CA1338501C - Method of detecting antibody against htlv-iii - Google Patents
Method of detecting antibody against htlv-iiiInfo
- Publication number
- CA1338501C CA1338501C CA000530796A CA530796A CA1338501C CA 1338501 C CA1338501 C CA 1338501C CA 000530796 A CA000530796 A CA 000530796A CA 530796 A CA530796 A CA 530796A CA 1338501 C CA1338501 C CA 1338501C
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- Prior art keywords
- htlv
- iii
- immunoadsorbent
- antibody
- protein
- Prior art date
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- C07K14/005—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from viruses
-
- 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
- G01N33/569—Immunoassay; Biospecific binding assay; Materials therefor for microorganisms, e.g. protozoa, bacteria, viruses
- G01N33/56983—Viruses
- G01N33/56988—HIV or HTLV
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K38/00—Medicinal preparations containing peptides
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N2740/00—Reverse transcribing RNA viruses
- C12N2740/00011—Details
- C12N2740/10011—Retroviridae
- C12N2740/16011—Human Immunodeficiency Virus, HIV
- C12N2740/16211—Human Immunodeficiency Virus, HIV concerning HIV gagpol
- C12N2740/16222—New viral proteins or individual genes, new structural or functional aspects of known viral proteins or genes
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- 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
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- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S435/00—Chemistry: molecular biology and microbiology
- Y10S435/974—Aids related test
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- 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
- Y10S436/807—Apparatus included in process claim, e.g. physical support structures
- Y10S436/808—Automated or kit
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- 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
- Y10S436/811—Test for named disease, body condition or organ function
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- 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
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- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S530/00—Chemistry: natural resins or derivatives; peptides or proteins; lignins or reaction products thereof
- Y10S530/82—Proteins from microorganisms
- Y10S530/826—Viruses
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- 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
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- Y10S930/00—Peptide or protein sequence
- Y10S930/01—Peptide or protein sequence
- Y10S930/22—Viral peptide or viral protein
- Y10S930/221—Retrovirus related, or human immunodeficiency virus related, or simian immunodeficiency virus related
Abstract
Immunochemical assays for detection of anti-bodies against HTLV-III core proteins are described.
The assays are based upon recombinant HTLV-III core proteins expressed by cloned DNA segments of the gag region of the HTLV-III genome. Immunoreactive, chimeric HTLV-III core proteins and methods of producing these proteins are also described.
The assays are based upon recombinant HTLV-III core proteins expressed by cloned DNA segments of the gag region of the HTLV-III genome. Immunoreactive, chimeric HTLV-III core proteins and methods of producing these proteins are also described.
Description
METHOD OF DETECTING ANTIBODY AGAINST HTLV-III
Field of the Invention This invention is in the fields of immunology and virology and pertains to immunochemical detec-05 tion of AIDS virus infection hased upon recombinantHTLV-III core antigens.
Background of the Invention Since the identification of human T cell lymphotropic virus Type III (~ITLV-III) (also called lymphadenopathy virus (LAV) or AIDS-associated retrovirus (ARV)) as the probable cause of infec-tious Acquired Immunodeficiency Syndrome (AIDS) and the establishment of a permissive T cell line for mass production of the virus, substantial progress has been made in characterizing the virus. - The complete nucleotide sequence of molecular clones of various provirus isolates have been deciphered. See Ratner _ al., (1985) Nature 313, 277-284; Wain-Hobson et al., (1985) Cell 40, 9-17; Sanches-Pescador et al., (1985) Science 227, 484-492;
Muesing et al., (1985) Nature 313, 450-458. The provirus is 9734-9749 base pairs (bp) in length including two long terminal repeat (LTR) sequences.
HTLV-III contains many characteristic structural features of other retroviruses: the long terminal repeats, a core protein gene (~), a gene region (pol) encoding the virion RNA-dependent DNA
polymerase and a gene encoding the virus envelope glycoproteins (env). Unlike other retroviruses the EITLV-III viruses contain two additional small open reading frames (SOR-I and 3'ORF) which may play a 05 role in its unusual cytopathogenicity. See Ratner et al., supra.
HTLV-III gag proteins are synthesized in the form of a polyprotein precursor of 512 amino acids which is proteolytically processed to individual gag proteins pl7, p24 and pl5. Data obtained from the analysis of nucleotide structure and the gag gene products of HTLV-III and ARV indicate that the pl7, p24 and pl5 proteins are 134, 230 and 122 amino acids long respectively. See Ratner et al., Wain-Elobson et al., Sanchez-Pescador et al., and Muesing _ al., supra. Two precursors, p70 and p55, have been detected in HTLV-III infected cells in culture and were shown to share peptide homology with the p24 gag protein Roby et al., (1985). Recently the p24 protein has been isolated from HTLV-III. Casey J.M., et al., (1985), J. Virol., 55 (2), 417-423.
Several methods for the detection of HTLV-III
~ infection also have been developed. Solid-phase immunoassays employing inactivated EITLV-III as a whole virus antigen immunoadsorbent have been developed for the detection of antibodies against HTLV-III in sera of patients. Such assays have been shown to detect antibodies in more than 80% of sera from patients with AIDS or AIDS-related complex ~ARC), or from individuals infected with HTLV-III
-~3~ 1338~01 and these are useful for diagnosing AIDS and for screening contaminated blood.
Assays employing the whole virus, however, have several drawbacks. Large quantities of the virus 05 must be cultivated as supply for test reagents.
Although rigorous safety measures can be instituted, there are dangers associated with large scale cultivation of the infectious virus. Further, there exists a risk, however small, that test reagents prepared with the inactivated virus can be contami-nated with live virus. Thus, persons who handle the reagents may be subjected to the risk of HTLV-III
infection.
Isolated viral p24 protein has been used in an immunoprecipitation assay for detection of anti-HTLV-III antibody in sera of AIDS patients. High serum titer of antibody was found in 73% AIDS
patients. Casey, J.M., et al., supra. Assays employing isolated viral components such as the p24 protein, however, do not eliminate the need for production of the virus. Large scale production of the virus is required for isolation of sufficient quantity of the viral protein for preparation of assay reagents.
Disclosure of the Invention This invention pertains to recombinant HTLV-III
antigenic polypeptides expressed by cloned DNA
segments of the ~ region of the HTLV-III genome and to immunochemical assays for detecting antibody against HTLV-III core protein employing the _, -polypeptides. The recombinant HTLV-III core proteins are immunoreactive with anti-HTLV-III core protein antibodies in the serum HTLV-III infected individuals. Because of this, the recombinant core proteins can be used to detect antibodies against HTLV-III core proteins in a biological fluid. In addition, they can be used in conjunction with immunoreactive recombinant HTLV-III envelop proteins for combined assay of antibody against HTLV-III core and envelop protein.
According to one aspect of the invention, there is thus provided a method of detecting antibody against HTLV-III core protein in a biological fluid, comprising the steps of:
(a) providing an antigen immunoadsorbent comprising a solid phase to which is attached a recombinant HTLV-III core antigen which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein;
b) incubating the immunoadsorbent with a sample of the biological fluid to be tested under conditions which allow antibody in the sample to complex with the antigen immunoadsorbent;
c) separating the immunoadsorbent from the sample; and d) determining antibody bound to the immunoadsorbent as an indication of antibody against HTLV-III core protein in the sample.
According to a further aspect of the invention, - 1338~01 there is provided a method of detecting antibody against HTLV-III core protein in human plasma or serum, comprising the steps of:
a) providing an antigen immunoadsorbent comprising a polystyrene bead coated with an essentially homogeneous purified preparation of pG2 polypeptide;
b) incubating the immunoadsorbent with a sample of human plasma or serum under conditions which permit anti-HTLV-III core protein antibody in the sample to complex with the pG2 polypeptide;
c) separating the immunoadsorbent from the sample;
d) incubating the immunoadsorbent with a solution of labeled anti-human Ig antibody;
e) separating the immunoadsorbent from the solution of labeled antibody; and f) detecting the label associated with the immunoadsorbent as an indication of anti-HTLV-III
core protein antibody in the sample.
The present invention also provides, in another aspect thereof, an immunoadsorbent comprising a solid phase support having attached thereto a recombinant HTLV-III core protein which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein.
Three HTLV-III recombinant core antigens were expressed in bacterial cells. Restriction fragments of HTLV-III gag gene were cloned into E. Coli.
E~
133~01 (Strain JA221) cells to produce three clonal cell lines. One clonal cell line, designated pG1, produces a hybrid protein containing 13 amino acid residues on the C-terminal of the 17Kd virion protein, the entire p24 polypeptide and 74 amino acid residues of the amino terminal of the 15Kd core ribonucleoprotein.
The second clone, pG2, produces a protein similar to pG1 except that it contains no pl7 sequences and lacks the NH2-terminal 77 amino acid residues of the p24. The third clone pG3 expresses a protein similar to pG2 except all but 56 amino acids of the C-terminal of p24 are absent. Thus, the antigens are chimeric molecules made up of portions of the virion pl7, p24 and pl5 core proteins.
The recombinant proteins are expressed by these clones as fusion proteins made up of the HTLV-III
polypeptide (encoded by the cloned gag gene segment) flanked by exogenous (vector supplied) polypeptide elements at the amino and carboxyl terminals. The fusion proteins pG1, pG2 and pG3 are strongly reactive towards anti-gag protein antibodies present in pooled sera from AIDS patients. The immunore-activity of the pG1, pG2 and pG3 proteins indicates that strong antigenic determinants are present between amino acid residues 77 and 175 of the viral p24 protein and residues 1 and 74 of the pl5 proteins.
L~
133~501 The bacterially expressed pG2 protein can be purified to virtual homogeneity. This can be accomplished by dissolution of the protein in a buffer containing a strong denaturant (8M Urea) and by subsequent dialysis and repetitive gel filtration chromotography in the presence of the denaturant. The pG2 protein purified by this technique is immunoreactive with antibody in AIDS patient sera. In strip assays, detection of anti-p24 antibody by pG2 protein correlates with detection of the antibody with whole virus.
The recombinant core antigens provide immuno-chemical methods for detection of antibody against HTLV-III core proteins Immunochemical assays for detection of antibody against HTLV-III core protein can take several forms, including immunometric assays and antigen sandwich assays. The preferred type of assay is a solid phase immunometric (double antibody) assay. The purified ~ derived polypeptide is immobilized by attaching it to solid phase to form an antigen immunoadsorbent.
38~01 The immunoadsorbent is used to adsorb anti-EITLV-III
core protein antibody in a sample of the biological fluid. The adsorbed anti-HTLV-III antibody is detected with an anti-(human IgG) antibody which is 05 labeled radioisotopica]ly, enzymatically, fluoro-metrically or in other ways. This second antibody, directed generally against human IgG, binds to anti-HTLV-III antibody adsorbed to the immuno-adsorbent and provides a detectable signal which can be evaluated as an indication of the presence of anti-HTLV-III core protein antibody in the sample.
HTLV-III core protein can be used in conjunc-tion with ~ITLV-III envelop proteins (e.g. HTLV-III
polypeptide 121) to enhance detection of antibody against the virus. For this purpose, the approxi-mately equimolar amounts of the core protein (e.g.
pG2) and the envelope protein can be affixed to a solid phase to form a dual antigen immunoadsorbent for use in an immunometric assay.
Expression of the pG1, pG2 and pG3 proteins in bclcterial cells and demonstration of the immunoreac-tivity of these proteins establishes that the antigenicity of HTLV-III core proteins can be retained when the proteins are expressed in a host cell system. Further, expression of these proteins enabled identification of certain antigenic regions of p24 and pl5 which can aid in rational design of additional recombinant HTLV-III core antigens. For example, other chimeric core proteins which embody these antigenic protein domains can be produced.
385~1 ,~ji ,. =!
Immunochemical assays employing the ~g derived polypeptides for detection of anti-E~V~T-III core protein antibodies provide several advantages over those based on the whole virus or on isolated viral 05 components. Viral components produced in safe host cells eliminate the need to grow large quantity of the infectious virus for preparation of assay reagents. This alleviates the risk associated with this process. Assay reagents based upon the HTLV-III
antigens rather than the whole virus will help mitigate the real or perceived risk of contracting AIDS by technicians who perform the assay. Addi-tionally, homogenous preparations of core protein can provide for less variability in assay perfor-mance. In whole virus preparation the level of coreprotein may vary and affect the sensitivity of the assay.
Brief Description of the Drawings Figure 1 is a schematic representation of the construction of the HTLV-III ~ gene clones Figure 2 shows SDS-PAGE analysis of HTLV-III
gag gene hybrid proteins, pGl, pG2 and pG3.
Figure 3 shows a Western blot analysis of the immunoreactivity of the pG1, pG2 and pG3 HTLV-III
~ gene clones.
Figure 4 shows SDS-PAGE analysis of purified pG2.
Flgur~ ~ sh~ws the predicted amino acid se-quence for the pG2 protein.
1 1~8SOl Figure 6 illustrates RIA results for antibodies against purified pG2 protein in sera from AIDS/~RC
patients and healthy individuals.
Best Mode of Carrying out the Invention 05 Three recombinant HTLV-III core proteins, designated pGl, pG2 and pG3 were produced by cloning and expressing three segments of DNA from the ~
gene of HTLV-III in E. Coli. The ~ gene of HTLV-III is capable of encoding a protein of 512 amino acid residues. The pl7 protein spans amino acid residues 1-132, the p24 is derived from amino acid residues 133-363 and the pl5 from amino acid residues 378-512. ~mino acids 364-377 are not present in processed, mature viral gag proteins, but are present in pGl, pG2 and pG3 proteins.
The segments were obtained by restriction endonuclease digestion of HTLV-III D~IA. HTLV-III
DNA was excised by Sst I digestion from ~BH-10, a recombinant phage comprising a 9 kb segment of the HTLV-III genome inserted into the vectorlgt WESlB.
See B.H. Haha et al., Nature, 312, 166 (1984). The SstI fragment is shown with the nucleotide numbers above the restriction enzyme designation in Figure 1.
The pGl, pG2 and pG3 gene constructs were made by further digestion of the Sst I fragment. The three constructs are illustrated schematically in Figure 1. The Sst I fragment from ABH-10 was digested with the restriction endonucleases Pvu II
and Bg1 II or Pst I and Bg1 II. PVU II/Bgl II
digestion yielded a 949 bp fragment (corresponding ; 1338501 , `
....
to nucleotide 692 through 1641 of the HTLV-III
genome) and Pst I/Bgl II digestion gave a 677 bp fragment (nucleotides 964-1641). The fragments were inserted into a the "REV" expression vector (Rep-05 ligen, Cambridge, MA) to give plasmid pGl and pG2,respectively.
Plasmid pG3 was constructed from pG2. pG2 DNA
was digested with Pst I and E~ind III, end repaired and ligated, resulting in excision of the Pst I-Hind 10 III fragment from pG2.
E. coli cells were transformed with the recom-binant vectors. Bacterial cells containing the plasmids pG1, pG2 and pG3 expressed proteins of 41Kd, 33Kd and 18Kd, respectively. The expressed 15 proteins were fusion proteins containing a methio-nine residue plus 33 vector encoded amino acid residues at the NH2 terminal of the HTLV-III poly-peptide and 14 vector encoded amino acids at the COOH terminal. The fusion proteins were made in large quantities by the transformed bacterial cell lines (over 10% of total cellular protein). The expressed fusion proteins were tested for reactivity with pooled ~IDS patient sera by Western blot analysis. Each protein was immunoreactive.
The immunoreactivity of the pGl, pG2 and pG3 proteins indicate that these proteins exhibit strong HTLV-III antigenic determinants. The determinants are present between amino acid residues 77-175 of p24 protein and residues 1-74 of the pl5 proteins.
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The pG2 protein was purified to greater than 98% homogeneity by the following procedure. Soluble cellular protein was removed from pG2 cell lysates by extraction with a nondenaturant buffer. The 05 fusion protein pG2 was contained in the insoluble cell pellet at approximately 20% purity. The pG2 protein was solubilized by suspending the cell pellet in an extraction buffer comprising 50 mM
Tris-HCl, 8 M Urea, lM ~laCl, lOmM DL dithiothreitol (DTT) and 0.05% EDTA disodium salt. The suspension was homogenized and centrifuged. pG2 in the super-natant was purified by gel filtration chromatography in the extraction buffer, subsequent dialysis against distilled water, and further gel filtration chromatography in the extraction buffer. The major peak eluted from final gel filtration column con-tained the pG2 protein at greater than 98% purity as judged by SDS-PAGE.
Purified pG2 protein was used in a strip immunoassay to characterize sera from healthy individuals in the high risk population and sera from patients with AIDS or ARC. pG2 protein ad-sorbed onto mitrocellulose strips was incubated with human serum to be tested, washed, then contacted with labeled anti-human IgG to detect antibody bound to the strip. The assay was also performed with dirupted whole virus. pG2 was equally as effective as the whole virus in detecting anti-core protein antibody in sera (100% correlation). Of seroposi-tive healthy homosexuals tested (i.e. those showingantibody reactive with the whole virus), 81% had - 1~ 1338501 ~, .. .
.. ...
antibodies reactive with pG2; the percentage dropped to 56~ for AIDS and ARC patients.
The pG1, pG2 and pG3 proteins are hybrid proteins containing parts of naturally occurring 05 HTLV-III antigens (i.e. the viral pl7, p24 and pl5 core proteins). The success achieved in e~pression of the immunoreactive chimeric core proteins pGl, pG2 and pG3 indicate that the pl7, p24 and plS
proteins themselves can be expressed in host cell systems. In addition, other chimeric HTLV-III core proteins, especially proteins which encompass the identified antigenic domains of the virion proteins p24 and pl5 can be produced. Further, the DNA
segments encoding these polypeptides may be modified (e.g., by deletion, insertion or substitution of nucleotides) to design other HTLV-III core polypep-tides. As used herein, the term "recomhinant core protein" is intended to be inclusive all forms of viral core polypeptides which are expressed by genetically engineered host cells and which are immunoreactive with anti-core protein antibody.
Recombinant HTLV-III core proteins, including the pG1, pG2 and pG3 polypeptides, or equivalent type polypeptides can be produced de novo by recom-binant DNA techniques. HTLV-III now can be rou-tinely and reproducibly isolated from patients with AIDS and propagated in a line of permissive T cells developed for this purpose. M. Popovic et al.
Science 224, 4S7 ~1984); R. C. Gallo et al. Science 224, 500 (1984). From such cells HTLV-III proviral 13385~1 DNA can be obtained and cloned. The designated gag regions of the HTLV-III genome, identified to encode antigenic determinants, can be excised from the proviral DNA (generally by restriction enzyme 05 digestion), inserted into an expression vector, preferably one which can express the polypeptide at high levels, to form a recombinant expression vector containing gag gene sequence. Appropriate host cells transformed by the vector can provide a system for expression of the gene product.
Alternatively, gag DNA segments encoding antigenic regions of the core proteins can be synthesized chemically. Several techniques are available for synthesizing DNA of desired nucleotide sequences. See, e.g., Matteucci et al.~J. Am. Chem.
Soc. (1981) 103:3185; Alvarado-Urbina _ al.~Science (1980) 214:270. Synthesized segments of viral DNA
can be adapted and inserted into an expression vector which can be used to transform vector com-patible host cells and provide for expression of thegene product.
Core proteins containing the identified anti-genic regions of p24 and pl5 can be synthesized chemically. The predicted amino acid sequence of the pG2 protein, for example, is shown in Figure 5; the protein, or proteins, thereof, can be synthesized by the solid phase procedure of Merrifield.
When expressed as heterologous protein in a host cell system, any of several purification techniques, in addition to the techniques described herein for purification of pG2, can be used to purify the recomhinant core proteins. For use in immunoassays, the protein must be purified to substantial immunological purity. Importantly, the preparation should be free of host cell contaminants 05 which might be reactive with antibody in human sera.
Such contaminants could yield a high level of false positive results which would detract from the accuracy of the assay.
Immunochemical assays employing the polypep-tides can take a variety of forms. The preferred type is a solid phase immunometric assay. In assays of this type, the purified recombinant polypeptide is immobilized on a solid phase to form an antigen-immunoadsorbent. The immunoadsorbent is incubated with the sample to be tested. The duration and conditions of the incubation are standard, those appropriate for the formation of the antigen-anti-body complex. The immunoadsorbent is then separated from the sample and a labeled anti-(human IgG) anti-body is used to detect human anti-HTLV-III antibody bound to the immunoadsorbent. The amount of label associated with the immunoadsorbent is compared to positive and negative controls to assess the pre-sence or absence of anti-HTLV-III antibody.
The immunoadsorbent can be prepared by adsorb-ing or coupling purified polypeptide to a solid phase. Various solid phases can be used, such as beads formed of glass, polystyrene, polypropylene, dextran or other material. Other suitable solid phases include tubes or plates formed from or coated with these materials.
1338~01 The recombinant core proteins can be either covalently or non-covalently bound to the solid phase by techniques such as covalent bonding via an amide or ester linkage or adsorption. After the 05 HTLV-III polypeptide is affixed to the solid phase, the solid phase can be post-coated with an animal protein, e.g., 3% fish gelatin. This provides a blocking protein which reduces nonspecific adsorp-tion of protein to the immunoadsorbent surface.
The immunoadsorbent functions to insolubilize anti-core protein antibody in the liquid sample tested. In blood screening for anti-HTLV-III
antibody, the immunoadsorbent is incubated with blood plasma or serum. Before incubation, plasma or serum is diluted with normal animal plasma or serum.
The diluent plasma or serum is derived from the same animal species that is the source of the anti-(human IgG) antibody. The preferred anti-(human IgG) antibody is goat anti-(human IgG) antibody. Thus, in the preferred format, the diluent would be goat serum or plasma. The optimal dilution factor for human plasma and serum is about 10-11 fold.
The conditions of incubation, e.g. pH and temperature, and the duration of incubation are not crucial. These parameters can be optimized by - routine experimentation. Generally, the incubation will be run for 1-2 hours at about 45C in a buffer of pH 7-8.
After incubation, the immunoadsorbent and the sample are separated. Separation can be accom-plished by any conventional separation technique 1~
~ - 1338501 ~,. C .
such as sedimentation or centrifugation. The immunoadsorbent then may be washed free of sample to eliminate any interfering substances.
To assess human antibody bound to the immuno-05 adsorbent, the immunoadsorbent is incubated with thelabeled anti-(human IgG) antibody (tracer). Gene-rally, the immunoadsorbent is incubated with a solution of the labeled anti-(human IgG) antibody which contains a small amount (about 1~) of the 10 serum or plasma of the animal species which serves as the source of the anti-(human IgG) antibody.
Anti-(human IgG) antibody can be obtained from any animal source. However, goat anti-(human IgG) antibody is preferred. The anti-(human IgG) anti-15 body can be an antibody against the Fcfragment ofhuman IgG, for example, goat anti-(human IgG) Fc antibody.
The anti-(human IgG) antibody or anti-(human IgG)F can be labeled with a radioactive material such as l25Iodine; labeled with an optical label, such as a fluorescent material; or labeled with an enzyme such as horse radish peroxidase. The anti-human antibody can also be biotinylated and labeled avidin used to detect its binding to the immuno-adsorbent.
~ fter incubation with the labeled antibody, theimmunoadsorbent is separated from the solution and the label associated with the immunoadsorbent is evaluated. Depending upon the choice of label, the evaluation can be done in a variety of ways. The label may be detected by a gamma counter if the g-1338SOl label is a radioactive gamma emitter, or by a fluorimeter, if the label is a fluorescent material.
In the case of an enzyme label detection may be done colorimetrically employing a substrate for the 05 enzyme.
The amount of label associated with the immuno-adsorbent is compared with positive and negative controls in order to determine the presence of anti-HTLV-III core protein antibody. The controls are generally run concomitantly with the sample to be tested. A positive control is a serum containing antibody against I~TLV-III core protein; a negative control is a serum from healthy individuals which do not contain antibody against HTLV-III core protein.
For convenience and standardization, reagents for the performance of the immunometric assay can be assembled in assay kits. A kit for screening blood, for example, can include:
a~ an immunoadsorbent e.g. a polystyrene bead coated with a recombinant HTLV-III core polypep-tide;
b) a diluent for the serum or plasma sample, e.g. normal goat serum or plasma;
c) an anti-(human IgG) antibody e.g. goat anti-(human IgG) antibody in buffered, aqueous solution containing about 1~ goat serum or plasma;
d) a positive control i.e. serum containing antibody against polypeptide 121; and ~9 13~8501 e) a negative control e.g. pooled sera from healthy individuals which does not contain antibody against polypeptide 121.
If the label is an enzyme, an additional element of 05 the kit can be the substrate for the enzyme.
Another type of assay for anti-HTLV-III anti-body is an antigen sandwich assay. In this assay, a labeled HTLV-III recombinant polypeptide is used in place of anti-(human IgG) antibody to detect anti-10 HTLV-III antibody bound to the immunoadsorbent. The assay is based in principle on the bivalency of antibody molecules. One binding site of the anti-body binds the antigen affixed to the solid phase;
the second is available for binding the labeled 15 antigen. The assay procedure is essentially the same as described for the immunometric assay except that after incubation with the sample, the immuno-adsorbent is incubated with a solution of labeled core polypeptide. The HTLV-III polypeptide can be labeled with radioisotope, an enzyme, etc. for this type of assay.
In a third format, the bacterial protein, Protein A, which binds the Fc segment of an IgG
molecule without interfering with the antigen-25 antibody interaction can be used as the labeled tracer to detect anti-HTLV-III-antibody adsorbed to the immunoadsorbent. Protein A can be readily labeled with a radioisotope, enzyme or other detect-a~le species.
Some serum samples appear to show stronger reactivity towards HTLV-III core protein than toward - ~ 1338~01 HTLV-III envelop protein. This suggests that combined testing for antibody against both viral core and envelop proteins might enhance the overall sensitivity of a test for HTLV-III infection. The use of the combination of homogenous preparations of recombinant core and envelop protein, rather than the whole virus, for this purpose would eliminate false positives encountered with assays based on preparations of whole virus (which can contain host cell contaminants). This would reduce the waste of valuable blood units.
A combination assay can be used based upon homogenous polypeptide pG2 and recombinant env protein. A suitable HTLV-III env protein is HTLV-III
polypeptide 121 described in European Patent Application published under No. 199,438 on October 29, 1986. A mixture of pG2 and polypeptide 121, preferably containing approximately equimolar amounts of the two antigens, can be applied to a solid phase to form a double antigen immunoadsorbent for adsorption of antibody against either antigen. The assay would be conducted in the same manner as that described for the pG2 assay above.
Immunochemical assays employing recombinant HTLV-III core proteins for detection of antibodies against HTLV-III core protein have several advan-tages over those employing a whole (or disrupted) virus for this purpose. For one, assays based upon the polypeptide will alleviate the concern over growing large quantities of infectious virus and the inherent variability associated with cell culturing and virus production. Efficient expression of viral antigens in E. coli. as other host cell systems 05 provide a safe means of large scale production of assay reagents. Further, the assay will help mitigate the real or perceived fear of contracting AIDS by technicians in hospitals, clinics and blood banks who perform the test. As mentioned, reagents 10 for assays based upon the whole virus (e.g. whole virus antigen immunoadsorbent), even though they are made with a disrupted, inactivated virus, present a risk of contamination with live virus. For example, a possible source of live virus contamination may be 15 residual cell debris from the virus isolation process. Although extensive precautions can be taken to reduce the risk of contamination, it is virtually impossible to completely eliminate it.
Significantly, the risk, though minimal, may be 20 perceived as greater than it actually is by persons who handle the test reagents. Assay reagents without whole virus can help minimize this percep-tion of risk. Immunoassays based upon viral compo-nents in safe host cell systems provide a substitute for assays based on the whole virus which are at least comparable in sensitivity and specificity and superior in reproducibility.
Assays employing natural, isolated HTLV-III
core proteins, e.g. p24 protein, while they elimi-30 nate the use of whole virus from assay reagents,still require the growth of the virus on a large nr~
scale for a supply of the natural protein and thus do not eliminate the risks attendant to this proce-dure.
The invention is illustrated further by the 05 following Exemplifications.
Exemplification Bacterial strains and plasmids E. coli strain JA221 (lpp ) was used in all experiments as the host cell. Ghrayeb et al. (1984) 10 EMBO J. 3. 2437-2442. Cells were grown in L-Broth supplemented with ampicillin (100 g/ml). The REV
(Repligen, Cambridge, MA) expression vector was used for cloning of the HTLV-III DMA.
DNA manipulations Isolation of plasmid DNA and various manipula-tions were carried out as previously described by L.C. Ghrayeb et al., i.e. supra. Restriction enzymes were obtained from New England Biolabs. T4 DNA ligase was purchased from Boehringer Mannheim 20 Biochemicals. The DNAs were digested with restric-tion enzymes in conditions described by the manu-facturer.
Expression and analysis of the gag gene clones HTLV-III ~ proteins produced by recombinant 25 clones PGl, PG2 and PG3 were analyzed by SDS-poly-acrylamide gel electrophoresis ~SDS-PAGE) as de-scribed previously. See Chang, N. T. et al., (1985), Science, 228, 93-96. Cells were grown in 1 ml L-broth at 37C overnight and the cells were ~3 1338501 -harvested by centrifugation at 5000 x g for 10 minutes. The cell pellets were dissolved in 200 ul of loading buffer and 20 ul was applied to a 12%
SDS-polyacrylamide gel and electrophoresed under 05 reducing conditions. Unlabeled molecular weight markers were obtained from Biorad Laboratories.
[14C]-labeled molecular weight markers were obtained from Amersham. The expression of HTLV-III specific protein by the recombinant clones was detected by Western blotting analysis using sera from AIDS
patients. Bacterial proteins were separated on a 12% SDs-polyacrylamide gel and transferred to nitrocellulose and blotted as described below. The blot was incubated overnight at 4C with sera from AIDS patients or from healthy individuals. After washing, virus specific protein bands were vis-ualized by incubation with [ I]-labeled goat anti-human IgG (see below). The blots were air dried and exposed to Kodak X-AR5 at -70C with intensifying screens.
Purification of the pG2 protein For large scale growth, 20 ml of an overnight culture of pG2 were inoculated into 1 liter of L-BROTH containing 100 ~g/ml of ampicillin and 0.025% antifoam, and sha~en at 37C. The cells were ~ harvested after 8 hr and washed with 50 mM Tris-HCl p~I 8.5 (sonication buffer). 25 g of cell pellet were suspended in 70 ml of sonication buffer and sonicated in two portions at 70 W for eight 30 sec bursts with a 60 sec cooling period between each * Trade Mark.
~, , . .
~i 1338~01 t ~ ,~
burst. The lysed cells were then centrifuged at 10,000 xg for 30 min. All of the pG2 protein was found in the pellet and constituted approximately 20% of the total protein as judged by SDS-PAGE.
05 The pellet containing the pG2 protein was suspended in 50 mM Tris-HC1 pH 8.5 containing 8 ~
Urea, 1 M NaCl, 10 mM DL dithiothreitol (DTT) and 0.05~ EDT~ disodium salt (extraction buffer). The suspension was incubated at 45C for 60 min and centrifuged at 10,000 xg for 30 min. The resulting supernatant was applied to a SEPHACRYL S-300 gel filtration column (5 x 80 cm) previously equili-brated with extraction buffer containing 5 m~S DTT.
The column was eluted in the same buffer at a flow rate of 0.5 ml/min at room temperature and the fractions (lO ml) were monitored by U.V. absorption at 280 nm. The pG2 protein, found in the second main peak, was pooled and dialyzed exhaustively against distilled water at 4C. During dialysis, the pG2 protein was precipitated quantitatively.
The precipitated protein was then redissolved in 10 ml of extraction buffer containing lO mM DTT and incubated at 45C for 30 min. The resulting solu-tion was applied to a second SEPHACRYL S-300 column (2.6 x 65 cm) under identical conditions to the first column. The ma~or peak contained the pG2 protein which was 95~ pure as judged by SDS-PAGE.
The protein was further purified by repeating the second column purification under identical condi-tions. The main peak from the third S-300 column contained the pG2 protein in 98% purity. The yield * Trade Mark.
~i was 50 mg and this preparation was used for screening human sera (see below).
Immunoreactivity of pG2 with ~luman Sera 50~ g of pure pG2 protein or 430~g of purified 05 disrupted HTLV-III virus, were electrophoresed on a 12% SDS polyacrylamide gel (13 cm x 13 cm x 1.5 mm) and transferred to nitrocellulose using a Biorad Tran-Blot apparatus. The electroblotting buffer used was 20% aqueous methanol containing 0.016 M
Tris base and 0.13 M glycine, and transfer was performed at 40 volts at 4C overnight. The nitro-cellulose paper was then shaken for 2 hr at 37C
with 60 ml of PBS containing 5% non-fat dry milk, 0.1% sodium azide and 0.1% antifoam (milk buffer) and then for 2 hrs at room temperature with 60 ml of 5% normal goat serum in milk buffer. ~t this stage, the blocked nitrocellulose was either stored at -20C, or used directly for the strip assay. The nitrocellulose was cut into 13 cm x 0.5 cm strips, and each strip was rocked overnight at 4C with 4 ml of milk buffer containing 5~ normal goat serum and 40~1 of the human serum to be tested in a 15 ml disposable conical tube. The next day the milk solution was replaced with 10 ml of 0.15% sodium deoxycholate, O.lM NaCl, 0.5% triton X-100, 0.1 m~l phenylmethylsulfonyl fluoride in 10 mM sodium phosphate pH 7.5 (wash buffer) and the tubes were rocked for 1 hr. The wash buffer was removed and replaced with 4ml 5% goat serum in milk buffer and the tubes were rocked for 1 hr, at which time 125[I]-labeled goat anti-human IgG (10 cpm/ml) was ~ -~ 1338501 added. After 30 min, the strips were washed for 1 hr with 10 ml of wash buffer, air dried and exposed to Kodak XA~-5 film at -70C with intensifying screens.
05 Radioimmunoassay 96 well microtiter dishes were coated with the antigen at lOO~g/ml in 50 mM Tris-HCl pH 8Ø After an overnight incubation, the wells were washed three times with phosphate buffered saline (PBS). The 10 wells were then post coated with 200 ~1 3% fish gelatin (Norland Products, Inc.) in PBS containing 0.1% sodium azide. The fish gelatin solution was removed and each well was filled with 200 ~l of 1:5 or 1:10 dilutions of the test serum in PBS contain-15 ing 10% normal goat serum, 10% anti-E. coli goat serum and 1% fish gelatin. After one hour at room temperature, the wells were washed three times with PBS and 200~1 of [1 I]-labeled goat anti-human IgG
(Fc portion) in 1% normal goat serum, 1% fish 20 gelatin in PBS at 1.5x106 cpm/ml was added to each well. After one hour at room temperature, the plates were washed four times with PBS and once with distilled water and counted.
RESULTS
25 Construction of the HTI,V-III gag gene clones The isolation of recombinant phage clone BEI10 containing the unintegrated linear form of HTLV-III
proviral DNA has been reported previously. Shaw et al., (1985), Science, 226, 1165-1171. The 9 Kb ~i 133850~
HTLV-III insert of phage BHlO was released by SstI
cleavage within the R element of the LTR (See Figure 1). The SstI fragment was then digested with either PvuII and ~II or PstI and ~II. The 949 bp 05 PvuII-BglII fragment and the 677 bp PstI-~fragments were inserted into the REV expression vector ~Repligen, Cambridge, MA) to give pGl and pG2 respectively (Figure 1). Clone pG3 was constructed from pG2. pG2 DN~ was digested with PstI and HindIII, end repaired and ligated. Thus, in pG3 the PstI-H _ III fragment was deleted from the HTLV-III
DNA insert of pG2. As seen from Figure 1, the three constructs carry HTLV-III DNA that is predicted to code for chimeric peptides containing various portions of the pl7, p24 and pl5 viral gag proteins.
See Ratner et al., (1985), Nature, 313, 277-284.
The sizes of the expressed proteins are larger than predicted since the expression vector supplies the initiation methionine codon plus 35 amino residues at the NH2-terminus of each expressed protein.
Expression of the HTLV-III gag gene clones E. coli transformed with plasmids, pGl, pG2 or pG3 were found to produce proteins of 41kd, 33kd and 18kd, respectively, as demonstrated by SDS-polacryl-amide gel electrophoresis of total bacterial celllysates. SDS-PAGE analysis of HTLV-III gag gene proteins is shown in Figure 2. Cells from lml cultures were centrifuged and the pellets resus-pended in 200~1 of SDS sample buffer and analyzed by SDS-PAGE as described above. 20 lul of cell lysate ~-' 1338501 were loaded per lane and gels were stained with commassie brilliant blue R250. (Lane 1, molecular weight markers, lane 2, control cells with no plasmid, lane 3, pGl, lane 4, pG2, lane 5, pG3, lane 05 6, cells carrying the REV vector containing no HTLV-III D~IA. The number on the left designate the molecular weights in kilodaltons.) All three proteins were made in large quanti-tied (over 10~ of total cellular protein in these 10 cells) but were not detected in the host cell with or without the REV vector alone. The overproduction of the plasmid encoded HTLV-III ~ proteins caused a marked decrease in the rate of cell growth. The kinetics of the growth rate could be correlated with 15 the accumulation of the ~ gene products in the cytoplasm although no cell lysis was observed (data not shown). Maximum accumulation was observed at 8 hours after the start of the log phase growth period. In addition, the expressed ~ gene pro-20 ducts were present as aggregates containing membraneproteins after disruption of the cells. Depending on growth conditions, HTLV-III gag proteins of smaller size could be detected on SDS-PAGE gels (Figure 2). The products are likely due to the 25 degradation of the major high molecular weight proteins with increasing growth time.
Immunochemical characterization of the gag gene products The bacterial expressed EITLV-III ~-specific protein in cells carrying pGl, pG2 or pG3 were ., ~q 13385ol detected by Western blot analysis using sera pooled from AIDS patients. The results of this analysis are shown in Figure 3. SDS-PAGE analysis was performed exactly as in Figure 2. Transfer of 05 proteins to nitrocellulose paper, reaction with antibodies and detection of immunoreactive bands is described above. Figure 3 shows a blot in which lane 1 is control cells, lane 2 is pG1, lane 3 is pG2 and lane 4 is pG3. The blot was treated with 10 pooled sera from AIDS patients. The numbers on the left designate the relative position of the [14C]
molecular weight markers that were run along with the samples in lanes 1-4, but are not shown in the figure. The result clearly shows the synthesis of 15 specifically cross-reacting HTLV-III peptide in recombinant clones containing pG1, pG2 and pG3. The immunoreactive proteins in each clone corresponded to the expressed proteins, 41kd, 33kd, 18kd, seen in the Coomassie blue stained SDS-polyacrylamide gel 20 (Figure 2). There was no HTLV-III virion-specific peptide detected in lysate of control JA221 cells.
The products of pG2 was purified to greater than 98% homogeneity as judged by SDS-P~GE. Figure 4 shows SDS-PAGE analysis of pG2 purified as de-25 scribed above. PG-2 protein eluted from a sephacryl S-300 column in 50 mr~ Tris-HCL pH 8.5 containing 8M
Urea, lM NaCl and 5 mM DTT, was mixed with an equal volume of 2X SDS-PAGE sample buffer, heated at 100C
for 5 min and applied to two identical 12% SDS-PAGE
30 gels. One of the gels was stained with Coomassie Brilliant Blue (panel 7), while the other trans-~ 1338SOl ferred to nitrocellose and the blot treated withpooled sera from AIDS patients (panel B) as in Figure 3. Panel A, lane 1 is molecular weight markers, lane 2, 3, 4 are pure pG2 at 2, 5 and 10 05 g respectively. Panel B is identical to A except that lane 1 was run with 14[C]-labeled molecular weight markers.
The major band is of 33 kd while there is a minor band of 30 kd which is also seen in total cell lysates (Figure 2) and is most likely a degradation product. A very minor band of 65 kd can also be seen and is most likely to be the dimer form of pG2.
All the bands that are visible by Commassie blue staining are also immunoreactive towards HTLV-III
specific antibodies present in sera from AIDS
patients (Figure 4B) as well as the anti-P24 mouse monoclonal antibody (data not shown). We feel confident that the pG2 protein is essentially free of contaminating E. coli. proteins.
The purified pG2 protein was used to screen for antibodies directed towards the core p24 protein in human sera, using a strip assay based on tlle western blot technique. The same samples were also tested under identical conditions, using the purified, disrupted HTLV-III virus. The results are summa-rized in Table 1.
i, ~
~;
13~8~01 Table 1 No. Positive No. For p24 of No. Positive Clinical StatusTested HTLV-III Using pG2 Healthy donors 50 0 0 Elealthy homosexuals* 49 17 17 ARC** 51 28 28 AIDS*~ 34 19 19 *Only 21 of these donors were seropositive for antibodies to either p24 and/or gp41 of HTLV-III.
In addition, the same individuals who were positive 05 for p24 antibodies using the whole virus assay were also positive for antibodies to pG2.
**All these sera were positive for antibodies to gp41.
The results show that there is 100~ correlation between p24 antibodies detected by pG2 protein and those detected by the whole virus. In addition, none of the normal donor controls were reactive with pG2 protein. This indicates the recombinant pG2 protein can substitute adequately for the whole virus when detection of p24 antibodies is required.
The data presented in Table 1 also show that of the 21 seropositive healthy homosexuals tested, 17 (81~) had detectable antibodies to the p24. In both ARC
and AIDS patients, the percentage drops to 56~.
Whether the anti-p24 antibody titer is an indication of the progress of E~TLV-III infection remains to be studied. In this regard, the uses of pG2 protein in such studies would be preferable since the levels of p24 protein in different virus preparations may vary and may affect the sensitivity of the assay.
1~38~01 Partially purified pG2 protein was tested in a solid phase RIA. Details of the plate RIA assay are given above. The pG? protein preparation used was only "partially" purified. 24 sera from ~IDS/~RC
05 patients and 24 sera from healthy individuals were used in the assay and results were plotted on a semi-log scale. The horizontal dotted line desig-nates the cut-off points so that values below the line are considered negative while those above are considered positive. The results are shown in Figure 6. The results indicated that 18 out of the 24 AIDS or ARC patients' sera tested were reactive with the antigen. The 6 sera from patients with AIDS or ~RC that were negative in the RIA assay were found to contain no detecta~le amounts of anti-p24 _ antibodies as assayed by a strip immunoassay base on Western blot technique using the purified disrupted whole virus (data not shown). Of the 24 normal human sera tested in the RI~, only one was positive but was negative when tested ~ith the purified virus in a Western blot (data not shown). The reactivity of the one normal sample may be due to the presence of unusually high titre of anti-E. coli antibodies present in that particular serum and the fact that the pG2 antigen preparation contained trace amounts of E. coli protein impurities. This nonspecific immunoreactivity can be eliminated by absorption of this serum with SEPHAROSE 4B conjugated with E. coli extract. ~lternatively, better purified pG2 prepara-tions such as the preparation used in the stripassay can be used.
* Trade Mark.
33` 1338501 Equivalents Those skilled in the art will recognize, or be able to ascertain no more than routine experimenta-tion, many equivalents to the specific embodiments 05 of the invention described herein. Such equivalents are intended to be encompassed by the following c lalms .
Field of the Invention This invention is in the fields of immunology and virology and pertains to immunochemical detec-05 tion of AIDS virus infection hased upon recombinantHTLV-III core antigens.
Background of the Invention Since the identification of human T cell lymphotropic virus Type III (~ITLV-III) (also called lymphadenopathy virus (LAV) or AIDS-associated retrovirus (ARV)) as the probable cause of infec-tious Acquired Immunodeficiency Syndrome (AIDS) and the establishment of a permissive T cell line for mass production of the virus, substantial progress has been made in characterizing the virus. - The complete nucleotide sequence of molecular clones of various provirus isolates have been deciphered. See Ratner _ al., (1985) Nature 313, 277-284; Wain-Hobson et al., (1985) Cell 40, 9-17; Sanches-Pescador et al., (1985) Science 227, 484-492;
Muesing et al., (1985) Nature 313, 450-458. The provirus is 9734-9749 base pairs (bp) in length including two long terminal repeat (LTR) sequences.
HTLV-III contains many characteristic structural features of other retroviruses: the long terminal repeats, a core protein gene (~), a gene region (pol) encoding the virion RNA-dependent DNA
polymerase and a gene encoding the virus envelope glycoproteins (env). Unlike other retroviruses the EITLV-III viruses contain two additional small open reading frames (SOR-I and 3'ORF) which may play a 05 role in its unusual cytopathogenicity. See Ratner et al., supra.
HTLV-III gag proteins are synthesized in the form of a polyprotein precursor of 512 amino acids which is proteolytically processed to individual gag proteins pl7, p24 and pl5. Data obtained from the analysis of nucleotide structure and the gag gene products of HTLV-III and ARV indicate that the pl7, p24 and pl5 proteins are 134, 230 and 122 amino acids long respectively. See Ratner et al., Wain-Elobson et al., Sanchez-Pescador et al., and Muesing _ al., supra. Two precursors, p70 and p55, have been detected in HTLV-III infected cells in culture and were shown to share peptide homology with the p24 gag protein Roby et al., (1985). Recently the p24 protein has been isolated from HTLV-III. Casey J.M., et al., (1985), J. Virol., 55 (2), 417-423.
Several methods for the detection of HTLV-III
~ infection also have been developed. Solid-phase immunoassays employing inactivated EITLV-III as a whole virus antigen immunoadsorbent have been developed for the detection of antibodies against HTLV-III in sera of patients. Such assays have been shown to detect antibodies in more than 80% of sera from patients with AIDS or AIDS-related complex ~ARC), or from individuals infected with HTLV-III
-~3~ 1338~01 and these are useful for diagnosing AIDS and for screening contaminated blood.
Assays employing the whole virus, however, have several drawbacks. Large quantities of the virus 05 must be cultivated as supply for test reagents.
Although rigorous safety measures can be instituted, there are dangers associated with large scale cultivation of the infectious virus. Further, there exists a risk, however small, that test reagents prepared with the inactivated virus can be contami-nated with live virus. Thus, persons who handle the reagents may be subjected to the risk of HTLV-III
infection.
Isolated viral p24 protein has been used in an immunoprecipitation assay for detection of anti-HTLV-III antibody in sera of AIDS patients. High serum titer of antibody was found in 73% AIDS
patients. Casey, J.M., et al., supra. Assays employing isolated viral components such as the p24 protein, however, do not eliminate the need for production of the virus. Large scale production of the virus is required for isolation of sufficient quantity of the viral protein for preparation of assay reagents.
Disclosure of the Invention This invention pertains to recombinant HTLV-III
antigenic polypeptides expressed by cloned DNA
segments of the ~ region of the HTLV-III genome and to immunochemical assays for detecting antibody against HTLV-III core protein employing the _, -polypeptides. The recombinant HTLV-III core proteins are immunoreactive with anti-HTLV-III core protein antibodies in the serum HTLV-III infected individuals. Because of this, the recombinant core proteins can be used to detect antibodies against HTLV-III core proteins in a biological fluid. In addition, they can be used in conjunction with immunoreactive recombinant HTLV-III envelop proteins for combined assay of antibody against HTLV-III core and envelop protein.
According to one aspect of the invention, there is thus provided a method of detecting antibody against HTLV-III core protein in a biological fluid, comprising the steps of:
(a) providing an antigen immunoadsorbent comprising a solid phase to which is attached a recombinant HTLV-III core antigen which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein;
b) incubating the immunoadsorbent with a sample of the biological fluid to be tested under conditions which allow antibody in the sample to complex with the antigen immunoadsorbent;
c) separating the immunoadsorbent from the sample; and d) determining antibody bound to the immunoadsorbent as an indication of antibody against HTLV-III core protein in the sample.
According to a further aspect of the invention, - 1338~01 there is provided a method of detecting antibody against HTLV-III core protein in human plasma or serum, comprising the steps of:
a) providing an antigen immunoadsorbent comprising a polystyrene bead coated with an essentially homogeneous purified preparation of pG2 polypeptide;
b) incubating the immunoadsorbent with a sample of human plasma or serum under conditions which permit anti-HTLV-III core protein antibody in the sample to complex with the pG2 polypeptide;
c) separating the immunoadsorbent from the sample;
d) incubating the immunoadsorbent with a solution of labeled anti-human Ig antibody;
e) separating the immunoadsorbent from the solution of labeled antibody; and f) detecting the label associated with the immunoadsorbent as an indication of anti-HTLV-III
core protein antibody in the sample.
The present invention also provides, in another aspect thereof, an immunoadsorbent comprising a solid phase support having attached thereto a recombinant HTLV-III core protein which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein.
Three HTLV-III recombinant core antigens were expressed in bacterial cells. Restriction fragments of HTLV-III gag gene were cloned into E. Coli.
E~
133~01 (Strain JA221) cells to produce three clonal cell lines. One clonal cell line, designated pG1, produces a hybrid protein containing 13 amino acid residues on the C-terminal of the 17Kd virion protein, the entire p24 polypeptide and 74 amino acid residues of the amino terminal of the 15Kd core ribonucleoprotein.
The second clone, pG2, produces a protein similar to pG1 except that it contains no pl7 sequences and lacks the NH2-terminal 77 amino acid residues of the p24. The third clone pG3 expresses a protein similar to pG2 except all but 56 amino acids of the C-terminal of p24 are absent. Thus, the antigens are chimeric molecules made up of portions of the virion pl7, p24 and pl5 core proteins.
The recombinant proteins are expressed by these clones as fusion proteins made up of the HTLV-III
polypeptide (encoded by the cloned gag gene segment) flanked by exogenous (vector supplied) polypeptide elements at the amino and carboxyl terminals. The fusion proteins pG1, pG2 and pG3 are strongly reactive towards anti-gag protein antibodies present in pooled sera from AIDS patients. The immunore-activity of the pG1, pG2 and pG3 proteins indicates that strong antigenic determinants are present between amino acid residues 77 and 175 of the viral p24 protein and residues 1 and 74 of the pl5 proteins.
L~
133~501 The bacterially expressed pG2 protein can be purified to virtual homogeneity. This can be accomplished by dissolution of the protein in a buffer containing a strong denaturant (8M Urea) and by subsequent dialysis and repetitive gel filtration chromotography in the presence of the denaturant. The pG2 protein purified by this technique is immunoreactive with antibody in AIDS patient sera. In strip assays, detection of anti-p24 antibody by pG2 protein correlates with detection of the antibody with whole virus.
The recombinant core antigens provide immuno-chemical methods for detection of antibody against HTLV-III core proteins Immunochemical assays for detection of antibody against HTLV-III core protein can take several forms, including immunometric assays and antigen sandwich assays. The preferred type of assay is a solid phase immunometric (double antibody) assay. The purified ~ derived polypeptide is immobilized by attaching it to solid phase to form an antigen immunoadsorbent.
38~01 The immunoadsorbent is used to adsorb anti-EITLV-III
core protein antibody in a sample of the biological fluid. The adsorbed anti-HTLV-III antibody is detected with an anti-(human IgG) antibody which is 05 labeled radioisotopica]ly, enzymatically, fluoro-metrically or in other ways. This second antibody, directed generally against human IgG, binds to anti-HTLV-III antibody adsorbed to the immuno-adsorbent and provides a detectable signal which can be evaluated as an indication of the presence of anti-HTLV-III core protein antibody in the sample.
HTLV-III core protein can be used in conjunc-tion with ~ITLV-III envelop proteins (e.g. HTLV-III
polypeptide 121) to enhance detection of antibody against the virus. For this purpose, the approxi-mately equimolar amounts of the core protein (e.g.
pG2) and the envelope protein can be affixed to a solid phase to form a dual antigen immunoadsorbent for use in an immunometric assay.
Expression of the pG1, pG2 and pG3 proteins in bclcterial cells and demonstration of the immunoreac-tivity of these proteins establishes that the antigenicity of HTLV-III core proteins can be retained when the proteins are expressed in a host cell system. Further, expression of these proteins enabled identification of certain antigenic regions of p24 and pl5 which can aid in rational design of additional recombinant HTLV-III core antigens. For example, other chimeric core proteins which embody these antigenic protein domains can be produced.
385~1 ,~ji ,. =!
Immunochemical assays employing the ~g derived polypeptides for detection of anti-E~V~T-III core protein antibodies provide several advantages over those based on the whole virus or on isolated viral 05 components. Viral components produced in safe host cells eliminate the need to grow large quantity of the infectious virus for preparation of assay reagents. This alleviates the risk associated with this process. Assay reagents based upon the HTLV-III
antigens rather than the whole virus will help mitigate the real or perceived risk of contracting AIDS by technicians who perform the assay. Addi-tionally, homogenous preparations of core protein can provide for less variability in assay perfor-mance. In whole virus preparation the level of coreprotein may vary and affect the sensitivity of the assay.
Brief Description of the Drawings Figure 1 is a schematic representation of the construction of the HTLV-III ~ gene clones Figure 2 shows SDS-PAGE analysis of HTLV-III
gag gene hybrid proteins, pGl, pG2 and pG3.
Figure 3 shows a Western blot analysis of the immunoreactivity of the pG1, pG2 and pG3 HTLV-III
~ gene clones.
Figure 4 shows SDS-PAGE analysis of purified pG2.
Flgur~ ~ sh~ws the predicted amino acid se-quence for the pG2 protein.
1 1~8SOl Figure 6 illustrates RIA results for antibodies against purified pG2 protein in sera from AIDS/~RC
patients and healthy individuals.
Best Mode of Carrying out the Invention 05 Three recombinant HTLV-III core proteins, designated pGl, pG2 and pG3 were produced by cloning and expressing three segments of DNA from the ~
gene of HTLV-III in E. Coli. The ~ gene of HTLV-III is capable of encoding a protein of 512 amino acid residues. The pl7 protein spans amino acid residues 1-132, the p24 is derived from amino acid residues 133-363 and the pl5 from amino acid residues 378-512. ~mino acids 364-377 are not present in processed, mature viral gag proteins, but are present in pGl, pG2 and pG3 proteins.
The segments were obtained by restriction endonuclease digestion of HTLV-III D~IA. HTLV-III
DNA was excised by Sst I digestion from ~BH-10, a recombinant phage comprising a 9 kb segment of the HTLV-III genome inserted into the vectorlgt WESlB.
See B.H. Haha et al., Nature, 312, 166 (1984). The SstI fragment is shown with the nucleotide numbers above the restriction enzyme designation in Figure 1.
The pGl, pG2 and pG3 gene constructs were made by further digestion of the Sst I fragment. The three constructs are illustrated schematically in Figure 1. The Sst I fragment from ABH-10 was digested with the restriction endonucleases Pvu II
and Bg1 II or Pst I and Bg1 II. PVU II/Bgl II
digestion yielded a 949 bp fragment (corresponding ; 1338501 , `
....
to nucleotide 692 through 1641 of the HTLV-III
genome) and Pst I/Bgl II digestion gave a 677 bp fragment (nucleotides 964-1641). The fragments were inserted into a the "REV" expression vector (Rep-05 ligen, Cambridge, MA) to give plasmid pGl and pG2,respectively.
Plasmid pG3 was constructed from pG2. pG2 DNA
was digested with Pst I and E~ind III, end repaired and ligated, resulting in excision of the Pst I-Hind 10 III fragment from pG2.
E. coli cells were transformed with the recom-binant vectors. Bacterial cells containing the plasmids pG1, pG2 and pG3 expressed proteins of 41Kd, 33Kd and 18Kd, respectively. The expressed 15 proteins were fusion proteins containing a methio-nine residue plus 33 vector encoded amino acid residues at the NH2 terminal of the HTLV-III poly-peptide and 14 vector encoded amino acids at the COOH terminal. The fusion proteins were made in large quantities by the transformed bacterial cell lines (over 10% of total cellular protein). The expressed fusion proteins were tested for reactivity with pooled ~IDS patient sera by Western blot analysis. Each protein was immunoreactive.
The immunoreactivity of the pGl, pG2 and pG3 proteins indicate that these proteins exhibit strong HTLV-III antigenic determinants. The determinants are present between amino acid residues 77-175 of p24 protein and residues 1-74 of the pl5 proteins.
~r .,1~`.
", ~
The pG2 protein was purified to greater than 98% homogeneity by the following procedure. Soluble cellular protein was removed from pG2 cell lysates by extraction with a nondenaturant buffer. The 05 fusion protein pG2 was contained in the insoluble cell pellet at approximately 20% purity. The pG2 protein was solubilized by suspending the cell pellet in an extraction buffer comprising 50 mM
Tris-HCl, 8 M Urea, lM ~laCl, lOmM DL dithiothreitol (DTT) and 0.05% EDTA disodium salt. The suspension was homogenized and centrifuged. pG2 in the super-natant was purified by gel filtration chromatography in the extraction buffer, subsequent dialysis against distilled water, and further gel filtration chromatography in the extraction buffer. The major peak eluted from final gel filtration column con-tained the pG2 protein at greater than 98% purity as judged by SDS-PAGE.
Purified pG2 protein was used in a strip immunoassay to characterize sera from healthy individuals in the high risk population and sera from patients with AIDS or ARC. pG2 protein ad-sorbed onto mitrocellulose strips was incubated with human serum to be tested, washed, then contacted with labeled anti-human IgG to detect antibody bound to the strip. The assay was also performed with dirupted whole virus. pG2 was equally as effective as the whole virus in detecting anti-core protein antibody in sera (100% correlation). Of seroposi-tive healthy homosexuals tested (i.e. those showingantibody reactive with the whole virus), 81% had - 1~ 1338501 ~, .. .
.. ...
antibodies reactive with pG2; the percentage dropped to 56~ for AIDS and ARC patients.
The pG1, pG2 and pG3 proteins are hybrid proteins containing parts of naturally occurring 05 HTLV-III antigens (i.e. the viral pl7, p24 and pl5 core proteins). The success achieved in e~pression of the immunoreactive chimeric core proteins pGl, pG2 and pG3 indicate that the pl7, p24 and plS
proteins themselves can be expressed in host cell systems. In addition, other chimeric HTLV-III core proteins, especially proteins which encompass the identified antigenic domains of the virion proteins p24 and pl5 can be produced. Further, the DNA
segments encoding these polypeptides may be modified (e.g., by deletion, insertion or substitution of nucleotides) to design other HTLV-III core polypep-tides. As used herein, the term "recomhinant core protein" is intended to be inclusive all forms of viral core polypeptides which are expressed by genetically engineered host cells and which are immunoreactive with anti-core protein antibody.
Recombinant HTLV-III core proteins, including the pG1, pG2 and pG3 polypeptides, or equivalent type polypeptides can be produced de novo by recom-binant DNA techniques. HTLV-III now can be rou-tinely and reproducibly isolated from patients with AIDS and propagated in a line of permissive T cells developed for this purpose. M. Popovic et al.
Science 224, 4S7 ~1984); R. C. Gallo et al. Science 224, 500 (1984). From such cells HTLV-III proviral 13385~1 DNA can be obtained and cloned. The designated gag regions of the HTLV-III genome, identified to encode antigenic determinants, can be excised from the proviral DNA (generally by restriction enzyme 05 digestion), inserted into an expression vector, preferably one which can express the polypeptide at high levels, to form a recombinant expression vector containing gag gene sequence. Appropriate host cells transformed by the vector can provide a system for expression of the gene product.
Alternatively, gag DNA segments encoding antigenic regions of the core proteins can be synthesized chemically. Several techniques are available for synthesizing DNA of desired nucleotide sequences. See, e.g., Matteucci et al.~J. Am. Chem.
Soc. (1981) 103:3185; Alvarado-Urbina _ al.~Science (1980) 214:270. Synthesized segments of viral DNA
can be adapted and inserted into an expression vector which can be used to transform vector com-patible host cells and provide for expression of thegene product.
Core proteins containing the identified anti-genic regions of p24 and pl5 can be synthesized chemically. The predicted amino acid sequence of the pG2 protein, for example, is shown in Figure 5; the protein, or proteins, thereof, can be synthesized by the solid phase procedure of Merrifield.
When expressed as heterologous protein in a host cell system, any of several purification techniques, in addition to the techniques described herein for purification of pG2, can be used to purify the recomhinant core proteins. For use in immunoassays, the protein must be purified to substantial immunological purity. Importantly, the preparation should be free of host cell contaminants 05 which might be reactive with antibody in human sera.
Such contaminants could yield a high level of false positive results which would detract from the accuracy of the assay.
Immunochemical assays employing the polypep-tides can take a variety of forms. The preferred type is a solid phase immunometric assay. In assays of this type, the purified recombinant polypeptide is immobilized on a solid phase to form an antigen-immunoadsorbent. The immunoadsorbent is incubated with the sample to be tested. The duration and conditions of the incubation are standard, those appropriate for the formation of the antigen-anti-body complex. The immunoadsorbent is then separated from the sample and a labeled anti-(human IgG) anti-body is used to detect human anti-HTLV-III antibody bound to the immunoadsorbent. The amount of label associated with the immunoadsorbent is compared to positive and negative controls to assess the pre-sence or absence of anti-HTLV-III antibody.
The immunoadsorbent can be prepared by adsorb-ing or coupling purified polypeptide to a solid phase. Various solid phases can be used, such as beads formed of glass, polystyrene, polypropylene, dextran or other material. Other suitable solid phases include tubes or plates formed from or coated with these materials.
1338~01 The recombinant core proteins can be either covalently or non-covalently bound to the solid phase by techniques such as covalent bonding via an amide or ester linkage or adsorption. After the 05 HTLV-III polypeptide is affixed to the solid phase, the solid phase can be post-coated with an animal protein, e.g., 3% fish gelatin. This provides a blocking protein which reduces nonspecific adsorp-tion of protein to the immunoadsorbent surface.
The immunoadsorbent functions to insolubilize anti-core protein antibody in the liquid sample tested. In blood screening for anti-HTLV-III
antibody, the immunoadsorbent is incubated with blood plasma or serum. Before incubation, plasma or serum is diluted with normal animal plasma or serum.
The diluent plasma or serum is derived from the same animal species that is the source of the anti-(human IgG) antibody. The preferred anti-(human IgG) antibody is goat anti-(human IgG) antibody. Thus, in the preferred format, the diluent would be goat serum or plasma. The optimal dilution factor for human plasma and serum is about 10-11 fold.
The conditions of incubation, e.g. pH and temperature, and the duration of incubation are not crucial. These parameters can be optimized by - routine experimentation. Generally, the incubation will be run for 1-2 hours at about 45C in a buffer of pH 7-8.
After incubation, the immunoadsorbent and the sample are separated. Separation can be accom-plished by any conventional separation technique 1~
~ - 1338501 ~,. C .
such as sedimentation or centrifugation. The immunoadsorbent then may be washed free of sample to eliminate any interfering substances.
To assess human antibody bound to the immuno-05 adsorbent, the immunoadsorbent is incubated with thelabeled anti-(human IgG) antibody (tracer). Gene-rally, the immunoadsorbent is incubated with a solution of the labeled anti-(human IgG) antibody which contains a small amount (about 1~) of the 10 serum or plasma of the animal species which serves as the source of the anti-(human IgG) antibody.
Anti-(human IgG) antibody can be obtained from any animal source. However, goat anti-(human IgG) antibody is preferred. The anti-(human IgG) anti-15 body can be an antibody against the Fcfragment ofhuman IgG, for example, goat anti-(human IgG) Fc antibody.
The anti-(human IgG) antibody or anti-(human IgG)F can be labeled with a radioactive material such as l25Iodine; labeled with an optical label, such as a fluorescent material; or labeled with an enzyme such as horse radish peroxidase. The anti-human antibody can also be biotinylated and labeled avidin used to detect its binding to the immuno-adsorbent.
~ fter incubation with the labeled antibody, theimmunoadsorbent is separated from the solution and the label associated with the immunoadsorbent is evaluated. Depending upon the choice of label, the evaluation can be done in a variety of ways. The label may be detected by a gamma counter if the g-1338SOl label is a radioactive gamma emitter, or by a fluorimeter, if the label is a fluorescent material.
In the case of an enzyme label detection may be done colorimetrically employing a substrate for the 05 enzyme.
The amount of label associated with the immuno-adsorbent is compared with positive and negative controls in order to determine the presence of anti-HTLV-III core protein antibody. The controls are generally run concomitantly with the sample to be tested. A positive control is a serum containing antibody against I~TLV-III core protein; a negative control is a serum from healthy individuals which do not contain antibody against HTLV-III core protein.
For convenience and standardization, reagents for the performance of the immunometric assay can be assembled in assay kits. A kit for screening blood, for example, can include:
a~ an immunoadsorbent e.g. a polystyrene bead coated with a recombinant HTLV-III core polypep-tide;
b) a diluent for the serum or plasma sample, e.g. normal goat serum or plasma;
c) an anti-(human IgG) antibody e.g. goat anti-(human IgG) antibody in buffered, aqueous solution containing about 1~ goat serum or plasma;
d) a positive control i.e. serum containing antibody against polypeptide 121; and ~9 13~8501 e) a negative control e.g. pooled sera from healthy individuals which does not contain antibody against polypeptide 121.
If the label is an enzyme, an additional element of 05 the kit can be the substrate for the enzyme.
Another type of assay for anti-HTLV-III anti-body is an antigen sandwich assay. In this assay, a labeled HTLV-III recombinant polypeptide is used in place of anti-(human IgG) antibody to detect anti-10 HTLV-III antibody bound to the immunoadsorbent. The assay is based in principle on the bivalency of antibody molecules. One binding site of the anti-body binds the antigen affixed to the solid phase;
the second is available for binding the labeled 15 antigen. The assay procedure is essentially the same as described for the immunometric assay except that after incubation with the sample, the immuno-adsorbent is incubated with a solution of labeled core polypeptide. The HTLV-III polypeptide can be labeled with radioisotope, an enzyme, etc. for this type of assay.
In a third format, the bacterial protein, Protein A, which binds the Fc segment of an IgG
molecule without interfering with the antigen-25 antibody interaction can be used as the labeled tracer to detect anti-HTLV-III-antibody adsorbed to the immunoadsorbent. Protein A can be readily labeled with a radioisotope, enzyme or other detect-a~le species.
Some serum samples appear to show stronger reactivity towards HTLV-III core protein than toward - ~ 1338~01 HTLV-III envelop protein. This suggests that combined testing for antibody against both viral core and envelop proteins might enhance the overall sensitivity of a test for HTLV-III infection. The use of the combination of homogenous preparations of recombinant core and envelop protein, rather than the whole virus, for this purpose would eliminate false positives encountered with assays based on preparations of whole virus (which can contain host cell contaminants). This would reduce the waste of valuable blood units.
A combination assay can be used based upon homogenous polypeptide pG2 and recombinant env protein. A suitable HTLV-III env protein is HTLV-III
polypeptide 121 described in European Patent Application published under No. 199,438 on October 29, 1986. A mixture of pG2 and polypeptide 121, preferably containing approximately equimolar amounts of the two antigens, can be applied to a solid phase to form a double antigen immunoadsorbent for adsorption of antibody against either antigen. The assay would be conducted in the same manner as that described for the pG2 assay above.
Immunochemical assays employing recombinant HTLV-III core proteins for detection of antibodies against HTLV-III core protein have several advan-tages over those employing a whole (or disrupted) virus for this purpose. For one, assays based upon the polypeptide will alleviate the concern over growing large quantities of infectious virus and the inherent variability associated with cell culturing and virus production. Efficient expression of viral antigens in E. coli. as other host cell systems 05 provide a safe means of large scale production of assay reagents. Further, the assay will help mitigate the real or perceived fear of contracting AIDS by technicians in hospitals, clinics and blood banks who perform the test. As mentioned, reagents 10 for assays based upon the whole virus (e.g. whole virus antigen immunoadsorbent), even though they are made with a disrupted, inactivated virus, present a risk of contamination with live virus. For example, a possible source of live virus contamination may be 15 residual cell debris from the virus isolation process. Although extensive precautions can be taken to reduce the risk of contamination, it is virtually impossible to completely eliminate it.
Significantly, the risk, though minimal, may be 20 perceived as greater than it actually is by persons who handle the test reagents. Assay reagents without whole virus can help minimize this percep-tion of risk. Immunoassays based upon viral compo-nents in safe host cell systems provide a substitute for assays based on the whole virus which are at least comparable in sensitivity and specificity and superior in reproducibility.
Assays employing natural, isolated HTLV-III
core proteins, e.g. p24 protein, while they elimi-30 nate the use of whole virus from assay reagents,still require the growth of the virus on a large nr~
scale for a supply of the natural protein and thus do not eliminate the risks attendant to this proce-dure.
The invention is illustrated further by the 05 following Exemplifications.
Exemplification Bacterial strains and plasmids E. coli strain JA221 (lpp ) was used in all experiments as the host cell. Ghrayeb et al. (1984) 10 EMBO J. 3. 2437-2442. Cells were grown in L-Broth supplemented with ampicillin (100 g/ml). The REV
(Repligen, Cambridge, MA) expression vector was used for cloning of the HTLV-III DMA.
DNA manipulations Isolation of plasmid DNA and various manipula-tions were carried out as previously described by L.C. Ghrayeb et al., i.e. supra. Restriction enzymes were obtained from New England Biolabs. T4 DNA ligase was purchased from Boehringer Mannheim 20 Biochemicals. The DNAs were digested with restric-tion enzymes in conditions described by the manu-facturer.
Expression and analysis of the gag gene clones HTLV-III ~ proteins produced by recombinant 25 clones PGl, PG2 and PG3 were analyzed by SDS-poly-acrylamide gel electrophoresis ~SDS-PAGE) as de-scribed previously. See Chang, N. T. et al., (1985), Science, 228, 93-96. Cells were grown in 1 ml L-broth at 37C overnight and the cells were ~3 1338501 -harvested by centrifugation at 5000 x g for 10 minutes. The cell pellets were dissolved in 200 ul of loading buffer and 20 ul was applied to a 12%
SDS-polyacrylamide gel and electrophoresed under 05 reducing conditions. Unlabeled molecular weight markers were obtained from Biorad Laboratories.
[14C]-labeled molecular weight markers were obtained from Amersham. The expression of HTLV-III specific protein by the recombinant clones was detected by Western blotting analysis using sera from AIDS
patients. Bacterial proteins were separated on a 12% SDs-polyacrylamide gel and transferred to nitrocellulose and blotted as described below. The blot was incubated overnight at 4C with sera from AIDS patients or from healthy individuals. After washing, virus specific protein bands were vis-ualized by incubation with [ I]-labeled goat anti-human IgG (see below). The blots were air dried and exposed to Kodak X-AR5 at -70C with intensifying screens.
Purification of the pG2 protein For large scale growth, 20 ml of an overnight culture of pG2 were inoculated into 1 liter of L-BROTH containing 100 ~g/ml of ampicillin and 0.025% antifoam, and sha~en at 37C. The cells were ~ harvested after 8 hr and washed with 50 mM Tris-HCl p~I 8.5 (sonication buffer). 25 g of cell pellet were suspended in 70 ml of sonication buffer and sonicated in two portions at 70 W for eight 30 sec bursts with a 60 sec cooling period between each * Trade Mark.
~, , . .
~i 1338~01 t ~ ,~
burst. The lysed cells were then centrifuged at 10,000 xg for 30 min. All of the pG2 protein was found in the pellet and constituted approximately 20% of the total protein as judged by SDS-PAGE.
05 The pellet containing the pG2 protein was suspended in 50 mM Tris-HC1 pH 8.5 containing 8 ~
Urea, 1 M NaCl, 10 mM DL dithiothreitol (DTT) and 0.05~ EDT~ disodium salt (extraction buffer). The suspension was incubated at 45C for 60 min and centrifuged at 10,000 xg for 30 min. The resulting supernatant was applied to a SEPHACRYL S-300 gel filtration column (5 x 80 cm) previously equili-brated with extraction buffer containing 5 m~S DTT.
The column was eluted in the same buffer at a flow rate of 0.5 ml/min at room temperature and the fractions (lO ml) were monitored by U.V. absorption at 280 nm. The pG2 protein, found in the second main peak, was pooled and dialyzed exhaustively against distilled water at 4C. During dialysis, the pG2 protein was precipitated quantitatively.
The precipitated protein was then redissolved in 10 ml of extraction buffer containing lO mM DTT and incubated at 45C for 30 min. The resulting solu-tion was applied to a second SEPHACRYL S-300 column (2.6 x 65 cm) under identical conditions to the first column. The ma~or peak contained the pG2 protein which was 95~ pure as judged by SDS-PAGE.
The protein was further purified by repeating the second column purification under identical condi-tions. The main peak from the third S-300 column contained the pG2 protein in 98% purity. The yield * Trade Mark.
~i was 50 mg and this preparation was used for screening human sera (see below).
Immunoreactivity of pG2 with ~luman Sera 50~ g of pure pG2 protein or 430~g of purified 05 disrupted HTLV-III virus, were electrophoresed on a 12% SDS polyacrylamide gel (13 cm x 13 cm x 1.5 mm) and transferred to nitrocellulose using a Biorad Tran-Blot apparatus. The electroblotting buffer used was 20% aqueous methanol containing 0.016 M
Tris base and 0.13 M glycine, and transfer was performed at 40 volts at 4C overnight. The nitro-cellulose paper was then shaken for 2 hr at 37C
with 60 ml of PBS containing 5% non-fat dry milk, 0.1% sodium azide and 0.1% antifoam (milk buffer) and then for 2 hrs at room temperature with 60 ml of 5% normal goat serum in milk buffer. ~t this stage, the blocked nitrocellulose was either stored at -20C, or used directly for the strip assay. The nitrocellulose was cut into 13 cm x 0.5 cm strips, and each strip was rocked overnight at 4C with 4 ml of milk buffer containing 5~ normal goat serum and 40~1 of the human serum to be tested in a 15 ml disposable conical tube. The next day the milk solution was replaced with 10 ml of 0.15% sodium deoxycholate, O.lM NaCl, 0.5% triton X-100, 0.1 m~l phenylmethylsulfonyl fluoride in 10 mM sodium phosphate pH 7.5 (wash buffer) and the tubes were rocked for 1 hr. The wash buffer was removed and replaced with 4ml 5% goat serum in milk buffer and the tubes were rocked for 1 hr, at which time 125[I]-labeled goat anti-human IgG (10 cpm/ml) was ~ -~ 1338501 added. After 30 min, the strips were washed for 1 hr with 10 ml of wash buffer, air dried and exposed to Kodak XA~-5 film at -70C with intensifying screens.
05 Radioimmunoassay 96 well microtiter dishes were coated with the antigen at lOO~g/ml in 50 mM Tris-HCl pH 8Ø After an overnight incubation, the wells were washed three times with phosphate buffered saline (PBS). The 10 wells were then post coated with 200 ~1 3% fish gelatin (Norland Products, Inc.) in PBS containing 0.1% sodium azide. The fish gelatin solution was removed and each well was filled with 200 ~l of 1:5 or 1:10 dilutions of the test serum in PBS contain-15 ing 10% normal goat serum, 10% anti-E. coli goat serum and 1% fish gelatin. After one hour at room temperature, the wells were washed three times with PBS and 200~1 of [1 I]-labeled goat anti-human IgG
(Fc portion) in 1% normal goat serum, 1% fish 20 gelatin in PBS at 1.5x106 cpm/ml was added to each well. After one hour at room temperature, the plates were washed four times with PBS and once with distilled water and counted.
RESULTS
25 Construction of the HTI,V-III gag gene clones The isolation of recombinant phage clone BEI10 containing the unintegrated linear form of HTLV-III
proviral DNA has been reported previously. Shaw et al., (1985), Science, 226, 1165-1171. The 9 Kb ~i 133850~
HTLV-III insert of phage BHlO was released by SstI
cleavage within the R element of the LTR (See Figure 1). The SstI fragment was then digested with either PvuII and ~II or PstI and ~II. The 949 bp 05 PvuII-BglII fragment and the 677 bp PstI-~fragments were inserted into the REV expression vector ~Repligen, Cambridge, MA) to give pGl and pG2 respectively (Figure 1). Clone pG3 was constructed from pG2. pG2 DN~ was digested with PstI and HindIII, end repaired and ligated. Thus, in pG3 the PstI-H _ III fragment was deleted from the HTLV-III
DNA insert of pG2. As seen from Figure 1, the three constructs carry HTLV-III DNA that is predicted to code for chimeric peptides containing various portions of the pl7, p24 and pl5 viral gag proteins.
See Ratner et al., (1985), Nature, 313, 277-284.
The sizes of the expressed proteins are larger than predicted since the expression vector supplies the initiation methionine codon plus 35 amino residues at the NH2-terminus of each expressed protein.
Expression of the HTLV-III gag gene clones E. coli transformed with plasmids, pGl, pG2 or pG3 were found to produce proteins of 41kd, 33kd and 18kd, respectively, as demonstrated by SDS-polacryl-amide gel electrophoresis of total bacterial celllysates. SDS-PAGE analysis of HTLV-III gag gene proteins is shown in Figure 2. Cells from lml cultures were centrifuged and the pellets resus-pended in 200~1 of SDS sample buffer and analyzed by SDS-PAGE as described above. 20 lul of cell lysate ~-' 1338501 were loaded per lane and gels were stained with commassie brilliant blue R250. (Lane 1, molecular weight markers, lane 2, control cells with no plasmid, lane 3, pGl, lane 4, pG2, lane 5, pG3, lane 05 6, cells carrying the REV vector containing no HTLV-III D~IA. The number on the left designate the molecular weights in kilodaltons.) All three proteins were made in large quanti-tied (over 10~ of total cellular protein in these 10 cells) but were not detected in the host cell with or without the REV vector alone. The overproduction of the plasmid encoded HTLV-III ~ proteins caused a marked decrease in the rate of cell growth. The kinetics of the growth rate could be correlated with 15 the accumulation of the ~ gene products in the cytoplasm although no cell lysis was observed (data not shown). Maximum accumulation was observed at 8 hours after the start of the log phase growth period. In addition, the expressed ~ gene pro-20 ducts were present as aggregates containing membraneproteins after disruption of the cells. Depending on growth conditions, HTLV-III gag proteins of smaller size could be detected on SDS-PAGE gels (Figure 2). The products are likely due to the 25 degradation of the major high molecular weight proteins with increasing growth time.
Immunochemical characterization of the gag gene products The bacterial expressed EITLV-III ~-specific protein in cells carrying pGl, pG2 or pG3 were ., ~q 13385ol detected by Western blot analysis using sera pooled from AIDS patients. The results of this analysis are shown in Figure 3. SDS-PAGE analysis was performed exactly as in Figure 2. Transfer of 05 proteins to nitrocellulose paper, reaction with antibodies and detection of immunoreactive bands is described above. Figure 3 shows a blot in which lane 1 is control cells, lane 2 is pG1, lane 3 is pG2 and lane 4 is pG3. The blot was treated with 10 pooled sera from AIDS patients. The numbers on the left designate the relative position of the [14C]
molecular weight markers that were run along with the samples in lanes 1-4, but are not shown in the figure. The result clearly shows the synthesis of 15 specifically cross-reacting HTLV-III peptide in recombinant clones containing pG1, pG2 and pG3. The immunoreactive proteins in each clone corresponded to the expressed proteins, 41kd, 33kd, 18kd, seen in the Coomassie blue stained SDS-polyacrylamide gel 20 (Figure 2). There was no HTLV-III virion-specific peptide detected in lysate of control JA221 cells.
The products of pG2 was purified to greater than 98% homogeneity as judged by SDS-P~GE. Figure 4 shows SDS-PAGE analysis of pG2 purified as de-25 scribed above. PG-2 protein eluted from a sephacryl S-300 column in 50 mr~ Tris-HCL pH 8.5 containing 8M
Urea, lM NaCl and 5 mM DTT, was mixed with an equal volume of 2X SDS-PAGE sample buffer, heated at 100C
for 5 min and applied to two identical 12% SDS-PAGE
30 gels. One of the gels was stained with Coomassie Brilliant Blue (panel 7), while the other trans-~ 1338SOl ferred to nitrocellose and the blot treated withpooled sera from AIDS patients (panel B) as in Figure 3. Panel A, lane 1 is molecular weight markers, lane 2, 3, 4 are pure pG2 at 2, 5 and 10 05 g respectively. Panel B is identical to A except that lane 1 was run with 14[C]-labeled molecular weight markers.
The major band is of 33 kd while there is a minor band of 30 kd which is also seen in total cell lysates (Figure 2) and is most likely a degradation product. A very minor band of 65 kd can also be seen and is most likely to be the dimer form of pG2.
All the bands that are visible by Commassie blue staining are also immunoreactive towards HTLV-III
specific antibodies present in sera from AIDS
patients (Figure 4B) as well as the anti-P24 mouse monoclonal antibody (data not shown). We feel confident that the pG2 protein is essentially free of contaminating E. coli. proteins.
The purified pG2 protein was used to screen for antibodies directed towards the core p24 protein in human sera, using a strip assay based on tlle western blot technique. The same samples were also tested under identical conditions, using the purified, disrupted HTLV-III virus. The results are summa-rized in Table 1.
i, ~
~;
13~8~01 Table 1 No. Positive No. For p24 of No. Positive Clinical StatusTested HTLV-III Using pG2 Healthy donors 50 0 0 Elealthy homosexuals* 49 17 17 ARC** 51 28 28 AIDS*~ 34 19 19 *Only 21 of these donors were seropositive for antibodies to either p24 and/or gp41 of HTLV-III.
In addition, the same individuals who were positive 05 for p24 antibodies using the whole virus assay were also positive for antibodies to pG2.
**All these sera were positive for antibodies to gp41.
The results show that there is 100~ correlation between p24 antibodies detected by pG2 protein and those detected by the whole virus. In addition, none of the normal donor controls were reactive with pG2 protein. This indicates the recombinant pG2 protein can substitute adequately for the whole virus when detection of p24 antibodies is required.
The data presented in Table 1 also show that of the 21 seropositive healthy homosexuals tested, 17 (81~) had detectable antibodies to the p24. In both ARC
and AIDS patients, the percentage drops to 56~.
Whether the anti-p24 antibody titer is an indication of the progress of E~TLV-III infection remains to be studied. In this regard, the uses of pG2 protein in such studies would be preferable since the levels of p24 protein in different virus preparations may vary and may affect the sensitivity of the assay.
1~38~01 Partially purified pG2 protein was tested in a solid phase RIA. Details of the plate RIA assay are given above. The pG? protein preparation used was only "partially" purified. 24 sera from ~IDS/~RC
05 patients and 24 sera from healthy individuals were used in the assay and results were plotted on a semi-log scale. The horizontal dotted line desig-nates the cut-off points so that values below the line are considered negative while those above are considered positive. The results are shown in Figure 6. The results indicated that 18 out of the 24 AIDS or ARC patients' sera tested were reactive with the antigen. The 6 sera from patients with AIDS or ~RC that were negative in the RIA assay were found to contain no detecta~le amounts of anti-p24 _ antibodies as assayed by a strip immunoassay base on Western blot technique using the purified disrupted whole virus (data not shown). Of the 24 normal human sera tested in the RI~, only one was positive but was negative when tested ~ith the purified virus in a Western blot (data not shown). The reactivity of the one normal sample may be due to the presence of unusually high titre of anti-E. coli antibodies present in that particular serum and the fact that the pG2 antigen preparation contained trace amounts of E. coli protein impurities. This nonspecific immunoreactivity can be eliminated by absorption of this serum with SEPHAROSE 4B conjugated with E. coli extract. ~lternatively, better purified pG2 prepara-tions such as the preparation used in the stripassay can be used.
* Trade Mark.
33` 1338501 Equivalents Those skilled in the art will recognize, or be able to ascertain no more than routine experimenta-tion, many equivalents to the specific embodiments 05 of the invention described herein. Such equivalents are intended to be encompassed by the following c lalms .
Claims (18)
1. A method of detecting antibody against HTLV-III core protein in a biological fluid, comprising the steps of:
a) providing an antigen immunoadsorbent comprising a solid phase to which is attached a recombinant HTLV-III core antigen which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein;
b) incubating the immunoadsorbent with a sample of the biological fluid to be tested under conditions which allow antibody in the sample to complex with the antigen immunoadsorbent;
c) separating the immunoadsorbent from the sample; and d) determining antibody bound to the immunoadsorbent as an indication of antibody against HTLV-III core protein in the sample.
a) providing an antigen immunoadsorbent comprising a solid phase to which is attached a recombinant HTLV-III core antigen which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein;
b) incubating the immunoadsorbent with a sample of the biological fluid to be tested under conditions which allow antibody in the sample to complex with the antigen immunoadsorbent;
c) separating the immunoadsorbent from the sample; and d) determining antibody bound to the immunoadsorbent as an indication of antibody against HTLV-III core protein in the sample.
2. A method of claim 1, wherein the recombinant HTLV-III core antigen is a chimeric antigen consisting essentially of antigenic portions of HTLV-III p24, p17 and p15 proteins.
3. A method of claim 1, wherein the recombinant HTLV-III antigen is pG2 polypeptide.
4. A method of claim 1, wherein the biological fluid is human serum or plasma.
5. A method of claim 1, wherein the step of determining the antibody bound to the immunoadsorbent comprises:
a) incubating the immunoadsorbent with a labeled antibody against immunoglobulin of the species from which the biological fluid is derived;
b) separating the immunoadsorbent from the labeled antibody; and c) detecting the label associated with the immunoadsorbent as an indication of antibody against HTLV-III core protein in the sample.
a) incubating the immunoadsorbent with a labeled antibody against immunoglobulin of the species from which the biological fluid is derived;
b) separating the immunoadsorbent from the labeled antibody; and c) detecting the label associated with the immunoadsorbent as an indication of antibody against HTLV-III core protein in the sample.
6. A method of claim 5, wherein the biological fluid is human plasma or serum, and the labeled antibody is labeled anti-human Ig antibody.
7. A method of detecting antibody against HTLV-III core protein in human plasma or serum, comprising the steps of:
a) providing an antigen immunoadsorbent comprising a polystyrene bead coated with an essentially homogeneous purified preparation of pG2 polypeptide;
b) incubating the immunoadsorbent with a sample of human plasma or serum under conditions which permit anti-HTLV-III core protein antibody in the sample to complex with the pG2 polypeptide;
c) separating the immunoadsorbent from the sample;
d) incubating the immunoadsorbent with a solution of labeled anti-human Ig antibody;
e) separating the immunoadsorbent from the solution of labeled antibody; and f) detecting the label associated with the immunoadsorbent as an indication of anti-HTLV-III core protein antibody in the sample.
a) providing an antigen immunoadsorbent comprising a polystyrene bead coated with an essentially homogeneous purified preparation of pG2 polypeptide;
b) incubating the immunoadsorbent with a sample of human plasma or serum under conditions which permit anti-HTLV-III core protein antibody in the sample to complex with the pG2 polypeptide;
c) separating the immunoadsorbent from the sample;
d) incubating the immunoadsorbent with a solution of labeled anti-human Ig antibody;
e) separating the immunoadsorbent from the solution of labeled antibody; and f) detecting the label associated with the immunoadsorbent as an indication of anti-HTLV-III core protein antibody in the sample.
8. An immunoadsorbent comprising a solid phase support having attached thereto a recombinant HTLV-III core protein which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein.
9. An immunoadsorbent of claim 8, wherein the recombinant core protein is a chimeric protein consisting essentially of antigenic regions of the HTLV-III p24, p17 and p15 proteins.
10. An immunoadsorbent of claim 8, wherein the recombinant HTLV-III core protein is pG2 polypeptide.
11. An assay for antibody against HTLV-III
in a biological fluid comprising the steps of:
a) providing an immunoadsorbent comprising a solid phase to which is attached mixture of recombinant HTLV-III core protein which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein, and recombinant HTLV-III envelop protein immunoreactive with antibody against HTLV-III envelop protein;
b) incubating the immunoadsorbent with a sample of biological fluid;
c) separating the immunoadsorbent from the sample; and d) determining antibody bound to the immunoadsorbent as an indication of antibody against HTLV-III in the sample.
in a biological fluid comprising the steps of:
a) providing an immunoadsorbent comprising a solid phase to which is attached mixture of recombinant HTLV-III core protein which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein, and recombinant HTLV-III envelop protein immunoreactive with antibody against HTLV-III envelop protein;
b) incubating the immunoadsorbent with a sample of biological fluid;
c) separating the immunoadsorbent from the sample; and d) determining antibody bound to the immunoadsorbent as an indication of antibody against HTLV-III in the sample.
12. A method of claim 11, wherein the recombinant HTLV-III core protein is pG2 polypeptide and the recombinant HTLV-III envelop protein is HTLV-III polypeptide 121.
13. An assay for antibody against HTLV-III in a biological fluid, comprising the steps of:
a) providing an immunoadsorbent comprising a solid phase to which is attached approximately an equal amount of pG2 polypeptide and HTLV-III
polypeptide 121;
b) incubating the immunoadsorbent with a sample of biological fluid;
c) separating the immunoadsorbent from the sample;
d) incubating the immunoadsorbent with a solution of labeled anti-human Ig antibody;
e) separating the immunoadsorbent from the solution of labeled anti-human Ig antibody; and f) detecting the label associated with the immunoadsorbent as an indication of anti-HTLV-III antibody in the sample.
a) providing an immunoadsorbent comprising a solid phase to which is attached approximately an equal amount of pG2 polypeptide and HTLV-III
polypeptide 121;
b) incubating the immunoadsorbent with a sample of biological fluid;
c) separating the immunoadsorbent from the sample;
d) incubating the immunoadsorbent with a solution of labeled anti-human Ig antibody;
e) separating the immunoadsorbent from the solution of labeled anti-human Ig antibody; and f) detecting the label associated with the immunoadsorbent as an indication of anti-HTLV-III antibody in the sample.
14. An immunoadsorbent comprising a solid phase coated with an equal amount of pG2 polypeptide and polypeptide 121.
15. A recombinant HTLV-III core antigen which is a chimeric antigen encoded by insert of vector pG1, pG2 or pG3, the chimeric antigen being immunoreactive with antibody against HTLV-III core protein.
16. A HTLV-III core antigen of claim 15 which is a chimeric antigen consisting essentially of antigenic portions of HTLV-III p24, p17 and p15 proteins.
17. PG2 polypeptide.
18. An essentially homogeneous preparation of pG2 protein.
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US06/834,212 US4808536A (en) | 1986-02-27 | 1986-02-27 | Immunochemical method for detection of antibody against HTLV-III core protein based upon recombinant HTLV-III gag gene encoded protein |
| US834,212 | 1986-02-27 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA1338501C true CA1338501C (en) | 1996-07-30 |
Family
ID=25266391
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA000530796A Expired - Fee Related CA1338501C (en) | 1986-02-27 | 1987-02-27 | Method of detecting antibody against htlv-iii |
Country Status (5)
| Country | Link |
|---|---|
| US (1) | US4808536A (en) |
| EP (1) | EP0258404B1 (en) |
| JP (1) | JPH01500053A (en) |
| CA (1) | CA1338501C (en) |
| WO (1) | WO1987005399A1 (en) |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| GB8423659D0 (en) | 1984-09-19 | 1984-10-24 | Pasteur Institut | Cloned dna sequences |
| US7205102B1 (en) | 1983-09-15 | 2007-04-17 | Institut Pasteur | Cloned DNA sequences related to the genomic RNA of lymphadenopathy-associated virus (LAV) and proteins encoded by said LAV genomic RNA |
| US7232654B1 (en) | 1983-09-15 | 2007-06-19 | Institut Pasteur | DNA sequence of the LTR region of human immunodeficiency virus type 1 (HIV-1) |
| US5705612A (en) * | 1984-10-18 | 1998-01-06 | Institut Pasteur And Centre National De La Recherche Scientifique | NEF peptide encoded by human immunodefiency virus type 1 (HIV-1) |
| US7045130B1 (en) | 1984-10-18 | 2006-05-16 | Institut Pasteur | Antibodies against antigens of human immunodeficiency virus (HIV-1) |
| US6894152B1 (en) | 1984-11-16 | 2005-05-17 | Institut Pasteur | Cloned DNA sequences related to the genomic RNA of lymphadenopathy-associated-virus (LAV) and proteins encoded by said LAV genomic RNA |
| US6534285B1 (en) * | 1984-12-24 | 2003-03-18 | Genentech, Inc. | Molecularly cloned acquired immunodeficiency syndrome polypeptides and their methods of use |
| US5853978A (en) * | 1985-12-04 | 1998-12-29 | Genentech, Inc. | Molecularly cloned acquired immunodeficiency syndrome polypeptides and methods of use |
| DE3650011T2 (en) * | 1985-04-08 | 1994-11-17 | Genetic Systems Corp | EXPRESSION AND DIAGNOSIS WITH GAG-CODED PEPTIDES THAT ARE IMMUNOLOGICALLY REACTIVE WITH ANTIBODIES AGAINST LAV. |
| KR910002374B1 (en) | 1985-04-29 | 1991-04-20 | 제네틱 시스템즈 코포레이션 | Synthetic antigens for the detection of aids-relate disease |
| US4629783A (en) * | 1985-04-29 | 1986-12-16 | Genetic Systems Corporation | Synthetic antigen for the detection of AIDS-related disease |
| US4808536A (en) * | 1986-02-27 | 1989-02-28 | Centocor, Inc. | Immunochemical method for detection of antibody against HTLV-III core protein based upon recombinant HTLV-III gag gene encoded protein |
| US6130314A (en) * | 1986-03-26 | 2000-10-10 | Genetic Systems Corporation | Synthetic antigen for the detection of AIDS-related disease |
| US4925784A (en) * | 1986-04-04 | 1990-05-15 | Hoffmann-La Roche Inc. | Expression and purification of an HTLV-III gag/env gene protein |
| US4983387A (en) * | 1986-05-19 | 1991-01-08 | Viral Technologies Inc. | HIV related peptides, immunogenic antigens, and use therefor as subunit vaccine for AIDS virus |
| US5142025A (en) * | 1986-08-01 | 1992-08-25 | Repligen Corporation | Recombinant HTLV-III proteins and uses thereof |
| US5447837A (en) * | 1987-08-05 | 1995-09-05 | Calypte, Inc. | Multi-immunoassay diagnostic system for antigens or antibodies or both |
| US5149623A (en) * | 1988-02-09 | 1992-09-22 | Virotest, Inc. | Rapid, easy, and economical screening test for antibodies to human immunodeficiency virus |
| US5204259A (en) * | 1988-05-06 | 1993-04-20 | Pharmacia Genetic Engineering, Inc. | Methods and systems for producing HIV antigens |
| DE346022T1 (en) * | 1988-06-10 | 1990-05-23 | Medical Research Council, London, Gb | PEPTIDE FRAGMENTS OF HIV. |
| ATE105413T1 (en) * | 1989-02-01 | 1994-05-15 | Du Pont | HIV P17 TEST FOR MONITORING THE COURSE OF AIDS. |
| CA2072351A1 (en) * | 1990-01-05 | 1991-07-06 | Andrew J. Mcmichael | Hiv-1 core protein fragments |
| SE468168B (en) * | 1990-02-20 | 1992-11-16 | Replico Medical Ab | HIV-1, P24 PEPTIDES, DIAGNOSTIC ANTIGENS AND PROCEDURES FOR DIFFERENTIAL DIAGNOSTICS OF PRELIMINARY HIV-1 POSITIVE SERUM TESTS |
| US6228608B1 (en) * | 1991-02-28 | 2001-05-08 | Aquila Biopharmaceuticals, Inc. | Recombinant FIV glycoprotein 160 and P24 gag protein |
| EP0600018B1 (en) * | 1991-08-21 | 2001-07-11 | Abbott Laboratories | Hepatitis c assay utilizing recombinant antigens to c-100 region |
| KR0172970B1 (en) * | 1992-06-17 | 1999-02-01 | 김영길 | Chimeric proteins useful for an aids vaccine and the preparation thereof |
| IL108707A (en) * | 1993-02-19 | 1999-06-20 | Weiner David B | Pharmaceutical compositions and diagnostic kits comprising hiv protein vpr or proteins that bind to vpr |
| US5874225A (en) * | 1993-02-19 | 1999-02-23 | Trustees Of The University Of Pennsylvania | Identification of compounds that modulate HIV-1 vpr protein activity |
| WO1998029551A1 (en) * | 1997-01-02 | 1998-07-09 | Universidade Federal De Minas Gerais | THE PROCESS FOR EXPRESSION AND PRODUCTION OF RECOMBINANT PROTEIN HYBRID PROTEIN (p24/p17) DERIVED FROM HUMAN IMMUNODEFICIENCY VIRUSES (HIV-1) |
| JP4805511B2 (en) * | 1999-12-23 | 2011-11-02 | メディカル リサーチ カウンシル | Improvement in immune response to HIV or improvement in immune response |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| IE58321B1 (en) * | 1984-04-23 | 1993-09-08 | Us Health | Isolation of proteins of HTLV-III, serological detection of antibodies to HTLV-III in sera of patients with aids and pre-aids conditions, and detection of HTLV-III infection bi/immuno-assays using HTLV-III infection by immuno-assays using HTLV-III and its proteins |
| US4520113A (en) * | 1984-04-23 | 1985-05-28 | The United States Of America As Represented By The Secretary Of The Department Of Health And Human Services | Serological detection of antibodies to HTLV-III in sera of patients with AIDS and pre-AIDS conditions |
| US4689398A (en) * | 1984-06-20 | 1987-08-25 | Ortho Diagnostic Systems Inc. | HTLV test using synthetic peptides |
| CA1341482C (en) * | 1984-10-31 | 2005-05-10 | Paul A. Luciw | Process for preparing fragments of aids-associated retroviruses |
| US4774175A (en) * | 1985-03-01 | 1988-09-27 | Centocor, Inc. | Immunochemical methods for the detection of antibody against HTLV-III |
| DE3650011T2 (en) * | 1985-04-08 | 1994-11-17 | Genetic Systems Corp | EXPRESSION AND DIAGNOSIS WITH GAG-CODED PEPTIDES THAT ARE IMMUNOLOGICALLY REACTIVE WITH ANTIBODIES AGAINST LAV. |
| US4629783A (en) * | 1985-04-29 | 1986-12-16 | Genetic Systems Corporation | Synthetic antigen for the detection of AIDS-related disease |
| US4661445A (en) * | 1985-05-24 | 1987-04-28 | Saxinger W Carl | Competitive ELISA for the detection of HTLV-III antibodies |
| US4808536A (en) * | 1986-02-27 | 1989-02-28 | Centocor, Inc. | Immunochemical method for detection of antibody against HTLV-III core protein based upon recombinant HTLV-III gag gene encoded protein |
-
1986
- 1986-02-27 US US06/834,212 patent/US4808536A/en not_active Expired - Lifetime
-
1987
- 1987-02-20 JP JP62501548A patent/JPH01500053A/en active Pending
- 1987-02-20 WO PCT/US1987/000373 patent/WO1987005399A1/en not_active Application Discontinuation
- 1987-02-20 EP EP87901921A patent/EP0258404B1/en not_active Expired - Lifetime
- 1987-02-27 CA CA000530796A patent/CA1338501C/en not_active Expired - Fee Related
Also Published As
| Publication number | Publication date |
|---|---|
| EP0258404B1 (en) | 1992-05-20 |
| EP0258404A1 (en) | 1988-03-09 |
| JPH01500053A (en) | 1989-01-12 |
| WO1987005399A1 (en) | 1987-09-11 |
| US4808536A (en) | 1989-02-28 |
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