CA1073382A - Immobilized proteins and method of preparing same - Google Patents
Immobilized proteins and method of preparing sameInfo
- Publication number
- CA1073382A CA1073382A CA260,069A CA260069A CA1073382A CA 1073382 A CA1073382 A CA 1073382A CA 260069 A CA260069 A CA 260069A CA 1073382 A CA1073382 A CA 1073382A
- Authority
- CA
- Canada
- Prior art keywords
- enzyme
- filler particles
- composite
- microporous
- binder
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Expired
Links
Classifications
-
- 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
- C12N11/00—Carrier-bound or immobilised enzymes; Carrier-bound or immobilised microbial cells; Preparation thereof
- C12N11/14—Enzymes or microbial cells immobilised on or in an inorganic carrier
-
- 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
- C12N11/00—Carrier-bound or immobilised enzymes; Carrier-bound or immobilised microbial cells; Preparation thereof
- C12N11/02—Enzymes or microbial cells immobilised on or in an organic carrier
- C12N11/08—Enzymes or microbial cells immobilised on or in an organic carrier the carrier being a synthetic polymer
- C12N11/082—Enzymes or microbial cells immobilised on or in an organic carrier the carrier being a synthetic polymer obtained by reactions only involving carbon-to-carbon unsaturated bonds
-
- 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
- Y10S530/00—Chemistry: natural resins or derivatives; peptides or proteins; lignins or reaction products thereof
- Y10S530/81—Carrier - bound or immobilized peptides or proteins and the preparation thereof, e.g. biological cell or cell fragment as carrier
- Y10S530/811—Peptides or proteins is immobilized on, or in, an inorganic carrier
Abstract
ABSTRACT OF THE DISCLOSURE
A microporous member comprising a binder or matrix and finely divided filler particles dispersed throughout the binder and having proteinaceous substances coupled to at least some of said filler particles thereby immobilizing said proteinaceous substances and rendering them insoluble. Methods of preparing said immobilized protein system are also disclosed.
A microporous member comprising a binder or matrix and finely divided filler particles dispersed throughout the binder and having proteinaceous substances coupled to at least some of said filler particles thereby immobilizing said proteinaceous substances and rendering them insoluble. Methods of preparing said immobilized protein system are also disclosed.
Description
~ 733~2 The present invention relates generally -to enzyme systems, and more particularly, to method and means for immobiliz-ing enzymes by coupling or bonding same -to an insoluble support or carrier.
As is well documented in the art, enzymes are proteinaceous substances generally of high molecular weight, which function as biological catalysts capable of promoting a wide range of chemical reactions, e.g., reacting glucose with the enzyme glucose isomerase to produce fructese. Unfortunately, most enzymes are soluble in water making it difficult to remove them from solu-tion for repeated use and/or maintain their catalytic effectiveness over an extended period of time. In addition, enzymes are frequently relatively expensive to obtain or produce in commercial quantities. Accordingly, many techniques have been proposed heretofore to immobilize enzymes and render them insoluble -typically by bonding or coupling them to an insoluble support or carrier. As used herein, the terms "immobile"
or "immobilized" when applied to enzymes, refer to enzymes which have been made essentially water-insoluble through attachment to, or entrapment within, a water-insoluble carrier in such a manner that they retain their activity, can readily be removed from a reaction solu-tion, and can be repeatedly used.
Prior attempts to carry out catalytic reactions employing immobilized enzymes have met wi-th more or less success depending in part upon the method of coupling or bonding the enzymes to the insoluble carrier; the na-ture or physical and chemical properties of the carrier material itself; and the mass transfer mechanism under which a substrate is brought into con-tact with -the enzyme carrier. The term "substrate" as used herein means a substance upon which an enzyme reacts ca-talytically.
1C~73313Z
, .
For example, enzymes have been adsorbed to siliceous carriers such as porous glass beads (U.S. Patent No. 3,556,945) or have been chemically coupled to such porous beads by an intermediate silane coupling agent (U.S. Patent No. 3,519,538).
Porous ceramic beads have been suggested in lieu of glass wi-th the enzyme being coupled via adsorption (U.S. Patent No. 3,850,751).
However, because the aforementioned porous glass or ceramic beads are extremely small in size it is necessary in order to effect the enzymatic reaction to cause the substrate to f`low through a packed bed of many such discrete particles. Packed bed enzyme reactors are expensive, suscep-tible to clogging or channeling, present a rela-tively high resistance to flow, and tend to retain the substra-te within the pores due -to the latter's rela-tively small size thus presenting a contamination problem when a series of different substrates or samples are fed through the packed bed and the enzyme reaction is a relatively fast one.
Similarly, as further reported in the literature (U.S. Patent No. 3,824,150) enzymes have been immobilized by ~ ~-mechanical entrapment within a semi-permeable carrier such as a membrane, or by chemical coupling through an intermediate agent to natural or synthetic polymeric materials including cellulosic materials in the f`orm of filter paper. In the membrane or mechanical entrapment reactor, the enzymatic reaction can take place only be diffusion of the substrate solution through -the support, and furthermore, the use of such supports often do not impart any extra stability to the enzyme. The use of cellulosic filter paper and similar organic carriers having enzymes coupled or otherwise bonded thereto suffer from disadvantages inheren-t in such support materials inasmuch as -the la-t-ter usually are :, :: .. : , .
~73~
, fragile, are subject to chemical and microbial attack, and ca~not be easily sterilized without damage.
Still further, it is known to apply a water insoluble polymeric coating having nitrilo, acid amido, or ureido groups to a single phase macroporous pol~meric support and then couple enzymes by adsorption to the coated su;rface of such support (U.S.:
Patent No. 3,7~5,084). The preparation of such coated reactors, however, is time consuming and expensive; and the amount ~f enzymes which may be attached to a unit volume of the resulting reactor is somewhat limited by the fact that the support material is macro-poxous.
In accordance with the present invention there is providedan insoluble composite comprisiny a microporous member having at least a pair of opposed surfaces and a predetermined thickne~s, said microporous member comprising a polymeric resinous binder having finely divided filler particles dispersed through~ut said binder and a network of substantially i~terconnecked pores formed therein, said pores being formed within said resinous binder, between said filler particl~s and said xesinous binder, and between neighboring filler particles, said dispersed filler particles being present in said microporous member in an amount by weight of a~. least about 25%, the size distribution of said pores varying non-uniformly across each of said surfaaes and across said predetermined thickness through the range of about Q.01 micron to about lO0 microns as determined porosimetrically by the Mercury Intxusion Method, and a proteinaceous substance bound to at least some of said filler particles dispersed throughout said binder, said microporous member being pervious to the flow of a fluid through at least on~ of said surfaces wherein at least some of said filler particles to which said proteinaceous substance is bound is adapted to come into con-, . ~
tact with such fluid.
In accordance with the present invention there is provid-ed the method of carrying out a chemical process compri~ing the steps of reacting a substrate by placilg the substrake in contact with an in~oluble micropox~us mem~er having a proteinaceous sub-stanae whiah reaats wit~ said ~ubstrate bonded thereto, and recov~r-ing a product of the rea~tion, said inl301uble microporou~ member having at least a pair of opposed surfaaes and a predetermined thick-n~ss, said mioroporous member comprising a polymeric resinous binder having finely divided filler particle~ dispersed throughout said binder and a network of substantially interconnected pores formed therein, said pores being formed within said resinous binder, be-tween said filler particles and said resinous binder, and between neighboring filler partiales, said dispersed filler particles being pre~ent in said miaroporQus member in an amount by weight of at least about 25%, the size distribution of said pores varying non-uniformly across each o ~aid surfaces and across each of said pre-determined thickness ~hrough the range of about 0.01 micron to abou~ 100 microns a9 dete~mined porosimetrically by the Mercury Intru~ion Method, and a proteinaGeous subskance bound to at least some o said filler particles dispersed throughout said binder, said miaroporous member be:Lng parvious to the flow of said substrate through at least one o~ 6aid surfaces.
In aacardance with the pres~nt invention there i8 provided a method of immobilizing proteinaceous substanaes comprising the steps of providing an insoluble miaroporous member, having at lea9t a pair of opposed surfaGes and a predetermined thickness, ~aid mi~roporous member aomprisi~g a polymeric resinous binde~ having finely divided filler particles dispersed throughoùt said binder and a network ~f substantially interconnected pores formed therein, said pores baing formed wi~hin ~aid resinous binder, between said filler particlea and ~aid resinou~ binder~ and between neighboring filler particle~, Raid di~persed filler particles being pre~ent in said ~lcroporous member in an amount b~ weight of at lea~t a~out 25~, ~he size distri~u~ion o ~aid pore~ varying non-uni~ormly acroes eaah o~ ~ai~ ~uracas and acro~s said predatermin0d th~cknes~ through the rang~ o about 0.01 micron to about lOC micron~ as determined por~simatrically by ~he Mercury Intru3i.0n Method, and bonding a p~o-tei~aaeou~ ~ubatance to the surfa~e of at least som~of said plural-ity o di~perse~ fillar particles, ~aid microp~r0u~ membsr b~ingpervious to th~ flow of a fluid thxou~h at least ona of ~ai~ ~r-faces wharein at lea~t ome of said filler particlas to whlch said proteinaceou~ ~ub~tance iB bound i8 adapted to come into contact with ~aid 1u~d.
An example of a microporous ma~erial o the for~oing type and ona which i~ especially ~uitable and herefore particularly prQ-ferred for usa a~ an insolubla enzym~ carrier or ~upport in accord-anae wi~h the prasent inv~ntion i~ fully de~cribed in U.S. Patent NOO 3~862~030O AB i~ avid~nt from the '030 Patent, su¢h mi~ap~r~u~
material comprisa~ a n~rmally hydrophobic polymeric ma~rix ~e.g., polyvinyl ahloride), finely divided normally hydrophilic 1~1er partlclee ~e.gO, 3ilica) dlsp~r~d throughout the re~inous matrlx;
and a ne~work ~f intar¢onnected miaropore~ forme~ throughout ~he materlalO Tha network of in~arconnected micropore~, in turn, con-25 BiSti ~f micr~porss ~ormed betwe~n adjacent or neighboring p8rti~1e8of th~ di~perse~ inorganic iller, between parti~le~ o~ dispers~
filler and the re~inou~ matrix, and in the resinous matrix ~tself, with the size distribution of tha microporss typically ranging ov~r a relatively broad ra~ge ~rom about r~l micron to ab~ut 100 micron, 3~ and tha mean pore ~iam~ter of t~e mi~ropores typically being ln the _5_ ~'~ ' " ... ' '' ' ~ ' ;;
:l`
1~733~3Z
range o about 0.1 micron to about 0.2 micron as determined, poro-simetrically by the Mercury Intrusion Method. Furthermore, the total porosity of such material is typically within the range of about 50% to about 70%. Such microporous materials have been em-ployed hereto~ore, for example, in the fabrication of batteryseparators as disclosed in U.S. Patent No. 3,696,061, or more recently, as sub-micron filter media as disclosed in the afore-mentioned U.S. Patent No. 3,862,030.
It will be appreciated that microporous materials other than those disclosed in the '030 Patent may also be usad in practic-; ing the present invention, Thus~ for example, in lieu of the thermo-plastic binder cons ituent of the microporous material of the '030 Patent, synthetic ~r natural thermosetting rubber polymers or co-polymers thereof may bs employed~
If formed of rubber-like polymers, the latter, with additives such as antidegradants, cros~-linking agents~ inert fillers, or the like normally employed by those skilled in the -5a-.~9 ~73382 art of compounding thermosetting compounds, are intimately mixed using conventional methods with a suitable filler, such as silica hydrogel or precipitated hydrated silica (i.e., silicic acid (n Si
As is well documented in the art, enzymes are proteinaceous substances generally of high molecular weight, which function as biological catalysts capable of promoting a wide range of chemical reactions, e.g., reacting glucose with the enzyme glucose isomerase to produce fructese. Unfortunately, most enzymes are soluble in water making it difficult to remove them from solu-tion for repeated use and/or maintain their catalytic effectiveness over an extended period of time. In addition, enzymes are frequently relatively expensive to obtain or produce in commercial quantities. Accordingly, many techniques have been proposed heretofore to immobilize enzymes and render them insoluble -typically by bonding or coupling them to an insoluble support or carrier. As used herein, the terms "immobile"
or "immobilized" when applied to enzymes, refer to enzymes which have been made essentially water-insoluble through attachment to, or entrapment within, a water-insoluble carrier in such a manner that they retain their activity, can readily be removed from a reaction solu-tion, and can be repeatedly used.
Prior attempts to carry out catalytic reactions employing immobilized enzymes have met wi-th more or less success depending in part upon the method of coupling or bonding the enzymes to the insoluble carrier; the na-ture or physical and chemical properties of the carrier material itself; and the mass transfer mechanism under which a substrate is brought into con-tact with -the enzyme carrier. The term "substrate" as used herein means a substance upon which an enzyme reacts ca-talytically.
1C~73313Z
, .
For example, enzymes have been adsorbed to siliceous carriers such as porous glass beads (U.S. Patent No. 3,556,945) or have been chemically coupled to such porous beads by an intermediate silane coupling agent (U.S. Patent No. 3,519,538).
Porous ceramic beads have been suggested in lieu of glass wi-th the enzyme being coupled via adsorption (U.S. Patent No. 3,850,751).
However, because the aforementioned porous glass or ceramic beads are extremely small in size it is necessary in order to effect the enzymatic reaction to cause the substrate to f`low through a packed bed of many such discrete particles. Packed bed enzyme reactors are expensive, suscep-tible to clogging or channeling, present a rela-tively high resistance to flow, and tend to retain the substra-te within the pores due -to the latter's rela-tively small size thus presenting a contamination problem when a series of different substrates or samples are fed through the packed bed and the enzyme reaction is a relatively fast one.
Similarly, as further reported in the literature (U.S. Patent No. 3,824,150) enzymes have been immobilized by ~ ~-mechanical entrapment within a semi-permeable carrier such as a membrane, or by chemical coupling through an intermediate agent to natural or synthetic polymeric materials including cellulosic materials in the f`orm of filter paper. In the membrane or mechanical entrapment reactor, the enzymatic reaction can take place only be diffusion of the substrate solution through -the support, and furthermore, the use of such supports often do not impart any extra stability to the enzyme. The use of cellulosic filter paper and similar organic carriers having enzymes coupled or otherwise bonded thereto suffer from disadvantages inheren-t in such support materials inasmuch as -the la-t-ter usually are :, :: .. : , .
~73~
, fragile, are subject to chemical and microbial attack, and ca~not be easily sterilized without damage.
Still further, it is known to apply a water insoluble polymeric coating having nitrilo, acid amido, or ureido groups to a single phase macroporous pol~meric support and then couple enzymes by adsorption to the coated su;rface of such support (U.S.:
Patent No. 3,7~5,084). The preparation of such coated reactors, however, is time consuming and expensive; and the amount ~f enzymes which may be attached to a unit volume of the resulting reactor is somewhat limited by the fact that the support material is macro-poxous.
In accordance with the present invention there is providedan insoluble composite comprisiny a microporous member having at least a pair of opposed surfaces and a predetermined thickne~s, said microporous member comprising a polymeric resinous binder having finely divided filler particles dispersed through~ut said binder and a network of substantially i~terconnecked pores formed therein, said pores being formed within said resinous binder, between said filler particl~s and said xesinous binder, and between neighboring filler particles, said dispersed filler particles being present in said microporous member in an amount by weight of a~. least about 25%, the size distribution of said pores varying non-uniformly across each of said surfaaes and across said predetermined thickness through the range of about Q.01 micron to about lO0 microns as determined porosimetrically by the Mercury Intxusion Method, and a proteinaceous substance bound to at least some of said filler particles dispersed throughout said binder, said microporous member being pervious to the flow of a fluid through at least on~ of said surfaces wherein at least some of said filler particles to which said proteinaceous substance is bound is adapted to come into con-, . ~
tact with such fluid.
In accordance with the present invention there is provid-ed the method of carrying out a chemical process compri~ing the steps of reacting a substrate by placilg the substrake in contact with an in~oluble micropox~us mem~er having a proteinaceous sub-stanae whiah reaats wit~ said ~ubstrate bonded thereto, and recov~r-ing a product of the rea~tion, said inl301uble microporou~ member having at least a pair of opposed surfaaes and a predetermined thick-n~ss, said mioroporous member comprising a polymeric resinous binder having finely divided filler particle~ dispersed throughout said binder and a network of substantially interconnected pores formed therein, said pores being formed within said resinous binder, be-tween said filler particles and said resinous binder, and between neighboring filler partiales, said dispersed filler particles being pre~ent in said miaroporQus member in an amount by weight of at least about 25%, the size distribution of said pores varying non-uniformly across each o ~aid surfaces and across each of said pre-determined thickness ~hrough the range of about 0.01 micron to abou~ 100 microns a9 dete~mined porosimetrically by the Mercury Intru~ion Method, and a proteinaGeous subskance bound to at least some o said filler particles dispersed throughout said binder, said miaroporous member be:Lng parvious to the flow of said substrate through at least one o~ 6aid surfaces.
In aacardance with the pres~nt invention there i8 provided a method of immobilizing proteinaceous substanaes comprising the steps of providing an insoluble miaroporous member, having at lea9t a pair of opposed surfaGes and a predetermined thickness, ~aid mi~roporous member aomprisi~g a polymeric resinous binde~ having finely divided filler particles dispersed throughoùt said binder and a network ~f substantially interconnected pores formed therein, said pores baing formed wi~hin ~aid resinous binder, between said filler particlea and ~aid resinou~ binder~ and between neighboring filler particle~, Raid di~persed filler particles being pre~ent in said ~lcroporous member in an amount b~ weight of at lea~t a~out 25~, ~he size distri~u~ion o ~aid pore~ varying non-uni~ormly acroes eaah o~ ~ai~ ~uracas and acro~s said predatermin0d th~cknes~ through the rang~ o about 0.01 micron to about lOC micron~ as determined por~simatrically by ~he Mercury Intru3i.0n Method, and bonding a p~o-tei~aaeou~ ~ubatance to the surfa~e of at least som~of said plural-ity o di~perse~ fillar particles, ~aid microp~r0u~ membsr b~ingpervious to th~ flow of a fluid thxou~h at least ona of ~ai~ ~r-faces wharein at lea~t ome of said filler particlas to whlch said proteinaceou~ ~ub~tance iB bound i8 adapted to come into contact with ~aid 1u~d.
An example of a microporous ma~erial o the for~oing type and ona which i~ especially ~uitable and herefore particularly prQ-ferred for usa a~ an insolubla enzym~ carrier or ~upport in accord-anae wi~h the prasent inv~ntion i~ fully de~cribed in U.S. Patent NOO 3~862~030O AB i~ avid~nt from the '030 Patent, su¢h mi~ap~r~u~
material comprisa~ a n~rmally hydrophobic polymeric ma~rix ~e.g., polyvinyl ahloride), finely divided normally hydrophilic 1~1er partlclee ~e.gO, 3ilica) dlsp~r~d throughout the re~inous matrlx;
and a ne~work ~f intar¢onnected miaropore~ forme~ throughout ~he materlalO Tha network of in~arconnected micropore~, in turn, con-25 BiSti ~f micr~porss ~ormed betwe~n adjacent or neighboring p8rti~1e8of th~ di~perse~ inorganic iller, between parti~le~ o~ dispers~
filler and the re~inou~ matrix, and in the resinous matrix ~tself, with the size distribution of tha microporss typically ranging ov~r a relatively broad ra~ge ~rom about r~l micron to ab~ut 100 micron, 3~ and tha mean pore ~iam~ter of t~e mi~ropores typically being ln the _5_ ~'~ ' " ... ' '' ' ~ ' ;;
:l`
1~733~3Z
range o about 0.1 micron to about 0.2 micron as determined, poro-simetrically by the Mercury Intrusion Method. Furthermore, the total porosity of such material is typically within the range of about 50% to about 70%. Such microporous materials have been em-ployed hereto~ore, for example, in the fabrication of batteryseparators as disclosed in U.S. Patent No. 3,696,061, or more recently, as sub-micron filter media as disclosed in the afore-mentioned U.S. Patent No. 3,862,030.
It will be appreciated that microporous materials other than those disclosed in the '030 Patent may also be usad in practic-; ing the present invention, Thus~ for example, in lieu of the thermo-plastic binder cons ituent of the microporous material of the '030 Patent, synthetic ~r natural thermosetting rubber polymers or co-polymers thereof may bs employed~
If formed of rubber-like polymers, the latter, with additives such as antidegradants, cros~-linking agents~ inert fillers, or the like normally employed by those skilled in the -5a-.~9 ~73382 art of compounding thermosetting compounds, are intimately mixed using conventional methods with a suitable filler, such as silica hydrogel or precipitated hydrated silica (i.e., silicic acid (n Si
2 m H20) where n and m are integers) the latter being available commercially, for example, under the trademark Hi-Sil from PPG
Industries. The resultant compound is then formed into a sheet, preferably by calendering onto a suitable carrier (i.e., paper or ; a thin metal sheet or screen), wound on reels of convenient size, and then vulcanized under hydrostatic conditions in a steam au-to-clave to an appropriate state of cure using pressurized s-team as the source of heat. The vulcanized sheet is then dried in a warm dry air stream which also serves to dehydrate the silica. Such dehydration results in the formation of micropores in the sheet caused by the shrinkage of the silica thereby forming a normally hydrophilic microporous article.
In the finished state a typical thermoset rubber-like polymeric based microporous sheet contains abou-t 1 part of rubber-like polymer to about 0.5 parts silica by weight, and is about 60 percent porous of a volume basis. The pore size distribution is typically rather wide, varying from about 0.05 to lO microns for the most part according to mercury intrusion data, the mean pore -size being typically about 1.4 micron. Such thermoset rubber-like polymeric sheet are normally hydrophilic and liquid water soaks rapidly into the material, passing -through without any applied pressure, indicating tha-t the micropores are substantially interconnected. Such sheets, and the process of making same, are known in the prior art.
In broad aspect, the present invention contemplates utilization of the finely divided filler par-ticles dispersed throughout the binder or matrix of the microporous material as ........ . . .
733~;2 active sites to which enzymes may be coupled. Due to its poxous construction and the dispersion of the filler particlcs throughout the matrix or binder, such microporous material has a relatively large surface area, typically on the ordcr of about 80 M2~g, and the number of available enzyme coupling sites is relatively large; hence, the loading factor or amount of enzymes which may be coupled per unit volume .
.
I
, ;, , '~ .' 1 , '~
' `` ` ~.C~733~32 of such microporous material has been found to be correspondingly large. In addition, since each filler par-ticle is in effec-t sur-rounded by the interconnected network of varying sized micropores, a substrate in the form of a fluid or aqueous stream flowing ;~
through, for example, a relatively thin sheet of microporous material having enzymes coupled thereto will immediately come into contact with or gain access to a great many enzyme sites thus pro-moting extremely rapid enzymatic re~ctions with high product conversion efficiency. Thus, if the reaction efficiency-of the enzyme is relatively high, the sheet may be made quite thin and essentially complete reactions effected almost instantaneously upon passage of the substrate therethrough. By the same token, less efficiently reactive enzymes may necessitate slightly thicker sheets, and slightly longer reaction times to effect essen-tially complete product conversions. Owing to its high degree of poros-ity and the hydrophillic nature of the dispersed filler constitu-ent, the microporous material wets easily and is quite permeable to fluids flowing therethorugh. Thus, relatively low hydraulic pressures are required to pass a substrate through the material.
For example, as poin-ted out in the aforementioned Patent No.
Industries. The resultant compound is then formed into a sheet, preferably by calendering onto a suitable carrier (i.e., paper or ; a thin metal sheet or screen), wound on reels of convenient size, and then vulcanized under hydrostatic conditions in a steam au-to-clave to an appropriate state of cure using pressurized s-team as the source of heat. The vulcanized sheet is then dried in a warm dry air stream which also serves to dehydrate the silica. Such dehydration results in the formation of micropores in the sheet caused by the shrinkage of the silica thereby forming a normally hydrophilic microporous article.
In the finished state a typical thermoset rubber-like polymeric based microporous sheet contains abou-t 1 part of rubber-like polymer to about 0.5 parts silica by weight, and is about 60 percent porous of a volume basis. The pore size distribution is typically rather wide, varying from about 0.05 to lO microns for the most part according to mercury intrusion data, the mean pore -size being typically about 1.4 micron. Such thermoset rubber-like polymeric sheet are normally hydrophilic and liquid water soaks rapidly into the material, passing -through without any applied pressure, indicating tha-t the micropores are substantially interconnected. Such sheets, and the process of making same, are known in the prior art.
In broad aspect, the present invention contemplates utilization of the finely divided filler par-ticles dispersed throughout the binder or matrix of the microporous material as ........ . . .
733~;2 active sites to which enzymes may be coupled. Due to its poxous construction and the dispersion of the filler particlcs throughout the matrix or binder, such microporous material has a relatively large surface area, typically on the ordcr of about 80 M2~g, and the number of available enzyme coupling sites is relatively large; hence, the loading factor or amount of enzymes which may be coupled per unit volume .
.
I
, ;, , '~ .' 1 , '~
' `` ` ~.C~733~32 of such microporous material has been found to be correspondingly large. In addition, since each filler par-ticle is in effec-t sur-rounded by the interconnected network of varying sized micropores, a substrate in the form of a fluid or aqueous stream flowing ;~
through, for example, a relatively thin sheet of microporous material having enzymes coupled thereto will immediately come into contact with or gain access to a great many enzyme sites thus pro-moting extremely rapid enzymatic re~ctions with high product conversion efficiency. Thus, if the reaction efficiency-of the enzyme is relatively high, the sheet may be made quite thin and essentially complete reactions effected almost instantaneously upon passage of the substrate therethrough. By the same token, less efficiently reactive enzymes may necessitate slightly thicker sheets, and slightly longer reaction times to effect essen-tially complete product conversions. Owing to its high degree of poros-ity and the hydrophillic nature of the dispersed filler constitu-ent, the microporous material wets easily and is quite permeable to fluids flowing therethorugh. Thus, relatively low hydraulic pressures are required to pass a substrate through the material.
For example, as poin-ted out in the aforementioned Patent No.
3,862,030, flow through rates ranging from about 0.4 gallons/min./
sq. ft. to about 9 gallons/min./sq. ft. have been achieved through sheets of the preferred microporous material having a thickness of about 0.02 inches under a pressure gradient of only 10 psig, and having filler/binder ratios in the range from about 1/1 to about 2/1. Generally, an increase in the filler to binder ratio will result in increased pore size and greater total porosity thereby resulting in an increase in permeability of the material. Accord-ingly, the immobilized enzyme support of the present invention is ` ~7338Z
particularly suitable for use in the form of a so-called flow-through reactor core, -that is, a reactor core wherein the substrate solution penetrates one surface of the enzyme laden material, is catalytically reacted upon the enzyme, and the conver-ted product as well as any unreacted substrate exi-t through the same or another surface of the material.
Moreover, since as mentioned above, the pore size distri-bution of the microporous support material extends over a rela-tively wide range (i.e., about 0.01 micron -to about 100 micron) and the micropores are substantially interconnected, the material contains a multitude of sufficiently sized paths along which both substrate and/or converted product may easily flow. Product efflux from the material is thus quite rapid and may be terminated substantially simultaneously with end point flow of the substrate -through the support material. In other words, ca-taly-tic reactions produced with the enzyme support contemplated by the present inventibn have an ex-tremely sharp cutoff, and accordingly, many different substrate samples may be fed through the sarne immo- `-bilized enzyme support in rapid succession without the danger of contamination between successive samples, an extremely desirable advan-tage when immobilized enzymes are employed to carry out successive catalytic reactions on a series of different substrate samples as in medical or industrial analytical instruments, for example.
The foregoing cons-titutes a significant advantage of the present invention since in other known immobilized enzyme reactors such as the packed bed of porous glass beads, or the membrane reactor, for example, pore size is controlled quite uniformly and is of such small size that mass transfer through the reactor is accomplished by diffusion. In such diffusion limited enzyme ...;
,~ _g_ ,:
..
07~3~3Z
reactors, total efflux -time of the product may lag significantly behind the substrate sample termination poin-t, thus presenting a contamination problem should a succeeding substrate sample be fed into the reactor too rapidly.
In addi-tion to the foregoing advantages, the microporous enzyme support material of the present invention has excellent strength characteristics typically having a tensile strength of about 400 psi and a percentage of elongation under 20%, and thus may be handled quite easily during -the various s-tages of trea-t-ment necessary to bond or attach enzymes thereto as will beexplained in more detail below. Moreover, due to its excellent dimensional stability and strength, the microporous material of the present invention resists compaction under hydraulic pressures, and therefore is especially adapted -to be employed in large scale bulk processing reactors where large enzyme reaction areas are involved and large dynamic forces are exerted on the enzyme support member such as, for example, in commercial industrial or chemical processes uilitizing enzymatic reactions. Moreover, the preferred microporous material is resistant to a-ttack by chemicals such as acids and alcohols, for example, and is capable of being exposed to elevated temperatures without affecting its physical properties. In regard -to -the latter, it has been found possible, for example, to heat sterilize the preferred microporous material by emersion in steam at 15 psi and 2~0 F for 30 minu-tes without degrading the dimensional s-tability or physical properties of the material.
As more fully disclosed in the aforementioned '030 paten-t, the particularly preferred microporous material may be fabricated by admixing suitable quantities of a finely divided polymeric resin, 1~7338Z
:"`
a finely divided inorganic filler, a solvent (e.g., cyclohexanone) and a non-solvent (e.g.,water) under low shear conditions to ~orm a stable, damp, free-flowing powder. The powder mixture may then be extruded and calendered preferably -to form a substantially planar structure or sheet of desired dimensions which may next be passed through an aqueous bath to leach out the solvent, and then subsequently passed through a heated air oven to remove all -traces ; of moisture. In accordance with the present invention, the resulting article in the form of a microporous, dimensionally stable~ semi-rigid, insoluble, fluid permeable member may then be treated in such a manner as to couple or bond enzymes thereto.
As is generally known in the art, it is possible to bond or attach enzymes to an insoluble support or carrier by directly adsorbing the enzyme on the carrier, or by indirectly adsorbing or covalently bonding the enzyme to the carrier through an intermediate coupling agent. Due primarily to its dispersed silica filler component, the preferred microporous support material of the present invention has been found to exhibit a net negative charge as evidenced by substantial adsorption of proteins thereto at pH values below the isolectric point of the adsorbed protein. Thus, although direct adsorption of enzymes to the dis-persed filler particles in the material is feasible, the adsorp-tive in-teraction (direct) has been found to be of insufficient magnitude to prevent relatively rapid desorption during use and subsequently, loss of enzymatic activity from the enzyme composite.
Accordingly, in carrying out the present invention, i-t is preferred that the microporous material be treated in such a manner as to effect a chemical bond between the catalytically active enzyme and the insoluble microporous support material.
"
1~173382 In i-ts untreated condition, -the microporous ma-terial laeks -the organic funetionality necessary to effect such chemieal bonding to proteinaceous substances, hence, any known technique for imparting the required functionality to -the microporous material may be employed sinee the present in~ention in i-ts broades-t aspeet is eoneerned with the discovery -that the bonding of enzymes of the microporous starting material resul-ts in a superior immobilized `;
enzyme composite. Most known enzymes may be immobilized by covalently coupling or cross-linking free amino residues or groups on the enzyme molecule which are not essential -to the enzymatic activity of the enzyme to a carrier surface containing aliphatic primary or secondary amino or hydroxyl groups or residues. Still other known enzymes may be covalently coupled or cross-linked to a earrier surfaee in similar fashion via sueh o-ther fune-tional groups as, earboxyl, isonitrile, aldehyde or ketone, or anion, to name a few. Therefore, it will be understood that the term "ehemieal bond" or "chemieally bound" as used therein and in the appended elaims refers broadly -to the ehemical linkage between the cata-lytically active protein or enzyme and the functional groups or residues imparted -to the microporous starting material and is not -to be construed as being limited to a particular functional group or residue or to a partieular enzyme.
In one preferred embodiment of the present invention, a~iphatic primary amine functionality may be imparted to the mieroporous starting material by eovalently bonding directly to - the dispersed filler particles in the microporous material a ; bridging agent in the form of an organosilane such as gamma-aminopropyl-triethoxysilane, whereas in another alternatively preferred embodiment of the invention alipha-tic primary amine functionality may be imparted -to the microporous material by :
! .
` ~La,733~Z
irreversibly chemiadsorbing directly -to -the dispersed filler particles in the microporous material a bridging agent in the form of a macromolecular polyelectrolyte such as polyethylenemine (PEI~. Enzymes may -then be covalently bonded or cross-linked to the chemically modified microporous material and more specifically to the aliphatic primary amine residues impar-ted to the surface of the material by the aforementioned bridging agen-ts.
In the case where a bridging agent such as gamma- ;
aminopropyltriethoxysilane is employed, the latter is believed to be primarily covalently bonded directly to the hydrophilic inorganic filler particles dispersed through the polymeric binder constituent of the microporous material. Generally speaking the use of a silane bridging agent to bond or attach enzymes to siliceous materials is known in the art as disclosed, for example, in the aforementioned U.S. Paten-t No. 3,519,538.
In -the case where a bridging agent such as poly-ethylenemine is employed, the latter is believed to be attached or bonded to the dispersed hydrophilic inorganic filler constituen-ts of the microporous material via strong chemiadsorptive forces.
ZO Generally, the use of a macromolecular polyelectrolyte or poly-amine as a bridging agent to bond or attach enzymes to the surface of colloidal particles of silica, or to fibrous cellulose, is known in the art as respectively disclosed, for example, in U.S.
Patents Nos. 3,796,634 and 3,741,871. -In both cases, the enzyme is preferably cross-linked to ;~ the bridging agent by means of a bifunctional electrophilic : reagent such as glutaraldehyde or bisimidate esters to effect the :
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~0733~Z
desired covalent conjugation of the enzyme to -the functional amine groups which have been imparted to the external surfaces of the hydrophilic filler particles dispersed -throughout the microporous carrier or support via the bridging agent.
When using a carrier surface adsorptive bridging agen-t, in the form of -the aforementioned polyethylenimine, for example, or a bridging agent covalently bonded to the carrier surface such as the aforementioned gamma-aminopropyltriethoxysilane, for exam-ple, covalent conjugation of the enzyme and the carrier may be carried out in a single or two step producedure. In the single step procedure, the chemically modified carrier material may be simul-taneously treated with the bifunctional electrophilic reagent and the enzyme to effect simultaneous inter-molecular cross-linking of -the carrier surface reactive polymer and the enzyme. Commercial grades of glutaraldehyde, a typical bifunctional reagent as men--tioned above, con-tain significan-t amounts of soluble polymeric com-pounds formed from intermolecular aldol condensa-tions of the mono-meric dialdehyde, hence, each site of condensation results in a highly reactive alpha-beta unsaturated aldehyde moiety which will rapidly undergo Michael type addition reactions involving nucleo-philes such as aliphatic amines or other residues found on the surface of enzymes. In addition, free aliphatic aldehyde groups which are present in the carrier surface reactive polymer may also participate in the cross-linking reactions by combina-tion with aliphatic amino residues of the carrier or enzyme to form Schiff bases. Although the degree to which desired covalent conjugation of the enzyme competes with such undesired, unproductive reactions resulting in simple protein modification and cross-linking of carrier reactive surface residues may be empirically determined by varying experimental conditions such as pH, protein concentration :
~733~3Z
and cross-linking reagent concentration, it is difficult to selec-tively control such undesired, competetive reactions as -the bifunctional cross-linking reagent is always presen-t in a substan-tial molar excess during the reaction. In certain cases, there-fore, employment of the single step procedure may result in partial or -total enzyme inactivation due to extensive chemical modification of the enzyme or to chemical modification of the essential ac-tive site residues.
In situations where chemical modifica-tion results in extensive enzyme inactivation, the two s-tep procedure is recom-mended wherein the chemically modified carrier material is first cross-linked with the bifunctional reagent and then subsequently incubated with the enzyme. By using a sui-tably high concentration of -the cross-linking reagen-t, bimolecular reactions can become competitive for the surface amino residues relative to intramole-cular processes such as cross-linking. This results in a high surface density of pendant residues capable of reacting with nucleophilic side chain residues of enzymes. After removal of the excess unreacted cross-linking reagent, the enzyme of interest may then be incubated with the modified carrier resulting in covalent conjugation of the enzyme and the carrier. The fore-going two step procedure has been found to result in minimal modification of the enzyme since only residues in the vicinity of the contact region between the enzyme and the carrier reactive surface are involved.
It will be appreciated that various chemistries other than the electrophilic bifunctional reagen-ts mentioned above can be employed to covalently bond enzymes to the chemically modified carrier material. Such alternatives may include, for example, - 30 acylation of the alipha-tic amino group at the carrier reac-tive surface with succinic anhydride to produce a pendant aliphatic ~0733t3Z
carboxyl group which is subsequently reacted with nucleophilic side chain residues of enzymes in the presence of a water soluble carbodiimide; direct reaction of the amino group at -the carrier reactive surface with side chain carboxyl groups of enzymes in the presence of a water soluble carbodiimide; acylation of -the amino group at the carrier reactive surface with p-nitrobenzoyl chloride, reduction of the aryl nitro to an aryl amine via sodium dithionite, oxidation of the aryl amino group to an aryl diazonium salt via nitrous acid and subsequent reaction with aromatic side chain residues of proteins to form a stable azo linkage; acylation of the amino group at the carrier reactive surface with -terepthaloyl chloride, reaction of the pendan-t p-benzoyl acid halide with hydrazide to a benzoyl azide and subsequent reaction with nucleo-philic side chain res~dues of enzymes.
~ hen reacting the enzyme with the chemically modified carrier, the enzyme is preferably placed in a buffering solu-tion and the reaction carried out at temperatures sufficiently low to avoid deactivation of the enzyme or substantial changes in the latter's conformational state. Generally, tempera-tures in the ZO range of about 5 C to about 50 C are acceptable. As is known in the art, the pH of the enzyme reaction solution may be con-trolled at a desired level, by selec-ting suitable buffers, depending upon the particular enzyme being bound. Likewise, the concentration of enzyme in the buffered reac-tive solution and ,:!
. therefore, the extent to which the chemically modified carrier will be loaded with enzymes may be chosen depending upon the conversion rate of the enzyme, the concentration of the substrate, and the flow rate of the substrate through the reactor core.
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The present invention now will be further described with reference to the following examples -thereof, which latter are intended for illustration purposes only and are not to be cons-trued as limiting the scope of the invent:ion. ;
PREPARATI_N OF UNTREATED ENZYME SU _ORT M MBER
A sheet of microporous material was prepared by first dry blending 20.0 lbs. of Conoco 5385 polyvinyl chloride resin having a particle size of about 80 mesh, and 40.0 lbs. of Hi Sil 233, a precipitated hydrated silica, in a Patterson Kelley "low shear" liquids-solids blender for approximately 3 minutes.
Thereafter, and during continued agitation, 54.6 lbs. of solvent (cylohexanone) were added over a 20 minute period by means of a pump. Wa-ter in an amount of 59.0 lbs. was then added to the mix in the agitating blender over a subsequent 20-minute period to form a damp, stable, free-flowing powder. The powder was then introduced into a screw extruder having a barrel temperature of -approximately 120 F., and the extrudate passed between the rolls :, , of a calender to obtain a substantially flat sheet having a thickness of 0.02 inches (0.5mm). The sheet was then passed through an extraction bath of water at 170 F., and subsequently dried in a hot air oven at 225 F., for 6 minutes. The finished microporous sheet has a relatively wide pore size distribution extending from about 0.01 micron to about 100 micron, and a mean pore diameter in the range of about .15 micron to about .25 micron as determined by the Mercury Intrusion Method. In addition 9 the total porosity of this material is approxima-tely 65% by volume and the dispersed filler content (e.g., silica) comprises approximately 56% by weight. Liquid water soaked rapidly into the material without any applied pressure indicatlng that the micropores are 7338~
substantial~y interconnected rom sur~ace to surEace. From the resulting substantially flattened, semi-rigid, microporous shcet a plurality of untreated support members 5X5cm in size were cut and heat sterilized by immersion in a steam bath for one hour and allowed to cool and dry in open air.
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CHEMICA _ MODIFICATION BY COVALENT BONDING
An untreated support member prepared in accordance with Example 1 was incubated in a 10% vol/vol aqueous solution of gamma-aminopropyltriethoxysilane containing 1% vol/vol concen-trated HCl for 24 hours. The treated support member was flushed with water and 1 M NaCl to remove all unreacted reagents. The presence of aliphatic primary amino residues was then qualita-tively assessed by reacting the treated member with 0.5% wt/vol trinitrobenzene sulfonic acid in 0.1 M sodium tetraborate buffer at 70 F. and observing an intense orange trinitrophenyl amine derivative on the surface of the treated support member. Another un-treated support member prepared in accordance with Example 1 was similarly asseyed, but displayed no reac-tion -to this test.
Elemental analysis of` the treated support member yielded 0.5%
nitrogen by dry weight above that of the untreated support member.
The permanence of the amino functionality of the treated support member was evidenced by negligible nitrogen loss after storage in ~; water for a period of 12 months. The treated support member displayed identical flow properties with respectto the untreated support member and was not sensitive to differences in the buffers or ionic streng-th.
CHEMICAL MODIFICATION BY CHEMIADSORPTION
Another untreated support member prepared in accordance ~` with Example 1 was incubated in a 5% wt/vol aqueous solu-tion of 50,000 mol. wt. branched chain polyethyleneimine (PEI) at room temperature for one hour. The treated support was flushed with water and 1 m NaCl to remove any unadsorbed PEI. Assey was by the ,.
10733~3Z
same trinitrobenzene sulfonic acid test employed in Example 2 and an intense orange -trinitrophenyl amine derivative was observed on the surface of the treated support member demonstra-ting subs-tan tial aliphatic amino functionality. The nitrogen loading on the treated support member was quantitated by elemental analysis and was 1.25% nitrogen by dry weight versus 0.02% nitrogen by dry weight of an untreated suppor-t member. The chemiadsorption of PEI on the treated support member appeared virtually irreversible ; since it could not be removed by incubation with high ionic strength solutions (e.g., lM NaCl or 1 M K2 HP04/KH2P04) at pH
values between 3 and 9. Only in the case of strong acidic condi-tions (incubation in 1 M HCl for 2 hours) was there evidence of ~ partial desorption amounting to 50% of the nitrogen content as - indicated by elemental analysis. The surface area of the treated support by standard BET procedure was 55.4 M /g versus 81.1 M /g ~or the control. The support member treated with PEI displayed identical flow properties compared to an untreated support member irrespective of the buffer or ionic strength used.
, 20 ENZYME COUPLING REACTION
(Glucose Oxidase) -~ The support member treated in accordance with Example 3 was incubated for one hour in 10% vol/vol aqueous solu-tion of glutaraldehyde at pH 7. The support member was then rinsed with water and incubated for one hour in a solution of glucose oxidase which had been purified to homogeneity from Asper~llis n ger.
The conditions of the enzyme coupling reaction were as follows:
glucose oxidase concentration 20 mg/ml in 0.1 M K2HPO~/KH2P04 buffer pH 6.0 at ambient room temperature. Directly pumping -the enzyme solution through the support member under a positive ;, , . ', ~, ::
~07338Z , ;
hydraulic pressure did not improve enzyme loading rela-tive to ,~
that obtained by simple incubation. The tempera-ture of the coupling reaction was not found to be critical with the only requirement being that it did not exceed the -thermal inactivation region of 50 C for glucose oxidase. The support member was then extensively washed with water and 1 M NaCl to remove unreacted enzyme. Quenching of electrophilic residues on the support member surface was achieved by incubation of the immobilized enzyme com-posite with 0.1 M ethanolamine at p~ 7.0 containing 50 mM NaCNBH3.
The immobilized enzyme appears to have an indefinite shelf life when stored at 4 C in 0.1 M K2HP04 buffer pH 6Ø
SINGLE ENZYME REACTOR
The following reaction was carried out employing a pair ,;-, ~ of 1.5cm diameter disks prepared in accordance with Example 4 and . j mounted in a stacked configuration in a flow--thru reactor wherein the flow vector of the substrate was substantially perpendicular : :j to -the plane of each disk. The cross section of each mounted disk exposed to the fluid stream was 79mm . Glucose oxidase (E.C.1.1.3.4.) catalyzes the aerobic oxidation of glucose ~ -D-glucose + 2 -- ~ D-gluconolactone + H202 -~ Enzymatic activity in the stacked disk reactor conf`iguration was evaluated by measuring oxygen depletion downstream from the reactor with a Biological Oxygen Monitor, Model No. 53, obtained from Yellow Springs Instrument Company. A solu-tion of 0.15 mM glucose at anomeric equilibrium in air saturated 0.1 M Na acetate buffer pH 5.5 was pumped through the reactor at a flow rate of 2 ml/min.
The conversion of the limiting substrate,~ -D-glucose, was quantitative as measured by oxygen depletion downstream from the `` 1~733~3;Z `~
reactor. The residence time of the sample stream in contact with the reactor was approximately 1.6 seconds. The integra-ted form of the rate equation for glucose oxidase under these experi-mental conditions ls known explicitly, and it can be calculated thatthe lower limit for the immobilized enzyme concentration is ; 10 mg/ml. The unusually high activity of the stacked disk reactor is attributed to the absence of internal mass transport effects, i.e., no evidence of internal mass transport constraints for the reactor was observed.
A second set of stacked disks were prepared in accor-dance with Example 4 and mounted in the flow-thru reactor; the disks, however, were prepared with substantially reduced concen- ' , tration of the immobilized enzyme, i.e., by a factor of 10. A
'jl l mM glucose solution in 0.1 M Na acetate buffer pH 5.5 was then pumped through the second disk reactor at flow rates sufficiently fas-t tha-t the reactor was operating in a kinetic mode with only partial conversion of glucose to gluconolactone. The steady-state level of substrate conversion by the reactor under this condition `
was found to be highly sensitive to the enzyme concentration.
When observed under continuous operation for a period of four hours, no change in the steady-state conversion level was observed indicating no loss of enzymatic activity from the reactor.
ENZYME COUPLING REACTION
(Alcohol Dehydrogenase) Another suppor-t member treated in accordance with Example 3 was incubated for one hour in a 10% vol/vol aqueous solution of glutaraldehyde at pH 7. The support member was then rinsed with water and incubated for one hour in a solution of alcohol dehydro-genase. The conditions of the enzyme coupling reaction were asfollows:
.. . . . .
" 10733~3Z
alcohol dehydrogenase concentration 5 mg/ml in 0.1 M K2HP04KH2P04 buffer pH 6.0 containing 0.1 mM EDTA and 10 ~ M NADH (reduced nicotinamide adenine dinucleotide) at ambient room -temperature.
The support member was then extensively washed with the reaction buffer and 1 M NaCl to remove unreacted enzyme. Unreacted electrophilic residues on the support member was quenched by incubation of the immobilized enzyme composi-te with 0.1 M ethano-lamine at pH 7.0 containing 50 mM NaCNBH3. The enzyme loading was ~.
11 mg/g of the carrier and was calculated by measuring the incre-mental increase in nitrogen upon the support member prior to the ,, quenching reaction.
~ Alcohol dehydrogenase (EC 1.1.1.1) catalyzes the - reversible oxidation of primary alcohols according to the equation ; alcohol + NA ~ ~ aldehyde + NADH +
Enzymatic activity in a stacked disk reactor configuration was evaluated by measuring spectrophotometrically the formation of NADH @ 340 nm downstream from the reactor with a flow-through Model UA-5 absorbance monitor obtained from Instrumentation Specialties Co. A single 1.5 cm disk of the immobilized enzyme was mounted into a flow t~rough reactor in the manner of Example 5.
A solution of 50 mM ethanol and 0.5 mM NAD~ in 0.1 M K2HP04/KH2P04 buffer pH 7.4 containing 10 ~ M EDTA was pumped through the reactor at a flow rate of 1 ml/min. The calculated equilibrium conversion for the reaction under these conditions is 16% of the starting NA ~ concentration. Complete equilibration was observed indicat-ing that a few milliseconds contact with the immobilized enzyme reactor were sufficient to achieve the thermodynamic limit of the ; reaction. In order to demonstrate the stability of the immobi-lized enzyme a set of conditions was chosen in which the reactor was operated for 24 hours in a kinetic mode. As the conversion ~[)733~3~
, of substrates to products is extremely sensitive to conservation ;
of the catalyst under these conditions, a decrease in the conVer-sion level indicates loss or inactivation of the enzyme. The conditions of the experiment were 5 mM ethanol and 50~ M NAD in 0.1 M K2HP04/KH2P04 buffer pH 7.0 containing -lO~ M EDTA. This solution was pumped through the reactor at a flow rate of ] ml/min ~ `~
for 24 hours with continuous monitoring and recording of the sub-strate conversion level. It was found tha-t the conversion remained constant during this period indicating complete conser~
vation of the immobilized enzyme.
TANDEM ENZYME REACTOR
A disk reactor system incorporating three differen-t immobilized enzyme composites was constructed for catalyzing the ~ reaction sequence shown below.
,1 (EC 3.2.1.26) . sucrose + H20 - - > ~-D~glucose + fructose : ~l . :' :~:
-D-glucose - - ~ ~ D glu `~
~, ` ;~ ,`
(E.C. 1.1.3.4.) -D-glucose + 2 - ) ~ D-gluconolactone + H202 ;~
The glucose oxidase was homogeneous and prepared from Aspergillis niger, -the aldose-1-epi.merase enzyme (EC 5.1.3.3) was prepared from hog kidney and was 20% wt/wt purity, and the ~-D-fr~cto-furanosidase (EC 3.2.1.26) was a high purity preparation from Candida utilis. Each of the aforementioned enzymes was covalently immobilized to a pair of 1.5cm disks in accordance with the method of Example 4 at an enzyme concentration of 20 mg/ml. The alde-hyde quenching reaction was not employed. The two sets of three disks, each disk in each set corresponding to one of the three enzymes in the coupled reaction and in -the sequence shown above, ' .
~73313Z
were then mounted in the flow-thru reactor of Example 5 in a stacked fashion. A 1 mM solution of ultrapure sucrose in 0.05 M
K2HP04 pH 6~0, air saturated at 25C. was then pumped through the reactor at a flow rate of 1.2 ml/min. The conversion as measured by oxygen depletion downstream from the reactor was lO~o the theoretical based upon the known stoichiometry o-f the overall reaction. The maximum conversion which could be obtained, how-ever, was 25% since dissolved oxygen is the limiting substrate (250~ M). Under the conditions employed for -this example, the aldose-1-epimerase is the rate limiting enzyme. At slower flow rates and consequently longer reactor residence times, measured conversions approaching 25% were obtained.
IMMOBILIZATION OF GLUCOSE ISOMERASE
ON MICROPOROUS CARRIER
Glucose isomerase (E.C. 5.3.1.5) catalyzes the revers-ible interconversion of ~-D-fructose to~-D-glucose in accordance ; with the following reaction:
~-D-fructose E.C. 5.3.1.5 ~-D-glucose ; 20 Four discs of 26 mm diameter were cut from a sheet of microporous material (Example 1) and treated in accordance with Example 3 and then mounted in stacked fashion into a standard Millipore filter holder without gasket seals to form a flow-thru reactor. The PEI
laden support discs were modified by pumping glutaraldehyde (10%
wt/vol pH adjusted to 8.0) through the reactor in a recycled mode from a 100 ml reservoir for 1 hour. The support member was then rinsed in-situ by pumping 500 ml (approximately 1/2 hour) of deionized water and 200 ml of Hepes buffer or equivalent (i.e.
2g/1 Mg S04.7H20 and 0.2g/1 CoS04.7H20 pH 7.0-7.5 in deionized water 1C~733~3Z
,~
through the reactor. A solution of glucose isomerase at pH 7.5 (30 ml containing 0.43 units/ml) was passed through a Millipore 0.65 micron fil-ter and circulated through the disc reactor for 1 ~;
hour at room temperature. The term "units" as used herein refers to units of activity and is de~`ined as that amount of enzyme 1 which catalyzes the conversion of 1 micromole of ~-D-fructose '~ to ~ D-flucose per minute at 25C. The reactor was rinsed with approximately 500 ml of Hepes buffer until no protein could be detected irl the effluent. The glucose isomerase enzyme immobil-' 10 ized in this Example was obtained as a lyophilized whole cell ;~
homogenate of Streptomyces albus from Novo Enzyme Corporation and purified by soluble protein isolation and fractionation with . ammonioum sulfate (AmS04~. Although the frac-tionation depends in part upon the initial protein concentration of the supernatant obtained from the protein isolation step, the major glucose activity is typically found in the 70-85% AmS04 pellet. The protein pellets containing the majority of the activity are dissolved in v20-30ml of Hepes buffer and dialyzed against 4 litres of buffer from 24 hours at 4 C. using standard cellulose acetate dialysis tubing. Although the enzyme preparation at this point is suitable for use in immobilization if desired, the above enzyme concentrate can be purified s-till further by standard gel permeation techniques. Protein assay of the rinse affluent solution was carried out by employing the following reaction - sequence:
a. ~-D-fructose ~ C~-D-glucose rate-limiting b. ~-D-glucose aldose-l-epimeras~ ~ -D-glucose fast c. ~-D-glucose + 1/2 2 glucose oxid ~ D-gluconolactone +
fast d- 2H202 c ~ 2H20 + 2 fast 733~2 ~ s mentioned, glucose isomcxase cata]yzes the revers-ible conversion of ~-D-fructose to ~-D-glucosc. At 25C. the equilibrium constant of this reaction is approximately unity and would result in an approximate 50-50 mi~ture of ~-D-fructose and a-D-glucose. The spontaneous epimerization of the intermediate ~-D-glucose to ~-D-glucose is not sufficiently fast under the conditions of the assay to prevent accumulation of this inter-mediate and thus aldose-l-epimerase is added to the assay solu-tion to facilitate this intermediate reac_ion. The reporter ~eaction of this analysis is the aerobic (~lucose cxidase) oxida--tion of ~-D-glucose to D-gluconolactone in the presence of cata-lase which results in an overall stoichiometry of two moles of ~-D-fructose per mole of oxygen (2) This final reaction is monitored by means of a biological oxygen monitor such as a YSI
Model 53.
The assay was carried out as follows. Into a reaction cell which was equilibrated to 25~C. 3 ml of 0.01 molar phosphate buffer, pH 8, was added and stirred at a setting of 5 on a Thomas stirrer. Then, 30 microlitres of Sigma glucose oxidase Type V concehtrated 10 fold and 100 microlitres of aldose-l-epimerase prepared according to Lepedes and Chasel or equivalent was added. Subsequently, 10 microlitres of Sigma-C-100 catalase ~5 mg/ml concentration), and 20 microlitres of 72% (4.0 molar) ~-D-fructose were added to the cell. After the resulting solu-tion had been stirred for a total of 3 to 5 minutes, the elec-trode of a Model 53 YSI biological oxygen monitor was carefully inserted into the cell making sure that no air bubbles were retained; such as adhering to ~he electrode, cell walls, or ~ "Aldose-l-Epimerase from Hog Kidney: Isolation and Evidence o Purity, Chemical Studies and Inhibition Kinetics", S. L.
Lapedes and A. M. Chase, Bio_lem. & B~oE~ys. Res._Co~n., 31 967 (196~) ~C)733~Z
~ under the stir bar. With t}le recorder of the Model 53 YSI
I biological o~y~en monitor operating at a chart speed of 1/2" per minute the trace was allowed to stabillæe; that is, give a linear base line. Once a linear base line was established 100 micro-litres of the buffer rinse was added to the reaction cell alld the recorder trace was again allowed to achieve linearity, The assay is linear up to 10 micromoles 2 per minute, although slower ; rates are routinely employed using expanding scale attachments on ; the oxygen monitcr. No shift in the slope of the recorder trace indicates lack of active enzyme in the buffer rinse.
A loading of 0.7 units of glucose isomerase per ml of reactor matrix was calculated based upon loss of activity from the protein solution used for immobilization.
.~ .
COMPARISON OF MICROPOROUS CARRIER
WITH CONTROLLED PORE GLASS (CPG) Controlled pore glass particles 40-80 mesh were ob--tained from Electronucleonics Corporation and chemically modified by standard methods2 to introduce covalenty bound, aliphatic amino functionality on the external and internal surfaces thereof.
Two grams of the amino modified CPG were degassed and suspended in 100 ml of Hepes buffer for 1/2 hour. The supernatant was aspi-rated away from the bed and the particles resuspended in 100 ml of 10% aqueous gluaraldehyde solution for 1 hour. The CPG par-ticles were extensively washed by suspension and decantation until the odor of glutaraldehyde was gone. rl'en (10) ml of the enzyme solution containing 0.43 units/ml p~l 7.5 was added to the particles and allowed to react for 1 hour. A 1.2 ml volume of 2 "Immobilized Enzymes: A Prototype Vevice for the Analysis of Glucose in Biolo~ica'~ I'luids Employin~ Immobilized Glucose Oxidase", M. X. Weibel et al., ~nal. ~iochem , 52 502 (1'~73) 33~2 ., .
~ the partic~.es was loaded into a small colulnll (0.6 centime~Lc : diameter) ~o form a packed bcd reactor, and rinsed with thc llepes buffer until no protein could be detected in the supernatant as . determined by the assay technique of ~xample 8. Based upon loss of activity from the reaction solution, the loadinc~ was 0.66 units/ml (CPG has a bulk density of 0.36 grams/ml) which is , substantially equivalent to that of the immobilized enzyme carrier of Example $. The relative volumes of the disc (Example 8) and pac~ed bed reacto-s were within 20~ being 1.0 and 1.2 ml, respec-tively. The reactors were empirically evaluated k~ measu~ing the dec3ree of conversion of a 7.2% wt/vol fructose solution !o . ~
molar) pl-l 7.0 at several flow rates in the Hepes buffer. Glucose was measured by diluting the reactor effl.uent lOOX into 0.1 molar sodium acetate pH 5.5 and measuring the endpoint oxygen consump-tion in the presence of reporter enzymes. Analysis for immobi-lized enzyme activity was done by the same technique as used for solutions as described in Example 8 above, excep-t that the first reaction has already been accomplished and one need only analyze for the amount of ~-D--glucose in the effl.uent stream of the reactor. Thus the reaction:
~-D-fructose ~I ~ a-D-c3].ucose had already been accomplished in the reactor and is carried out with a 7.2% fructose solution in Hepes buffer. The analytical sequence of the reactor effluent is the same as equations b, c, and d of the reaction sequence of the assay technique set forth in Example 8, above.
The assay of the reactor effluent for efficiency of conversion of ~-~-fructose to ~ lucose is as follows: Into the reaction cell whi.ch was equilibrat:ed at 25C., 3 ml of sodium acetate buffer pTI 5.5 was pipeted and stirred at a settincJ of 5 ~7338Z
on the Thomas stirrer. Then, 60 microlitres of glucose oxidase, 200 microlitres of aldose-l-epimerase, and 10 microlitres of catalase were added -to the cell. After the resulting solution had been stirred for a total of 3 to 5 minutes the electrode of the YSI oxygen monitor was carefully inser-ted into the cell making sure that no air bubbles were retained on the surface of the electrode, the cell, or in the solution itself. With the YSI ;
biological oxygen monitor recorder operating at a chart speed of 12" per minute the trace was allowed to stabilize to a constant baseline. Once a linear baseline was es-tablished, 30 microlitres of reactor effluent was injected into the reaction cell and the curve was again allowed to achieve a stable slope.
The results of the empirical evaluation are tabulated below. Both immobilization and reactor s-tudies were carried out in parallel on the same day to ensure that a direc-t comparison could be made. The performance of each reactor over a period of 6 hours was unchanged as determined by the constant steady state conversion of fructose to glucose when the two reactors were operated in a kinetic mode.
Packed Bed Reactor (volume 1.2 ml) :.
Flow _ ate % Conversion Residence Time 1. 30 ml/min 0. 38% 0 . 92 min 0.69 ml/min 0.56% 1.74 min ~; 0.20 ml/min 1.50% 6.00 min Disc Reactor (volume 1.0 ml) _---------- !
0.75 ml/min 0. 81~o 1. 33 min 0.37 ml/min 1.30% 2.72 min O .18 ml/min 2.45% 5.50 min 733~3Z
As can be seen from the above data, the efficiency of the packed bed reactor is consistently only 60-70% that of the s-tacked disc assembly when the residence times are normalized.
This is quite surprising in view of calcula-tions which indicate ;~
that the "bulk concentration" of the enzyme is for prac-tical purposes identical for both reactors. The disc reactor was allowed to remain at room -temperature in the presence of the substrate solution for 5 days. The transport characteristics of the reactor were unchanged and the percent conversion a-t 0.37 ml/min was slightly higher at 1.50%.
MICROPOROUS CARRIER HAVING THERMOSET MATRIX
-- _____ In order to demonstrate that the matrix or binder constituent of the microporous enzyme carrier of the present invention is not limited to a thermoplastic polymeric resin, a sheet of microporous material was prepared by thoroughly inter-mixing 100 parts by weight of natural rubber, 165.5 parts of silica hydrogel, 3.1 parts inert filler (rubber dust)~ 39.0 parts sulfur, 0.8 parts stearic acid, and 0.8 parts diphenylguanidine in a Banbury mixer to produce a homogeneous mixture. This mixture was then extruded into shee-t form and calendered to 0.047 inches thick nominal. The calendered sheet was wound on a reel and vulcanized in an autoclave for 35 minutes at 172C. and 155 psig.
The vulcanized sheet was then air-dried in an oven to remove all traces of moisture. The resuling microporous material is extremely porous having micropores which vary in siz.e from about 0.5 micron to about 5 microns, and has a mean pore diameter of approximately 1.5 microns as determined by the Mercury Intrusion Method. In addition, the total porosity of this material is approximately 56% by volume and the dispersed ,~ .
733~Z
filler content (e.g. silica) comprises approxima-tely 26% by weight. Sample specimens 1.3 centimetres in diameter were punched from the finished microporous sheet on a press and utilized to ; form single disc reactors as follows:
1. Reac-tor No. 1 - incubated in enzyme only 2. Reactor No. 2 - incubated in polyethyleneimine, glutaraldehyde and enzyme For comparison purposes, a third single disc reactor (Reactor No.
3) was prepared by forming a disc of the material of Example 1 having a diameter of 1.3 centimetres and incubating in poly-ethyleneimine, glutaraldehyde, and enzyme.
Each microporous reactor disc (Reactors Nos. 2 and 3 ;
only) having been cut to the appropriate size, was immersed in 20 --cc of 5% polyethyleneimine for 30 minutes and agitated frequently to remove air bubbles. The pieces were then washed for 30 minutes in a 1 molar solution of sodium chloride to fix the -~
polyethyleneimine and subsequently washed thoroughly in distilled water to remove all the sodium chloride from the reactor discs.
This required four washings, 50 ml and 10 minutes each. The reactor discs next were soaked in 50 cc of a 10% aqueous solution of glutaraldehyde at pH 9 and agitated frequently to ensure uniform pene-tration of the discs by the glutaraldehyde. After incubation in the glutaraldehyde, the discs were thoroughly washed in distilled water using four 50 ml washings for 10 minutes each. ~lucose oxidase (1270 units/ml) was diluted 50/50 with phosphate buffer (0.1 molar, pH 6). The resultilng solution (50 cc) was adjusted to pH 6 with dilute sodium hydroxide and the discs of Reactors Nos. 1, 2, and 3 were incubated in this solu-tion for 30 minutes. After the 30 minute incubation, the reactor discs were removed and thoroughly washed with distilled water to :; :
~073382 .
remove free enzyme from the porous material, leaving behind only the immobilized enzyme.
Each of the above three reactors were assayed f'or activity by conversion of ~-D-glucose to D-gluconolactone and monitoring the hydrogen peroxide concentration in the ef`fluent stream. The substrate solution ( ~D-glucose, 0.15 millimolar in 0.1 molar potassium phosphate buffer at pH 6) was pumped through the reactors at varying flow rates and the effluent stream collected and assayed for hydrogen peroxide which is generated according to the e~uation:
1/202 + H20 + ~-D-glucose Glucose Oxidase H202 + D-gluconolactone Into the analyzer cuvet-te is added 25 microlitres of the peroxi-dase solution (10 mg/5 ml in potassium phosphate buffer at pH 6) and 50 microlitres of reduced O-Dianisideine solution (2% in methanol). The cuvette is filled with the reactor effluent, agitated, and analyzed on a Bausch & Lomb Spectronic 20 at 460 millimicrons for optical density versus a blank standard. The observed results are summarized as follows:
Reactor No. 1 Minimum enzyme activity was exhibited by this reactor. The activity that did exist was readily washed out as the glucose solution was pumped through the reactor indica-ting that the enzyme was not bound to the media but rather trapped within the pores.
Reactor No. 2 This reactor exhibited good activity on the first day being almost as active as the control (Reactor No. 3) when normalized for silica content of the material. At a flow rate of 0.5 cc/min.
through a 1 centimetre diameter area, the disc showed an activity ~' ! , ' . 'i , ". ' ' ' ' " , ' ' : ~7,338Z
:.
of 0.65 units/gram of material. The activity seemed to drop off slightly on the second day but this was not quantified.
Reactor No~ 3 This reactor exhibited good activity and revealed a constant reaction rate both days. At 0.5 cc/min. flow rate through a 1 centimetre diameter area the disc showed an activity of 1.8 units/gram of material.
It will be noted that the activity of Reactor No. 2 was approximately half that of Reactor No. 3 and also, that the material of Reactor No. 2 contained roughly half the silica filler of Reactor No. 3. This indicates that the filler (silica) constituent in the microporous material constitutes the primary . :
binding species for the immobilized enzyme rather than the surrounding matrix, such as hard rubber or polyvinyl chloride, -for example.
Although certain of the foregoing Examples illustrate the immobilized enzyme system of the present invention in the -form of a so called stacked-disc or flow-through reactor, it will be appreciated that many other forms of reactors may be employed as well. For example, the microporous starting material may be formed into the shape of a hollow tube, and treated in the manner disclosed above to bond or attach catalytically active enzymes thereto. A substratemay then be caused to flow into the tube at one end, be enzymatically reacted upon as it ~lows along and comes into contact with the inner wall of the tube, and the resulting product caused -to flow out of the tube at its other end.
Similarly, in cases where the substrate has a relatively high viscosity, or it is otherwise desirable to utilize a lQ~3382 packed-bed, f]uidized-bed, or stirred tan~ type o~ reactor, ~or example, sheets of microporous st~rting material may have enzymes bound thereto and immobilized as above with the resulting sheets being subsequently cut-up or divided into small pieces of practically any desired siæe (e.g., pieces, granules, beads, powders, and so on). The resu:Lting divided immobilized ; enzyme particles may -then be utilized by those skilled ln the art in applications requiring such forms of immobilized enzyme carrier.
10Finally, as will be understood further, the immobiliza-tion principles of the present invention are applicable to proteinaceous substances other than enzymes, such as antibodies or antigens, for example. Accordingly, the present invention should be limited only by the true scope o the appended claims.
-35~
., ~ . . ,, , ,~ "
sq. ft. to about 9 gallons/min./sq. ft. have been achieved through sheets of the preferred microporous material having a thickness of about 0.02 inches under a pressure gradient of only 10 psig, and having filler/binder ratios in the range from about 1/1 to about 2/1. Generally, an increase in the filler to binder ratio will result in increased pore size and greater total porosity thereby resulting in an increase in permeability of the material. Accord-ingly, the immobilized enzyme support of the present invention is ` ~7338Z
particularly suitable for use in the form of a so-called flow-through reactor core, -that is, a reactor core wherein the substrate solution penetrates one surface of the enzyme laden material, is catalytically reacted upon the enzyme, and the conver-ted product as well as any unreacted substrate exi-t through the same or another surface of the material.
Moreover, since as mentioned above, the pore size distri-bution of the microporous support material extends over a rela-tively wide range (i.e., about 0.01 micron -to about 100 micron) and the micropores are substantially interconnected, the material contains a multitude of sufficiently sized paths along which both substrate and/or converted product may easily flow. Product efflux from the material is thus quite rapid and may be terminated substantially simultaneously with end point flow of the substrate -through the support material. In other words, ca-taly-tic reactions produced with the enzyme support contemplated by the present inventibn have an ex-tremely sharp cutoff, and accordingly, many different substrate samples may be fed through the sarne immo- `-bilized enzyme support in rapid succession without the danger of contamination between successive samples, an extremely desirable advan-tage when immobilized enzymes are employed to carry out successive catalytic reactions on a series of different substrate samples as in medical or industrial analytical instruments, for example.
The foregoing cons-titutes a significant advantage of the present invention since in other known immobilized enzyme reactors such as the packed bed of porous glass beads, or the membrane reactor, for example, pore size is controlled quite uniformly and is of such small size that mass transfer through the reactor is accomplished by diffusion. In such diffusion limited enzyme ...;
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07~3~3Z
reactors, total efflux -time of the product may lag significantly behind the substrate sample termination poin-t, thus presenting a contamination problem should a succeeding substrate sample be fed into the reactor too rapidly.
In addi-tion to the foregoing advantages, the microporous enzyme support material of the present invention has excellent strength characteristics typically having a tensile strength of about 400 psi and a percentage of elongation under 20%, and thus may be handled quite easily during -the various s-tages of trea-t-ment necessary to bond or attach enzymes thereto as will beexplained in more detail below. Moreover, due to its excellent dimensional stability and strength, the microporous material of the present invention resists compaction under hydraulic pressures, and therefore is especially adapted -to be employed in large scale bulk processing reactors where large enzyme reaction areas are involved and large dynamic forces are exerted on the enzyme support member such as, for example, in commercial industrial or chemical processes uilitizing enzymatic reactions. Moreover, the preferred microporous material is resistant to a-ttack by chemicals such as acids and alcohols, for example, and is capable of being exposed to elevated temperatures without affecting its physical properties. In regard -to -the latter, it has been found possible, for example, to heat sterilize the preferred microporous material by emersion in steam at 15 psi and 2~0 F for 30 minu-tes without degrading the dimensional s-tability or physical properties of the material.
As more fully disclosed in the aforementioned '030 paten-t, the particularly preferred microporous material may be fabricated by admixing suitable quantities of a finely divided polymeric resin, 1~7338Z
:"`
a finely divided inorganic filler, a solvent (e.g., cyclohexanone) and a non-solvent (e.g.,water) under low shear conditions to ~orm a stable, damp, free-flowing powder. The powder mixture may then be extruded and calendered preferably -to form a substantially planar structure or sheet of desired dimensions which may next be passed through an aqueous bath to leach out the solvent, and then subsequently passed through a heated air oven to remove all -traces ; of moisture. In accordance with the present invention, the resulting article in the form of a microporous, dimensionally stable~ semi-rigid, insoluble, fluid permeable member may then be treated in such a manner as to couple or bond enzymes thereto.
As is generally known in the art, it is possible to bond or attach enzymes to an insoluble support or carrier by directly adsorbing the enzyme on the carrier, or by indirectly adsorbing or covalently bonding the enzyme to the carrier through an intermediate coupling agent. Due primarily to its dispersed silica filler component, the preferred microporous support material of the present invention has been found to exhibit a net negative charge as evidenced by substantial adsorption of proteins thereto at pH values below the isolectric point of the adsorbed protein. Thus, although direct adsorption of enzymes to the dis-persed filler particles in the material is feasible, the adsorp-tive in-teraction (direct) has been found to be of insufficient magnitude to prevent relatively rapid desorption during use and subsequently, loss of enzymatic activity from the enzyme composite.
Accordingly, in carrying out the present invention, i-t is preferred that the microporous material be treated in such a manner as to effect a chemical bond between the catalytically active enzyme and the insoluble microporous support material.
"
1~173382 In i-ts untreated condition, -the microporous ma-terial laeks -the organic funetionality necessary to effect such chemieal bonding to proteinaceous substances, hence, any known technique for imparting the required functionality to -the microporous material may be employed sinee the present in~ention in i-ts broades-t aspeet is eoneerned with the discovery -that the bonding of enzymes of the microporous starting material resul-ts in a superior immobilized `;
enzyme composite. Most known enzymes may be immobilized by covalently coupling or cross-linking free amino residues or groups on the enzyme molecule which are not essential -to the enzymatic activity of the enzyme to a carrier surface containing aliphatic primary or secondary amino or hydroxyl groups or residues. Still other known enzymes may be covalently coupled or cross-linked to a earrier surfaee in similar fashion via sueh o-ther fune-tional groups as, earboxyl, isonitrile, aldehyde or ketone, or anion, to name a few. Therefore, it will be understood that the term "ehemieal bond" or "chemieally bound" as used therein and in the appended elaims refers broadly -to the ehemical linkage between the cata-lytically active protein or enzyme and the functional groups or residues imparted -to the microporous starting material and is not -to be construed as being limited to a particular functional group or residue or to a partieular enzyme.
In one preferred embodiment of the present invention, a~iphatic primary amine functionality may be imparted to the mieroporous starting material by eovalently bonding directly to - the dispersed filler particles in the microporous material a ; bridging agent in the form of an organosilane such as gamma-aminopropyl-triethoxysilane, whereas in another alternatively preferred embodiment of the invention alipha-tic primary amine functionality may be imparted -to the microporous material by :
! .
` ~La,733~Z
irreversibly chemiadsorbing directly -to -the dispersed filler particles in the microporous material a bridging agent in the form of a macromolecular polyelectrolyte such as polyethylenemine (PEI~. Enzymes may -then be covalently bonded or cross-linked to the chemically modified microporous material and more specifically to the aliphatic primary amine residues impar-ted to the surface of the material by the aforementioned bridging agen-ts.
In the case where a bridging agent such as gamma- ;
aminopropyltriethoxysilane is employed, the latter is believed to be primarily covalently bonded directly to the hydrophilic inorganic filler particles dispersed through the polymeric binder constituent of the microporous material. Generally speaking the use of a silane bridging agent to bond or attach enzymes to siliceous materials is known in the art as disclosed, for example, in the aforementioned U.S. Paten-t No. 3,519,538.
In -the case where a bridging agent such as poly-ethylenemine is employed, the latter is believed to be attached or bonded to the dispersed hydrophilic inorganic filler constituen-ts of the microporous material via strong chemiadsorptive forces.
ZO Generally, the use of a macromolecular polyelectrolyte or poly-amine as a bridging agent to bond or attach enzymes to the surface of colloidal particles of silica, or to fibrous cellulose, is known in the art as respectively disclosed, for example, in U.S.
Patents Nos. 3,796,634 and 3,741,871. -In both cases, the enzyme is preferably cross-linked to ;~ the bridging agent by means of a bifunctional electrophilic : reagent such as glutaraldehyde or bisimidate esters to effect the :
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~0733~Z
desired covalent conjugation of the enzyme to -the functional amine groups which have been imparted to the external surfaces of the hydrophilic filler particles dispersed -throughout the microporous carrier or support via the bridging agent.
When using a carrier surface adsorptive bridging agen-t, in the form of -the aforementioned polyethylenimine, for example, or a bridging agent covalently bonded to the carrier surface such as the aforementioned gamma-aminopropyltriethoxysilane, for exam-ple, covalent conjugation of the enzyme and the carrier may be carried out in a single or two step producedure. In the single step procedure, the chemically modified carrier material may be simul-taneously treated with the bifunctional electrophilic reagent and the enzyme to effect simultaneous inter-molecular cross-linking of -the carrier surface reactive polymer and the enzyme. Commercial grades of glutaraldehyde, a typical bifunctional reagent as men--tioned above, con-tain significan-t amounts of soluble polymeric com-pounds formed from intermolecular aldol condensa-tions of the mono-meric dialdehyde, hence, each site of condensation results in a highly reactive alpha-beta unsaturated aldehyde moiety which will rapidly undergo Michael type addition reactions involving nucleo-philes such as aliphatic amines or other residues found on the surface of enzymes. In addition, free aliphatic aldehyde groups which are present in the carrier surface reactive polymer may also participate in the cross-linking reactions by combina-tion with aliphatic amino residues of the carrier or enzyme to form Schiff bases. Although the degree to which desired covalent conjugation of the enzyme competes with such undesired, unproductive reactions resulting in simple protein modification and cross-linking of carrier reactive surface residues may be empirically determined by varying experimental conditions such as pH, protein concentration :
~733~3Z
and cross-linking reagent concentration, it is difficult to selec-tively control such undesired, competetive reactions as -the bifunctional cross-linking reagent is always presen-t in a substan-tial molar excess during the reaction. In certain cases, there-fore, employment of the single step procedure may result in partial or -total enzyme inactivation due to extensive chemical modification of the enzyme or to chemical modification of the essential ac-tive site residues.
In situations where chemical modifica-tion results in extensive enzyme inactivation, the two s-tep procedure is recom-mended wherein the chemically modified carrier material is first cross-linked with the bifunctional reagent and then subsequently incubated with the enzyme. By using a sui-tably high concentration of -the cross-linking reagen-t, bimolecular reactions can become competitive for the surface amino residues relative to intramole-cular processes such as cross-linking. This results in a high surface density of pendant residues capable of reacting with nucleophilic side chain residues of enzymes. After removal of the excess unreacted cross-linking reagent, the enzyme of interest may then be incubated with the modified carrier resulting in covalent conjugation of the enzyme and the carrier. The fore-going two step procedure has been found to result in minimal modification of the enzyme since only residues in the vicinity of the contact region between the enzyme and the carrier reactive surface are involved.
It will be appreciated that various chemistries other than the electrophilic bifunctional reagen-ts mentioned above can be employed to covalently bond enzymes to the chemically modified carrier material. Such alternatives may include, for example, - 30 acylation of the alipha-tic amino group at the carrier reac-tive surface with succinic anhydride to produce a pendant aliphatic ~0733t3Z
carboxyl group which is subsequently reacted with nucleophilic side chain residues of enzymes in the presence of a water soluble carbodiimide; direct reaction of the amino group at -the carrier reactive surface with side chain carboxyl groups of enzymes in the presence of a water soluble carbodiimide; acylation of -the amino group at the carrier reactive surface with p-nitrobenzoyl chloride, reduction of the aryl nitro to an aryl amine via sodium dithionite, oxidation of the aryl amino group to an aryl diazonium salt via nitrous acid and subsequent reaction with aromatic side chain residues of proteins to form a stable azo linkage; acylation of the amino group at the carrier reactive surface with -terepthaloyl chloride, reaction of the pendan-t p-benzoyl acid halide with hydrazide to a benzoyl azide and subsequent reaction with nucleo-philic side chain res~dues of enzymes.
~ hen reacting the enzyme with the chemically modified carrier, the enzyme is preferably placed in a buffering solu-tion and the reaction carried out at temperatures sufficiently low to avoid deactivation of the enzyme or substantial changes in the latter's conformational state. Generally, tempera-tures in the ZO range of about 5 C to about 50 C are acceptable. As is known in the art, the pH of the enzyme reaction solution may be con-trolled at a desired level, by selec-ting suitable buffers, depending upon the particular enzyme being bound. Likewise, the concentration of enzyme in the buffered reac-tive solution and ,:!
. therefore, the extent to which the chemically modified carrier will be loaded with enzymes may be chosen depending upon the conversion rate of the enzyme, the concentration of the substrate, and the flow rate of the substrate through the reactor core.
:
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The present invention now will be further described with reference to the following examples -thereof, which latter are intended for illustration purposes only and are not to be cons-trued as limiting the scope of the invent:ion. ;
PREPARATI_N OF UNTREATED ENZYME SU _ORT M MBER
A sheet of microporous material was prepared by first dry blending 20.0 lbs. of Conoco 5385 polyvinyl chloride resin having a particle size of about 80 mesh, and 40.0 lbs. of Hi Sil 233, a precipitated hydrated silica, in a Patterson Kelley "low shear" liquids-solids blender for approximately 3 minutes.
Thereafter, and during continued agitation, 54.6 lbs. of solvent (cylohexanone) were added over a 20 minute period by means of a pump. Wa-ter in an amount of 59.0 lbs. was then added to the mix in the agitating blender over a subsequent 20-minute period to form a damp, stable, free-flowing powder. The powder was then introduced into a screw extruder having a barrel temperature of -approximately 120 F., and the extrudate passed between the rolls :, , of a calender to obtain a substantially flat sheet having a thickness of 0.02 inches (0.5mm). The sheet was then passed through an extraction bath of water at 170 F., and subsequently dried in a hot air oven at 225 F., for 6 minutes. The finished microporous sheet has a relatively wide pore size distribution extending from about 0.01 micron to about 100 micron, and a mean pore diameter in the range of about .15 micron to about .25 micron as determined by the Mercury Intrusion Method. In addition 9 the total porosity of this material is approxima-tely 65% by volume and the dispersed filler content (e.g., silica) comprises approximately 56% by weight. Liquid water soaked rapidly into the material without any applied pressure indicatlng that the micropores are 7338~
substantial~y interconnected rom sur~ace to surEace. From the resulting substantially flattened, semi-rigid, microporous shcet a plurality of untreated support members 5X5cm in size were cut and heat sterilized by immersion in a steam bath for one hour and allowed to cool and dry in open air.
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CHEMICA _ MODIFICATION BY COVALENT BONDING
An untreated support member prepared in accordance with Example 1 was incubated in a 10% vol/vol aqueous solution of gamma-aminopropyltriethoxysilane containing 1% vol/vol concen-trated HCl for 24 hours. The treated support member was flushed with water and 1 M NaCl to remove all unreacted reagents. The presence of aliphatic primary amino residues was then qualita-tively assessed by reacting the treated member with 0.5% wt/vol trinitrobenzene sulfonic acid in 0.1 M sodium tetraborate buffer at 70 F. and observing an intense orange trinitrophenyl amine derivative on the surface of the treated support member. Another un-treated support member prepared in accordance with Example 1 was similarly asseyed, but displayed no reac-tion -to this test.
Elemental analysis of` the treated support member yielded 0.5%
nitrogen by dry weight above that of the untreated support member.
The permanence of the amino functionality of the treated support member was evidenced by negligible nitrogen loss after storage in ~; water for a period of 12 months. The treated support member displayed identical flow properties with respectto the untreated support member and was not sensitive to differences in the buffers or ionic streng-th.
CHEMICAL MODIFICATION BY CHEMIADSORPTION
Another untreated support member prepared in accordance ~` with Example 1 was incubated in a 5% wt/vol aqueous solu-tion of 50,000 mol. wt. branched chain polyethyleneimine (PEI) at room temperature for one hour. The treated support was flushed with water and 1 m NaCl to remove any unadsorbed PEI. Assey was by the ,.
10733~3Z
same trinitrobenzene sulfonic acid test employed in Example 2 and an intense orange -trinitrophenyl amine derivative was observed on the surface of the treated support member demonstra-ting subs-tan tial aliphatic amino functionality. The nitrogen loading on the treated support member was quantitated by elemental analysis and was 1.25% nitrogen by dry weight versus 0.02% nitrogen by dry weight of an untreated suppor-t member. The chemiadsorption of PEI on the treated support member appeared virtually irreversible ; since it could not be removed by incubation with high ionic strength solutions (e.g., lM NaCl or 1 M K2 HP04/KH2P04) at pH
values between 3 and 9. Only in the case of strong acidic condi-tions (incubation in 1 M HCl for 2 hours) was there evidence of ~ partial desorption amounting to 50% of the nitrogen content as - indicated by elemental analysis. The surface area of the treated support by standard BET procedure was 55.4 M /g versus 81.1 M /g ~or the control. The support member treated with PEI displayed identical flow properties compared to an untreated support member irrespective of the buffer or ionic strength used.
, 20 ENZYME COUPLING REACTION
(Glucose Oxidase) -~ The support member treated in accordance with Example 3 was incubated for one hour in 10% vol/vol aqueous solu-tion of glutaraldehyde at pH 7. The support member was then rinsed with water and incubated for one hour in a solution of glucose oxidase which had been purified to homogeneity from Asper~llis n ger.
The conditions of the enzyme coupling reaction were as follows:
glucose oxidase concentration 20 mg/ml in 0.1 M K2HPO~/KH2P04 buffer pH 6.0 at ambient room temperature. Directly pumping -the enzyme solution through the support member under a positive ;, , . ', ~, ::
~07338Z , ;
hydraulic pressure did not improve enzyme loading rela-tive to ,~
that obtained by simple incubation. The tempera-ture of the coupling reaction was not found to be critical with the only requirement being that it did not exceed the -thermal inactivation region of 50 C for glucose oxidase. The support member was then extensively washed with water and 1 M NaCl to remove unreacted enzyme. Quenching of electrophilic residues on the support member surface was achieved by incubation of the immobilized enzyme com-posite with 0.1 M ethanolamine at p~ 7.0 containing 50 mM NaCNBH3.
The immobilized enzyme appears to have an indefinite shelf life when stored at 4 C in 0.1 M K2HP04 buffer pH 6Ø
SINGLE ENZYME REACTOR
The following reaction was carried out employing a pair ,;-, ~ of 1.5cm diameter disks prepared in accordance with Example 4 and . j mounted in a stacked configuration in a flow--thru reactor wherein the flow vector of the substrate was substantially perpendicular : :j to -the plane of each disk. The cross section of each mounted disk exposed to the fluid stream was 79mm . Glucose oxidase (E.C.1.1.3.4.) catalyzes the aerobic oxidation of glucose ~ -D-glucose + 2 -- ~ D-gluconolactone + H202 -~ Enzymatic activity in the stacked disk reactor conf`iguration was evaluated by measuring oxygen depletion downstream from the reactor with a Biological Oxygen Monitor, Model No. 53, obtained from Yellow Springs Instrument Company. A solu-tion of 0.15 mM glucose at anomeric equilibrium in air saturated 0.1 M Na acetate buffer pH 5.5 was pumped through the reactor at a flow rate of 2 ml/min.
The conversion of the limiting substrate,~ -D-glucose, was quantitative as measured by oxygen depletion downstream from the `` 1~733~3;Z `~
reactor. The residence time of the sample stream in contact with the reactor was approximately 1.6 seconds. The integra-ted form of the rate equation for glucose oxidase under these experi-mental conditions ls known explicitly, and it can be calculated thatthe lower limit for the immobilized enzyme concentration is ; 10 mg/ml. The unusually high activity of the stacked disk reactor is attributed to the absence of internal mass transport effects, i.e., no evidence of internal mass transport constraints for the reactor was observed.
A second set of stacked disks were prepared in accor-dance with Example 4 and mounted in the flow-thru reactor; the disks, however, were prepared with substantially reduced concen- ' , tration of the immobilized enzyme, i.e., by a factor of 10. A
'jl l mM glucose solution in 0.1 M Na acetate buffer pH 5.5 was then pumped through the second disk reactor at flow rates sufficiently fas-t tha-t the reactor was operating in a kinetic mode with only partial conversion of glucose to gluconolactone. The steady-state level of substrate conversion by the reactor under this condition `
was found to be highly sensitive to the enzyme concentration.
When observed under continuous operation for a period of four hours, no change in the steady-state conversion level was observed indicating no loss of enzymatic activity from the reactor.
ENZYME COUPLING REACTION
(Alcohol Dehydrogenase) Another suppor-t member treated in accordance with Example 3 was incubated for one hour in a 10% vol/vol aqueous solution of glutaraldehyde at pH 7. The support member was then rinsed with water and incubated for one hour in a solution of alcohol dehydro-genase. The conditions of the enzyme coupling reaction were asfollows:
.. . . . .
" 10733~3Z
alcohol dehydrogenase concentration 5 mg/ml in 0.1 M K2HP04KH2P04 buffer pH 6.0 containing 0.1 mM EDTA and 10 ~ M NADH (reduced nicotinamide adenine dinucleotide) at ambient room -temperature.
The support member was then extensively washed with the reaction buffer and 1 M NaCl to remove unreacted enzyme. Unreacted electrophilic residues on the support member was quenched by incubation of the immobilized enzyme composi-te with 0.1 M ethano-lamine at pH 7.0 containing 50 mM NaCNBH3. The enzyme loading was ~.
11 mg/g of the carrier and was calculated by measuring the incre-mental increase in nitrogen upon the support member prior to the ,, quenching reaction.
~ Alcohol dehydrogenase (EC 1.1.1.1) catalyzes the - reversible oxidation of primary alcohols according to the equation ; alcohol + NA ~ ~ aldehyde + NADH +
Enzymatic activity in a stacked disk reactor configuration was evaluated by measuring spectrophotometrically the formation of NADH @ 340 nm downstream from the reactor with a flow-through Model UA-5 absorbance monitor obtained from Instrumentation Specialties Co. A single 1.5 cm disk of the immobilized enzyme was mounted into a flow t~rough reactor in the manner of Example 5.
A solution of 50 mM ethanol and 0.5 mM NAD~ in 0.1 M K2HP04/KH2P04 buffer pH 7.4 containing 10 ~ M EDTA was pumped through the reactor at a flow rate of 1 ml/min. The calculated equilibrium conversion for the reaction under these conditions is 16% of the starting NA ~ concentration. Complete equilibration was observed indicat-ing that a few milliseconds contact with the immobilized enzyme reactor were sufficient to achieve the thermodynamic limit of the ; reaction. In order to demonstrate the stability of the immobi-lized enzyme a set of conditions was chosen in which the reactor was operated for 24 hours in a kinetic mode. As the conversion ~[)733~3~
, of substrates to products is extremely sensitive to conservation ;
of the catalyst under these conditions, a decrease in the conVer-sion level indicates loss or inactivation of the enzyme. The conditions of the experiment were 5 mM ethanol and 50~ M NAD in 0.1 M K2HP04/KH2P04 buffer pH 7.0 containing -lO~ M EDTA. This solution was pumped through the reactor at a flow rate of ] ml/min ~ `~
for 24 hours with continuous monitoring and recording of the sub-strate conversion level. It was found tha-t the conversion remained constant during this period indicating complete conser~
vation of the immobilized enzyme.
TANDEM ENZYME REACTOR
A disk reactor system incorporating three differen-t immobilized enzyme composites was constructed for catalyzing the ~ reaction sequence shown below.
,1 (EC 3.2.1.26) . sucrose + H20 - - > ~-D~glucose + fructose : ~l . :' :~:
-D-glucose - - ~ ~ D glu `~
~, ` ;~ ,`
(E.C. 1.1.3.4.) -D-glucose + 2 - ) ~ D-gluconolactone + H202 ;~
The glucose oxidase was homogeneous and prepared from Aspergillis niger, -the aldose-1-epi.merase enzyme (EC 5.1.3.3) was prepared from hog kidney and was 20% wt/wt purity, and the ~-D-fr~cto-furanosidase (EC 3.2.1.26) was a high purity preparation from Candida utilis. Each of the aforementioned enzymes was covalently immobilized to a pair of 1.5cm disks in accordance with the method of Example 4 at an enzyme concentration of 20 mg/ml. The alde-hyde quenching reaction was not employed. The two sets of three disks, each disk in each set corresponding to one of the three enzymes in the coupled reaction and in -the sequence shown above, ' .
~73313Z
were then mounted in the flow-thru reactor of Example 5 in a stacked fashion. A 1 mM solution of ultrapure sucrose in 0.05 M
K2HP04 pH 6~0, air saturated at 25C. was then pumped through the reactor at a flow rate of 1.2 ml/min. The conversion as measured by oxygen depletion downstream from the reactor was lO~o the theoretical based upon the known stoichiometry o-f the overall reaction. The maximum conversion which could be obtained, how-ever, was 25% since dissolved oxygen is the limiting substrate (250~ M). Under the conditions employed for -this example, the aldose-1-epimerase is the rate limiting enzyme. At slower flow rates and consequently longer reactor residence times, measured conversions approaching 25% were obtained.
IMMOBILIZATION OF GLUCOSE ISOMERASE
ON MICROPOROUS CARRIER
Glucose isomerase (E.C. 5.3.1.5) catalyzes the revers-ible interconversion of ~-D-fructose to~-D-glucose in accordance ; with the following reaction:
~-D-fructose E.C. 5.3.1.5 ~-D-glucose ; 20 Four discs of 26 mm diameter were cut from a sheet of microporous material (Example 1) and treated in accordance with Example 3 and then mounted in stacked fashion into a standard Millipore filter holder without gasket seals to form a flow-thru reactor. The PEI
laden support discs were modified by pumping glutaraldehyde (10%
wt/vol pH adjusted to 8.0) through the reactor in a recycled mode from a 100 ml reservoir for 1 hour. The support member was then rinsed in-situ by pumping 500 ml (approximately 1/2 hour) of deionized water and 200 ml of Hepes buffer or equivalent (i.e.
2g/1 Mg S04.7H20 and 0.2g/1 CoS04.7H20 pH 7.0-7.5 in deionized water 1C~733~3Z
,~
through the reactor. A solution of glucose isomerase at pH 7.5 (30 ml containing 0.43 units/ml) was passed through a Millipore 0.65 micron fil-ter and circulated through the disc reactor for 1 ~;
hour at room temperature. The term "units" as used herein refers to units of activity and is de~`ined as that amount of enzyme 1 which catalyzes the conversion of 1 micromole of ~-D-fructose '~ to ~ D-flucose per minute at 25C. The reactor was rinsed with approximately 500 ml of Hepes buffer until no protein could be detected irl the effluent. The glucose isomerase enzyme immobil-' 10 ized in this Example was obtained as a lyophilized whole cell ;~
homogenate of Streptomyces albus from Novo Enzyme Corporation and purified by soluble protein isolation and fractionation with . ammonioum sulfate (AmS04~. Although the frac-tionation depends in part upon the initial protein concentration of the supernatant obtained from the protein isolation step, the major glucose activity is typically found in the 70-85% AmS04 pellet. The protein pellets containing the majority of the activity are dissolved in v20-30ml of Hepes buffer and dialyzed against 4 litres of buffer from 24 hours at 4 C. using standard cellulose acetate dialysis tubing. Although the enzyme preparation at this point is suitable for use in immobilization if desired, the above enzyme concentrate can be purified s-till further by standard gel permeation techniques. Protein assay of the rinse affluent solution was carried out by employing the following reaction - sequence:
a. ~-D-fructose ~ C~-D-glucose rate-limiting b. ~-D-glucose aldose-l-epimeras~ ~ -D-glucose fast c. ~-D-glucose + 1/2 2 glucose oxid ~ D-gluconolactone +
fast d- 2H202 c ~ 2H20 + 2 fast 733~2 ~ s mentioned, glucose isomcxase cata]yzes the revers-ible conversion of ~-D-fructose to ~-D-glucosc. At 25C. the equilibrium constant of this reaction is approximately unity and would result in an approximate 50-50 mi~ture of ~-D-fructose and a-D-glucose. The spontaneous epimerization of the intermediate ~-D-glucose to ~-D-glucose is not sufficiently fast under the conditions of the assay to prevent accumulation of this inter-mediate and thus aldose-l-epimerase is added to the assay solu-tion to facilitate this intermediate reac_ion. The reporter ~eaction of this analysis is the aerobic (~lucose cxidase) oxida--tion of ~-D-glucose to D-gluconolactone in the presence of cata-lase which results in an overall stoichiometry of two moles of ~-D-fructose per mole of oxygen (2) This final reaction is monitored by means of a biological oxygen monitor such as a YSI
Model 53.
The assay was carried out as follows. Into a reaction cell which was equilibrated to 25~C. 3 ml of 0.01 molar phosphate buffer, pH 8, was added and stirred at a setting of 5 on a Thomas stirrer. Then, 30 microlitres of Sigma glucose oxidase Type V concehtrated 10 fold and 100 microlitres of aldose-l-epimerase prepared according to Lepedes and Chasel or equivalent was added. Subsequently, 10 microlitres of Sigma-C-100 catalase ~5 mg/ml concentration), and 20 microlitres of 72% (4.0 molar) ~-D-fructose were added to the cell. After the resulting solu-tion had been stirred for a total of 3 to 5 minutes, the elec-trode of a Model 53 YSI biological oxygen monitor was carefully inserted into the cell making sure that no air bubbles were retained; such as adhering to ~he electrode, cell walls, or ~ "Aldose-l-Epimerase from Hog Kidney: Isolation and Evidence o Purity, Chemical Studies and Inhibition Kinetics", S. L.
Lapedes and A. M. Chase, Bio_lem. & B~oE~ys. Res._Co~n., 31 967 (196~) ~C)733~Z
~ under the stir bar. With t}le recorder of the Model 53 YSI
I biological o~y~en monitor operating at a chart speed of 1/2" per minute the trace was allowed to stabillæe; that is, give a linear base line. Once a linear base line was established 100 micro-litres of the buffer rinse was added to the reaction cell alld the recorder trace was again allowed to achieve linearity, The assay is linear up to 10 micromoles 2 per minute, although slower ; rates are routinely employed using expanding scale attachments on ; the oxygen monitcr. No shift in the slope of the recorder trace indicates lack of active enzyme in the buffer rinse.
A loading of 0.7 units of glucose isomerase per ml of reactor matrix was calculated based upon loss of activity from the protein solution used for immobilization.
.~ .
COMPARISON OF MICROPOROUS CARRIER
WITH CONTROLLED PORE GLASS (CPG) Controlled pore glass particles 40-80 mesh were ob--tained from Electronucleonics Corporation and chemically modified by standard methods2 to introduce covalenty bound, aliphatic amino functionality on the external and internal surfaces thereof.
Two grams of the amino modified CPG were degassed and suspended in 100 ml of Hepes buffer for 1/2 hour. The supernatant was aspi-rated away from the bed and the particles resuspended in 100 ml of 10% aqueous gluaraldehyde solution for 1 hour. The CPG par-ticles were extensively washed by suspension and decantation until the odor of glutaraldehyde was gone. rl'en (10) ml of the enzyme solution containing 0.43 units/ml p~l 7.5 was added to the particles and allowed to react for 1 hour. A 1.2 ml volume of 2 "Immobilized Enzymes: A Prototype Vevice for the Analysis of Glucose in Biolo~ica'~ I'luids Employin~ Immobilized Glucose Oxidase", M. X. Weibel et al., ~nal. ~iochem , 52 502 (1'~73) 33~2 ., .
~ the partic~.es was loaded into a small colulnll (0.6 centime~Lc : diameter) ~o form a packed bcd reactor, and rinsed with thc llepes buffer until no protein could be detected in the supernatant as . determined by the assay technique of ~xample 8. Based upon loss of activity from the reaction solution, the loadinc~ was 0.66 units/ml (CPG has a bulk density of 0.36 grams/ml) which is , substantially equivalent to that of the immobilized enzyme carrier of Example $. The relative volumes of the disc (Example 8) and pac~ed bed reacto-s were within 20~ being 1.0 and 1.2 ml, respec-tively. The reactors were empirically evaluated k~ measu~ing the dec3ree of conversion of a 7.2% wt/vol fructose solution !o . ~
molar) pl-l 7.0 at several flow rates in the Hepes buffer. Glucose was measured by diluting the reactor effl.uent lOOX into 0.1 molar sodium acetate pH 5.5 and measuring the endpoint oxygen consump-tion in the presence of reporter enzymes. Analysis for immobi-lized enzyme activity was done by the same technique as used for solutions as described in Example 8 above, excep-t that the first reaction has already been accomplished and one need only analyze for the amount of ~-D--glucose in the effl.uent stream of the reactor. Thus the reaction:
~-D-fructose ~I ~ a-D-c3].ucose had already been accomplished in the reactor and is carried out with a 7.2% fructose solution in Hepes buffer. The analytical sequence of the reactor effluent is the same as equations b, c, and d of the reaction sequence of the assay technique set forth in Example 8, above.
The assay of the reactor effluent for efficiency of conversion of ~-~-fructose to ~ lucose is as follows: Into the reaction cell whi.ch was equilibrat:ed at 25C., 3 ml of sodium acetate buffer pTI 5.5 was pipeted and stirred at a settincJ of 5 ~7338Z
on the Thomas stirrer. Then, 60 microlitres of glucose oxidase, 200 microlitres of aldose-l-epimerase, and 10 microlitres of catalase were added -to the cell. After the resulting solution had been stirred for a total of 3 to 5 minutes the electrode of the YSI oxygen monitor was carefully inser-ted into the cell making sure that no air bubbles were retained on the surface of the electrode, the cell, or in the solution itself. With the YSI ;
biological oxygen monitor recorder operating at a chart speed of 12" per minute the trace was allowed to stabilize to a constant baseline. Once a linear baseline was es-tablished, 30 microlitres of reactor effluent was injected into the reaction cell and the curve was again allowed to achieve a stable slope.
The results of the empirical evaluation are tabulated below. Both immobilization and reactor s-tudies were carried out in parallel on the same day to ensure that a direc-t comparison could be made. The performance of each reactor over a period of 6 hours was unchanged as determined by the constant steady state conversion of fructose to glucose when the two reactors were operated in a kinetic mode.
Packed Bed Reactor (volume 1.2 ml) :.
Flow _ ate % Conversion Residence Time 1. 30 ml/min 0. 38% 0 . 92 min 0.69 ml/min 0.56% 1.74 min ~; 0.20 ml/min 1.50% 6.00 min Disc Reactor (volume 1.0 ml) _---------- !
0.75 ml/min 0. 81~o 1. 33 min 0.37 ml/min 1.30% 2.72 min O .18 ml/min 2.45% 5.50 min 733~3Z
As can be seen from the above data, the efficiency of the packed bed reactor is consistently only 60-70% that of the s-tacked disc assembly when the residence times are normalized.
This is quite surprising in view of calcula-tions which indicate ;~
that the "bulk concentration" of the enzyme is for prac-tical purposes identical for both reactors. The disc reactor was allowed to remain at room -temperature in the presence of the substrate solution for 5 days. The transport characteristics of the reactor were unchanged and the percent conversion a-t 0.37 ml/min was slightly higher at 1.50%.
MICROPOROUS CARRIER HAVING THERMOSET MATRIX
-- _____ In order to demonstrate that the matrix or binder constituent of the microporous enzyme carrier of the present invention is not limited to a thermoplastic polymeric resin, a sheet of microporous material was prepared by thoroughly inter-mixing 100 parts by weight of natural rubber, 165.5 parts of silica hydrogel, 3.1 parts inert filler (rubber dust)~ 39.0 parts sulfur, 0.8 parts stearic acid, and 0.8 parts diphenylguanidine in a Banbury mixer to produce a homogeneous mixture. This mixture was then extruded into shee-t form and calendered to 0.047 inches thick nominal. The calendered sheet was wound on a reel and vulcanized in an autoclave for 35 minutes at 172C. and 155 psig.
The vulcanized sheet was then air-dried in an oven to remove all traces of moisture. The resuling microporous material is extremely porous having micropores which vary in siz.e from about 0.5 micron to about 5 microns, and has a mean pore diameter of approximately 1.5 microns as determined by the Mercury Intrusion Method. In addition, the total porosity of this material is approximately 56% by volume and the dispersed ,~ .
733~Z
filler content (e.g. silica) comprises approxima-tely 26% by weight. Sample specimens 1.3 centimetres in diameter were punched from the finished microporous sheet on a press and utilized to ; form single disc reactors as follows:
1. Reac-tor No. 1 - incubated in enzyme only 2. Reactor No. 2 - incubated in polyethyleneimine, glutaraldehyde and enzyme For comparison purposes, a third single disc reactor (Reactor No.
3) was prepared by forming a disc of the material of Example 1 having a diameter of 1.3 centimetres and incubating in poly-ethyleneimine, glutaraldehyde, and enzyme.
Each microporous reactor disc (Reactors Nos. 2 and 3 ;
only) having been cut to the appropriate size, was immersed in 20 --cc of 5% polyethyleneimine for 30 minutes and agitated frequently to remove air bubbles. The pieces were then washed for 30 minutes in a 1 molar solution of sodium chloride to fix the -~
polyethyleneimine and subsequently washed thoroughly in distilled water to remove all the sodium chloride from the reactor discs.
This required four washings, 50 ml and 10 minutes each. The reactor discs next were soaked in 50 cc of a 10% aqueous solution of glutaraldehyde at pH 9 and agitated frequently to ensure uniform pene-tration of the discs by the glutaraldehyde. After incubation in the glutaraldehyde, the discs were thoroughly washed in distilled water using four 50 ml washings for 10 minutes each. ~lucose oxidase (1270 units/ml) was diluted 50/50 with phosphate buffer (0.1 molar, pH 6). The resultilng solution (50 cc) was adjusted to pH 6 with dilute sodium hydroxide and the discs of Reactors Nos. 1, 2, and 3 were incubated in this solu-tion for 30 minutes. After the 30 minute incubation, the reactor discs were removed and thoroughly washed with distilled water to :; :
~073382 .
remove free enzyme from the porous material, leaving behind only the immobilized enzyme.
Each of the above three reactors were assayed f'or activity by conversion of ~-D-glucose to D-gluconolactone and monitoring the hydrogen peroxide concentration in the ef`fluent stream. The substrate solution ( ~D-glucose, 0.15 millimolar in 0.1 molar potassium phosphate buffer at pH 6) was pumped through the reactors at varying flow rates and the effluent stream collected and assayed for hydrogen peroxide which is generated according to the e~uation:
1/202 + H20 + ~-D-glucose Glucose Oxidase H202 + D-gluconolactone Into the analyzer cuvet-te is added 25 microlitres of the peroxi-dase solution (10 mg/5 ml in potassium phosphate buffer at pH 6) and 50 microlitres of reduced O-Dianisideine solution (2% in methanol). The cuvette is filled with the reactor effluent, agitated, and analyzed on a Bausch & Lomb Spectronic 20 at 460 millimicrons for optical density versus a blank standard. The observed results are summarized as follows:
Reactor No. 1 Minimum enzyme activity was exhibited by this reactor. The activity that did exist was readily washed out as the glucose solution was pumped through the reactor indica-ting that the enzyme was not bound to the media but rather trapped within the pores.
Reactor No. 2 This reactor exhibited good activity on the first day being almost as active as the control (Reactor No. 3) when normalized for silica content of the material. At a flow rate of 0.5 cc/min.
through a 1 centimetre diameter area, the disc showed an activity ~' ! , ' . 'i , ". ' ' ' ' " , ' ' : ~7,338Z
:.
of 0.65 units/gram of material. The activity seemed to drop off slightly on the second day but this was not quantified.
Reactor No~ 3 This reactor exhibited good activity and revealed a constant reaction rate both days. At 0.5 cc/min. flow rate through a 1 centimetre diameter area the disc showed an activity of 1.8 units/gram of material.
It will be noted that the activity of Reactor No. 2 was approximately half that of Reactor No. 3 and also, that the material of Reactor No. 2 contained roughly half the silica filler of Reactor No. 3. This indicates that the filler (silica) constituent in the microporous material constitutes the primary . :
binding species for the immobilized enzyme rather than the surrounding matrix, such as hard rubber or polyvinyl chloride, -for example.
Although certain of the foregoing Examples illustrate the immobilized enzyme system of the present invention in the -form of a so called stacked-disc or flow-through reactor, it will be appreciated that many other forms of reactors may be employed as well. For example, the microporous starting material may be formed into the shape of a hollow tube, and treated in the manner disclosed above to bond or attach catalytically active enzymes thereto. A substratemay then be caused to flow into the tube at one end, be enzymatically reacted upon as it ~lows along and comes into contact with the inner wall of the tube, and the resulting product caused -to flow out of the tube at its other end.
Similarly, in cases where the substrate has a relatively high viscosity, or it is otherwise desirable to utilize a lQ~3382 packed-bed, f]uidized-bed, or stirred tan~ type o~ reactor, ~or example, sheets of microporous st~rting material may have enzymes bound thereto and immobilized as above with the resulting sheets being subsequently cut-up or divided into small pieces of practically any desired siæe (e.g., pieces, granules, beads, powders, and so on). The resu:Lting divided immobilized ; enzyme particles may -then be utilized by those skilled ln the art in applications requiring such forms of immobilized enzyme carrier.
10Finally, as will be understood further, the immobiliza-tion principles of the present invention are applicable to proteinaceous substances other than enzymes, such as antibodies or antigens, for example. Accordingly, the present invention should be limited only by the true scope o the appended claims.
-35~
., ~ . . ,, , ,~ "
Claims (33)
1. An insoluble composite comprising a microporous member having at least a pair of opposed surfaces and a predetermined thickness, said microporous member comprising a polymeric resinous binder having finely divided filler particles dispersed throughout said binder and a network of substantially interconnected pores formed therein, said pores being formed within said resinous binder, between said filler particles and said resinous binder, and between neighboring filler particles, said dispersed filler par-ticles being present in said microporous member in an amount by weight of at least about 25%, the size distribution of said pores varying non-uniformly across each of said sur-faces and across said predetermined thickness through the range of about 0.01 micron to about 100 microns as deter-mined porosimetrically by the Mercury Intrusion Method, and a proteinaceous substance bound to at least some of said filler particles dispersed throughout said binder, said microporous member being pervious to the flow of a fluid through at least one of said surfaces wherein at least some of said filler particles to which said proteinaceous substance is bound is adapted to come into contact with such fluid.
2. The composite of claim 1, wherein said dis-persed filler particles comprise silicious material.
3. The composite of claim 1, wherein said binder comprises polyvinyl chloride.
4. The composite of claim 1, wherein said binder comprises hard rubber.
5. The composite of claim 1, wherein said protein-aceous substance is a catalytically active enzyme.
6. The composite of claim 5, wherein said cata-lytically active enzyme is chemically bound to said at least some of said dispersed filler particles through an intermediate coupling agent.
7. The composite of claim 6, wherein said intermedi-ate coupling agent is covalently bonded to said filler particles and said catalytically active enzyme is covalently bonded or crosslinked to said intermediate coupling agent.
8. The composite of claim 6, wherein said inter-mediate coupling agent is chemiadsorbed to the surface of said at least some of said dispersed filler particles and said catalytically active enzyme is covalently bonded or cross-linked to said intermediate coupling agent.
9. The composite of claim 5, wherein said enzyme is glucose oxidase.
10. The composite of claim 5, wherein said enzyme is aldose-l-epimerase.
11. The composite of claim 5, wherein said enzyme is .alpha.-D-fructofuranosidase.
12. The composite of claim 5, wherein said enzyme is alcohol dehydrogenase.
13. The composite of claim 5, wherein said enzyme is glucose isomerase.
14. The composite of claim 1, wherein said finely divided filler particles comprise inorganic material.
15. The method of carrying out a chemical process comprising the steps of reacting a substrate by placing the substrate in contact with an insoluble microporous member having a proteinaceous substance which reacts with said substrate bonded thereto, and recovering a product of the reaction, said insoluble microporous member having at least a pair of opposed surfaces and a predetermined thickness, said microporous member comprising a polymeric resinous binder having finely divided filler particles dispersed throughout said binder and a network of substan-tially interconnected pores formed therein, said pores being formed within said resinous binder, between said filler particles and said resinous binder, and between neighboring filler particles, said dispersed filler par-ticles being present in said microporous member in an amount by weight of at least about 25%, the size distribu-tion of said pores varying non-uniformly across each of said surfaces and across each of said predetermined thickness through the range of about 0.01 micron to about 100 microns as determined porosimetrically by the Mercury Intrusion Method, and a proteinaceous substance bound to at least some of said filler particles dispersed throughout said binder, said microporous member being pervious to the flow of said sub-strate through at least one of said surfaces.
16. The method of claim 15, wherein said micro-porous member is in the form of a reactor core comprising a sheet having said at least pair of opposed surfaces ex-tending substantially parallel to one another, and said step of reacting a substrate comprises passing said sub-strate through said sheet in a direction substantially normal to said parallel surfaces.
17. The method of claim 15, wherein said microporous member is in the form of a reactor core comprising a hollow tube having an inlet end and an outlet end, said step of enzymatically reacting a substrate comprises passing said substrate through said inlet end to contact the interior surface of said tube, and said product being recovered through said outlet end of said tube.
18. The method of claim 15, wherein said microporous member is in the form of a plurality of divided particles, and said step of enzymatically reacting a substrate com-prises contacting said substrate with a plurality of said divided particles.
19. The method of claim 15, wherein said filler particles comprise inorganic material.
20. A method of immobilizing proteinaceous sub stances comprising the steps of providing an insoluble microporous member, having at least a pair of opposed surfaces and a predetermined thickness, said microporous member comprising a polymeric resinous binder having finely divided filler particles dispersed throughout said binder and a network of substantially interconnected pores formed therein, said pores being formed within said resinous binder, between said filler particles and said resinous binder, and between neighboring filler particles, said dispersed filler particles being present in said microporous member in an amount by weight of at least about 25%, the size distribution of said pores varying non-uniformly across each of said surfaces and across said pre-determined thickness through the range of about 0.01 micron to about 100 microns as determined porosimetrically by the Mercury Intrusion Method, and bonding a proteinaceous substance to the surface of at least some of said plurality of dispersed filler particles, said microporous member being pervious to the flow of a fluid through at least one of said surfaces wherein at least some of said filler particles to which said proteinaceous substance is bound is adapted to come into contact with said fluid.
21. The method of claim 20, wherein said proteinaceous substance is a catalytically active enzyme.
22. The method of claim 21, wherein said catalytically active enzyme is chemically bound to said surface of said filler particles by treating said support member with an intermediate coupling agent to form organic functional groups covalently bonded to said surface, and said treated support member is exposed to a solution including said enzyme to covalently bond said enzyme to said organic functional groups on the surface of said filler particles.
23. The method of claim 22, wherein said treated support member is exposed to a cross-linking agent prior to being exposed to said enzyme solution.
24. The method of claim 22, wherein said treated support member is exposed simultaneously to said enzyme solution and a cross-linking agent.
25. The method of claim 22, wherein said intermediate coupling agent is an organosilane.
26. The method of claim 25, wherein said organosilane is gamma-aminopropyltriethoxysilane.
27. The method of claim 23 or 24, wherein said intermediate coupling agent is a gamma-aminopropyltriethoxy-silane and said cross-linking agent is glutaraldehyde.
28. The method of claim 21, wherein said catalyti-cally active enzyme is chemically bound to said surface of said filler particles by treating said support member with an intermediate coupling agent to form organic func-tional groups chemiadsorbed to said surface, and said treated support member is exposed to a solution including said enzyme to covalently bond said enzyme to said organic functional groups on the surface of said filler particles.
29. The method of claim 28, wherein said treated support member is exposed to a cross-linking agent prior to being exposed to said enzyme solution.
30. The method of claim 28, wherein said treated support member is exposed simultaneously to said enzyme solution and a cross-linking agent.
31. The method of claim 28, wherein said inter-mediate coupling agent is a polyelectrolyte.
32. The method of claim 31, wherein said poly-electrolyte is polyethelenimine.
33. The method of claim 29 or 30, wherein said intermediate coupling agent is polyethelenimine and said cross-linking agent is glutaraldehyde.
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US60907775A | 1975-08-29 | 1975-08-29 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA1073382A true CA1073382A (en) | 1980-03-11 |
Family
ID=24439269
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA260,069A Expired CA1073382A (en) | 1975-08-29 | 1976-08-27 | Immobilized proteins and method of preparing same |
Country Status (9)
| Country | Link |
|---|---|
| US (1) | US4102746A (en) |
| JP (1) | JPS6029474B2 (en) |
| BR (1) | BR7605647A (en) |
| CA (1) | CA1073382A (en) |
| DE (1) | DE2639234C2 (en) |
| DK (1) | DK149312C (en) |
| FR (1) | FR2322156A1 (en) |
| GB (1) | GB1550128A (en) |
| IT (1) | IT1075203B (en) |
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| US4251631A (en) * | 1978-02-23 | 1981-02-17 | Research Products Rehovot Ltd. | Cross-linked enzyme membrane |
| US4343901A (en) * | 1980-10-22 | 1982-08-10 | Uop Inc. | Magnetic support matrix for enzyme immobilization |
| DE3130924A1 (en) * | 1981-08-05 | 1983-02-17 | Röhm GmbH, 6100 Darmstadt | SURFACE-BASED SYSTEMS FOR FIXING SUBSTRATES CONTAINING NUCLEOPHILE GROUPS |
| US4557900A (en) * | 1982-09-28 | 1985-12-10 | Cardiovascular Devices, Inc. | Optical sensor with beads |
| US4474879A (en) * | 1982-11-16 | 1984-10-02 | Eli Lilly And Company | Process for 3-hydroxymethyl cephalosporin sulfones |
| US4663163A (en) * | 1983-02-14 | 1987-05-05 | Hou Kenneth C | Modified polysaccharide supports |
| AU580548B2 (en) * | 1983-02-14 | 1989-01-19 | Cuno Incorporated | Polymer modified polysaccharide |
| DK317483D0 (en) * | 1983-07-08 | 1983-07-08 | Superfos As | IMMOBILIZED ENZYME PREPARATION AND PROCEDURES FOR PRODUCING THEREOF |
| US4724207A (en) * | 1984-02-02 | 1988-02-09 | Cuno Incorporated | Modified siliceous chromatographic supports |
| US4687820A (en) * | 1984-08-22 | 1987-08-18 | Cuno Incorporated | Modified polypeptide supports |
| DE3662830D1 (en) | 1985-01-30 | 1989-05-24 | Kao Corp | A fastener tape for disposable diaper |
| US4861714A (en) * | 1985-04-04 | 1989-08-29 | Verax Corporation | Weighted collagen microsponge for immobilizing bioactive material |
| US5100783A (en) * | 1985-05-10 | 1992-03-31 | Verax Corporation | Weighted microsponge for immobilizing bioactive material |
| WO1987000199A1 (en) * | 1985-07-10 | 1987-01-15 | Clyde Robert A | Process and apparatus for enhancing biological and chemical reactions from high area inorganic base silica on fibers |
| US4861644A (en) * | 1987-04-24 | 1989-08-29 | Ppg Industries, Inc. | Printed microporous material |
| US4833172A (en) * | 1987-04-24 | 1989-05-23 | Ppg Industries, Inc. | Stretched microporous material |
| US4927802A (en) * | 1988-12-09 | 1990-05-22 | Ppg Industries, Inc. | Pressure-sensitive multi-part record unit |
| US5019270A (en) * | 1989-07-06 | 1991-05-28 | Perseptive Biosystems, Inc. | Perfusive chromatography |
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|---|---|---|---|---|
| US2772322A (en) * | 1953-08-05 | 1956-11-27 | Us Rubber Co | Microporous vinyl chloride resin and method of making same |
| GB954202A (en) | 1959-06-08 | 1964-04-02 | Electric Storage Battery Co | Microporous thermoplastic material |
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| US3696061A (en) * | 1970-04-13 | 1972-10-03 | Amerace Esna Corp | Method for forming flowable powder processable into microporous object |
| US3791927A (en) * | 1971-07-14 | 1974-02-12 | American Cyanamid Co | Entrapped carrier bound enzymes |
| US3766013A (en) * | 1971-08-24 | 1973-10-16 | American Cyanamid Co | Preparation of water-insoluble carrier bound enzymes |
| US3862030A (en) * | 1972-12-13 | 1975-01-21 | Amerace Esna Corp | Microporous sub-micron filter media |
-
1976
- 1976-08-16 US US05/714,291 patent/US4102746A/en not_active Expired - Lifetime
- 1976-08-17 GB GB34237/76A patent/GB1550128A/en not_active Expired
- 1976-08-26 IT IT51030/76A patent/IT1075203B/en active
- 1976-08-27 DE DE2639234A patent/DE2639234C2/en not_active Expired
- 1976-08-27 DK DK389376A patent/DK149312C/en not_active IP Right Cessation
- 1976-08-27 CA CA260,069A patent/CA1073382A/en not_active Expired
- 1976-08-27 BR BR7605647A patent/BR7605647A/en unknown
- 1976-08-30 JP JP51102726A patent/JPS6029474B2/en not_active Expired
- 1976-08-30 FR FR7626168A patent/FR2322156A1/en active Granted
Also Published As
| Publication number | Publication date |
|---|---|
| DE2639234A1 (en) | 1977-03-10 |
| DK149312B (en) | 1986-04-28 |
| FR2322156B1 (en) | 1981-12-11 |
| JPS5234978A (en) | 1977-03-17 |
| IT1075203B (en) | 1985-04-22 |
| BR7605647A (en) | 1977-08-09 |
| DE2639234C2 (en) | 1984-04-12 |
| DK149312C (en) | 1986-09-15 |
| US4102746A (en) | 1978-07-25 |
| DK389376A (en) | 1977-03-01 |
| FR2322156A1 (en) | 1977-03-25 |
| GB1550128A (en) | 1979-08-08 |
| JPS6029474B2 (en) | 1985-07-10 |
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