]([C@@H](O)[C@@H](O2)N2C3=NC=NC(N)=C3N=C2)O)O1 BOPGDPNILDQYTO-NNYOXOHSSA-N 0.000 description 3
- NBIIXXVUZAFLBC-UHFFFAOYSA-K phosphate Chemical compound [O-]P([O-])([O-])=O NBIIXXVUZAFLBC-UHFFFAOYSA-K 0.000 description 3
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- NGNBDVOYPDDBFK-UHFFFAOYSA-N 2-[2,4-di(pentan-2-yl)phenoxy]acetyl chloride Chemical compound CCCC(C)C1=CC=C(OCC(Cl)=O)C(C(C)CCC)=C1 NGNBDVOYPDDBFK-UHFFFAOYSA-N 0.000 description 2
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- ZXFXBSWRVIQKOD-UHFFFAOYSA-N trans-heptachlor epoxide Chemical class ClC1=C(Cl)C2(Cl)C3C4OC4C(Cl)C3C1(Cl)C2(Cl)Cl ZXFXBSWRVIQKOD-UHFFFAOYSA-N 0.000 description 1
- 238000012546 transfer Methods 0.000 description 1
- 238000011282 treatment Methods 0.000 description 1
- 150000003626 triacylglycerols Chemical class 0.000 description 1
- 229960003726 vasopressin Drugs 0.000 description 1
- 235000019155 vitamin A Nutrition 0.000 description 1
- 239000011719 vitamin A Substances 0.000 description 1
- 235000019166 vitamin D Nutrition 0.000 description 1
- 239000011710 vitamin D Substances 0.000 description 1
- 150000003710 vitamin D derivatives Chemical class 0.000 description 1
- 235000019165 vitamin E Nutrition 0.000 description 1
- 229940046009 vitamin E Drugs 0.000 description 1
- 239000011709 vitamin E Substances 0.000 description 1
- 229940045997 vitamin a Drugs 0.000 description 1
- 229940046008 vitamin d Drugs 0.000 description 1
- 239000011800 void material Substances 0.000 description 1
Classifications
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07J—STEROIDS
- C07J51/00—Normal steroids with unmodified cyclopenta(a)hydrophenanthrene skeleton not provided for in groups C07J1/00 - C07J43/00
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/10—Dispersions; Emulsions
- A61K9/127—Liposomes
- A61K9/1271—Non-conventional liposomes, e.g. PEGylated liposomes, liposomes coated with polymers
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N33/00—Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
- G01N33/48—Biological material, e.g. blood, urine; Haemocytometers
- G01N33/50—Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
- G01N33/53—Immunoassay; Biospecific binding assay; Materials therefor
- G01N33/536—Immunoassay; Biospecific binding assay; Materials therefor with immune complex formed in liquid phase
- G01N33/542—Immunoassay; Biospecific binding assay; Materials therefor with immune complex formed in liquid phase with steric inhibition or signal modification, e.g. fluorescent quenching
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S435/00—Chemistry: molecular biology and microbiology
- Y10S435/81—Packaged device or kit
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S435/00—Chemistry: molecular biology and microbiology
- Y10S435/966—Chemistry: molecular biology and microbiology involving an enzyme system with high turnover rate or complement magnified assay, e.g. multi-enzyme systems
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S435/00—Chemistry: molecular biology and microbiology
- Y10S435/975—Kit
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S436/00—Chemistry: analytical and immunological testing
- Y10S436/829—Liposomes, e.g. encapsulation
Abstract
1044, 40 SSKa Abstract of the Disclosure An immunoassay method utilizes antigen tagged, enzyme encapsulating liposomes which are immunospecifically ruptured in the presence of cognate antibody and active complement. A
homogeneous phase reaction occurs with the antibody and complement acting to release the enzyme if an immunospecific antigen-anti-body complex is formed at the surface of the liposome. The posi-tions of the antigen and antibody can be reversed.
homogeneous phase reaction occurs with the antibody and complement acting to release the enzyme if an immunospecific antigen-anti-body complex is formed at the surface of the liposome. The posi-tions of the antigen and antibody can be reversed.
Description
~L~7~
Background of the Invention There hasalways been a need ~or high volume screening assays to identify the presence or absence of antigenic materials, anti-bodies and analytes in a large nu~ber of different sampling situa-tions. Various test methods have been used in the past includinggas chromatography, mass spectrometry, liquid chromatography and various bioassay methods. Often these methods are time consuming, expensive and cannot be applied to large scale screening programs in an efficient manner.
It has been suggested that immunoassay methods could be used for such screening since immunoassays are known to be easily designed to be specific, highly sensitlve and simple to perform. Radioim-munoassays for example have found a large market and use in connection with clinical diagnostics. However, RIA procedures arP often in-compatible with large scale screening programs. Radiotracers used have inherently limited stability and special disposal and personnel screening procedures are often required. Sophisticated instrumenta-tion is often necessary. For certain uses RIA may create potential hazards as in food processing environments.
Other techniques have been developed such as fluorescent or enzymatic immunoassay techniques whicn are useful in that potentially hazardous reagents are avoided. However, often these ~ethods require separation by filtration or centrifugation steps in proced~ures used.
. ~
c4 ~o ss~ 75t7 Such separations make test procedures inherently slower and diffi-cult to automate.
In a more recent development, enzyme labeled antigen is used which requires no bound-free separation and thus can be performed quickly with excellent sensitivity. Such a system can be automated for high volume assays as in EMIT system d;sclosed by Rosenthal, A.F., Vargas, M.G. and Klass, C.S. (1976) Clin Chem. 22, 1899.
This system utilizes a mode of coupling antigen to enzyme which is quite critical and can result in the system being not readily adapted to different analyses without extens;ve development for each new system.
Recently, there have been reports of liposomes which can carry enzymes or substrates and be labeled with antigens or anti-bodies. Liposomes labeled with` antigens at ~heir external surface and containing an enzyme entrapped in their internal volume are reported-ly mixed with cognate antibody and complement to determine whether or not the liposomes permit release of the entrapped envme. This determination is reported made by detecting enzymatic activity which is physically released from the liposomes after separating liposomes from surrounding medium. See Uemura, K. and Kinsky, S.C. (1972) Biochemistry, 11, 4085-4094 and Kataoka, T., William-son, J. and Kinsky, S. (1973) BiochemicsetBiophysica Acta 298, 158-179. However, there has been no recognition that such lipo-somes when suitably formed with suitable high signal to noise ratios can be useful for immunoassay procedures which avoid the use of separation steps and permit testing in homogeneous phase reactions. Moreover there are reported difficulties in preparing pr;or art immunospec;fic liposomes, G.H. Strejan, P.M. Smith, C.W. Grant and D. Surlan, "Naturally Occurring Antibodies To Lipo-somes", The Journal of Immunology, Vol. 123, No. 1, July 1979, 370-378. Furthermore, it has long been established that dif-fusion of macromolecules such as enzymes through lesions produced by complement in bilayer membranes is very much slower than that of small molecules (Green,H., Barrow,P. and Goldberg, B. [1959] J. Exp. Med. _10, 699).
lC44/7~0 .~S~
-3- ~ ~ 7S~
1 Summary of the Invention It is an object of this invention to provide immunoassay products and methods for use in rapid and simplified testing procedures which can quantitatively and/or qualitatively determ-ine the presence or absence of antigenic materials or antibodies.
It is another object of this invention to provide methods inaccordance with the preceding object which can be carried out by relatively untrained personnel with test results determined in a single step with ease of resulting readout and without the need for any separation step after the test reaction.
It is another object of this invention to provide a homo-geneous phase reaction in which antigen or antibody-tagged enzyme-laden liposomes are immunospecifically caused to release enzyme in the presence of cognate antigen or antibody and active complement.
It is still another object of this invention to provide lipo-somes labeled with an antigen or antibody and carrying an enzyme yet having a signal to noise ratio no less than 5 and preferably having a stability of at least about 60 days when carried in a liquid.
According to the invention a liposome is labeled with an anti-gen or antibody and carries an enzyme, yet, has a signal to noiseratio of no less than 5. The enzyme is encapsulated within the liposome. Preferably the liposome is carried in a liquid nedia and is stable for a period of at least 6~ days. Pref-erably the liposome signal to noise ratio is high and above 60 with stability over six months at 4~C under inert gas atmosphere. In a kit form the liposome of this invention is sold along with vials of cognate antibodies or antigen which are immunospecific for the antigen or antibody attached to the surface of the liposome, and complement.
According to the method of this invention, an immunoassay method comprises forming a mixture of (a) liposomes labeled with an antigen or antibody carrying an enzyme and having a signal to noise ratio of no less than 5, (b) a substrate for said enzyme, (c) a test material to be tested for specif~c antigen or antibody activity and (d) complement. The mixture is observed and the presence of enzymatic activity detected as by color change visible to the eye, spectro-scopic readout or the like. Preferably, additional cognate antigen or antibody as attached to the liposomes is admixed with the mixture lC44/740 SS.~ `
1/7/&1 _4_ ~L~7~ 3 1 and the test is carried out for the same antigen or antibody as is attached to the liposornes. If immunospecif;c antigen or anti-body tested for, is present in the test material, the free anti-body or antigen as the case may be, in the mixture reacts with that antigen or antibody leaving the liposome ;ntact, thus pre-venting complement attack while if the cognate is not present in the test material the liposome label is reacted and en y me ac-tivity becomes detectable. The amount of cognate in the test sample if present can permit some complement attack if insuf-ficient to react with all of the free cognate in the test mix-ture, and a portion of the enzymatic actiYity can then be detected.
In some cases, the immunoassay method may bc employed directly to detect any of the elements of the group antigen, antibody or complement. In the direct method an incomplete mixture lacking but one element of the group antigen, antibody or comDlement is prepared and the presence of the missing element in a test sample is assessed by the extent to which addition of the sample to the incomplete mixture promotes lysis of the liposome by immune spec;fic attack on the liposomal membrane or exposure of the encapsulated enzyme - 20 to the fluid around the liposon~e. When the test material is to be tested for the cognate antibody or antigen to that which acts as a label for the liposome, no antigen or antibody need be added to the mixture. A direct immunoassay rnethod for antigen or anti-body would comprise a mixture of:
(a) li~osomes labeled with one of an antigen ~r its cocnate antibody, carrying an enzyrne and having a signal to noise of no less than 5, (b) a substrate for said enzyme, (c) a test material to be tested for the one antigen or cog-3~ nate antibody, (d) complement.
If the aim of a direct immunoassay is to assess the active complement in a test sample the method ~ould comprise a mixture of:
1~44/732 SSK~
1/2/~
-4A- ~L~17~
1 (a) liposomes labeled with one of an antigen or its cognate antibody, carrying an enzyme and having a signal to noise of no less than 5, (b) a substrate for said enzyme, (c) a test material to be tested for complement, (d) free cognate of the other of said one antigen or antibody.
A preferred immunoassay method preferably comprises, forming a mixture of:
(a) liposomes labeled with one of an antigen or its cognate antibody carrying an enzyme and having a signal to noise ratio of no less than 5, (b) a substrate for said enzyme, (c) a test material to be tested for the one antigen or cognate antibody, (d) complement, and (e) free cognate of the other of said one antigen Dr anti-body, and detecting the presence or absence of enzymatic activity in said mixture. In this method the antigen to be tested for can be used to label the liposomes and free cognate antibody used. Alternately .......
~"-" ,.
b lC44 `
SSKa 1 2/28/7g l the antibody to be tested for can be used to label the liposome and free cognate antibody used.
Pre~erably the method is carried out as a one-step method and all mater;als are added to a single vial with incubation at standard immunological conditions as for example 37~C, or in a range of from 4C to 45C for periods o~ from about l second to 120 minu~es.
Alternately all but the enzyme substrate are adm;xed and incubated for 5 to about 120 minutes or more and then this admixture is added to an enzyme substrate and the result determined.
A kit for detecting one of an antigen or ;ts cognate antibody preferably has a first container carrying liposomes labeled with one of the antigen or its cognate antibody suspended in an appropriate buffer. A second container carries powderedlyophilized or frozen concentrated antibody or antigen which is the cognate of that on the liposome. A third vial carries powdered or frozen concentrated complement which can be in the ~orm of guinea pig serum and a fourth container carries an enzyme substrate ~or the enzyme which may be in liquid or powder form. Buffer is also included in another con-tainer.
A one-step method can be uséd where all component$ are mixed and incubated. However, in some cases, the procedure may be carried out in two or more steps with some o~ the materials incubated together prior to comple~e mixing. In all cases, no separation is carried out a~ter the immune reaction or ab~ence o~ it and a direct reading is made of the reaction materials to determine the presence or absence of the antigen or antibody 1n the test specimen, by detect-ing enzyme activity or reaction with the substrate.
It is a feature of ~his inventlon that the test can be carried out quickly by untrained personnel at relatively low cost. The readout can be subjective, e.g.7 visual as by a color change when qualitative readouts lC4 `~ ~L~7 ~2/29/80 1 are~desired. Semi-quantitative readouts may be obtained subjectively, as when deep to light color changes may occur. Spectrophotometric methods and the like can also be used to detect the presence or ab-sence of enzymatic activity in the presence of substrate which indi-cates lysing of the liposome or immune specific attack on the lipo-somal membrane so as to expose the enzyme to the substrate.
The exposure of enzyme activity will occur when the immune reac-tion occurs to form an immune complex and affect the bilayer or enzyme enclosing membrane of the liposomes. When the antibody or antigen, as the case may be, in the system reacts with the op-posite with which the liposome~is labeled in the presence of active complement, the enzyme is released. However, if the test sample contains the antigen or antibody to be tested for, reaction ot tne cognate in the media prevents or reduces reaction with the cognate label and thus prevents the enzyme fram being detected in the sub-strate indicating a positive for the antigen or antibody being tested for.
Brief Description of Preferred Embod-ments The liposomes of the present invent~on are sometimes called smectic mesophases or synthetic vesicles. They are in fact dry lipid films suspended in aqueous media as have been described by Uemura, K. and Kinsky, S.C. (1972) Biochemistry 11~ 40~5-4094. Liposomes are believed to consist of 1ipid bilayers which separate an internal aqueous compartment from an external aqueous media and are in fact prototypes of biological membranes. The liposomes mimic the prop-erties of biological membranes. As is known, they can be made to contain either enV me substrates or enzymes. For purposes of the present invention, the liposomes contain an enzyme and have an outer surface substant;ally free of the enzyme which outer surface encloses the enzyme such that the catalytic action of the enzyme is not detectable unless the outer surface encapsulating the membrane is disrupted and is labeled with an antigen or its cognate antibody depending upon the test to be carried out. Preferably if one lC44/740 SS~
_7_ ~ ~ 7 ~r~
1 is testing for the antibody, the liposome will be labeled with that antibody while if one is testing for the antigen, the liposome will be labeled with the antigen.
Liposomes have been known in the art. However, the art is not believed to have previously obtained liposomes haYing enzymes contained therein which liposomes have signal to noise rat;os of no less than 5. This is probably so since the art has not recog-nized the advantage of obtaining such liposomes for use in immuno-assay procedures~
The signal to noise ratio should be 5 or higher such as pref-erably at least 60, and can be 1,000 or more so that the lipo-somes contain and sequester the enzyme from the substrate. Thus no detectable enzymatic activity occurs in the absence of an antigen-antibody complex or immune complex being formed to rupture or render porous the liposome membrane. In some cases, the signal to noise ratio can be 5 or higher in liposomes in accordance with this invention, so long as no detectable enzymatic activity occurs in the absence of an antigen-antibody complex or immune complex being formed. The signal to noise ratio as known in the art is obtained by comparing a first vial or noise vial, of liposome labeled with one of antigen or cognate antibody suspended in an isotonic buffer in the presence of enzyme substrate as compared to a second or signal vial containing enzyme substrate, liposome as previously described, in the presence o~ a known lysing agent such as a strong detergent. The signal to noise ratio is the test result of the enzyme reaction observed. Preferably the noise tube not containing the lysing agent is as low as possible indicating no noise thus little or no enzyme activity.
Preferably the noise is maintained low or non-existent for as long a time period as possible. In the preferred form, the noise tevel is at zero or close thereto after storage for at least sixty days or the signal to noise ratio is no less than 5. This gives good shelf life which is desirable ~hen selling test kits for use in the present invention.
1 C4~Ka ` ) ;~ 7~r7~f~3 1 In the immunoassay methods of this invention the l;posome sequesters the enzyme from the substrate and through the mediat;on of immunospecifically activated complement, otherwise latent (hidden) enzyme activity becomes apparent. The liposome en-capsulates the enzyme, i.e., the enzyme is physically trapped within a space delimited by a bilayer membrane. The physical en-capsulation also acts to sequester the enzymatic activity. Para-Nitrophenyl-phosphate (pNPP) is a substrate for the enzyme alkaline phosphatase (AP). Under alkaline conditions (pH greater than 7) AP will snip off the phosphate group from pNPP (which is colorless) producing para-Nitrophenol which under alkaline condi-t;ons is ;ntensely yellow colored. Thus, if one prepares an aqueous solution of pNPP, this solution is colorless. If one then adds AP to this solution an intense yellow color is produced quite rapidly. The liposomes used in this invention are such that they encapsulate AP and sequester this AP away from pNPP
in the surrounding aqueous solution. Thus, the l;posomes with encapsulated AP can be disperâed in pNPP solutions and very little yellow color is produced, while if the same quantity of AP which is encapsulated were to be introduced, directly, considerable color would be developed quite rapidly.
For the above reasons in constructing liposomes, enzymes whose activity can be effectively sequestered by the intact lipid bilayer are selected resulting in a signal to noise ratio greater than 5. It is preferred not to use enzymes which:
(a) would be ~dsorbed to the outer surface o~ the lipo-some membrane, and thus at all times accessible to sub-strate in the surrounding medium.
(b) would be included in the bilayer itself such that it would span both the internal and external media and might lC4~ ~0 SSka 1?/29/80 g 1 likewise be readily accessible to substrate in the sur-rounding medium.
(c) react w;th substrates which can read;ly diffuse through an intact lipid bilayer (typically such would be non-polar, lipid-soluble, small molecules). In this case even though the enzyme might be encapsulated, its activi-ty would not be sequestered ;nasmuch as substrate in the : surrounding medium, by diffusion through the lipid bilayer, could gain access to the enapsulated enzyme.
The structure of sequestration is important in the context of an immunoassay using the present invention. It is because this sequestration can be broken immunospecifically that one may obtain a homogeneous assay, i.e., it is not necessary to have physical separation of bound from free signal by centrifugation, chromatography, filtration, solid phase immob;lization, etc.
Such separations are time-consuming, require special instrumenta-tion or apparatus, and are difficult to automate.
Liposomes are prepared from amphiphilic lipids. Lipids may be defined generally as molecules of intermediate molecular weight 1 C~
SSka 12/28/79 ~7~7~
1 (150-3,000 daltons) consisting mainly of saturated or unsaturated and/or aromatic or aliphat;c hydrocarbon moieties. Amphilic lipids are those which contain both water soluble and water insoluble regions.
Small (J. Am. Oil Chem. Soc. 4S, 108-117 ~1968]) provides a classification of lipids based upon their interaction with water, both in bulk and at the surface. Such lipids useful in the present invention are defined below:
Class I - Insoluble, Non-Swelling Amphiphilic Lipids di- and triglycerides, long chain protonated fatty acids, sterol esters, long-chain alcohols, phytols, retinals, Vitamin A, Yitamin K, Vitamin E and many sterols such as cholesterol, - desmosterol, Vitamin D, and a number of hormones.
Class II - Insoluble, Swelling Amphiphilic Lipids Lecithins, phosphatidyl ethanolam~nes, phosphatidyl inositol, sphingo~yelin, cerebrosides, phosphatidic acid, plasmalogens, phosphatidyl serine, cardiolipins, and certain plant sulfo-lipids.
Class III A - Soluble Amphiphiles, Type A
Form liquid crystalllne phases when small quantities of water are added (lyotropic mesomorph~sm). Includes many of the classic anionic, cationic and nonlonic detergents.
Class III B -Soluble Amphiphiles Type B
Will not form liquld crystals, no clear-cut polarity - bile salts.
Class II lipids are particularly appropriate for the formation of 1iposomes, and the latter can often be prepared from such lipids alone. For example~ quite large vesicles can be prepared from phosphatidyl ethanolamine or phosphatidyl serine according to.Papahadjopoulos Annals N.Y. Acad. of Sc~. 308, lg78. In some cases, however, it is useful to incorporate Class I or Class III lipids into the vesicle lC4 1S2/28/79 ~L~ G~
-tl-1 bilayer for structural purposes - to produce less fluid bilayers e.g. by incorporation of cholesterol or to promote greater spacing between adjacent bilayers as for example by electrostatic repulsion resultant from the incorporation of anionic - dicetyl phosphate -or cationic-stearylamine lipids into the bilayers. Procedures for preparing a variety of vesicular structures have been described (Szoka and Papahadjopoulos Proc. Nat. Acad. Sci. 75, 4194-4198 C1978]). Many of these structures with appropriate modification can be adapted to the present inventions. In selecting an appropriate mode of preparation, several criteria are preferably applied as follows:
1. The mode of incorporation of enzyme into the liposomes should not result in inactivation or denaturation of the enzyme.
Thus, prolonged exposure to elevated temperatures or denaturing organic solvents is to be avoided.
Background of the Invention There hasalways been a need ~or high volume screening assays to identify the presence or absence of antigenic materials, anti-bodies and analytes in a large nu~ber of different sampling situa-tions. Various test methods have been used in the past includinggas chromatography, mass spectrometry, liquid chromatography and various bioassay methods. Often these methods are time consuming, expensive and cannot be applied to large scale screening programs in an efficient manner.
It has been suggested that immunoassay methods could be used for such screening since immunoassays are known to be easily designed to be specific, highly sensitlve and simple to perform. Radioim-munoassays for example have found a large market and use in connection with clinical diagnostics. However, RIA procedures arP often in-compatible with large scale screening programs. Radiotracers used have inherently limited stability and special disposal and personnel screening procedures are often required. Sophisticated instrumenta-tion is often necessary. For certain uses RIA may create potential hazards as in food processing environments.
Other techniques have been developed such as fluorescent or enzymatic immunoassay techniques whicn are useful in that potentially hazardous reagents are avoided. However, often these ~ethods require separation by filtration or centrifugation steps in proced~ures used.
. ~
c4 ~o ss~ 75t7 Such separations make test procedures inherently slower and diffi-cult to automate.
In a more recent development, enzyme labeled antigen is used which requires no bound-free separation and thus can be performed quickly with excellent sensitivity. Such a system can be automated for high volume assays as in EMIT system d;sclosed by Rosenthal, A.F., Vargas, M.G. and Klass, C.S. (1976) Clin Chem. 22, 1899.
This system utilizes a mode of coupling antigen to enzyme which is quite critical and can result in the system being not readily adapted to different analyses without extens;ve development for each new system.
Recently, there have been reports of liposomes which can carry enzymes or substrates and be labeled with antigens or anti-bodies. Liposomes labeled with` antigens at ~heir external surface and containing an enzyme entrapped in their internal volume are reported-ly mixed with cognate antibody and complement to determine whether or not the liposomes permit release of the entrapped envme. This determination is reported made by detecting enzymatic activity which is physically released from the liposomes after separating liposomes from surrounding medium. See Uemura, K. and Kinsky, S.C. (1972) Biochemistry, 11, 4085-4094 and Kataoka, T., William-son, J. and Kinsky, S. (1973) BiochemicsetBiophysica Acta 298, 158-179. However, there has been no recognition that such lipo-somes when suitably formed with suitable high signal to noise ratios can be useful for immunoassay procedures which avoid the use of separation steps and permit testing in homogeneous phase reactions. Moreover there are reported difficulties in preparing pr;or art immunospec;fic liposomes, G.H. Strejan, P.M. Smith, C.W. Grant and D. Surlan, "Naturally Occurring Antibodies To Lipo-somes", The Journal of Immunology, Vol. 123, No. 1, July 1979, 370-378. Furthermore, it has long been established that dif-fusion of macromolecules such as enzymes through lesions produced by complement in bilayer membranes is very much slower than that of small molecules (Green,H., Barrow,P. and Goldberg, B. [1959] J. Exp. Med. _10, 699).
lC44/7~0 .~S~
-3- ~ ~ 7S~
1 Summary of the Invention It is an object of this invention to provide immunoassay products and methods for use in rapid and simplified testing procedures which can quantitatively and/or qualitatively determ-ine the presence or absence of antigenic materials or antibodies.
It is another object of this invention to provide methods inaccordance with the preceding object which can be carried out by relatively untrained personnel with test results determined in a single step with ease of resulting readout and without the need for any separation step after the test reaction.
It is another object of this invention to provide a homo-geneous phase reaction in which antigen or antibody-tagged enzyme-laden liposomes are immunospecifically caused to release enzyme in the presence of cognate antigen or antibody and active complement.
It is still another object of this invention to provide lipo-somes labeled with an antigen or antibody and carrying an enzyme yet having a signal to noise ratio no less than 5 and preferably having a stability of at least about 60 days when carried in a liquid.
According to the invention a liposome is labeled with an anti-gen or antibody and carries an enzyme, yet, has a signal to noiseratio of no less than 5. The enzyme is encapsulated within the liposome. Preferably the liposome is carried in a liquid nedia and is stable for a period of at least 6~ days. Pref-erably the liposome signal to noise ratio is high and above 60 with stability over six months at 4~C under inert gas atmosphere. In a kit form the liposome of this invention is sold along with vials of cognate antibodies or antigen which are immunospecific for the antigen or antibody attached to the surface of the liposome, and complement.
According to the method of this invention, an immunoassay method comprises forming a mixture of (a) liposomes labeled with an antigen or antibody carrying an enzyme and having a signal to noise ratio of no less than 5, (b) a substrate for said enzyme, (c) a test material to be tested for specif~c antigen or antibody activity and (d) complement. The mixture is observed and the presence of enzymatic activity detected as by color change visible to the eye, spectro-scopic readout or the like. Preferably, additional cognate antigen or antibody as attached to the liposomes is admixed with the mixture lC44/740 SS.~ `
1/7/&1 _4_ ~L~7~ 3 1 and the test is carried out for the same antigen or antibody as is attached to the liposornes. If immunospecif;c antigen or anti-body tested for, is present in the test material, the free anti-body or antigen as the case may be, in the mixture reacts with that antigen or antibody leaving the liposome ;ntact, thus pre-venting complement attack while if the cognate is not present in the test material the liposome label is reacted and en y me ac-tivity becomes detectable. The amount of cognate in the test sample if present can permit some complement attack if insuf-ficient to react with all of the free cognate in the test mix-ture, and a portion of the enzymatic actiYity can then be detected.
In some cases, the immunoassay method may bc employed directly to detect any of the elements of the group antigen, antibody or complement. In the direct method an incomplete mixture lacking but one element of the group antigen, antibody or comDlement is prepared and the presence of the missing element in a test sample is assessed by the extent to which addition of the sample to the incomplete mixture promotes lysis of the liposome by immune spec;fic attack on the liposomal membrane or exposure of the encapsulated enzyme - 20 to the fluid around the liposon~e. When the test material is to be tested for the cognate antibody or antigen to that which acts as a label for the liposome, no antigen or antibody need be added to the mixture. A direct immunoassay rnethod for antigen or anti-body would comprise a mixture of:
(a) li~osomes labeled with one of an antigen ~r its cocnate antibody, carrying an enzyrne and having a signal to noise of no less than 5, (b) a substrate for said enzyme, (c) a test material to be tested for the one antigen or cog-3~ nate antibody, (d) complement.
If the aim of a direct immunoassay is to assess the active complement in a test sample the method ~ould comprise a mixture of:
1~44/732 SSK~
1/2/~
-4A- ~L~17~
1 (a) liposomes labeled with one of an antigen or its cognate antibody, carrying an enzyme and having a signal to noise of no less than 5, (b) a substrate for said enzyme, (c) a test material to be tested for complement, (d) free cognate of the other of said one antigen or antibody.
A preferred immunoassay method preferably comprises, forming a mixture of:
(a) liposomes labeled with one of an antigen or its cognate antibody carrying an enzyme and having a signal to noise ratio of no less than 5, (b) a substrate for said enzyme, (c) a test material to be tested for the one antigen or cognate antibody, (d) complement, and (e) free cognate of the other of said one antigen Dr anti-body, and detecting the presence or absence of enzymatic activity in said mixture. In this method the antigen to be tested for can be used to label the liposomes and free cognate antibody used. Alternately .......
~"-" ,.
b lC44 `
SSKa 1 2/28/7g l the antibody to be tested for can be used to label the liposome and free cognate antibody used.
Pre~erably the method is carried out as a one-step method and all mater;als are added to a single vial with incubation at standard immunological conditions as for example 37~C, or in a range of from 4C to 45C for periods o~ from about l second to 120 minu~es.
Alternately all but the enzyme substrate are adm;xed and incubated for 5 to about 120 minutes or more and then this admixture is added to an enzyme substrate and the result determined.
A kit for detecting one of an antigen or ;ts cognate antibody preferably has a first container carrying liposomes labeled with one of the antigen or its cognate antibody suspended in an appropriate buffer. A second container carries powderedlyophilized or frozen concentrated antibody or antigen which is the cognate of that on the liposome. A third vial carries powdered or frozen concentrated complement which can be in the ~orm of guinea pig serum and a fourth container carries an enzyme substrate ~or the enzyme which may be in liquid or powder form. Buffer is also included in another con-tainer.
A one-step method can be uséd where all component$ are mixed and incubated. However, in some cases, the procedure may be carried out in two or more steps with some o~ the materials incubated together prior to comple~e mixing. In all cases, no separation is carried out a~ter the immune reaction or ab~ence o~ it and a direct reading is made of the reaction materials to determine the presence or absence of the antigen or antibody 1n the test specimen, by detect-ing enzyme activity or reaction with the substrate.
It is a feature of ~his inventlon that the test can be carried out quickly by untrained personnel at relatively low cost. The readout can be subjective, e.g.7 visual as by a color change when qualitative readouts lC4 `~ ~L~7 ~2/29/80 1 are~desired. Semi-quantitative readouts may be obtained subjectively, as when deep to light color changes may occur. Spectrophotometric methods and the like can also be used to detect the presence or ab-sence of enzymatic activity in the presence of substrate which indi-cates lysing of the liposome or immune specific attack on the lipo-somal membrane so as to expose the enzyme to the substrate.
The exposure of enzyme activity will occur when the immune reac-tion occurs to form an immune complex and affect the bilayer or enzyme enclosing membrane of the liposomes. When the antibody or antigen, as the case may be, in the system reacts with the op-posite with which the liposome~is labeled in the presence of active complement, the enzyme is released. However, if the test sample contains the antigen or antibody to be tested for, reaction ot tne cognate in the media prevents or reduces reaction with the cognate label and thus prevents the enzyme fram being detected in the sub-strate indicating a positive for the antigen or antibody being tested for.
Brief Description of Preferred Embod-ments The liposomes of the present invent~on are sometimes called smectic mesophases or synthetic vesicles. They are in fact dry lipid films suspended in aqueous media as have been described by Uemura, K. and Kinsky, S.C. (1972) Biochemistry 11~ 40~5-4094. Liposomes are believed to consist of 1ipid bilayers which separate an internal aqueous compartment from an external aqueous media and are in fact prototypes of biological membranes. The liposomes mimic the prop-erties of biological membranes. As is known, they can be made to contain either enV me substrates or enzymes. For purposes of the present invention, the liposomes contain an enzyme and have an outer surface substant;ally free of the enzyme which outer surface encloses the enzyme such that the catalytic action of the enzyme is not detectable unless the outer surface encapsulating the membrane is disrupted and is labeled with an antigen or its cognate antibody depending upon the test to be carried out. Preferably if one lC44/740 SS~
_7_ ~ ~ 7 ~r~
1 is testing for the antibody, the liposome will be labeled with that antibody while if one is testing for the antigen, the liposome will be labeled with the antigen.
Liposomes have been known in the art. However, the art is not believed to have previously obtained liposomes haYing enzymes contained therein which liposomes have signal to noise rat;os of no less than 5. This is probably so since the art has not recog-nized the advantage of obtaining such liposomes for use in immuno-assay procedures~
The signal to noise ratio should be 5 or higher such as pref-erably at least 60, and can be 1,000 or more so that the lipo-somes contain and sequester the enzyme from the substrate. Thus no detectable enzymatic activity occurs in the absence of an antigen-antibody complex or immune complex being formed to rupture or render porous the liposome membrane. In some cases, the signal to noise ratio can be 5 or higher in liposomes in accordance with this invention, so long as no detectable enzymatic activity occurs in the absence of an antigen-antibody complex or immune complex being formed. The signal to noise ratio as known in the art is obtained by comparing a first vial or noise vial, of liposome labeled with one of antigen or cognate antibody suspended in an isotonic buffer in the presence of enzyme substrate as compared to a second or signal vial containing enzyme substrate, liposome as previously described, in the presence o~ a known lysing agent such as a strong detergent. The signal to noise ratio is the test result of the enzyme reaction observed. Preferably the noise tube not containing the lysing agent is as low as possible indicating no noise thus little or no enzyme activity.
Preferably the noise is maintained low or non-existent for as long a time period as possible. In the preferred form, the noise tevel is at zero or close thereto after storage for at least sixty days or the signal to noise ratio is no less than 5. This gives good shelf life which is desirable ~hen selling test kits for use in the present invention.
1 C4~Ka ` ) ;~ 7~r7~f~3 1 In the immunoassay methods of this invention the l;posome sequesters the enzyme from the substrate and through the mediat;on of immunospecifically activated complement, otherwise latent (hidden) enzyme activity becomes apparent. The liposome en-capsulates the enzyme, i.e., the enzyme is physically trapped within a space delimited by a bilayer membrane. The physical en-capsulation also acts to sequester the enzymatic activity. Para-Nitrophenyl-phosphate (pNPP) is a substrate for the enzyme alkaline phosphatase (AP). Under alkaline conditions (pH greater than 7) AP will snip off the phosphate group from pNPP (which is colorless) producing para-Nitrophenol which under alkaline condi-t;ons is ;ntensely yellow colored. Thus, if one prepares an aqueous solution of pNPP, this solution is colorless. If one then adds AP to this solution an intense yellow color is produced quite rapidly. The liposomes used in this invention are such that they encapsulate AP and sequester this AP away from pNPP
in the surrounding aqueous solution. Thus, the l;posomes with encapsulated AP can be disperâed in pNPP solutions and very little yellow color is produced, while if the same quantity of AP which is encapsulated were to be introduced, directly, considerable color would be developed quite rapidly.
For the above reasons in constructing liposomes, enzymes whose activity can be effectively sequestered by the intact lipid bilayer are selected resulting in a signal to noise ratio greater than 5. It is preferred not to use enzymes which:
(a) would be ~dsorbed to the outer surface o~ the lipo-some membrane, and thus at all times accessible to sub-strate in the surrounding medium.
(b) would be included in the bilayer itself such that it would span both the internal and external media and might lC4~ ~0 SSka 1?/29/80 g 1 likewise be readily accessible to substrate in the sur-rounding medium.
(c) react w;th substrates which can read;ly diffuse through an intact lipid bilayer (typically such would be non-polar, lipid-soluble, small molecules). In this case even though the enzyme might be encapsulated, its activi-ty would not be sequestered ;nasmuch as substrate in the : surrounding medium, by diffusion through the lipid bilayer, could gain access to the enapsulated enzyme.
The structure of sequestration is important in the context of an immunoassay using the present invention. It is because this sequestration can be broken immunospecifically that one may obtain a homogeneous assay, i.e., it is not necessary to have physical separation of bound from free signal by centrifugation, chromatography, filtration, solid phase immob;lization, etc.
Such separations are time-consuming, require special instrumenta-tion or apparatus, and are difficult to automate.
Liposomes are prepared from amphiphilic lipids. Lipids may be defined generally as molecules of intermediate molecular weight 1 C~
SSka 12/28/79 ~7~7~
1 (150-3,000 daltons) consisting mainly of saturated or unsaturated and/or aromatic or aliphat;c hydrocarbon moieties. Amphilic lipids are those which contain both water soluble and water insoluble regions.
Small (J. Am. Oil Chem. Soc. 4S, 108-117 ~1968]) provides a classification of lipids based upon their interaction with water, both in bulk and at the surface. Such lipids useful in the present invention are defined below:
Class I - Insoluble, Non-Swelling Amphiphilic Lipids di- and triglycerides, long chain protonated fatty acids, sterol esters, long-chain alcohols, phytols, retinals, Vitamin A, Yitamin K, Vitamin E and many sterols such as cholesterol, - desmosterol, Vitamin D, and a number of hormones.
Class II - Insoluble, Swelling Amphiphilic Lipids Lecithins, phosphatidyl ethanolam~nes, phosphatidyl inositol, sphingo~yelin, cerebrosides, phosphatidic acid, plasmalogens, phosphatidyl serine, cardiolipins, and certain plant sulfo-lipids.
Class III A - Soluble Amphiphiles, Type A
Form liquid crystalllne phases when small quantities of water are added (lyotropic mesomorph~sm). Includes many of the classic anionic, cationic and nonlonic detergents.
Class III B -Soluble Amphiphiles Type B
Will not form liquld crystals, no clear-cut polarity - bile salts.
Class II lipids are particularly appropriate for the formation of 1iposomes, and the latter can often be prepared from such lipids alone. For example~ quite large vesicles can be prepared from phosphatidyl ethanolamine or phosphatidyl serine according to.Papahadjopoulos Annals N.Y. Acad. of Sc~. 308, lg78. In some cases, however, it is useful to incorporate Class I or Class III lipids into the vesicle lC4 1S2/28/79 ~L~ G~
-tl-1 bilayer for structural purposes - to produce less fluid bilayers e.g. by incorporation of cholesterol or to promote greater spacing between adjacent bilayers as for example by electrostatic repulsion resultant from the incorporation of anionic - dicetyl phosphate -or cationic-stearylamine lipids into the bilayers. Procedures for preparing a variety of vesicular structures have been described (Szoka and Papahadjopoulos Proc. Nat. Acad. Sci. 75, 4194-4198 C1978]). Many of these structures with appropriate modification can be adapted to the present inventions. In selecting an appropriate mode of preparation, several criteria are preferably applied as follows:
1. The mode of incorporation of enzyme into the liposomes should not result in inactivation or denaturation of the enzyme.
Thus, prolonged exposure to elevated temperatures or denaturing organic solvents is to be avoided.
2. The liposomes should be sufficiently large to incorporate enzyme activity. Structures less than 50-100 A in diameter would not encapsulate more than a few enzyme molecules in most cases and are not preferred.
3. The liposomal bilayer should be stable and relatively im-permeable. It has been shown (Kitagawa T. and Inoue K. Nature 254, 254-6 ~1975]) that incorporation o~ Class I lipid such as sterols leads to a condensing of the bilayers with resultant greater rigidity and stability and are more susceptible to complement mediated lysis.
lC44 SSka 12/28/79 ~al~7S~7~r3 1 In preparing liposomes, it is necessary that lipids - such as those of Class II - which are insoluble in water be introduced into an aqueous environment. Th;s can be ach;eved by a var;ety of methods.
By one such known method, l;p;ds are phys;cally dispersed ;nto an aqueous solution. A dry th;n film of lipids is formed on the interior surface of a suitable vessel. The aqueous solution contain-ing the substances to be entrapped with;n the l;posomes ;s then placed ;n the vessel in contact with the lipid film. The lip;d f;lm is then dispersed into the aqueous solution by vigorous ag;tation of the vessel (glass beads approximately 0.1 mm in diameter may be included ;n the vessel to accelerate this dispersion). Also, dispers;on of the lip;d f;lm may be enhanced by sonication through immersion of the vessel ;n a bath type sontcator or by immersing the probe of a sonifier lnto the aqueous solut;on. E~cess;ve sonication may in-activate enzyme and can produce very small liposomes.
Alternatively, the lipids may be dlssolved in an aqueous solutlon containing a detergent lipid of Class III A or B such as laurylsulfate or sod;um deoxycholate. The detergent is then removed (e,g. by dialysis), and the liposome b;layers are formed. ~noch and Strittmatter (Proc. Nat. Acad. Sci. 76, 145-149) have described the preparation of 1000 A diameter, s;ngle-bilayer liposomes using sod;um doxycholate as the detergent wh;ch is d;alyzed.
Another known technique involves the addition of aqueous solution to a mixture of l;p;d and a volatlle organic solvent which solvent is subsequently removed by evaporation at reduced pressure.
Szoka and Papahadjopoulos (Proc. Nat. Acad. Sci. 75, 4194-4198 ~1978]) have described preparation of liposomes wlth very large internal aqueous space by means of evaporation of organic solvents diethyl ether or ;sopropyl ether.
The physical and detergent dialys;s methods are particularly appropriate to the present invention, as these produce acceptably lC44, '-SSKa 12/2~/79 ~L~L7~7~3 1 large vesicles and are quite gentle, thus unlikely to inactivate the enzymes. In cases where organic solvent evaporation is to be employed, it is necessary that the enzyme to be encapsulated should be insensitive to that solvent. For example, vesicles of this type can be prepared containing alkaline phosphatase which enzyme is not denatured by the diethyl ether used in the process.
Enzymes suitable for use in the present invention include any of those which will result in low noise levels. A large number of known enzymes may be employed in the present invention. These vary widely in their substrates, the nature of the reaction catalyzed, stability, turnover rate, optimal reaction conditions (pH, ionic strength, temperature), and the like. The International Union of Biochemists has classified various enzymes according to the nature of the reaction catalyzed.
There are a number of criteria which may be applied in the selection of a given enzyme for commerclal application. These enzymes which are at present available in but trace amounts, are less desirable than those which are abundant and may be purchased from commercial sources. The enzyme should be stable when stored at temperatures which are convenient at the site of commercial application, e.g.
4C, for a period of at least 3 months. The catalytic activity or turnover number of the enzyme should be sufficiently high as to provide detectable reaction in a relatively short time period, i.e.
a few secondsto 120 minutes. The cataly~ic activity of the enzyme should be conveniently detectable by mPans available to the commercial user, e.g. the catalyzed reaction produces an increase or decrease in the absorption of light in the ultraviolet or the visible region, i.e.
in the range of 250-750 nm.
Preferably the enzyme should be one which is not present at significant levels in the sample to be tested and is not susceptible lC4 ~0 SSk~
12~2~/80 ~ ~L~ 7~C~
1 to inh;bition by substances commonly found in the test sample.
The enzyme should not be inactivated or poisoned by the lipids employed in liposome preparation and is not inactivated or de-natured durin~ the liposome preparation. The enzyme selected should be one which may be fully encapsulated. Such enzymes in nature are found in the cellular cytoplasm or circulate freely in extracellular fluids. Not desirable are the natural membrane proteins. These in nature are found in association ~ith cellular membranes and have hydrophobic surface(s) which anchor them to the bilayer. Commonly such enzymes span the bilayer with their catalytic sites exposed to the surrounding aqueous medium.
The following table indicates enzymes of particular interest classified according to the International Union of Biochemists:
1. Oxidoreductases 1.1 Acting on the CH-OH group of donors 1.1.1 With NAD or NADP as acceptor 1. alcohol dehydrogenase 6. glycerol dehydrogenase 26. glyoxylate reductase 27. L-lactate dehydrogenase 37. malate dehydrogenase 49. glucose 6-phosphate dehydrogenase 17. mannitol l-phosphate dehydrogenase 1.1.2 With cytochrome as an acceptor 3. L-lactate dehydrogenase 1.1.3 With 2 as acceptor
lC44 SSka 12/28/79 ~al~7S~7~r3 1 In preparing liposomes, it is necessary that lipids - such as those of Class II - which are insoluble in water be introduced into an aqueous environment. Th;s can be ach;eved by a var;ety of methods.
By one such known method, l;p;ds are phys;cally dispersed ;nto an aqueous solution. A dry th;n film of lipids is formed on the interior surface of a suitable vessel. The aqueous solution contain-ing the substances to be entrapped with;n the l;posomes ;s then placed ;n the vessel in contact with the lipid film. The lip;d f;lm is then dispersed into the aqueous solution by vigorous ag;tation of the vessel (glass beads approximately 0.1 mm in diameter may be included ;n the vessel to accelerate this dispersion). Also, dispers;on of the lip;d f;lm may be enhanced by sonication through immersion of the vessel ;n a bath type sontcator or by immersing the probe of a sonifier lnto the aqueous solut;on. E~cess;ve sonication may in-activate enzyme and can produce very small liposomes.
Alternatively, the lipids may be dlssolved in an aqueous solutlon containing a detergent lipid of Class III A or B such as laurylsulfate or sod;um deoxycholate. The detergent is then removed (e,g. by dialysis), and the liposome b;layers are formed. ~noch and Strittmatter (Proc. Nat. Acad. Sci. 76, 145-149) have described the preparation of 1000 A diameter, s;ngle-bilayer liposomes using sod;um doxycholate as the detergent wh;ch is d;alyzed.
Another known technique involves the addition of aqueous solution to a mixture of l;p;d and a volatlle organic solvent which solvent is subsequently removed by evaporation at reduced pressure.
Szoka and Papahadjopoulos (Proc. Nat. Acad. Sci. 75, 4194-4198 ~1978]) have described preparation of liposomes wlth very large internal aqueous space by means of evaporation of organic solvents diethyl ether or ;sopropyl ether.
The physical and detergent dialys;s methods are particularly appropriate to the present invention, as these produce acceptably lC44, '-SSKa 12/2~/79 ~L~L7~7~3 1 large vesicles and are quite gentle, thus unlikely to inactivate the enzymes. In cases where organic solvent evaporation is to be employed, it is necessary that the enzyme to be encapsulated should be insensitive to that solvent. For example, vesicles of this type can be prepared containing alkaline phosphatase which enzyme is not denatured by the diethyl ether used in the process.
Enzymes suitable for use in the present invention include any of those which will result in low noise levels. A large number of known enzymes may be employed in the present invention. These vary widely in their substrates, the nature of the reaction catalyzed, stability, turnover rate, optimal reaction conditions (pH, ionic strength, temperature), and the like. The International Union of Biochemists has classified various enzymes according to the nature of the reaction catalyzed.
There are a number of criteria which may be applied in the selection of a given enzyme for commerclal application. These enzymes which are at present available in but trace amounts, are less desirable than those which are abundant and may be purchased from commercial sources. The enzyme should be stable when stored at temperatures which are convenient at the site of commercial application, e.g.
4C, for a period of at least 3 months. The catalytic activity or turnover number of the enzyme should be sufficiently high as to provide detectable reaction in a relatively short time period, i.e.
a few secondsto 120 minutes. The cataly~ic activity of the enzyme should be conveniently detectable by mPans available to the commercial user, e.g. the catalyzed reaction produces an increase or decrease in the absorption of light in the ultraviolet or the visible region, i.e.
in the range of 250-750 nm.
Preferably the enzyme should be one which is not present at significant levels in the sample to be tested and is not susceptible lC4 ~0 SSk~
12~2~/80 ~ ~L~ 7~C~
1 to inh;bition by substances commonly found in the test sample.
The enzyme should not be inactivated or poisoned by the lipids employed in liposome preparation and is not inactivated or de-natured durin~ the liposome preparation. The enzyme selected should be one which may be fully encapsulated. Such enzymes in nature are found in the cellular cytoplasm or circulate freely in extracellular fluids. Not desirable are the natural membrane proteins. These in nature are found in association ~ith cellular membranes and have hydrophobic surface(s) which anchor them to the bilayer. Commonly such enzymes span the bilayer with their catalytic sites exposed to the surrounding aqueous medium.
The following table indicates enzymes of particular interest classified according to the International Union of Biochemists:
1. Oxidoreductases 1.1 Acting on the CH-OH group of donors 1.1.1 With NAD or NADP as acceptor 1. alcohol dehydrogenase 6. glycerol dehydrogenase 26. glyoxylate reductase 27. L-lactate dehydrogenase 37. malate dehydrogenase 49. glucose 6-phosphate dehydrogenase 17. mannitol l-phosphate dehydrogenase 1.1.2 With cytochrome as an acceptor 3. L-lactate dehydrogenase 1.1.3 With 2 as acceptor
4. glucose oxidase 9. galactose oxidase 1.2 Acting on the CH-NH2group of donors 1.4.3 With 2 as acceptor 2. L-amino acid oxidase 3. D-amino acid oxidase 1.6 Acting on reduced NAD or NADP as donor 1.6.99 With other acceptors diaphorase 1.10 Acting on diphenols and related substances as donors 1.10.3 With 02as acceptor 1. polyphenol oxidase 3. ascorbate oxidase lC44/
SSKa 1 1.11 Acting on H202 as acceptor 1 .11 .1 . catalase 7. peroxidase 3. Hydrolases 3.1 Acting on ester bonds 3.1.1 Carboxylic ester hydrolases 7. cholinesterase 3.1.3 Phosphoric monoester hydrolase 1. alkaline phosphatase 3.1.4 Phosphoric diester hydrolase 3. phospholipase C
3.2 Acting on glycosyl compounds 3.2.1 Glycoside hydrolases 1. ~-amylase 4. cellulase 17. lysozyme 23. ~-galactosidase 27. amyloglucosidase 31. ~-glucuronidase 3.4 Acting on peptide bonds 3.4.2 Peptidyl-amlno acid hydrolase 1. carboxypeptidase A
3.4.4 Peptidyl-peptide hydrolase
SSKa 1 1.11 Acting on H202 as acceptor 1 .11 .1 . catalase 7. peroxidase 3. Hydrolases 3.1 Acting on ester bonds 3.1.1 Carboxylic ester hydrolases 7. cholinesterase 3.1.3 Phosphoric monoester hydrolase 1. alkaline phosphatase 3.1.4 Phosphoric diester hydrolase 3. phospholipase C
3.2 Acting on glycosyl compounds 3.2.1 Glycoside hydrolases 1. ~-amylase 4. cellulase 17. lysozyme 23. ~-galactosidase 27. amyloglucosidase 31. ~-glucuronidase 3.4 Acting on peptide bonds 3.4.2 Peptidyl-amlno acid hydrolase 1. carboxypeptidase A
3.4.4 Peptidyl-peptide hydrolase
5. ~-chymotrypsin 10. papain 3.5 Acting on C-N bonds other than peptide bonds 3.5.1 In linear amides 5. urease 3.6 Acting on acid anhydride bonds lC44, 1/2/80 ~7~j ~f~3 1 3.6.1 In phosphoryl-containing anhydrides 1. inorganic pyrophosphatase 4. Lyases 4.1 Carbon-carbon lyases 4.1.2 Aldehyde lyases 7. aldolase 4.2 Carbon-oxygen lyases 4.2.1 Hydrolases 1. carbonic anhydrase 4.3 Carbon-nitrogen lyases 4~3.1 Ammonia lyases 3. histidase lC4 '~0 12/29/80 ~ ~ 7~7~3 1 Substrates useful in this invention include those reactive with the enzymes selected for use as known in the art and thus include for example p-nitrophenyl phosphate and 4-methyl umbelliferyl phosphate for alkaline phosphatase; 4 aminosalicylic acid or o-dianiside and hydrogen peroxide for peroxidase; and o- or p-nitrophenyl glycosides for glycosidases. nther useful substrates include those listed by Bergmeyer, Methods for Enzymatic Analysis, Academic Press N.~. 1965.
Not desirahle are those substrates which would readily diffuse through an intact membrane bilayer. Generally such substrates would be small molecules which are soluble in lipid solvents.
Antigens which can be tested for or used as labels for the liposomes in accordance with this invention are numerous. There are a number of antigens, the quantitation of which is of significance in clinical diagnostics. Many of these are now assayed by radio-isotopic methods. Assays for these by the present invention would be a considerable improvement inasmuch as hazardous, unstable re-agents are not employed.
The present invention would be beneFicially applied to the detection and estimation of circulating hormones as indicators of endocrine function. A partial listing of these would include:
thyroid hormones - thyroxineand triidothyronine, parathyroid hormone and calcitonin.
pancreatic hormones - insulin, proinsulin, and glucagon.
pituitary hormones - prolactin, adrenocorticotropic hormone, tyro-tropin, oxytocin and vasopressin.
uterine and placental hormones - chorionic gonadotropin, placental lactogens, chorionic thyrotropin and relaxin.
steroid ho~mones - Estradiol, Estrone, Estriol, Testosterone and Dihydrotestosterone.
growth factors - Urogastrone, Nerve growth factor and the somato-medins.
The method may be usefully applied to the intracellular messen-gers, the cyclic nucleotides and prostaglandins.
The present invention may also be applied to the screening of lC4a- ~2 -~l3L7~7~
1 circulating levels of therapeutic drugs, e.g. the cardiac glycosides;
digoxin, digitoxin, anticonvulsants, diphenylhydantoin, mesantoin, phenobarbital, and mephobarbital. Of particular interest are those drugs with narrow therapeutic index i.e. a certain minimal circulating level is required for therapeutic efficacy while a moderately higher level elicits toxic or harmful reactions.
The procedure may also be adapted to screening for antibiotics such as penicillin, streptomycin, and tetracyclines, chlortetra-cycline, oxytetracycline, and tetracycline, chloramphenicol, erythro-mycin, caromycin, polymyxin B. The aminoglycoside antibioticsgentamycin, amikacin, tobramycin, kanamycin and neomicin employed in the management of aerobic Gram negative bacillary infections can be conveniently assayed by the present invention.
This method may also be applied to the detection and estimation of drugs of a~use such as opiates-morphine, heroin, meperidine and methadone; ergot alkaloids, such as lysergic acid diethylamide, marijuana, barbiturates and cocaine and its derivatives.
Inasmuch as the present invention is very simple in performance and does not employ unstable or hazardous reagents, the assay method is applicable in environments which are less well-equipped and sophis-ticated than diagnostic laboratories. For example, the assay method can be applied to screening food and environmental toxins. In food screening, important antigens would be mycotoxins and natural toxicants. This area involves such major toxins as aflatoxins, ochratoxin, patulin, penicillic acid, zearelonone; and tricothecene toxins, as well as toxic metabolites such as ipomeamerone that occur naturally in foods. Beyond the natural toxicants there are a wide variety of environmental contaminants, the presence of which in foods even in trace amounts poses a significant threat to mankind.
These may be industrial byproducts or pesticides e.g.polychlorinated lC44 -~2 ~7~7~
l/2/80 l biphenyls, chlorinated dibenzo-p-dioxins, chlorinated dibenzofurans, heptachlorepoxide, dieldrin, and DDT 1,1'-2,2,2-Trichloroethylidene)-bis~3-chlorobenzene]; l,l,l trichloro-2,2 bis (p-chlorophenyl) ethane.
Other food contaminants ofconcern are the antibiotlcs - penicil-lin, chloramphenicol and tetracycline.
The method need not be restricted to small molecules as it has been shown (Humphries and McConnell Proc. Nat. Acad. Sci. 71, 1691-1694, 1974) that macromolecular antigens such as egg albumin may be coupled to the surface of immunoreactive liposomes. Thus, the present invention may also be applied to detection of macromolecular antigens - plasma proteins, hepatitis associated antigens, histo-compatibility markers.
Antigens and antigenic materials which are to be analyzed for purposes of this application include any which by themselves or with other products will produce antibodies cognate therefor and thus detectableby the immune reaction. For example, digoxin is considered an antigen because it with another material will produce antibodies such that the antibody to digoxin can be used in a test with either the antibody or digoxin used as the label depending upon whether one is testing for the digoxin or the cognate antibody. Such materials as bovine serum albumin, key hole limpet heomocyanin or other macro-molecular carriers are covalently coupled to the digoxin or other "antigen" in forming antibodies. Thus the word "antigen" as used herein is meant to include all antigenic materials whether antigenic by themselves or in combination with other materials to produce cognate antibodies in animals such as man, rabbits, goats, sheep, guinea pigs, bovine species and other mammals.
The present invention may be employed to detect and quantitate specific antibodies directed against various antigens. The presence as well as the amounts of such antibodies may be taken as indicators of the potential of immunity to various infectious disease, previous exposure to disease, or active lnfection.
~Lt7~79~C~
sc~a 740 _19_ 1 For example, the present invention readily lends itself to the detection of Syphillis antibodies (directed against Treponema Pallidum) as these antibodies are reactive against cardiolipin (extracted from beef heart) which is read;ly incorporated into liposomes.
Antibodles directed against infectious disease agents - virus, bacteria, parasites may also be detected by coupling the surface antigenic markers from those to the liposome surface.
~n some cases, the presence of antibodies directed against specific macromolecule(s) can indicate autoimmune disorders - e.g.
antibodies reactive to nucleic acids polydeoxyribonucleic acids and polyribonucleic acids, collagen, gamma globulins, thyroglobulin, para-thyroid antigens, mitochondrinal antigens, smooth muscle antigens are all potential indicators o~ artoimmune diseases.
Antibodies are produced by introducing an immunogenic substance into the bloodstream of a living animal. The animal responds with the production of antibodies which bind to the immuno~en as the first step in the detoxification of the immunogen. Many antigens are direct-ly immunogenic and elicit antibody production directly. However, a number of substances are not in themselves immunogenic and re-quire mod~fication (coupling to a su~table carrier). Methods for the production of antibodies are described in considerable detail by Landsteiner Speficity of Serological Reactions, Dover Publications N. Y. 1962 and Weir.
Complement (a group of at least 9 different proteins) is a key component of a hosts immune defense against invading cellu-lar pathogens. Complement, once activated (alerted to the presence of a cellular invader) attaches to the outer membrane and creates small lesions in this membrane. In effect complement carves little holes all over the surface of membrane. These holes are quite small, on the order of 100 A (100 x 10~8cm) in diameter.
Very small molecules such as water and simple salts may readily 1 C ` 740 ~ 7~4~
SS 1~
diffuse through such lesions. However, macromolecules such as proteins are commonly about the same size or larger than these lesions 40-250 ~, so that such macromolecules cannot diffuse through these lesions or do so exceedingly slowly, see Green H., 5 Barrow P., and Goldberg, B., (1959) J. Exp. Med. 110, 699. In the present invention the complement used permits an antigen anti-body reaction to effectively poke holes in the liposome encapsulating layer. It is believed that this permits the substrate to enter the liposome bilayer and react with the enzyme therein, Thus an enzymatic reaction occurs even if no complete lysis of the bilayer occurs. The complement permits the reaction either by aiding in lysis or acting to form the holes which permit reaction without lysis. The term "lysis" is used herein to denote the breakdown and complete rupture of the liposome bilayer as well as the expo-sure of the encapsulated enzyme to substrate through holes formed in the bilayer by the immune reaction.
In a typical kit to detect anttgen, a vial contains a liposomes labeled with an antigen suspended in an appropriate buffer, as for example in a volume of from .1 to 10 ml. The concentration of the liposome in the buffer will normally vary from 1 to 50 millimolar~
Useful buffers include phosphate buffered saline or otherisotonicbuffer.
A second vial contains lyophilized powder form or frozen concentrate of the cognate antibody to the antigen. In the case where antibody ~ 'A0 ~L1L~ 7 ~3 1 is to be detected by the direct method, this vial would represent the positive control for the assay. A third vial contains lyo-philized powder or frozen concentrate of complement. Conventional complement for the antigen-antibody complex to be formed is used as S known in the art. For example, such complement can be guinea pig serum. Another vial contains the enzyme substrate which can be a liquid, powder, or the like, at a su~ficient concentration to enable ease of detection of enzymatic activity if the enzyme contained within the liposome is released. Another vial can contain a buffer to use in diluting the materials during the tests of thls invention.
In the simplest and most preferred test, all of the materials including the substrate are added to a single vial, incubated and a color change or the absence of a color change is detected to de-termine whether or not the test material which can, for example, be serum of an individual, contains or does not contain a specific antigen or antibody. In some cases, all of the materials except the substrate are added to a single vial, incubated and then ad-mixed with enzyme substrates and a color change or the absence of a color change is detected to determine whether or not the test mater-ial which can, for example, be serum of an individual, contains or does not contain a specific antigen or antibody. Particularly desirable enzymes are alkaline phosphatase and peroxidase because their reaction with p-nitrophenyl phosphate and 4-aminosalicylic acid give color reactions easily detectable to the eye.
In cases where inhibition of complement lysis is employed for analyte quantitation, there are some limitations on the order of addition. This results from the fact that once liposomes bearing antigen or antibody, complement, and the partner antibody or antigen are brought together, lysis begins. For purposes of quantitation accuracy, it is preferred that the sample to be analy-zed be added to the vial before the complement can act. Thus, useful orders of addition would be: (1) antibody, (2) liposomes, (3) sample, (4) complement. Entries 1, 2 and ~ can be permuted but sample is preferably always added before antibody comple-ment and liposomes are combined.
lC4~l7A0 ~2/29/80 3L~L7574~
1 In all cases,it is preferred to include a known positive test to be run as a check with the test. For example, if the test is a test for digoxin, a standard digoxin vial will be included in the test kit. Where the test is to be a quantitative test as well as a qualitative test, the test kit can include several samples of the material being tested at different concentrations, so that the color change obtained, if any, in the test sample can be compared with the color change or other enzymatic activity of each standard sample when the standards are tested along with the test sample in an ana-lytic procedure.
SSka 1 The determination of enzyme activity is well-known for a large variety of enzymes. Such known tests can be used to monitor enzyme activity following testing in accordance with this invention. A list of assay methods for many of these is given by Bergmeyer, Methods for Enzymatic Analysis, Academic Press N.Y. 1965. Most favored amongst the types of assays would be these which offer either high sensi-tfvity or convenient packaging.
To determine activity oF malate dehydrogenase (E.C. 1.1.1.40) the enzyme is reacted with substrates L~malic acid and nicotinamide adeninine dinucleotide and the progress of the reaction is monitored at 340 nm as in the following procedure;
Into cuvettes are placed the following:
Test Control Phosphate buffer 2.6 ml 2.7 ml NADH2 0.2 ml 0.2 ml Enzyme (diluted) 0.1 ml 0.1 ml Substrate 0.1 ml Enzyme - dilute with 0.1 M phosphate buffer, pH 7.4, to a concentra-tion of 0.1 - 0.3 units/ml.
Substrate - 0.006 M oxaloacetate (freshly prepared). Dissolve 6.7 m~
of the acid in 1 ml phosphate buffer (1.0 M pH 7.4), titrate to pH 7.4 with NaOH, and make to volume of 10 ml.
NADH2 - 0.00375 M. Dissolve 50 mg of NADH2 and 240 mg of THAM in 15 ml of H20, titrate to pH 7.4 in HCl, and make to volume of 20 ml.
Phosphate buffer - 0.1 M, pH 7.4.
Prior to adding the substrate, the instrument is balanced with control cuvette at an absorbancy of 0.200. Readings are taken at 15-second intervals for 2 minutes and the initial rate of change of absorbancy per minute is determined.
~L3L'~ 3 lC44 ?
SSKa 1 This enzyme has a very high turnover number, and therefore, lends itself to highly sensitive assays.
Many other enzyme assays could be selected because they lend themselves to convenient assay ~ormats or substrate packaging. Amongst these are:
Alkaline Phosphatase (E.C. 3.1.3.1). The synthetic substrate p-n;trophenylphosphate ;s used and this can be conveniently packaged in capsule form.
Pipette 3.0 ml of substrate into each of two l-cm cuvettes.
Adjust spectrophotometer to read zero absorbancy at 410 m~.
Enzyme - dilute with water to contain approximately 0.005 mg/ml.
mg/ml = A278 X 1.43 (Plocke, et al~ 1962) Substrate - 0.001 M p-nitrophe~nyl phosphate in 1.0 M Tris buffer, pH 8.0 At zero time, add 0.1 ml of enzyme solution to test cuvette and record absorbancy change. Molar absorbancy index for p-nitro-phenol in 1.0 M Tris, pH 8.0, is 1.62 X 104. One unit is that ac-tivity liberating one micromole p-nitrophenol per minute under the defined conditions at 25C. In this reaction a yellow-colored product is formed which is detectable by direct visual examination.
Also useful because of its widespread availability is the enzyme horseradish peroxidase (E.C. 1.11.1.7). A multiplicity of sub-strates and assay formats are available for this enzyme. One example is:
Add 0.05 ml o~ dye to 6.0 ml of substrate. Transfer 2.9 ml to test cuvette and pour remainder into control cuvette. At zero time add 0.1 ml of diluted enzyme. Introduce the enzyme into the cuvette from a 0.1 ml pipette with the tip below the surface. Mix by inverting cuvette with wax paper over top. Record absorbancy at 15-second intervals for 1-2 minutes and determine rate of change per lC44 ~ L~7 SSKa 1/2/8~
1 minute.
Substrate - Stock: 1 ml of 30% H202 (Merck's Superoxol) diluted to 100 ml with H20. To use, dllute 1 ml of stock H202 to 100 ml with 0.01 M phosphate buffer, pH 6.0 (fresh daily).
Dye - 1% o-dianisidine in methyl alcohol (fresh, in amber bottle).
Enzyme ~ Stock solution: 1 mg/ml in water. Immediately before using, dilute 0.1 ml to 250 ml.
One unit of peroxidase activity is that amount of enzyme decomposing 1 micromole of peroxide per minute at 25~C.
~n order for the llposomes to function in immunoassay, it is necessary that they be sensltized and labeled at their surface with the appropriate antigens. Antigens may be covalently bonded or in some cases absorbed to the surface of preformed liposomes. Alternatively, the antigen may be covalently linked to an appropriate amphiphile and this complex included in the lipid mixture from which the lipo-somes are for~ed. In the latter case, the amphiphile is incorporated into the lipid bilayer, and the attached antigen extends into the surrounding aqueous solution.
When liposomes are preformed, they can have at their external surface several chemical functionalities to which antigens may be covalently linked. Foremost amongst these are: amino groups derived from phosphatidyl ethanolamine, hydroxyl groups provided by phos-phatidyl inositol, and carboxyl groups provided by fatty ac;ds or phosphatidyl serine. These are preclsely the functionalities avail-able on proteins which are exploited in coupling small antigens to produce immunogens. Thus, antigens may be coupled to preformed liposomes by traditional chemical reactions - using bifunctional coupling agents such as: glutaraldehyde, diimide esters, aromatic and aliphatic diisocyanates, B~s-p-nitrophenyl esters of dicarboxy1ic acids, aromatic disulfonyl chlorides and bifunctional arylhalides lC44/ ~L~7~7~
SSKa 1/2l80 1 such as 1,5-difluoro-2,4-dinitrobenzene; p,p'-difluoro m,m~-di-nifrodiphenyl sulfone. Appropriate reactions which may be applied to such couplings are described in Williams et al Methods in Immunologv and Immunochemistry Vol. 1, Academic Press, Ne~ York 1967.
In some cases, antigens may be absorbed to the liposome surface.
Such is the case with certain lipopolysaccharides as was shown by Uemura and Kinsky (Biochemistry 11, 4085-4094 1972). This also obtains for antigens coupled with the Class III amphiphile lysolecithin.
The fact that an antigen may first be coupled to a selected amphiphile e.g. phosphatidyl - ethanolamine, serine - or inositol -and then included in the lipid mixture from which the liposomes are formed is most relevant inasmuch as this coupling reaction may be performed ;n a Yariety of solvents In coupling antigens to pre-formed liposomes or to proteins (as in preparing antigen), the reaction must almost always be performed in aqueous solutions as organic solvents will inactivate or denature or rupture proteins or lipo-somes. For example, if one wishes to couple an antigen containing a carboxyl residue, one may prepare the acid chloride of the antigen using thionyl chloride. This acid chloride may then be coupled to phosphatidyl ethanolamlne in benzene as solvent. This flexibility in choice of solvent will perm~t a broad range of antigens to be coupled to the liposomes.
The following Examples are given to illustrate the present invention and are not to be considered as limiting thereof.
EXAMPLE I
To prepare immunoreactive liposomes labeled at their surface with dinitrophenyl groups~ a mixture containing 40 milligrams of L-~-lecithin (Products #P5763 Sigma Chemical Co. of St. Louis, Mis-souri ) 11.6 mg of cholesterol (Products #CH-S Sigma Chemical Co.
Lot 57C - 7190), 2.18 mg of dicetyl phosphate (Product #D 2631 Sigma lC44~732 1/2/~u 1 Chemical Co. lot 28 [0460]) and 2 mg of N-dinitrophenyl aminocaproyl phosphatidylethanolamine (Avanti Biochemicals of Birmingham, Alabama, lot DCPE 17) in 6 milliliters of chloroform was prepared.
Solvent was evaporated under reduced pressure (water aspirator) in a 50 ml flask on a rotary evaporator producing a thin film of dry lipid on the interior surface of the flask. In order to insure complete removal of the solvent, evaporation was continued for 30 minutes beyond the point where the lipid film was visibly dry. A solution of 4 milligrams of alkaline phosphatase (E.C. 3.1.3.1 ) in 4 ml of O.OlM phosphate buffer pH 7.5 containing 0.3M glucose was added to the flask which was purged and sealed under argon. The sealed flask was gently swirled to dispersethe lipid film. The lipid film gradually disappears from the surface of the flask and the aqueous phase grows progressively turbid. At this point, the flask is held at 4C for 2 hours. Liposomes containing entrapped alkaline phosphatase are then separated from free enzyme by centrifugation at 27,0009 for 60 minutes. The liquid supernatant is decanted and the pellet containing the liposomes is resuspended in isotonic saline buffer (O.OlM phosphate pH 7.5 containing .15M sodium chloride). Further purification is obtained by repeated centrifugation and resuspension.
The extent to which enzyme is encapsulated within such lipo-somes is measured by detergent lysis assay. In the presence of the detergent Triton X-100* a product of Rohm and Haas Co. ~h;ch acts as a detergent, the liposomes are ruptured and the contents are liberated.
A 10 ~1 aliquot of the purified liposomes is added to 1 ml of lg Triton X-100 in deionized water. As a control, 10 ~1 of liposomes are added to 1 ml of isotonic saline. Enzyme is then measured by adding 50-100 l~l aliquots of these dilutions to 1 ml of a solution of 0.4mg/ml of the substrate paranitrophenyl phosphate in 0.1l~ borate pH 9Ø The hydrolysis of substrate is monitored by the appearance * Trademark lC4~ '2 ~7~7~
SSK~
l/2l80 1 of paranitrophenol and ;ncreasing absorbance of light at 410 nm.
This reaction is allowed to proceed for lO minutes and is then terminated by the addition o~ l ml of 2 N NaOH. The enzyme activity produced by the detergent lysls is compared to the control as a measure of the signal to noise characteristic of the liposomes. For the prep-aration de~cribed, this ratio exceeded 150 i.e. the absorbancy in-crease produced in lO minutes by the detergent lysed liposomes was 1.5, the control produced less than 0.01 unit of absorbancy increase.
In subsequent experiments, similar ~iposomes were purified by gel filtration chromatography rather than centrifugation. Three ml of the liposome preparation was layered over a column 40 x l cm of Sephadex G-200 equilibrated with phosphate buffered saline. The liposomes were then eluted from the column appearing with the void volume (approx. 15 ml), well separated from free enzym~ which emerged at 30 m1.
EXAMPLE II
Liposomes are prepared b~ a detergent dialysis method. A dry film from a mixture of 50 mg egg lecithin 3.5 mg cholesterol and 0.5 mg dinitrophenyl aminocaproylphosphatidyl ethanolamine in chloro-form was prepared as described in Example I. To this film was added 5.5 ml of solution contain1ng l mg/ml of alkaline phosphatase in .05 M sodium phosphate buffer pH 7.5, along with 3.6 ml of lOmM
sodium deoxycholate in water. The flask containing this mixture was placed in a sonicator bath at 35PC for 5 minutes and sonicated under argon. A transparent opalescent suspension was obtained. The de-oxycholate detergent was then removed by diafiltration using a Milli-pore Immersible separator. Thlrty volumes of 0.05M phosphate pH 7.5 were exchanged into the suspension while maintaining a constant volume of 9.1 ml. The liposomes were then ~urther purified by gel filtration lC44~ ~ ~L3L~ t7 ~3 ~SKa 1 chromatography as described in Example I. In this case, a signal to noise ratio of 225 was obtained.
EXAMPLE III
In this Example, we sought to show that with appropriately prepared liposomes, antibodies directed against a specific antigen could be detected by liberation of enzyme activity concomitant with immune specific lysis. Multilamellar vesicles are prepared as described in Example I and labeled with N-dinitrophenyl aminocaproyl phosphatidyl ethanolamine (5% of lecithin concentration). Five ~1 of these were mixed with 100 ~1 of complement (guinea pig serum) 345 ~1 o~ a buffer consisting of 50mM tris (hydroxymethyl) aminomethane pH 7.5 containing 0.15M sodium chloride, 0.15mM calcium chloride and 0.5mM magnesium chloride and 50 ~1 of various dilutions of rabbit antiserum to di-nitrophenylated bovine serum albumin. As controls there were included mixtures in which normal rabbit serum replaced the immune serum.
As a further control mixtures were prepared in which the complement had been inactivated by lncubation at 56C for 30 minutes were also prepared. These mixtures were incubated at 25C for 15 minutes at which point 100 ~1 aliquots were removed and added to tubes contain-ing 1 ml of a solution of 0.4 mg/ml paranitrophenylphosphate in O.lM sod;um borate pH 9Ø These tubes were incubated for 5 minutes at 25C. The phosphatase reaction was then termina~ed by the addition of 1 ml of 2M sodium hydroxide. The absorbance of the several tubes at 410 nm was then determined spectrophotometrically. The greater the absorbance, the more phosphatase which had been liberated and the greater the extent of immune specific lysis.
MIXTURE A8SORBANCE AT 410 nm Control:
Mixture containing non-immune (normal)rabbit serum .01 - 3L~75 ~7~3 lC44 j2 SSka 1 Control:
Mixture containing heat-inactivated (normal) rabbit serum .01 Test mixture containing antiserum to dinitrophenylated bovine serum albumin 1.2 EXAMPLE IV
In this Example, the immune specific lysis of liposomes is applied to the determination of relative concentrations of specific antibody. All conditions were identical to those of Example III
but various dilutions of the DNP-BSA antiserum were employed in order to assess the effect of different antibody concentrations upon the extent of complement mediated lysls.
The extent of absorbance increase at 410 nm in 5 minutes was recorded at various dilutions.
Antiserum Dilution 410 1:50 1.5 20 1:75 1-4 1:~00 1.15 1:200 .65 1:300 .30 Thus, this method can be employed to assess specific antibody levels.
EXAMPLE V
To test whether antigen would inhibit complement mediated lysis and whether such inhibition could be employed to quantitate antigen levels in a test sample, the protocol of Example III was modified to allow for inclusion of 50 ~1. of DNP Lysine solutions at various ~ - `
lC4~ ~
SSKa 1 concentrations in the initial incubation mixture. If the absorbancy increase at 410 nm in the absence of free DNP-Lysine is taken as 100% lysis, then at various levels of free antigen the following per-centages of lysis were recorded:
5Free DNP-lysine(Dicomoles) % Lysis
Not desirahle are those substrates which would readily diffuse through an intact membrane bilayer. Generally such substrates would be small molecules which are soluble in lipid solvents.
Antigens which can be tested for or used as labels for the liposomes in accordance with this invention are numerous. There are a number of antigens, the quantitation of which is of significance in clinical diagnostics. Many of these are now assayed by radio-isotopic methods. Assays for these by the present invention would be a considerable improvement inasmuch as hazardous, unstable re-agents are not employed.
The present invention would be beneFicially applied to the detection and estimation of circulating hormones as indicators of endocrine function. A partial listing of these would include:
thyroid hormones - thyroxineand triidothyronine, parathyroid hormone and calcitonin.
pancreatic hormones - insulin, proinsulin, and glucagon.
pituitary hormones - prolactin, adrenocorticotropic hormone, tyro-tropin, oxytocin and vasopressin.
uterine and placental hormones - chorionic gonadotropin, placental lactogens, chorionic thyrotropin and relaxin.
steroid ho~mones - Estradiol, Estrone, Estriol, Testosterone and Dihydrotestosterone.
growth factors - Urogastrone, Nerve growth factor and the somato-medins.
The method may be usefully applied to the intracellular messen-gers, the cyclic nucleotides and prostaglandins.
The present invention may also be applied to the screening of lC4a- ~2 -~l3L7~7~
1 circulating levels of therapeutic drugs, e.g. the cardiac glycosides;
digoxin, digitoxin, anticonvulsants, diphenylhydantoin, mesantoin, phenobarbital, and mephobarbital. Of particular interest are those drugs with narrow therapeutic index i.e. a certain minimal circulating level is required for therapeutic efficacy while a moderately higher level elicits toxic or harmful reactions.
The procedure may also be adapted to screening for antibiotics such as penicillin, streptomycin, and tetracyclines, chlortetra-cycline, oxytetracycline, and tetracycline, chloramphenicol, erythro-mycin, caromycin, polymyxin B. The aminoglycoside antibioticsgentamycin, amikacin, tobramycin, kanamycin and neomicin employed in the management of aerobic Gram negative bacillary infections can be conveniently assayed by the present invention.
This method may also be applied to the detection and estimation of drugs of a~use such as opiates-morphine, heroin, meperidine and methadone; ergot alkaloids, such as lysergic acid diethylamide, marijuana, barbiturates and cocaine and its derivatives.
Inasmuch as the present invention is very simple in performance and does not employ unstable or hazardous reagents, the assay method is applicable in environments which are less well-equipped and sophis-ticated than diagnostic laboratories. For example, the assay method can be applied to screening food and environmental toxins. In food screening, important antigens would be mycotoxins and natural toxicants. This area involves such major toxins as aflatoxins, ochratoxin, patulin, penicillic acid, zearelonone; and tricothecene toxins, as well as toxic metabolites such as ipomeamerone that occur naturally in foods. Beyond the natural toxicants there are a wide variety of environmental contaminants, the presence of which in foods even in trace amounts poses a significant threat to mankind.
These may be industrial byproducts or pesticides e.g.polychlorinated lC44 -~2 ~7~7~
l/2/80 l biphenyls, chlorinated dibenzo-p-dioxins, chlorinated dibenzofurans, heptachlorepoxide, dieldrin, and DDT 1,1'-2,2,2-Trichloroethylidene)-bis~3-chlorobenzene]; l,l,l trichloro-2,2 bis (p-chlorophenyl) ethane.
Other food contaminants ofconcern are the antibiotlcs - penicil-lin, chloramphenicol and tetracycline.
The method need not be restricted to small molecules as it has been shown (Humphries and McConnell Proc. Nat. Acad. Sci. 71, 1691-1694, 1974) that macromolecular antigens such as egg albumin may be coupled to the surface of immunoreactive liposomes. Thus, the present invention may also be applied to detection of macromolecular antigens - plasma proteins, hepatitis associated antigens, histo-compatibility markers.
Antigens and antigenic materials which are to be analyzed for purposes of this application include any which by themselves or with other products will produce antibodies cognate therefor and thus detectableby the immune reaction. For example, digoxin is considered an antigen because it with another material will produce antibodies such that the antibody to digoxin can be used in a test with either the antibody or digoxin used as the label depending upon whether one is testing for the digoxin or the cognate antibody. Such materials as bovine serum albumin, key hole limpet heomocyanin or other macro-molecular carriers are covalently coupled to the digoxin or other "antigen" in forming antibodies. Thus the word "antigen" as used herein is meant to include all antigenic materials whether antigenic by themselves or in combination with other materials to produce cognate antibodies in animals such as man, rabbits, goats, sheep, guinea pigs, bovine species and other mammals.
The present invention may be employed to detect and quantitate specific antibodies directed against various antigens. The presence as well as the amounts of such antibodies may be taken as indicators of the potential of immunity to various infectious disease, previous exposure to disease, or active lnfection.
~Lt7~79~C~
sc~a 740 _19_ 1 For example, the present invention readily lends itself to the detection of Syphillis antibodies (directed against Treponema Pallidum) as these antibodies are reactive against cardiolipin (extracted from beef heart) which is read;ly incorporated into liposomes.
Antibodles directed against infectious disease agents - virus, bacteria, parasites may also be detected by coupling the surface antigenic markers from those to the liposome surface.
~n some cases, the presence of antibodies directed against specific macromolecule(s) can indicate autoimmune disorders - e.g.
antibodies reactive to nucleic acids polydeoxyribonucleic acids and polyribonucleic acids, collagen, gamma globulins, thyroglobulin, para-thyroid antigens, mitochondrinal antigens, smooth muscle antigens are all potential indicators o~ artoimmune diseases.
Antibodies are produced by introducing an immunogenic substance into the bloodstream of a living animal. The animal responds with the production of antibodies which bind to the immuno~en as the first step in the detoxification of the immunogen. Many antigens are direct-ly immunogenic and elicit antibody production directly. However, a number of substances are not in themselves immunogenic and re-quire mod~fication (coupling to a su~table carrier). Methods for the production of antibodies are described in considerable detail by Landsteiner Speficity of Serological Reactions, Dover Publications N. Y. 1962 and Weir.
Complement (a group of at least 9 different proteins) is a key component of a hosts immune defense against invading cellu-lar pathogens. Complement, once activated (alerted to the presence of a cellular invader) attaches to the outer membrane and creates small lesions in this membrane. In effect complement carves little holes all over the surface of membrane. These holes are quite small, on the order of 100 A (100 x 10~8cm) in diameter.
Very small molecules such as water and simple salts may readily 1 C ` 740 ~ 7~4~
SS 1~
diffuse through such lesions. However, macromolecules such as proteins are commonly about the same size or larger than these lesions 40-250 ~, so that such macromolecules cannot diffuse through these lesions or do so exceedingly slowly, see Green H., 5 Barrow P., and Goldberg, B., (1959) J. Exp. Med. 110, 699. In the present invention the complement used permits an antigen anti-body reaction to effectively poke holes in the liposome encapsulating layer. It is believed that this permits the substrate to enter the liposome bilayer and react with the enzyme therein, Thus an enzymatic reaction occurs even if no complete lysis of the bilayer occurs. The complement permits the reaction either by aiding in lysis or acting to form the holes which permit reaction without lysis. The term "lysis" is used herein to denote the breakdown and complete rupture of the liposome bilayer as well as the expo-sure of the encapsulated enzyme to substrate through holes formed in the bilayer by the immune reaction.
In a typical kit to detect anttgen, a vial contains a liposomes labeled with an antigen suspended in an appropriate buffer, as for example in a volume of from .1 to 10 ml. The concentration of the liposome in the buffer will normally vary from 1 to 50 millimolar~
Useful buffers include phosphate buffered saline or otherisotonicbuffer.
A second vial contains lyophilized powder form or frozen concentrate of the cognate antibody to the antigen. In the case where antibody ~ 'A0 ~L1L~ 7 ~3 1 is to be detected by the direct method, this vial would represent the positive control for the assay. A third vial contains lyo-philized powder or frozen concentrate of complement. Conventional complement for the antigen-antibody complex to be formed is used as S known in the art. For example, such complement can be guinea pig serum. Another vial contains the enzyme substrate which can be a liquid, powder, or the like, at a su~ficient concentration to enable ease of detection of enzymatic activity if the enzyme contained within the liposome is released. Another vial can contain a buffer to use in diluting the materials during the tests of thls invention.
In the simplest and most preferred test, all of the materials including the substrate are added to a single vial, incubated and a color change or the absence of a color change is detected to de-termine whether or not the test material which can, for example, be serum of an individual, contains or does not contain a specific antigen or antibody. In some cases, all of the materials except the substrate are added to a single vial, incubated and then ad-mixed with enzyme substrates and a color change or the absence of a color change is detected to determine whether or not the test mater-ial which can, for example, be serum of an individual, contains or does not contain a specific antigen or antibody. Particularly desirable enzymes are alkaline phosphatase and peroxidase because their reaction with p-nitrophenyl phosphate and 4-aminosalicylic acid give color reactions easily detectable to the eye.
In cases where inhibition of complement lysis is employed for analyte quantitation, there are some limitations on the order of addition. This results from the fact that once liposomes bearing antigen or antibody, complement, and the partner antibody or antigen are brought together, lysis begins. For purposes of quantitation accuracy, it is preferred that the sample to be analy-zed be added to the vial before the complement can act. Thus, useful orders of addition would be: (1) antibody, (2) liposomes, (3) sample, (4) complement. Entries 1, 2 and ~ can be permuted but sample is preferably always added before antibody comple-ment and liposomes are combined.
lC4~l7A0 ~2/29/80 3L~L7574~
1 In all cases,it is preferred to include a known positive test to be run as a check with the test. For example, if the test is a test for digoxin, a standard digoxin vial will be included in the test kit. Where the test is to be a quantitative test as well as a qualitative test, the test kit can include several samples of the material being tested at different concentrations, so that the color change obtained, if any, in the test sample can be compared with the color change or other enzymatic activity of each standard sample when the standards are tested along with the test sample in an ana-lytic procedure.
SSka 1 The determination of enzyme activity is well-known for a large variety of enzymes. Such known tests can be used to monitor enzyme activity following testing in accordance with this invention. A list of assay methods for many of these is given by Bergmeyer, Methods for Enzymatic Analysis, Academic Press N.Y. 1965. Most favored amongst the types of assays would be these which offer either high sensi-tfvity or convenient packaging.
To determine activity oF malate dehydrogenase (E.C. 1.1.1.40) the enzyme is reacted with substrates L~malic acid and nicotinamide adeninine dinucleotide and the progress of the reaction is monitored at 340 nm as in the following procedure;
Into cuvettes are placed the following:
Test Control Phosphate buffer 2.6 ml 2.7 ml NADH2 0.2 ml 0.2 ml Enzyme (diluted) 0.1 ml 0.1 ml Substrate 0.1 ml Enzyme - dilute with 0.1 M phosphate buffer, pH 7.4, to a concentra-tion of 0.1 - 0.3 units/ml.
Substrate - 0.006 M oxaloacetate (freshly prepared). Dissolve 6.7 m~
of the acid in 1 ml phosphate buffer (1.0 M pH 7.4), titrate to pH 7.4 with NaOH, and make to volume of 10 ml.
NADH2 - 0.00375 M. Dissolve 50 mg of NADH2 and 240 mg of THAM in 15 ml of H20, titrate to pH 7.4 in HCl, and make to volume of 20 ml.
Phosphate buffer - 0.1 M, pH 7.4.
Prior to adding the substrate, the instrument is balanced with control cuvette at an absorbancy of 0.200. Readings are taken at 15-second intervals for 2 minutes and the initial rate of change of absorbancy per minute is determined.
~L3L'~ 3 lC44 ?
SSKa 1 This enzyme has a very high turnover number, and therefore, lends itself to highly sensitive assays.
Many other enzyme assays could be selected because they lend themselves to convenient assay ~ormats or substrate packaging. Amongst these are:
Alkaline Phosphatase (E.C. 3.1.3.1). The synthetic substrate p-n;trophenylphosphate ;s used and this can be conveniently packaged in capsule form.
Pipette 3.0 ml of substrate into each of two l-cm cuvettes.
Adjust spectrophotometer to read zero absorbancy at 410 m~.
Enzyme - dilute with water to contain approximately 0.005 mg/ml.
mg/ml = A278 X 1.43 (Plocke, et al~ 1962) Substrate - 0.001 M p-nitrophe~nyl phosphate in 1.0 M Tris buffer, pH 8.0 At zero time, add 0.1 ml of enzyme solution to test cuvette and record absorbancy change. Molar absorbancy index for p-nitro-phenol in 1.0 M Tris, pH 8.0, is 1.62 X 104. One unit is that ac-tivity liberating one micromole p-nitrophenol per minute under the defined conditions at 25C. In this reaction a yellow-colored product is formed which is detectable by direct visual examination.
Also useful because of its widespread availability is the enzyme horseradish peroxidase (E.C. 1.11.1.7). A multiplicity of sub-strates and assay formats are available for this enzyme. One example is:
Add 0.05 ml o~ dye to 6.0 ml of substrate. Transfer 2.9 ml to test cuvette and pour remainder into control cuvette. At zero time add 0.1 ml of diluted enzyme. Introduce the enzyme into the cuvette from a 0.1 ml pipette with the tip below the surface. Mix by inverting cuvette with wax paper over top. Record absorbancy at 15-second intervals for 1-2 minutes and determine rate of change per lC44 ~ L~7 SSKa 1/2/8~
1 minute.
Substrate - Stock: 1 ml of 30% H202 (Merck's Superoxol) diluted to 100 ml with H20. To use, dllute 1 ml of stock H202 to 100 ml with 0.01 M phosphate buffer, pH 6.0 (fresh daily).
Dye - 1% o-dianisidine in methyl alcohol (fresh, in amber bottle).
Enzyme ~ Stock solution: 1 mg/ml in water. Immediately before using, dilute 0.1 ml to 250 ml.
One unit of peroxidase activity is that amount of enzyme decomposing 1 micromole of peroxide per minute at 25~C.
~n order for the llposomes to function in immunoassay, it is necessary that they be sensltized and labeled at their surface with the appropriate antigens. Antigens may be covalently bonded or in some cases absorbed to the surface of preformed liposomes. Alternatively, the antigen may be covalently linked to an appropriate amphiphile and this complex included in the lipid mixture from which the lipo-somes are for~ed. In the latter case, the amphiphile is incorporated into the lipid bilayer, and the attached antigen extends into the surrounding aqueous solution.
When liposomes are preformed, they can have at their external surface several chemical functionalities to which antigens may be covalently linked. Foremost amongst these are: amino groups derived from phosphatidyl ethanolamine, hydroxyl groups provided by phos-phatidyl inositol, and carboxyl groups provided by fatty ac;ds or phosphatidyl serine. These are preclsely the functionalities avail-able on proteins which are exploited in coupling small antigens to produce immunogens. Thus, antigens may be coupled to preformed liposomes by traditional chemical reactions - using bifunctional coupling agents such as: glutaraldehyde, diimide esters, aromatic and aliphatic diisocyanates, B~s-p-nitrophenyl esters of dicarboxy1ic acids, aromatic disulfonyl chlorides and bifunctional arylhalides lC44/ ~L~7~7~
SSKa 1/2l80 1 such as 1,5-difluoro-2,4-dinitrobenzene; p,p'-difluoro m,m~-di-nifrodiphenyl sulfone. Appropriate reactions which may be applied to such couplings are described in Williams et al Methods in Immunologv and Immunochemistry Vol. 1, Academic Press, Ne~ York 1967.
In some cases, antigens may be absorbed to the liposome surface.
Such is the case with certain lipopolysaccharides as was shown by Uemura and Kinsky (Biochemistry 11, 4085-4094 1972). This also obtains for antigens coupled with the Class III amphiphile lysolecithin.
The fact that an antigen may first be coupled to a selected amphiphile e.g. phosphatidyl - ethanolamine, serine - or inositol -and then included in the lipid mixture from which the liposomes are formed is most relevant inasmuch as this coupling reaction may be performed ;n a Yariety of solvents In coupling antigens to pre-formed liposomes or to proteins (as in preparing antigen), the reaction must almost always be performed in aqueous solutions as organic solvents will inactivate or denature or rupture proteins or lipo-somes. For example, if one wishes to couple an antigen containing a carboxyl residue, one may prepare the acid chloride of the antigen using thionyl chloride. This acid chloride may then be coupled to phosphatidyl ethanolamlne in benzene as solvent. This flexibility in choice of solvent will perm~t a broad range of antigens to be coupled to the liposomes.
The following Examples are given to illustrate the present invention and are not to be considered as limiting thereof.
EXAMPLE I
To prepare immunoreactive liposomes labeled at their surface with dinitrophenyl groups~ a mixture containing 40 milligrams of L-~-lecithin (Products #P5763 Sigma Chemical Co. of St. Louis, Mis-souri ) 11.6 mg of cholesterol (Products #CH-S Sigma Chemical Co.
Lot 57C - 7190), 2.18 mg of dicetyl phosphate (Product #D 2631 Sigma lC44~732 1/2/~u 1 Chemical Co. lot 28 [0460]) and 2 mg of N-dinitrophenyl aminocaproyl phosphatidylethanolamine (Avanti Biochemicals of Birmingham, Alabama, lot DCPE 17) in 6 milliliters of chloroform was prepared.
Solvent was evaporated under reduced pressure (water aspirator) in a 50 ml flask on a rotary evaporator producing a thin film of dry lipid on the interior surface of the flask. In order to insure complete removal of the solvent, evaporation was continued for 30 minutes beyond the point where the lipid film was visibly dry. A solution of 4 milligrams of alkaline phosphatase (E.C. 3.1.3.1 ) in 4 ml of O.OlM phosphate buffer pH 7.5 containing 0.3M glucose was added to the flask which was purged and sealed under argon. The sealed flask was gently swirled to dispersethe lipid film. The lipid film gradually disappears from the surface of the flask and the aqueous phase grows progressively turbid. At this point, the flask is held at 4C for 2 hours. Liposomes containing entrapped alkaline phosphatase are then separated from free enzyme by centrifugation at 27,0009 for 60 minutes. The liquid supernatant is decanted and the pellet containing the liposomes is resuspended in isotonic saline buffer (O.OlM phosphate pH 7.5 containing .15M sodium chloride). Further purification is obtained by repeated centrifugation and resuspension.
The extent to which enzyme is encapsulated within such lipo-somes is measured by detergent lysis assay. In the presence of the detergent Triton X-100* a product of Rohm and Haas Co. ~h;ch acts as a detergent, the liposomes are ruptured and the contents are liberated.
A 10 ~1 aliquot of the purified liposomes is added to 1 ml of lg Triton X-100 in deionized water. As a control, 10 ~1 of liposomes are added to 1 ml of isotonic saline. Enzyme is then measured by adding 50-100 l~l aliquots of these dilutions to 1 ml of a solution of 0.4mg/ml of the substrate paranitrophenyl phosphate in 0.1l~ borate pH 9Ø The hydrolysis of substrate is monitored by the appearance * Trademark lC4~ '2 ~7~7~
SSK~
l/2l80 1 of paranitrophenol and ;ncreasing absorbance of light at 410 nm.
This reaction is allowed to proceed for lO minutes and is then terminated by the addition o~ l ml of 2 N NaOH. The enzyme activity produced by the detergent lysls is compared to the control as a measure of the signal to noise characteristic of the liposomes. For the prep-aration de~cribed, this ratio exceeded 150 i.e. the absorbancy in-crease produced in lO minutes by the detergent lysed liposomes was 1.5, the control produced less than 0.01 unit of absorbancy increase.
In subsequent experiments, similar ~iposomes were purified by gel filtration chromatography rather than centrifugation. Three ml of the liposome preparation was layered over a column 40 x l cm of Sephadex G-200 equilibrated with phosphate buffered saline. The liposomes were then eluted from the column appearing with the void volume (approx. 15 ml), well separated from free enzym~ which emerged at 30 m1.
EXAMPLE II
Liposomes are prepared b~ a detergent dialysis method. A dry film from a mixture of 50 mg egg lecithin 3.5 mg cholesterol and 0.5 mg dinitrophenyl aminocaproylphosphatidyl ethanolamine in chloro-form was prepared as described in Example I. To this film was added 5.5 ml of solution contain1ng l mg/ml of alkaline phosphatase in .05 M sodium phosphate buffer pH 7.5, along with 3.6 ml of lOmM
sodium deoxycholate in water. The flask containing this mixture was placed in a sonicator bath at 35PC for 5 minutes and sonicated under argon. A transparent opalescent suspension was obtained. The de-oxycholate detergent was then removed by diafiltration using a Milli-pore Immersible separator. Thlrty volumes of 0.05M phosphate pH 7.5 were exchanged into the suspension while maintaining a constant volume of 9.1 ml. The liposomes were then ~urther purified by gel filtration lC44~ ~ ~L3L~ t7 ~3 ~SKa 1 chromatography as described in Example I. In this case, a signal to noise ratio of 225 was obtained.
EXAMPLE III
In this Example, we sought to show that with appropriately prepared liposomes, antibodies directed against a specific antigen could be detected by liberation of enzyme activity concomitant with immune specific lysis. Multilamellar vesicles are prepared as described in Example I and labeled with N-dinitrophenyl aminocaproyl phosphatidyl ethanolamine (5% of lecithin concentration). Five ~1 of these were mixed with 100 ~1 of complement (guinea pig serum) 345 ~1 o~ a buffer consisting of 50mM tris (hydroxymethyl) aminomethane pH 7.5 containing 0.15M sodium chloride, 0.15mM calcium chloride and 0.5mM magnesium chloride and 50 ~1 of various dilutions of rabbit antiserum to di-nitrophenylated bovine serum albumin. As controls there were included mixtures in which normal rabbit serum replaced the immune serum.
As a further control mixtures were prepared in which the complement had been inactivated by lncubation at 56C for 30 minutes were also prepared. These mixtures were incubated at 25C for 15 minutes at which point 100 ~1 aliquots were removed and added to tubes contain-ing 1 ml of a solution of 0.4 mg/ml paranitrophenylphosphate in O.lM sod;um borate pH 9Ø These tubes were incubated for 5 minutes at 25C. The phosphatase reaction was then termina~ed by the addition of 1 ml of 2M sodium hydroxide. The absorbance of the several tubes at 410 nm was then determined spectrophotometrically. The greater the absorbance, the more phosphatase which had been liberated and the greater the extent of immune specific lysis.
MIXTURE A8SORBANCE AT 410 nm Control:
Mixture containing non-immune (normal)rabbit serum .01 - 3L~75 ~7~3 lC44 j2 SSka 1 Control:
Mixture containing heat-inactivated (normal) rabbit serum .01 Test mixture containing antiserum to dinitrophenylated bovine serum albumin 1.2 EXAMPLE IV
In this Example, the immune specific lysis of liposomes is applied to the determination of relative concentrations of specific antibody. All conditions were identical to those of Example III
but various dilutions of the DNP-BSA antiserum were employed in order to assess the effect of different antibody concentrations upon the extent of complement mediated lysls.
The extent of absorbance increase at 410 nm in 5 minutes was recorded at various dilutions.
Antiserum Dilution 410 1:50 1.5 20 1:75 1-4 1:~00 1.15 1:200 .65 1:300 .30 Thus, this method can be employed to assess specific antibody levels.
EXAMPLE V
To test whether antigen would inhibit complement mediated lysis and whether such inhibition could be employed to quantitate antigen levels in a test sample, the protocol of Example III was modified to allow for inclusion of 50 ~1. of DNP Lysine solutions at various ~ - `
lC4~ ~
SSKa 1 concentrations in the initial incubation mixture. If the absorbancy increase at 410 nm in the absence of free DNP-Lysine is taken as 100% lysis, then at various levels of free antigen the following per-centages of lysis were recorded:
5Free DNP-lysine(Dicomoles) % Lysis
6 33 13.5 56 Over this range, there is a linear relationship between the percent lysis and the logarithm of the antigen concentration. Analyzed by linear least squares regression the linear relationship is characterized by the follow-ing parameters:
slope = -33.3 y intercept = 143 correlation coefficient = .998 50~ occurs at 16.2 picomole.
EXAMPLE VI
Quantitative immunoassay is performed according to a one-step format, i.e. all reagents including enzyme substrate are mixed together at once so that lytic and enzymatic reactions occur coterminously. Such a single step ~ormat is simple in practice and can be easily automated.
Twenty-five milligrams of L-~-Lecithin-Dipalmitoyl (Cal-biochem-Behring Corp., LaJolla, California)8.6 mg cholesterol (Sigma), 1.6 mg dicetyl phosphate (Sigma), and 1.5 mg of Di-nitrophenyl aminocaproyl phosphatidyl ethanolamine (Avanti) were 1C'' 740 ~ ~ 7~7 SSK~ -' l mixed in chloroform solvent. The solvent was removed under re-duced pressure in a rotary eYaporator, and a thin film af lipids was formed on the interior of a 50 ml. round bottomed flask. This film was then dispersed in an aqueous solution containing 5 milli-grams of alkaline phosphatase (Sigma) in 3 ml. of PBS-Dextrose buffer.
The liposomes were then harvested by centrifugation as in the previous examples.
To a single tube were added 2 microliter of these liposomes (20 nanomole of phospholipid), 100 microliter of guinea pig comple-ment (diluted 1.8 in complement lysis buffer, 50 microliter of Rabbit antiserum to DNP, 100 microliter of buffer or standard solution and l ml. of phosphatase substrate. The reaction mix-ture was incubated at 37C for ten minutes whereupon 1 ml. of 0.5N sodium hydroxide was added to terminate the enzyme reaction.
The absorbance at 405 nm was obtained spectrophotometrically.
The extent of reaction was dependent on the quant1ty of DNP-Lysine (Sigma),as follows:
Amount of DNP-Lysine~pmole) Abs. at 405 nm -0 .95 202.0 .902 2.5 .811 4 .573 .430 6 .311
slope = -33.3 y intercept = 143 correlation coefficient = .998 50~ occurs at 16.2 picomole.
EXAMPLE VI
Quantitative immunoassay is performed according to a one-step format, i.e. all reagents including enzyme substrate are mixed together at once so that lytic and enzymatic reactions occur coterminously. Such a single step ~ormat is simple in practice and can be easily automated.
Twenty-five milligrams of L-~-Lecithin-Dipalmitoyl (Cal-biochem-Behring Corp., LaJolla, California)8.6 mg cholesterol (Sigma), 1.6 mg dicetyl phosphate (Sigma), and 1.5 mg of Di-nitrophenyl aminocaproyl phosphatidyl ethanolamine (Avanti) were 1C'' 740 ~ ~ 7~7 SSK~ -' l mixed in chloroform solvent. The solvent was removed under re-duced pressure in a rotary eYaporator, and a thin film af lipids was formed on the interior of a 50 ml. round bottomed flask. This film was then dispersed in an aqueous solution containing 5 milli-grams of alkaline phosphatase (Sigma) in 3 ml. of PBS-Dextrose buffer.
The liposomes were then harvested by centrifugation as in the previous examples.
To a single tube were added 2 microliter of these liposomes (20 nanomole of phospholipid), 100 microliter of guinea pig comple-ment (diluted 1.8 in complement lysis buffer, 50 microliter of Rabbit antiserum to DNP, 100 microliter of buffer or standard solution and l ml. of phosphatase substrate. The reaction mix-ture was incubated at 37C for ten minutes whereupon 1 ml. of 0.5N sodium hydroxide was added to terminate the enzyme reaction.
The absorbance at 405 nm was obtained spectrophotometrically.
The extent of reaction was dependent on the quant1ty of DNP-Lysine (Sigma),as follows:
Amount of DNP-Lysine~pmole) Abs. at 405 nm -0 .95 202.0 .902 2.5 .811 4 .573 .430 6 .311
7 .257 In the absorbance at 405 nm is plotted against the logarithm of the amount of DNP-Lysine a straight lineis derived with slope-66.8, intercept 143 and correlation coefficient .995. Fifty per-cent inhibition of lysis is achieved with 4 pmole of DNP-Lysine.
1C44k ~ 9~L~5 In an example of kinetic mode quantitat;on liposomes as described in the previous example are applied to quantitation of antigens by measuring the rate of the enzymatic reaction. In this case the reagents in quantities described in Example VI are mixed in a spectrophotometer cuvette. The time course of the enzymatic reaction may then be monitored directly. After a characteristic lag phase, the rate Q~ increase in absorbance at 405 becomes a linear function of the free antibody concentration.
Typically, one adds to a spectrophotometer cuvette .75 ml. of phosphatase substrate solution,50 microliter of antibody,0.1 ml. of complement and 5 microliter of iiposomes. The cuvette is then a thermostatted spectrophotometer and the absorbance at 405 nm is recorded. A characteristic lag phase of 2-3 minutes occurs during which the absorbance changes slightly. After this lag, the absorbance increases rapldly. Beyond 5 minutes, the rate at increase is a function of the amount of antibody avail-able.
Proteins and other macromolecules can be coupled to lipo-somes. Such liposomes with proteins attached to the outer sur-face are susceptible to complement mediated lysis in the presence of antibodies to the attached pro~eins. Liposomes can be pre-pared having within the membrane b~layer lipids suitable for coupling with proteins and other macromolecules. Typically, lipids such as phosphatidyl ethanolamine, phosphatidyl serine or phosphatidyl inositol would be suitable.
EXAMPLE YIII
The method described in Example I is employed to prepare liposomes containing alkaline phosphatase. In this case the lipid SSka ~L~ r~ 3 l mixture consists of 25 milligrams of dipalmitoyl phosphatidyl choline, 10 milligrams of phosphatidyl ethanolamine and 8.6 milli-grams of cholesterol. These liposomes are purified by repeated centrifugation after which they are resuspended in 2 ml. of 0.1 5 M borate buffer pH ~.5. To this suspension is added 20 micro-liter of 25% glutaraldehyde. After 10 minutes at room tempera-ture, the mixture is dialyzed overnight against 2 liters of borate buffer. The activated liposomes are then added to 2.4 milligrams of bovine serum albumin in 1 ml. borate buffer. The mixture is then incubated overnight at 4C whereupon the lipo-somes with protein attached are separated from unbound protein by centrifugation at 25,000 9 for 30 minutes. Following the assay method described in Examples III and IV and using rabbit antibody to bovine serum albumin~ an immune lysis assay can be prepared which will detect albumin in samples quantitatively in the range of from .1 to 2 ~9 1 ml.
EXAMPLE IX
-In order to assay the cardiac glycoside-digoxin was coupled 20 to dipalmitoylphosphatidylethanolamine. To this end mixture containing 0.5 grams (0.64 mmole)of Digoxin in 20 m1. of Ethanol/
Dioxane (4:1,v/v) was added to 60 ml. of 0.1 M sodium metaperiodate.
The mixture was stirred for 30 minutes at room temperature where-upon 4.5 ml. of ethylene glycol was added. This mixture was 25 stirred for one-half hour at room temperature and evaporated under reduced pressure. The resultant solid was then extracted 3 times with 50 ml. of chloroform. The extracts were pooled ~total volume 150 ml.) and solvent evaporated under reduced pressure, produc-ing 0.9 gm of oily residue. Twenty-five mg of this crude product of digoxin dialdehyde in l ml. oF ethanol/chloroform (1:4) was lC4` " ao ~7S7~
ss~ .
1 added to 20 mg of dipalm;toylphosphatidylethanolamine in 1 ml of ethanol/chloroform (1:2). Four drops of triethylamine were added and the reaction mixture (p~l 9) was incubated overnight at 37C and finally evaporated to a dry residue under reduced pressure. This residue was suspended in 2 ml. of ethanol/chloro-form (1:1) and 4 milligram of sodium borohydride was added.
This mixture was stirred for 30 minutes and then evaporated to dryness under reduced pressure. This residue was then tri-turated with ethanol and filtered to give a filtrate which upon evaporation yielded 45 milligrams of dipalmitoylphosphatidyl-phosphatidylethanolamine-digoxin conjugat;on product.
EXAMPLE X
The conjugate of digoxin anddipalmitoylphosphatidylethanol-amine is employed to prepare liposomes with digoxin. In this case 22 milligrams of dimyristoylphosphatidyl choline, 8.6 milli-grams of cholesterol, 1.6 milligrams of dicetylphosphate, and 2.5 milligrams of Digoxin-dipalmitoylphosphatidylethanolamine con-jugate were dissolved in 3 ml. o~ chloroform. Solvent was evap-orated under reduced pressure and the lipids deposited as a thinfilm on the internal wall of a 100 ml. round-bottomed flask. T~e lipid film was then dispersed in (solution as in Example I
lines 8-10 and purified also as in Example I).
Assays were performed as in Example VI. Inhibition by digoxin in test samples was observed in range of ~.5-10 ng/ml digoxin in the test sample.
Liposomes can be frozen successfully if they are first suspended in an isotonic medium - 0.01 M phosphate buffer con-taining 0.15 M sodium chloride. Also useful are solutions lC4 ~0 ~ ~L 7~ 3 ~SKa 1 buffered in the range From pH 4 to pH 10 containing 0.3 M glucose or like carbohydrate. However, liposomes frozen in proteinaceous media e.g. containing bovine serum albumin of rabbit gamma globu-lins are not preferred as these show elevated levels of enzyme activity in the absence of lytic reagents - detergent or comple-ment plus antibody. 8est results are achieved with rapid freez-ing at a rate of at least 5C per minute. Prior to freezing lipo-somes are suspended in isotonic media at concentrations of 1-10 mg/
ml. For example liposomes prepared as in Example I are suspended in 0.01 M sodium phosphate buffer containing 0.15 M sodium chloride.
This suspension contains 2.5 mg of total lipid in 1 ml of liquid.
0.1 ml aliquots of this mixture are placed in a 5 ml. vial. These are then frozen to -20C at a rate of 5C per minute. The lipo-somes can be thawed and used after long periods of storage.
While specific embodiments of this invention have been shown and described, it will be understood that many variations are possible.
Particular concentrat;ons, combinations and materials can vary greatly 90 long as the signal to noise ratio minimums of the inven-tion are maintained which aids in preventing false readings. A wide variety of materials can be tested in a wide variety of high volume screening test by relatively unskilled personnel.
The material to be tested can be body fluids or mixtures of all kinds. When serum is tested it is preferably treated chemically and/or with heat to remove undesirable inhibition. Prior treat-ment with amino groups is one such chemical method. Typically,0.1 ml of 2.54 M ammonia is added to 1.9 ml of serum which is then neutralized by the addition of 0.1 ml of 2.54 M hydrochloric acid. Also sulthydryl blocking reagents can be useful. In this case 0.1 ml of 0.2 M mercaptoethanolin phosphate buffered saline is added to 1 ml of serum. Then 1 ml of 0.2 M iodoacetamide is - ~L~ 7 lC~ ,740 SSKa 1 is added. Similarly useful is the sulfonic acid azo dye chlora-zol fast pink which selectively inhibits human complement activa-tion but not guinea pig complement. Heat treatment of at least about 58C for at least 30 and preferably 60 minutes is also useful to prevent unwanted inhibltion of the complement reaction.
.
1C44k ~ 9~L~5 In an example of kinetic mode quantitat;on liposomes as described in the previous example are applied to quantitation of antigens by measuring the rate of the enzymatic reaction. In this case the reagents in quantities described in Example VI are mixed in a spectrophotometer cuvette. The time course of the enzymatic reaction may then be monitored directly. After a characteristic lag phase, the rate Q~ increase in absorbance at 405 becomes a linear function of the free antibody concentration.
Typically, one adds to a spectrophotometer cuvette .75 ml. of phosphatase substrate solution,50 microliter of antibody,0.1 ml. of complement and 5 microliter of iiposomes. The cuvette is then a thermostatted spectrophotometer and the absorbance at 405 nm is recorded. A characteristic lag phase of 2-3 minutes occurs during which the absorbance changes slightly. After this lag, the absorbance increases rapldly. Beyond 5 minutes, the rate at increase is a function of the amount of antibody avail-able.
Proteins and other macromolecules can be coupled to lipo-somes. Such liposomes with proteins attached to the outer sur-face are susceptible to complement mediated lysis in the presence of antibodies to the attached pro~eins. Liposomes can be pre-pared having within the membrane b~layer lipids suitable for coupling with proteins and other macromolecules. Typically, lipids such as phosphatidyl ethanolamine, phosphatidyl serine or phosphatidyl inositol would be suitable.
EXAMPLE YIII
The method described in Example I is employed to prepare liposomes containing alkaline phosphatase. In this case the lipid SSka ~L~ r~ 3 l mixture consists of 25 milligrams of dipalmitoyl phosphatidyl choline, 10 milligrams of phosphatidyl ethanolamine and 8.6 milli-grams of cholesterol. These liposomes are purified by repeated centrifugation after which they are resuspended in 2 ml. of 0.1 5 M borate buffer pH ~.5. To this suspension is added 20 micro-liter of 25% glutaraldehyde. After 10 minutes at room tempera-ture, the mixture is dialyzed overnight against 2 liters of borate buffer. The activated liposomes are then added to 2.4 milligrams of bovine serum albumin in 1 ml. borate buffer. The mixture is then incubated overnight at 4C whereupon the lipo-somes with protein attached are separated from unbound protein by centrifugation at 25,000 9 for 30 minutes. Following the assay method described in Examples III and IV and using rabbit antibody to bovine serum albumin~ an immune lysis assay can be prepared which will detect albumin in samples quantitatively in the range of from .1 to 2 ~9 1 ml.
EXAMPLE IX
-In order to assay the cardiac glycoside-digoxin was coupled 20 to dipalmitoylphosphatidylethanolamine. To this end mixture containing 0.5 grams (0.64 mmole)of Digoxin in 20 m1. of Ethanol/
Dioxane (4:1,v/v) was added to 60 ml. of 0.1 M sodium metaperiodate.
The mixture was stirred for 30 minutes at room temperature where-upon 4.5 ml. of ethylene glycol was added. This mixture was 25 stirred for one-half hour at room temperature and evaporated under reduced pressure. The resultant solid was then extracted 3 times with 50 ml. of chloroform. The extracts were pooled ~total volume 150 ml.) and solvent evaporated under reduced pressure, produc-ing 0.9 gm of oily residue. Twenty-five mg of this crude product of digoxin dialdehyde in l ml. oF ethanol/chloroform (1:4) was lC4` " ao ~7S7~
ss~ .
1 added to 20 mg of dipalm;toylphosphatidylethanolamine in 1 ml of ethanol/chloroform (1:2). Four drops of triethylamine were added and the reaction mixture (p~l 9) was incubated overnight at 37C and finally evaporated to a dry residue under reduced pressure. This residue was suspended in 2 ml. of ethanol/chloro-form (1:1) and 4 milligram of sodium borohydride was added.
This mixture was stirred for 30 minutes and then evaporated to dryness under reduced pressure. This residue was then tri-turated with ethanol and filtered to give a filtrate which upon evaporation yielded 45 milligrams of dipalmitoylphosphatidyl-phosphatidylethanolamine-digoxin conjugat;on product.
EXAMPLE X
The conjugate of digoxin anddipalmitoylphosphatidylethanol-amine is employed to prepare liposomes with digoxin. In this case 22 milligrams of dimyristoylphosphatidyl choline, 8.6 milli-grams of cholesterol, 1.6 milligrams of dicetylphosphate, and 2.5 milligrams of Digoxin-dipalmitoylphosphatidylethanolamine con-jugate were dissolved in 3 ml. o~ chloroform. Solvent was evap-orated under reduced pressure and the lipids deposited as a thinfilm on the internal wall of a 100 ml. round-bottomed flask. T~e lipid film was then dispersed in (solution as in Example I
lines 8-10 and purified also as in Example I).
Assays were performed as in Example VI. Inhibition by digoxin in test samples was observed in range of ~.5-10 ng/ml digoxin in the test sample.
Liposomes can be frozen successfully if they are first suspended in an isotonic medium - 0.01 M phosphate buffer con-taining 0.15 M sodium chloride. Also useful are solutions lC4 ~0 ~ ~L 7~ 3 ~SKa 1 buffered in the range From pH 4 to pH 10 containing 0.3 M glucose or like carbohydrate. However, liposomes frozen in proteinaceous media e.g. containing bovine serum albumin of rabbit gamma globu-lins are not preferred as these show elevated levels of enzyme activity in the absence of lytic reagents - detergent or comple-ment plus antibody. 8est results are achieved with rapid freez-ing at a rate of at least 5C per minute. Prior to freezing lipo-somes are suspended in isotonic media at concentrations of 1-10 mg/
ml. For example liposomes prepared as in Example I are suspended in 0.01 M sodium phosphate buffer containing 0.15 M sodium chloride.
This suspension contains 2.5 mg of total lipid in 1 ml of liquid.
0.1 ml aliquots of this mixture are placed in a 5 ml. vial. These are then frozen to -20C at a rate of 5C per minute. The lipo-somes can be thawed and used after long periods of storage.
While specific embodiments of this invention have been shown and described, it will be understood that many variations are possible.
Particular concentrat;ons, combinations and materials can vary greatly 90 long as the signal to noise ratio minimums of the inven-tion are maintained which aids in preventing false readings. A wide variety of materials can be tested in a wide variety of high volume screening test by relatively unskilled personnel.
The material to be tested can be body fluids or mixtures of all kinds. When serum is tested it is preferably treated chemically and/or with heat to remove undesirable inhibition. Prior treat-ment with amino groups is one such chemical method. Typically,0.1 ml of 2.54 M ammonia is added to 1.9 ml of serum which is then neutralized by the addition of 0.1 ml of 2.54 M hydrochloric acid. Also sulthydryl blocking reagents can be useful. In this case 0.1 ml of 0.2 M mercaptoethanolin phosphate buffered saline is added to 1 ml of serum. Then 1 ml of 0.2 M iodoacetamide is - ~L~ 7 lC~ ,740 SSKa 1 is added. Similarly useful is the sulfonic acid azo dye chlora-zol fast pink which selectively inhibits human complement activa-tion but not guinea pig complement. Heat treatment of at least about 58C for at least 30 and preferably 60 minutes is also useful to prevent unwanted inhibltion of the complement reaction.
.
Claims
T? ?40 SSKa The embodiments of the invention in which an exclusive property or privilege is claimed are defined as follows:-1. An immunoreactive liposome labeled with one of an anti-gen or its cognate antibody sequestering an enzyme and having a signal to noise ratio of no less than 5.
2. An immunoreactive liposome in accordance with claim 1 and having in combination therewith the other of said antigen or antibody.
3. The liposome combination of claim 2 and further comprising a plurality of like liposomes being in the presence of a substrate for said enzyme and uniformly dispersed therein.
4. A liposome in combination as set forth in claim 3 and further comprising said liposomes being labeled with an antigen.
5. A liposome as set-forth in claim 3 and further comprising said liposomes being labeled with said antibody.
6. A liposome in accordance with claim 3 wherein said signal to noise ratio is in the range of from 5 to 1,000.
7. A liposome in accordance with claim 3 wherein said antigen is of use in clinical diagnostics.
?C44 ??2 SSKa ?/2/80 8. A liposome in accordance with claim 1 wherein said enzyme is selected from the group consisting essentially of oxidoreductases, hydrolases or mixtures thereof.
9. A liposome in accordance with claim 8 wherein said enzyme is selected from the group consisting essentially of alkaline phos-phates, peroxidase, malate dehydrogenase or mixtures thereof.
10. A liposome in accordance with the liposome of claim 1 , wherein said liposome is formed of a lipid which is a member of the group consisting essentially of water insoluble, swelling amphiphiles of Class II of the Small classification of lipids, with a sterol or similar Class I of the Small classification of lipids, non-swelling amphiphile.
11. An immuno test method comprising forming a mixture of a) a liposome labeled with one of an antigen or its cognate antibody sequestering an enzyme and having a signal to noise ratio of no less than 5;
b) a substrate for said enzyme c) a test material to be tested for specific activity of the said one antigen or cognate antibody; and d) complement, and detecting the presence or absence of enzymatic activity in said mixture under conditions which permit an immune reac-tion to expose said enzyme to said substrate.
1C? ?0 SSKa 12. The test method of claim 11 wherein said detecting is carried out in a homogeneous phase without the need for mechanical separation or purification steps.
13. A test method in accordance with claim 11 and further comprising incorporating in said mixture the other of said antigen and cognate antibody to test for presence or absence of said one cognate.
14. The test method of claim 13 wherein said detecting is carried out in a homogeneous phase.
15. A test method in accordance with the method of claim 13 wherein a plurality of tests are carried out with different concen-trations of said last-mentioned cognate so as to permit a quanti-tative determination of the cognate in said test material.
15. An immuno test method comprising forming a mixture of a) a liposome labeled with one of an antigen or its cognate antibody carrying an enzyme and having a signal to noise ratio of no less than 65;
b) a substrate for said enzyme c) a test material to be tested for specific activity of the other of said one antigen or cognate antibody; and d) complement, and detecting the presence or absence of enzymatic activity in said mixture in a homogenous phase.
17. A test method in accordance with claim 16 and further comprising incorporating in said mixture the other of said antigen and cognate antibody to test for presence or absence of said one cognate.
lC44/740C
SSka 18. An immunoassay test kit for detecting an antigen or its cognate antibody in a test sample, said test kit comprising, a container carrying liposomes labeled with one of antigen or cognate antibody which is to be the subject of the test determination and sequestering an enzyme while having a signal to noise ratio of no less than 5.
19. An immunoassay test kit in accordance with claim 18 and further comprising a container carrying a substrate for said enzyme, and a container carrying complement for said antibody or antigen.
20. An immunoassay test kit in accordance with claim 19 and further comprising a container carrying the cognate of said antibody or antigen.
21. An immunoassay test kit in accordance with claim 19 and further comprising a predetermined concentration of the cognate of said antibody or antigen and acting as a quantitative mechanism for carrying out an immunoassay test.
lC44 32 SSK
22. An immunoassay test kit in accordance with claim 19 and further comprising substrate for said enzyme.
23. An immunoassay test kit in accordance with any of claims 19 to 21wherein said signal to raise ratio is no less than 60.
24. An immunoreactive liposome in accordance with claim 1 wherein said signal to noise ratio is no less than 60.
25. An immunoreactive liposome in accordance with claim 1 wherein said signal to noise ratio is no less than 10.
26. An immunoreactive liposome in accordance with claim 3 wherein said signal to noise ratio is no less than 10.
27. An immunoreactive liposome in accordance with claim 4 wherein said signal to noise ratio is no less than 10.
28. An immunoreactive liposome in accordance with claim 5 wherein said signal to noise ratio is no less than 10.
lC44/740C
SSka 29. An immuno test method in accordance with claim 11 wherein said signal to noise ratio is no less than 10.
30. An immuno test method in accordance with claim 12 wherein said signal to noise ratio is no less than 10.
31. An immuno test method in accordance with claim 16 wherein said signal to noise ratio is no less than 10.
32. An immunoassay test kit in accordance with claim 18 wherein said enzyme has a signal to noise ratio of no less than 10.
33. In an immuno test method for determining antigen or its cognate, the steps comprising combining a liposome labeled with one of the antigen or its cognate antibody and sequestering an enzyme having a signal to noise ratio no less than 5, with a substrate and a material to be tested along with an agent for permitting exposure of the substrate to the enzyme under certain test conditions.
lC4??40 SSKa 34. A test method in accordance with the test method of claim 33 wherein said method is a homogeneous test method.
2. An immunoreactive liposome in accordance with claim 1 and having in combination therewith the other of said antigen or antibody.
3. The liposome combination of claim 2 and further comprising a plurality of like liposomes being in the presence of a substrate for said enzyme and uniformly dispersed therein.
4. A liposome in combination as set forth in claim 3 and further comprising said liposomes being labeled with an antigen.
5. A liposome as set-forth in claim 3 and further comprising said liposomes being labeled with said antibody.
6. A liposome in accordance with claim 3 wherein said signal to noise ratio is in the range of from 5 to 1,000.
7. A liposome in accordance with claim 3 wherein said antigen is of use in clinical diagnostics.
?C44 ??2 SSKa ?/2/80 8. A liposome in accordance with claim 1 wherein said enzyme is selected from the group consisting essentially of oxidoreductases, hydrolases or mixtures thereof.
9. A liposome in accordance with claim 8 wherein said enzyme is selected from the group consisting essentially of alkaline phos-phates, peroxidase, malate dehydrogenase or mixtures thereof.
10. A liposome in accordance with the liposome of claim 1 , wherein said liposome is formed of a lipid which is a member of the group consisting essentially of water insoluble, swelling amphiphiles of Class II of the Small classification of lipids, with a sterol or similar Class I of the Small classification of lipids, non-swelling amphiphile.
11. An immuno test method comprising forming a mixture of a) a liposome labeled with one of an antigen or its cognate antibody sequestering an enzyme and having a signal to noise ratio of no less than 5;
b) a substrate for said enzyme c) a test material to be tested for specific activity of the said one antigen or cognate antibody; and d) complement, and detecting the presence or absence of enzymatic activity in said mixture under conditions which permit an immune reac-tion to expose said enzyme to said substrate.
1C? ?0 SSKa 12. The test method of claim 11 wherein said detecting is carried out in a homogeneous phase without the need for mechanical separation or purification steps.
13. A test method in accordance with claim 11 and further comprising incorporating in said mixture the other of said antigen and cognate antibody to test for presence or absence of said one cognate.
14. The test method of claim 13 wherein said detecting is carried out in a homogeneous phase.
15. A test method in accordance with the method of claim 13 wherein a plurality of tests are carried out with different concen-trations of said last-mentioned cognate so as to permit a quanti-tative determination of the cognate in said test material.
15. An immuno test method comprising forming a mixture of a) a liposome labeled with one of an antigen or its cognate antibody carrying an enzyme and having a signal to noise ratio of no less than 65;
b) a substrate for said enzyme c) a test material to be tested for specific activity of the other of said one antigen or cognate antibody; and d) complement, and detecting the presence or absence of enzymatic activity in said mixture in a homogenous phase.
17. A test method in accordance with claim 16 and further comprising incorporating in said mixture the other of said antigen and cognate antibody to test for presence or absence of said one cognate.
lC44/740C
SSka 18. An immunoassay test kit for detecting an antigen or its cognate antibody in a test sample, said test kit comprising, a container carrying liposomes labeled with one of antigen or cognate antibody which is to be the subject of the test determination and sequestering an enzyme while having a signal to noise ratio of no less than 5.
19. An immunoassay test kit in accordance with claim 18 and further comprising a container carrying a substrate for said enzyme, and a container carrying complement for said antibody or antigen.
20. An immunoassay test kit in accordance with claim 19 and further comprising a container carrying the cognate of said antibody or antigen.
21. An immunoassay test kit in accordance with claim 19 and further comprising a predetermined concentration of the cognate of said antibody or antigen and acting as a quantitative mechanism for carrying out an immunoassay test.
lC44 32 SSK
22. An immunoassay test kit in accordance with claim 19 and further comprising substrate for said enzyme.
23. An immunoassay test kit in accordance with any of claims 19 to 21wherein said signal to raise ratio is no less than 60.
24. An immunoreactive liposome in accordance with claim 1 wherein said signal to noise ratio is no less than 60.
25. An immunoreactive liposome in accordance with claim 1 wherein said signal to noise ratio is no less than 10.
26. An immunoreactive liposome in accordance with claim 3 wherein said signal to noise ratio is no less than 10.
27. An immunoreactive liposome in accordance with claim 4 wherein said signal to noise ratio is no less than 10.
28. An immunoreactive liposome in accordance with claim 5 wherein said signal to noise ratio is no less than 10.
lC44/740C
SSka 29. An immuno test method in accordance with claim 11 wherein said signal to noise ratio is no less than 10.
30. An immuno test method in accordance with claim 12 wherein said signal to noise ratio is no less than 10.
31. An immuno test method in accordance with claim 16 wherein said signal to noise ratio is no less than 10.
32. An immunoassay test kit in accordance with claim 18 wherein said enzyme has a signal to noise ratio of no less than 10.
33. In an immuno test method for determining antigen or its cognate, the steps comprising combining a liposome labeled with one of the antigen or its cognate antibody and sequestering an enzyme having a signal to noise ratio no less than 5, with a substrate and a material to be tested along with an agent for permitting exposure of the substrate to the enzyme under certain test conditions.
lC4??40 SSKa 34. A test method in accordance with the test method of claim 33 wherein said method is a homogeneous test method.
Applications Claiming Priority (4)
Application Number | Priority Date | Filing Date | Title |
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US11786480A | 1980-02-04 | 1980-02-04 | |
US117,864 | 1980-02-04 | ||
US06/222,815 US4342826A (en) | 1980-02-04 | 1981-01-12 | Immunoassay products and methods |
US222,815 | 1981-01-12 |
Publications (1)
Publication Number | Publication Date |
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CA1175740A true CA1175740A (en) | 1984-10-09 |
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Family Applications (1)
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CA000369832A Expired CA1175740A (en) | 1980-02-04 | 1981-01-30 | Immunolabelled liposomes |
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US (1) | US4342826A (en) |
AU (1) | AU551950B2 (en) |
CA (1) | CA1175740A (en) |
CH (1) | CH659136A5 (en) |
DE (1) | DE3103826C2 (en) |
DK (1) | DK436781A (en) |
FR (1) | FR2485038A1 (en) |
GB (1) | GB2069133B (en) |
SE (1) | SE8105827L (en) |
WO (1) | WO1981002344A1 (en) |
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- 1981-01-13 WO PCT/US1981/000040 patent/WO1981002344A1/en unknown
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- 1981-01-13 CH CH6401/81A patent/CH659136A5/en not_active IP Right Cessation
- 1981-01-30 FR FR8101894A patent/FR2485038A1/en active Granted
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- 1981-02-03 GB GB8103282A patent/GB2069133B/en not_active Expired
- 1981-02-04 DE DE3103826A patent/DE3103826C2/en not_active Expired - Fee Related
- 1981-10-02 DK DK436781A patent/DK436781A/en not_active Application Discontinuation
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FR2485038B1 (en) | 1985-03-15 |
DE3103826C2 (en) | 1995-03-16 |
FR2485038A1 (en) | 1981-12-24 |
DE3103826A1 (en) | 1981-12-03 |
AU6785981A (en) | 1981-08-31 |
WO1981002344A1 (en) | 1981-08-20 |
CH659136A5 (en) | 1986-12-31 |
SE8105827L (en) | 1981-10-02 |
US4342826A (en) | 1982-08-03 |
GB2069133A (en) | 1981-08-19 |
GB2069133B (en) | 1984-01-18 |
AU551950B2 (en) | 1986-05-15 |
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