GB2122621A - Enhanced immobilization of glucose isomerase - Google Patents

Enhanced immobilization of glucose isomerase Download PDF

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GB2122621A
GB2122621A GB08218483A GB8218483A GB2122621A GB 2122621 A GB2122621 A GB 2122621A GB 08218483 A GB08218483 A GB 08218483A GB 8218483 A GB8218483 A GB 8218483A GB 2122621 A GB2122621 A GB 2122621A
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magnesium
support matrix
glucose isomerase
solution
matrix
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John Russell Teague
Aronson Leonard Huebner
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Honeywell UOP LLC
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N11/00Carrier-bound or immobilised enzymes; Carrier-bound or immobilised microbial cells; Preparation thereof
    • C12N11/14Enzymes or microbial cells immobilised on or in an inorganic carrier

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  • Immobilizing And Processing Of Enzymes And Microorganisms (AREA)

Abstract

The immobilization of glucose isomerase onto a support matrix is enhanced by pretreating the support matrix with divalent magnesium ions. In one embodiment, the support matrix is an inorganic oxide impregnated with a polyamine which is subsequently cross-linked with an excess of a bifunctional reagent so as to furnish a plurality of pendant function groups, and the wash solution is magnesium sulfate.

Description

SPECIFICATION Enhanced immobilization of glucose isomerase This invention relates to a method of enhancing the subsequent immobilization of glucose isomerase onto a support matrix and to a method of preparing an immobilized glucose isomerase.
Enzyme-catalyzed reactions have the advantages of proceeding with great chemical specificity under relatively mild conditions, and often accomplish what man finds difficult, if not impossible, to duplicate in the laboratory. For such reasons there is increasing emphasis on the use of enzymatic processes on a commercial scale. One example, of many which could be cited, is the conversion of glucose to fructose using glucose isomerase.
Enzymes are water soluble, and if they are merely used in aqueous solutions recovery of enzymes for reuse is difficult and expensive. Using the enzyme only once affords a process which is relatively expensive. Consequently, many techniques have been developed for immobilizing the enzyme in such a way that substantial enzymatic activity is displayed while the enzyme itself remains rigidly attached to some water-insoluble support, thereby permitting reuse of the enzyme over substantial periods of time and for substantial amounts of feedstock. One illustration of a method for immobilizing an enzyme is found in U.S.Patent No. 4,141,857, where a polyamine is absorbed on a metal oxide such as alumina, treated with an excess of a bifunctional reagent, such as glutaraldehyde, so as to cross-link the amine, and then contacting the mass with enzyme to form covalent bonds between the pendant aldehyde groups and an amino group on the enzyme. The support matrix prepared according to the aforementioned invention has great utility in immobilizing reactive chemical entities, enzymes being but one class of such reactive chemical entities.
Generally, immobilized enzyme systems are prepared by contacting a suitable solution containing -the enzyme with the support matrix, removing the excess of enzyme solution, and recovering the resulting immobilized enzyme system. Because of the relatively high cost of enzymes, it is highly desirable to maximize enzyme utilization. Among the identifiable characteristics measuring enzyme utilization in an immobilized enzyme system are included the activity and half life of the immobilized enzyme system, and the coupling efficiency of the enzyme to the support matrix. A discovery leading to the present invention is that pretreatment of a support matrix with a source of divalent magnesium ions enhances the utilization and immobilization of glucose isomerase.
According to one aspect of the present invention, a method of enhancing the subsequent immobilization of glucose isomerase on a support matrix comprises impregnating the matrix, prior to contact with said glucose isomerase, with at least 0.1 millimoles of divalent magnesium ions per g of support matrix, and recovering the resulting magnesium impregnated support matrix.
According to a further aspect of the present invention, a method of preparing immobilized glu cose isomerase comprises impregnating a porous refractory inorganic oxide with a polyamine, contact ing the impregnated inorganic oxide with an excess of a bifunctional reagent so as to cross-link the polyamine and furnish a plurality of pendantfunctional groups, removing the excess of said bifunctional reagents, impregnating the resulting support matrix with at least 0.1 millimoles divalent magne sium ion per g support matrix, contacting the magnesium impregnated support matrix with a solution containing glucose isomerase at a temperature of from 0 C. to 70"C. until immobilization is complete, and recovering the resulting immobilized glucose isomerase.
According to a still further aspect of the present invention, a method of preparing an immobilized glucose isomerase comprises impregnating a porous refractory inorganic oxide with a polyamine, contacting the impregnated inorganic oxide with a solution comprising an excess of a bifunctional reagent and divalent magnesium ions so as to cross-linkthe polyamine and furnish a plurality of pendant functional groups while impregnating the resulting support matrix with magnesium ions, removing the excess of said solution, contacting the resulting support matrix with a solution containing glucose isomerase at a temperature of from 0 C. to 70"C. until immobilization is complete, and recovering the resulting immobilized glucose isomerase.
An immobilized enzyme system consists of a support matrix on which there is bound an enzyme.
A support matrix is a structure characterized as having good physical integrity and favorable properties toward liquid flow under conditions experienced in fixed bed reactors, and further characterized by having the ability to bind or immobilize enzymes with minimum perturbation of enzymatic action. By an immobilized enzyme system is meant the structure which results from immobilization of an enzyme on a support matrix.
The binding or immobilization of enzymes to support matrices is represented by the extremes of physical and chemical binding forces. It is to be recognized that in most cases enzyme immobilization arises from a combination of such binding forces, although often one such force predominates.
The nature of enzyme immobilization generally is determined by the nature of the support matrix. As an example, when the support matrix is a resin, such as one of the phenol formaldehyde type, binding is predominantly through physical forces. A similar result is obtained when the support matrix is of an ion exchange type. Where the support matrix is comprised of refractory inorganic material, such as inorganic oxides, glass, and ceramics, bearing or impregnated with organic material, for example, polyamines, either bearing pendant functional groups themselves or cross-linked with a bifunctional reagent which provides pendant functional groups, enzyme immobilization arises mainly by chemical reaction of a site on the enzyme with the pendant functional group so as to form a covalent bond. In such an instance binding is, at least predominantly, by chemical means.
It is a discovery of this invention that impregnating the support matrix with divalent magnesium ions, such as by contacting the support matrix with a solution furnishing divalent magnesium ions, enhances subsequent immobilization of glucose isomerase onto the support matrix, the enhancement being manifested primarily by an increased half life of the immobilized glucose isomerase.
Additionally, pretreatment may result in a decreased time for immobilization of glucose isomerase. It is apparent that manifestation of increased half life is highly advantageous and leads to a substantial improvement in an immobilized glucose isomerase system.
The method of this invention is applicable to all support matrices, regardless of their nature. It is especially applicable to support matrices comprised of porous, refractory inorganic oxides, such as alumina, thoria, magnesia, silica, and combinations thereof, glass, or ceramics bearing or impregnated with a polyamine reacted with an excess of a bifunctional reagent so as to cross-link the polyamine and furnish a plurality of functional groups pendant to the formed polymer. Among the suitable polyamines are included materials such as polyethyleneimine, polypropyleneimine, tet raethylenepentamine, ethylenediamine, diethylenet riamine, triethylenetetramine, pentaethylenehexamine, hexamethylenediamine, phenylenediamine, and amino(polystyrene), with polyethyleneimine being an especially preferred polyamine.Among the bifunctional reagents used are glutaraldehyde, succindialdehyde, terephthaldehyde, and toluenediisocyanate, glutaraldehyde often being the bifunctional reagent of choice.
Briefly described, the invention herein comprises impregnating a support matrix with divalent magnesium ions, such as by contacting a support matrix with a solution furnishing divalent magnesium ions, removing the excess of said solution, and recovering the resulting magnesium impregnated support mat rix. This impregnation of the support matrix with divalent magnesium ions is performed prior to immobilization of glucose isomerase thereon. By "priorto" is meantthatsuch impregnation is a process stage performed before immobilization of the enzyme. It is preferred that the impregnation is performed immediately prior to immobilization, in the context of a process stage and in the context of time.However, it is to be understood that such impregnation may occur earlier, in both contexts, so long as subsequent events do not leach out or otherwise substantially decrease the amount of impregnated magnesium ion.
As stated above, the support matrix is impre gnated with divalent magnesium ions by contacting said matrix with a solution containing a source of magnesium ion. Inorganic and organic salts are a convenient source of magnesium ion, and their nature is not critical to the success of this invention so long as they are unreactive toward the support matrix and do not interfere with the activity of the subsequently bound enzyme. Among the salts which may be used are the magnesium halides, such as magnesium chloride, bromide, and iodide, magnesium sulfate, magnesium nitrate, magnesium hypophosphite, magnesium fluorosilicate, magnesium acetate and magnesium lactate. Magnesium sulfate frequently is preferred because of its great solubility and relatively low cost.
The concentration of divalent magnesium ion in the contacting solution is not critical, and at least the upper limit may be dictated by the solubility of the source of the divalent magnesium ions. Concentrations from 1 to 25 millimolar in magnesium ion have been found convenient to use, although both higher and lower concentrations are not necessarily deleterious to the practice of this invention.
Of far greater significance is the total amount of divalent magnesium ion impregnated per gram of support matrix. This amount may depend on the type of support matrix used, the temperature of contacting, and the constitution of the enzyme solution offered, among other factors. In general, where the support matrix has not been prior contacted with divalent magnesium ion, or does not independently contain divalent magnesium ion, the support matrix should be impregnated with at least 0.1 millimoles of divalent magnesium ion per gram of support matrix. In a preferred embodiment the support matrix is impregnated with divalent magnesium ion in an amount from 0.1 to 2 millimoles ion per gram of support matrix.There does not seem to be an upper limit to the amount of magnesium ion impregnation which is necessaryforthe practice of this invention, but further increase in impregnation does not necessarily lead to further increments in advantageous effect.
The contact time will depend on such things as the concentration of magnesium in the solution, the support matrix used, and the relative amounts of solution and support matrix. For example, where the support matrix is of the cross-linked polyamine type, and the solution is a 5 millimolar magnesium sulfate solution, and contacting is performed by passing the solution over a bed of the support matrix at a rate such that there is 1 bed volume about every 4 minutes, then equilibrium is attained after about7 to 8 bed volumes have been passed. Generally, a sufficiently large excess of solution is used so that equilibrium may be attained in from about 15 to 30 minutes. By equilibrium is meant that state in'which the support matrix no longer takes up magnesium from the contacting solution.
The method of this invention is practiced as follows. A solution is prepared from material furnishing a source of divalent magnesium ion. As mentioned previously, inorganic and organic salts of magnesium are the most convenient source of magnesium ions. The support matrix is then contacted with this solution for a sufficient time to ensure attainment of equilibrium in impregnation of magnesium ion. The temperature does not seem to have an important effect; contacting may be performed from about 0 C. to about 90 C., and generally is performed at ambient temperature. Such contacting may be as a batch operation, where the support matrix and the solution are mixed at least intermittently. Alternatively, the solution may be passed through a fixed bed of the support matrix.Other variations, where contacting is done by fluidized bed, expanded bed, and the like, will be recognized by the skilled artisan.
The practice of this invention is not limited to a particular type of support matrix. In a preferred embodiment, the support matrix is an inorganic oxide impregnated with a polyamine subsequently cross-linked with an excess of a bifunctional reagent so as to furnish a plurality of pendant functional groups. For example, an inorganic oxide, such as gamma alumina, may be contacted with an aqueous solution of a polyamine, such as polyethyleneimine, where the polyamine is present at a concentration from about 1% to about 50%. Excess liquid is removed by suitable means, as by decantation. The oxide may be washed with water to remove excess polyamine, but it is preferred to merely dry the material by evaporation of the water.An aqueous solution of cross-linking agent, such as glutaraldehyde, containing from about 1% to about 25% of the bifunctional reagent is added in an amount sufficient to provide an excess of from about 3 to about 50 or more moles of said bifunctional reagent per mole of polyamine. This solution is contacted, with occasional mixing, with the polyamine-coated oxide for a time sufficient to ensure equilibrium, generally from about 5 minutes to about 5 hours. Liquid is then removed from the oxide support by suitable means, such as by decantation, and the solid support is washed well with water to remove adhering, but not chemically bound, bifunctional reagent.
Where the preferred support matrix is utilized, magnesium impregnation may be performed as described above. However, a variant comprises incorporating a source furnishing divalent magnesium ions into the solution of bifunctional reagent, so that cross-linking, furnishing of a plurality of pendant functional groups, and impregnation with magnesium ion are carried out concurrently.
The immobilized enzyme system such as a glucose isomerase enzyme system may be prepared by contacting the magnesium impregnated support matrix with a solution containing glucose isomerase at a temperature from about 0 C. to about 70 C. for a time sufficient to ensure complete immobilization.
Contacting may be performed by intermittent mixing when the operation is done in a batch mode.
Alternately, contacting may be done by passing the enzyme solution through a fixed orfluidized bed of the support matrix. Immobilization by other means, such as by an expanded bed, will be apparent to those skilled in the art and such alternate means are intended to be encompassed herein. Immobilization generally is complete within about 30 hours, depending upon the temperature, the immobilization procedure, concentration of enzyme in the offering solution, support matrix, and so forth. After immobilization is complete adhering but unbound enzyme is removed by washing the system with, for example, de-ionized water, a solution of strong electrolyte, or feedstock.
The invention will now be described by way of example with reference to the following nonlimitative Examples.
Example 1 A support matrix was prepared in the following way. Alumina, 400 g of 60/80 mesh, ABD 0.3, was mixed with a 1.5% by weight solution of polyethyleneimine in water in an amount sufficient to yield 0.117 g polyamine per g alumina. After thorough mixing, water was evaporated and the polyamine-impregnated alumina was loaded into a glass column of 5 cm internal diameter.
An aqueous solution of glutaraldehyde, 2.5% by weight, 8 1 total volume, was circulated upflow at 40 ml per minute for 18 minutes, then recycled downflow at 400 ml per minute for 60 minutes. The bed was then washed with deionized water circulating downflow at 400 ml per minute for 4 hours 40 minutes to thoroughly remove excess glutaraldehyde. At the end of this wash the effluent gives a negative fuchsin aldehyde test. The support matrix so prepared is in a state ready for immobilization of enzyme and is relatively free of magnesium.
Example 2 An immobilized glucose isomerase system was prepared from the magnesium-free support matrix prepared as described in Example 1 in the following way. A total of 8.5 1 of an aqueous solution at 60"C.
containing 3500 units glucose isomerase per g support matrix was recycled upflowthrough a bed of support matrix from 400 g alumina for 25 minutes at 400 ml per minute. Flow was then reversed and the enzyme solution was recycled downflow for 23 hours. Excess adhering but unbound enzyme was removed by washing with a salt solution, prepared by dissolving 12 g magnesium sulfate and 20 g sodium sulfite in 20 1 deionized water, by washing the bed with 6 1 of this solution downflow at 400 ml per minute for 15 minutes. The column was further washed with 41 of salt solution recycled flow for 30 minutes at 400 ml per minute, after which this solution was discarded, and the wash procedure was repeated three more times until the entire salt solution was used.
Example 3 A magnesium impregnated matrix was prepared by first preparing a magnesium-free support matrix as described in Example 1.
The matrix was then contacted with a solution of magnesium salt. For example, the matrix was loaded into a glass column of 5 cm internal diameter and a solution of 0.005 M magnesium sulfate was circulated downflow at 400 ml per minute for 4 hours 40 minutes. After about 30 minutes very little additional magnesium was deposited on the matrix, as shown by the effluent magnesium level being about the same as the initial solution. The resulting support matrix contained 0.13 m moles magnesium per g of support matrix.
When higher concentrations of magnesium sulfate were used in the wash solution, higher levels of magnesium impregnation were obtained. For example, using a 0.010 M magnesium sulfate solution afforded a matrix containing 1.3 m moles magnesium per g support matrix.
Example 4 An immobilized glucose isomerase system was prepared from the support matrix impregnated with 0.13 m moles magnesium per g matrix, prepared as described in Example 3, in the following way. A total of 8.51 of an aqueous solution at 60"C. containing 3500 units glucose isomerase per g support matrix was recycled upflow through a bed of support matrix from 400 g alumina for 25 minutes at 400 ml per minute. Flow was then reversed and the enzyme solution was recycled downflow for 23 hours. Excess adhering but unbound enzyme was removed by washing with a salt solution, prepared by dissolving 12 g magnesium sulfate and 20 g sodium sulfite in 20 I deionized water, by washing the bed with 61 of this solution downflow at 400 ml per minute for 15 minutes.The column was further washed with 41 of salt solution recycled upflow for 30 minutes at 400 ml per minute, after which this solution was discarded, and the wash procedure was repeated three more times until the entire salt solution was used.
The magnesium-free immobilized glucose isomerase system prepared as described in Example 2 and the magnesium impregnated immobilized glucose isomerase system prepared as described in Example 4were used as fixed bed reactors for the conversion of glucose to fructose. The feedstock was Cerelose feed at 45% by weight dry solids, and conversions were performed at 600C. under nitrogen and pH 8.0 8.3 to a level of 42% fructose in the effluent. Initial activities for both systems were 2000 - 2100 units per g. The half life for the magnesium-free system was 58 days, whereas that for the system impregnated with 0.13 m mole magnesium ion per g support matrix was 78 days. Thus it is seen that magnesium impregnation atthis level increases the half life of the immobilized glucose isomerase system by over 34%.

Claims (27)

1. A method of enhancing the subsequent immobilization of glucose isomerase onto a support matrix comprising impregnating said matrix, prior to contact with said glucose isomerase, with at least 0.1 millimoles divalent magnesium ion per g of support matrix, and recovering the resulting magnesium impregnated support matrix.
2. A method as claimed in claim 1 wherein the impregnation of said matrix is effected essentially by contacting said matrix with a solution furnishing divalent magnesium ions, and removing the excess of said solution.
3. A method as claimed in claim 2 wherein the solution furnishing divalent magnesium ions is a solution of an inorganic or organic salt of divalent magnesium.
4. A method as claimed in claim 3 wherein said salt is selected from the group consisting of magnesium halides, magnesium sulfate, magnesium nitrate, magnesium hypophosphite, magnesium fluorosilicate, magnesium acetate and magnesium lactate.
5. A method as claimed in claim 4 wherein said salt is magnesium sulfate.
6. A method as claimed in any of claims 2 to 5 wherein the solution is from 1 to 25 millimolar in divalent magnesium ion.
7. A method as claimed in any of the preceding claims wherein the support matrix is impregnated with from 0.1 to 2 millimoles of divalent magnesium ion per g of support matrix.
8. A method as claimed in any of the preceding claims wherein the support matrix is an inorganic oxide impregnated with a polyamine cross-linked with an excess of a bifunctional reagent so as to furnish a plurality of pendant functional groups.
9. A method of enhancing the subsequent immobilization of glucose isomerase onto a support matrix substantially as described in the foregoing Example 3.
10. A magnesium impregnated support matrix prepared by a method as claimed in any of the preceding claims.
11. A method of preparing immobilized glucose isomerase comprising: a) impregnating a porous refractory inorganic oxide with a polyamine; b) contacting the impregnated inorganic oxide with an excess of a bifunctional reagent so as to cross-linkthe polyamine and furnish a plurality of pendant functional groups; c) removing the excess of said bifunctional reagent; d) impregnating the resulting support matrix with at least 0.1 millimoles divalent magnesium ion per g support matrix; e) contacting the magnesium impregnated support matrix with a solution containing glucose isomerase at a temperature from 0 C. to 70"C. until immobilization is complete; and f) recovering the resulting immobilized glucose isomerase.
12. A method of preparing an immobilized glucose isomerase comprising: a) impregnating a porous refractory inorganic oxide with a polyamine; b) contacting the impregnated inorganic oxide with a solution comprising an excess of a bifunctional reagent and divalent magnesium ions so as to cross-link the polyamine and furnish a plurality of pendant functional groups while impregnating the resulting support matrix with magnesium ions; c) removing the excess of said solution; d) contacting the resulting support matrix with a solution containing glucose isomerase at a temperature from 0 C. to 70"C. until immobilization is complete; e) and recovering the resulting immobilized glucose isomerase.
13. A method as claimed in claim 11 wherein the impregnation of said matrix consists essentially of contacting said matrix with a solution furnishing divalent magnesium ions, and removing the excess of said solution.
14. A method as claimed in any of claims 11 to 13 wherein the inorganic oxide is selected from the group consisting of alumina, thoria, magnesia, silica and combinations thereof.
15. A method as claimed in any of claims 11 to 14 wherein the polyamine is selected from the group consisting of polyethyleneimine, polypropyleneimine, tetraethylenepentamine, ethylenediamine, diethylenetriamine, triethylenetetramine, pentaethylenehexamine, hexamethylenediamine, phenylenediamine and amino(polystyrene).
16. A method as claimed in any of claims 11 to 15 wherein the bifunctional reagent is selected from the group consisting of glutaraldehyde, succindialdehyde, terephthaldehyde and toluenediisocyanate.
17. A method as claimed in claim 12, 13 or 17, or any of claims 14 to 16 when dependent upon claim 12 or 13, wherein the solution furnishing divalent magnesium ions is a solution of an inorganic or organic salt of divalent magnesium.
18. A method as claimed in claim 17 wherein said salt is selected from the group consisting of magnesium halides, magnesium sulfate, magnesium nitrate, magnesium hypophosphite, magnesium fluorosilicate, magnesium acetate and magnesium lactate.
19. A method as claimed in claim 18 wherein said salt is magnesium sulfate.
20. A method as claimed in any of claims 12, 13, 17,18Or19,oranyofclaims14to16when dependent upon claim 12 or 13, wherein the solution containing divalent magnesium ions is from 1 to 25 millimolar in divalent magnesium ion.
21. A method as claimed in any of claims 11 to 20 wherein the support matrix is impregnated with at least 0.13 millimoles divalent magnesium ion per g of support matrix.
22. A method of preparing an immobilized glucose isomerase system substantially as described in the foregoing Example 4.
23. An immobilized glucose isomerase system prepared by a method as claimed in any of claims 11 to 22.
24. An immobilized glucose isomerase system as claimed in claim 23 wherein the polyamine is polyethyleneimine.
25. An immobilized glucose isomerase system as claimed in claim 23 or 24 wherein the bifunctional reagent is glutaraldehyde.
26. A method of enhancing the subsequent immobilization of glucose isomerase onto a support matrix comprising contacting said matrix with a solution furnishing divalent magnesium ions, removing the excess of said solution, and recovering the resulting magnesium impregnated support matrix.
27. A method of preparing an immobilized glucose isomerase comprising preparing a magnesium impregnated support matrix as claimed in claim 26, contacting the magnesium impregnated support matrix with a solution containing glucose isomerase at a temperature of from 0 C. to 70"C. until immobilization is complete, and recovering the resulting immobilized glucose isomerase.
GB08218483A 1982-06-25 1982-06-25 Enhanced immobilization of glucose isomerase Expired GB2122621B (en)

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Cited By (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP0261836A1 (en) * 1986-09-17 1988-03-30 Beecham Group Plc Immobilised enzyme preparation and its use
US5283182A (en) * 1986-09-17 1994-02-01 Beecham Group Plc Preparation of immobilized hydantoinase stabilized with divalent metal ions

Citations (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
GB1346631A (en) * 1971-02-10 1974-02-13 Ranks Hovis Mcdougall Ltd Enzymes
GB1352739A (en) * 1971-09-01 1974-05-08 Aspro Nicholas Ltd Polymer-enzyme complexes
GB1454850A (en) * 1973-09-27 1976-11-03 Rhone Poulenc Sa Process for the enzymatic isomerisation of glucose to levulose
GB1598686A (en) * 1977-04-29 1981-09-23 Dia Prosim Enzymes immobilised on a resin via chelation with a metal

Patent Citations (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
GB1346631A (en) * 1971-02-10 1974-02-13 Ranks Hovis Mcdougall Ltd Enzymes
GB1352739A (en) * 1971-09-01 1974-05-08 Aspro Nicholas Ltd Polymer-enzyme complexes
GB1454850A (en) * 1973-09-27 1976-11-03 Rhone Poulenc Sa Process for the enzymatic isomerisation of glucose to levulose
GB1598686A (en) * 1977-04-29 1981-09-23 Dia Prosim Enzymes immobilised on a resin via chelation with a metal

Cited By (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP0261836A1 (en) * 1986-09-17 1988-03-30 Beecham Group Plc Immobilised enzyme preparation and its use
US5283182A (en) * 1986-09-17 1994-02-01 Beecham Group Plc Preparation of immobilized hydantoinase stabilized with divalent metal ions

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