AU2002331014A1 - Stabilized biocompatible membranes of block copolymers and fuel cells produced therewith - Google Patents

Stabilized biocompatible membranes of block copolymers and fuel cells produced therewith Download PDF

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AU2002331014A1
AU2002331014A1 AU2002331014A AU2002331014A AU2002331014A1 AU 2002331014 A1 AU2002331014 A1 AU 2002331014A1 AU 2002331014 A AU2002331014 A AU 2002331014A AU 2002331014 A AU2002331014 A AU 2002331014A AU 2002331014 A1 AU2002331014 A1 AU 2002331014A1
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polypeptide
biocompatible membrane
membrane
anode
synthetic polymer
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AU2002331014A
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Rosalyn Ritts
Hoi-Cheong Steve Sun
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PowerZyme Inc
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PowerZyme Inc
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Priority claimed from US10/123,008 external-priority patent/US20030087141A1/en
Priority claimed from US10/123,022 external-priority patent/US20030198859A1/en
Priority claimed from US10/213,477 external-priority patent/US20030049511A1/en
Application filed by PowerZyme Inc filed Critical PowerZyme Inc
Publication of AU2002331014A1 publication Critical patent/AU2002331014A1/en
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    • HELECTRICITY
    • H01ELECTRIC ELEMENTS
    • H01MPROCESSES OR MEANS, e.g. BATTERIES, FOR THE DIRECT CONVERSION OF CHEMICAL ENERGY INTO ELECTRICAL ENERGY
    • H01M8/00Fuel cells; Manufacture thereof
    • H01M8/10Fuel cells with solid electrolytes
    • H01M8/1016Fuel cells with solid electrolytes characterised by the electrolyte material
    • H01M8/1018Polymeric electrolyte materials
    • H01M8/102Polymeric electrolyte materials characterised by the chemical structure of the main chain of the ion-conducting polymer
    • H01M8/103Polymeric electrolyte materials characterised by the chemical structure of the main chain of the ion-conducting polymer having nitrogen, e.g. sulfonated polybenzimidazoles [S-PBI], polybenzimidazoles with phosphoric acid, sulfonated polyamides [S-PA] or sulfonated polyphosphazenes [S-PPh]
    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08JWORKING-UP; GENERAL PROCESSES OF COMPOUNDING; AFTER-TREATMENT NOT COVERED BY SUBCLASSES C08B, C08C, C08F, C08G or C08H
    • C08J5/00Manufacture of articles or shaped materials containing macromolecular substances
    • C08J5/20Manufacture of shaped structures of ion-exchange resins
    • C08J5/22Films, membranes or diaphragms
    • C08J5/2206Films, membranes or diaphragms based on organic and/or inorganic macromolecular compounds
    • C08J5/2218Synthetic macromolecular compounds
    • C08J5/2256Synthetic macromolecular compounds based on macromolecular compounds obtained by reactions other than those involving carbon-to-carbon bonds, e.g. obtained by polycondensation
    • HELECTRICITY
    • H01ELECTRIC ELEMENTS
    • H01MPROCESSES OR MEANS, e.g. BATTERIES, FOR THE DIRECT CONVERSION OF CHEMICAL ENERGY INTO ELECTRICAL ENERGY
    • H01M8/00Fuel cells; Manufacture thereof
    • H01M8/10Fuel cells with solid electrolytes
    • H01M8/1016Fuel cells with solid electrolytes characterised by the electrolyte material
    • H01M8/1018Polymeric electrolyte materials
    • H01M8/102Polymeric electrolyte materials characterised by the chemical structure of the main chain of the ion-conducting polymer
    • H01M8/1027Polymeric electrolyte materials characterised by the chemical structure of the main chain of the ion-conducting polymer having carbon, oxygen and other atoms, e.g. sulfonated polyethersulfones [S-PES]
    • HELECTRICITY
    • H01ELECTRIC ELEMENTS
    • H01MPROCESSES OR MEANS, e.g. BATTERIES, FOR THE DIRECT CONVERSION OF CHEMICAL ENERGY INTO ELECTRICAL ENERGY
    • H01M8/00Fuel cells; Manufacture thereof
    • H01M8/10Fuel cells with solid electrolytes
    • H01M8/1016Fuel cells with solid electrolytes characterised by the electrolyte material
    • H01M8/1018Polymeric electrolyte materials
    • H01M8/102Polymeric electrolyte materials characterised by the chemical structure of the main chain of the ion-conducting polymer
    • H01M8/1037Polymeric electrolyte materials characterised by the chemical structure of the main chain of the ion-conducting polymer having silicon, e.g. sulfonated crosslinked polydimethylsiloxanes
    • HELECTRICITY
    • H01ELECTRIC ELEMENTS
    • H01MPROCESSES OR MEANS, e.g. BATTERIES, FOR THE DIRECT CONVERSION OF CHEMICAL ENERGY INTO ELECTRICAL ENERGY
    • H01M8/00Fuel cells; Manufacture thereof
    • H01M8/10Fuel cells with solid electrolytes
    • H01M8/1016Fuel cells with solid electrolytes characterised by the electrolyte material
    • H01M8/1018Polymeric electrolyte materials
    • H01M8/1041Polymer electrolyte composites, mixtures or blends
    • H01M8/1044Mixtures of polymers, of which at least one is ionically conductive
    • HELECTRICITY
    • H01ELECTRIC ELEMENTS
    • H01MPROCESSES OR MEANS, e.g. BATTERIES, FOR THE DIRECT CONVERSION OF CHEMICAL ENERGY INTO ELECTRICAL ENERGY
    • H01M8/00Fuel cells; Manufacture thereof
    • H01M8/10Fuel cells with solid electrolytes
    • H01M8/1016Fuel cells with solid electrolytes characterised by the electrolyte material
    • H01M8/1018Polymeric electrolyte materials
    • H01M8/1069Polymeric electrolyte materials characterised by the manufacturing processes
    • H01M8/1081Polymeric electrolyte materials characterised by the manufacturing processes starting from solutions, dispersions or slurries exclusively of polymers
    • HELECTRICITY
    • H01ELECTRIC ELEMENTS
    • H01MPROCESSES OR MEANS, e.g. BATTERIES, FOR THE DIRECT CONVERSION OF CHEMICAL ENERGY INTO ELECTRICAL ENERGY
    • H01M8/00Fuel cells; Manufacture thereof
    • H01M8/16Biochemical fuel cells, i.e. cells in which microorganisms function as catalysts
    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08JWORKING-UP; GENERAL PROCESSES OF COMPOUNDING; AFTER-TREATMENT NOT COVERED BY SUBCLASSES C08B, C08C, C08F, C08G or C08H
    • C08J2383/00Characterised by the use of macromolecular compounds obtained by reactions forming in the main chain of the macromolecule a linkage containing silicon with or without sulfur, nitrogen, oxygen, or carbon only; Derivatives of such polymers
    • C08J2383/10Block- or graft-copolymers containing polysiloxane sequences
    • HELECTRICITY
    • H01ELECTRIC ELEMENTS
    • H01MPROCESSES OR MEANS, e.g. BATTERIES, FOR THE DIRECT CONVERSION OF CHEMICAL ENERGY INTO ELECTRICAL ENERGY
    • H01M2300/00Electrolytes
    • H01M2300/0017Non-aqueous electrolytes
    • H01M2300/0065Solid electrolytes
    • H01M2300/0082Organic polymers
    • YGENERAL 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
    • Y02TECHNOLOGIES OR APPLICATIONS FOR MITIGATION OR ADAPTATION AGAINST CLIMATE CHANGE
    • Y02EREDUCTION OF GREENHOUSE GAS [GHG] EMISSIONS, RELATED TO ENERGY GENERATION, TRANSMISSION OR DISTRIBUTION
    • Y02E60/00Enabling technologies; Technologies with a potential or indirect contribution to GHG emissions mitigation
    • Y02E60/30Hydrogen technology
    • Y02E60/50Fuel cells
    • YGENERAL 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
    • Y02TECHNOLOGIES OR APPLICATIONS FOR MITIGATION OR ADAPTATION AGAINST CLIMATE CHANGE
    • Y02PCLIMATE CHANGE MITIGATION TECHNOLOGIES IN THE PRODUCTION OR PROCESSING OF GOODS
    • Y02P70/00Climate change mitigation technologies in the production process for final industrial or consumer products
    • Y02P70/50Manufacturing or production processes characterised by the final manufactured product

Description

WO 03/054995 PCT/USO2/25148 1 DESCRIPTION STABILIZED BIOCOMPATIBLE MEMBRANES OF BLOCK COPOLYMERS AND FUEL CELLS PRODUCED THEREWITH 5 BACKGROUND OF THE INVENTION In one series of articles by Meier et al., various constructions were proposed for polymer based membranes, which included functional proteins. While such membranes had been the subject of speculation in the past, this is believed to be the 10 first successful biological protein containing polymer based membrane that included an imbedded enzyme that retained its functionality. See Corinne Nardin, Wolfgang Meier et al., 39 Angew Chem. Int. Ed., 4599-602 ( 2000 ); Langmuir, 16 1035-41 (2000); and Langmuir, 16 7708-12 (2000). These articles 15 describe a functionalized poly(2-methyloxazoline)-block-poly (dimethylsiloxane)-block-poly(2-methyloxazoline) triblock copolymer in which a protein (a "porin" -- a non-selective, passive pore-forming molecule) is embedded. The Meier et al. work is unique and limited in scope. It 20 does not broadly discuss the use of polymers, nor suggest that even the polymer membrane disclosed could be used in conjunction with even other enzymes. Certainly nothing in these articles suggests the possibility of creating a synthetic membrane containing an embedded biological species capable of 25 participating in oxidation or reduction, or "polypeptide mediated transporting of active molecules, atoms, protons or electrons across the membrane." Indeed, the narrowness of the disclosure and the lack of other successes offer little reason for optimism that other biological materials could be 30 successfully embedded into polymer membranes. The creation of membranes for the study of membrane associated proteins has long been known. See Functional WO 03/054995 PCT/US02/25148 2 Assembly of Membrane Proteins in Planar Lipid Bilayers, 14 Quart. Rev. Biophys. 1-79 (1981). Indeed, transmembrane and redox proteins were embedded in biologically based membranes, e.g., membranes produced of molecules found in living cells or 5 organisms, for purposes of studying their structure and mechanism. The use of lipid bilayers containing embedded enzyme complexes such as NADH dehydrogenase from E. coli, which can transport protons across the membrane and/or participate in redox reactions has also been described. See Liberatore et al., 10 U.S. Patent Application Publication No. US 2002/0001739 Al, published January 3, 2002. Indeed, Liberatore et al. described the use of such membranes as part of a battery. Neither the existence of biological membranes containing enzyme complexes nor the discovery of a single combination of a 15 polymer membrane and a specific enzyme offers much hope for the development of a broad class of synthetic, biocompatible polymer membranes, which are stable and functional. See also G. Tayhas et al. "A Methanol/Dioxogen Biofuel Cell That Uses NAD+ Dependent Dehydrogenases as Catalysts: Application of an 20 Electro-Enzymatic Method to Regenerate Nicotinamide Adenine Dinucleotide at Low Overpotentials," 43 J. Electroanalytical Chem. 155-161 (1998). SUMMARY OF THE INVENTION The present invention relates to a biocompatible membrane 25 including at least one layer of a synthetic polymer material having a first side and a second side. The biocompatible membrane includes at least one polypeptide associated therewith. In a preferred aspect, the present invention relates to a biocompatible membrane wherein the polypeptide is capable of 30 participating in a chemical reaction, participating in the transporting of molecules, atoms, protons or electrons from the first side of the at least one layer to the second side of the WO 03/054995 PCT/US02/25148 3 same layer or participating in the formation of molecular structures that facilitate such reactions or transport. In an even more particularly preferred aspect of the invention, the polypeptide is a redox enzyme and/or is an enzyme capable of 5 participating in the transmembrane transport of protons. Indeed, the polypeptide may have both the ability to cause the liberation of electrons and to participate in transporting protons across the membrane. When discussing transporting protons across a biocompatible membrane, it will be appreciated 10 that neither the exact mechanism, nor the exact species transferred is known. The transferred species might be a proton per se, a positively charged hydrogen, a hydronium ion, H 3 0' or indeed some other charged species. For convenience, however, these will be collectively discussed herein as "protons." 15 Any synthetic polymer material which is a block copolymer, copolymer or polymer or mixtures thereof may be used in accordance with the present invention so long as they are capable of forming biocompatible membrane. In one preferred aspect of the present invention, the synthetic polymer material 20 consists exclusively of at least one block copolymer. Mixtures of block copolymers are also contemplated. Optionally, the synthetic polymer material will include at least one additive. In a second preferred embodiment in accordance with the present invention, the synthetic polymer material includes at least one 25 polymer, copolymer or block copolymer. However, if a block copolymer is present, the synthetic polymer material also includes at least one polymer or copolymer. An optional additive is also contemplated. In another preferred embodiment of the present invention, the synthetic polymer material can be 30 any polymer material capable of forming a biocompatible membrane and includes in addition thereto at least one stabilizing polymer.
WO 03/054995 PCT/US2/25148 4 In another aspect of the present invention, the synthetic polymer material is a block copolymer, a mixture of block copolymers or a mixture of one or more block copolymers and a hydrogen bonding rich stabilizing polymer. Preferably, the 5 polypeptide is embedded in the synthetic polymer material so as to form a biocompatible membrane. "Biocompatible membrane" as used herein is one or more layers of a synthetic polymeric material forming a sheet, plug or other structure that can be used as a membrane and is 10 associated with a polypeptide or other molecule, often of biological origin. By "biocompatible," it is meant that the membrane itself is made of synthetic polymer materials that will not incapacitate or otherwise block all of the functionality of a polypeptide when they are associated with one another. A 15 "membrane" as used herein is a structure such as a sheet, layer or plug of a material that includes, at least as its major structural component, synthetic polymer materials and can be used to selectively segregate space, fluids (liquids or gases), solids and the like. A membrane as used herein may include 20 permeable materials that allow the passage or diffusion of some species from one side to the other. A membrane used in a fuel cell, for example, prevents the passage of some components from within a cathode compartment into the anode compartment and/or prevents some components within the anode compartment from 25 passing into the cathode compartment. Other components, however, may pass freely. At the same time, as exemplified in one embodiment of a membrane in accordance with the present invention, it will permit and indeed facilitate the passage of protons from the anode compartment to the cathode compartment. 30 "Associated" in accordance with the present invention can mean a number of things depending on the circumstances. A polypeptide can be associated with a biocompatible membrane by WO 03/054995 PCT/USO2/25148 5 being bound to one or more of the surfaces thereof, and/or by being wedged or bound within one or more of the surfaces of the membrane (such as in recesses or pores). The "associated" polypeptide can be disposed within the interior of the membrane 5 or in a vesicle or lumen contained within the membrane. Polypeptides could also be disposed between successive layers. Polypeptides may be embedded in the membrane as well. Indeed, in a particularly preferred embodiment, the polypeptide is embedded or integrated in the membrane in such a way so that it 10 is at least partially exposed through at least one surface of the membrane and/or can participate in a redox reaction or in the polypeptide mediated transporting of a molecule, atom, proton or electron from one side of the membrane to the other. The term "participate" in the context of transporting a 15 molecule, atom, proton or electron, from one side of the membrane to the other includes active transport where, for example, the polypeptide physically or chemically "pumps" the molecule, atom, proton or electron across the membrane, usually, but not exclusively, against a pH, concentration or charge 20 gradient or any other active transport mechanism. However, participation need not be so limited. The mere presence of the polypeptide in the membrane may alter the structure or properties of the membrane sufficiently to allow a proton, for example, to be transported from a relatively high proton 25 concentration to a relatively low proton concentration on the other side of the membrane. This is not exclusively a passive, non-selective process such as might result from the use of non selective, passive pore formers or from simple diffusion. Indeed, in some cases, inactivation of the polypeptides in a 30 membrane provides results that are inferior to similar membranes made without polypeptides at all. These processes (excluding passive diffusion) are collectively referred to as "polypeptide WO 03/054995 PCT/USO2/25148 6 mediated transport" where the presence of the polypeptide plays a role in the transporting of a species across the membrane, in ways other than merely structurally providing a static channel. Stated another way, "polypeptide mediated transport" means that 5 the presence of the polypeptide results in effective transport from one side of the membrane to the other in response to something other than just concentration. "Participate," in the context of a redox reaction, means that the polypeptide causes or facilitates the oxidation and/or reduction of a species, or 10 conveys to or from that reaction protons, electrons or oxidized or reduced species. "Polypeptide(s)" includes at least one molecule composed of four or more amino acids that is capable of participating in a chemical reaction, often as a catalyst, or participating in the 15 transporting of a molecule, atom, proton or electron from one side of a membrane to another, or participating in the formation of molecular structures that facilitate or enable such reactions or transport. The polypeptide can be single stranded, multiple stranded, can exist in a single subunit or multiple subunits. 20 It can be made up of exclusively amino acids or combinations of amino acids and other molecules. This can include, for example, pegalated peptides, peptide nucleic acids, peptide mimetics, neucleoprotein complexes. Strands of amino acids that include such modifications as glycosolation are also contemplated. 25 Polypeptides in accordance with the present invention are generally biological molecules or derivatives or conjugates of biological molecules. Polypeptides can therefore include molecules that can be isolated, as well as molecules that can be produced by recombinant technology or which must be, in whole or 30 in part, chemically synthesized. The term therefore encompasses naturally occurring proteins and enzymes, mutants of same, derivatives and conjugates of same, as well as wholly synthetic WO 03/054995 PCT/US02/25148 7 amino acid sequences and derivatives and conjugates thereof. In one preferred embodiment, polypeptides in accordance with the present invention can participate in the transporting of molecules, atoms, protons and/or electrons from one side of a 5 membrane to another side thereof, can participate in oxidation or reduction, or are charge driven proton pumping polypeptides such as DH^ Complex I (also referred to as "Complex 1 "). The present invention stems from the recognition that it is possible to create biocompatible membranes using a wide range of 10 synthetic polymer materials and polypeptides. Biocompatible membranes, when produced in accordance with the present invention, can have advantages over their completely biological counterparts in that they can be more stable, longer lived, more durable and able to be placed in a wider range of useful 15 environments. Indeed, some of the biocompatible membranes of the invention can operate when in contact with solutions having very different and very extreme pHs on either side. They can also be formulated to be stable in the presence of certain oxidizing and/or reducing agents and useful at relative extremes 20 of temperature or other operating and storage conditions. They will facilitate the passage of current to a degree at least greater than that which would occur using the identical membrane without a polypeptide. Preferably, the biocompatible membranes of the present invention will provide at least about 10 25 picoamps/cm 2 (such as when the biocompatible membrane is used in a sensor) more preferably at least about 10 milliamps/cm 2 and even more preferably about 100 milliamps/cm 2 or more. These biocompatible membranes are also generally, but not exclusively, free-standing as a membrane in air and thus can be 30 at least partially desolvated. When used in a fuel cell, these biocompatible membranes will have a useful operating life of, preferably, at least 8 hours, more preferably, at least 3 days, WO 03/054995 PCT/USO2/25148 8 and even more preferably one month or more, and still more preferably, six months or more. Synthetic polymer membranes that are biocompatible and contain polypeptides capable of participating in a redox 5 reaction and/or participating in the transport of a molecule, atom, proton or electron from one side of the membrane to the other are particularly advantageous because they can be used in the creation of a wide range of batteries or fuel cells. These include batteries that are environmentally friendly, light, 10 compact and easily transportable. It is also possible to produce fuel cells that are very high in terms of power output. Preferably, a fuel cell produced in accordance with the present invention can generate at least 10 milliwatts/cm, preferably at least about 50 milliwatts/cm 2 and most preferably at least about 15 100 milliwatts/cm 2 when a circuit, usually with a load or resistance, is created between the anode and cathode. This is also referred to as being in electrical contact. Accordingly, another aspect of the present invention is a fuel cell. The fuel cell includes an anode compartment having 20 an anode and a cathode compartment having a cathode. The fuel cell also includes at least one biocompatible membrane, which can be disposed within the anode compartment, within the cathode compartment or between the anode and cathode compartments. The biocompatible membrane, as previously discussed, can include at 25 least one layer of a synthetic polymer material and at least one polypeptide associated therewith. Preferably, the polypeptide has the ability to participate in a redox reaction and/or to participate in the transporting of molecules, atoms, protons or electrons from one side of the membrane to the other. In a 30 particularly preferred embodiment, the polypeptide can participate in both a redox reaction and in transportation of a molecule, atom, proton or electron. Such a fuel cell may also WO 03/054995 PCT/US02/25148 include an electron carrier and a second polypeptide, both of which are disposed within the anode compartment. Another aspect of the present invention is the creation of solutions which are themselves useful for producing 5 biocompatible membranes in accordance with the present invention. The solutions include at least one synthetic polymer material and at least one polypeptide in a solvent system which often includes both organic solvents and water. Preferable, the synthetic polymer materials is present in an amount of between 10 about 1 and about 30% w/v, and more preferably, and between about 2 and about 20% w/v and most preferably between about 2 and about 10% w/v. Similarly, the polypeptide is present in the solution in an amount of between about 0.001 and about 10.0% w/v, more preferably between about 0.01 and about 15 7.0% w/v, and even more preferably between about 0.1 and about 5.0% w/v. The solution may also include a solubilizing detergent additives and other materials as desirable. The synthetic polymer material, in a preferred embodiment, consists of at least one block copolymer. In another preferred 20 embodiment, the synthetic polymer material includes at least one polymer, copolymer or block copolymer with the proviso that when the synthetic copolymer materials includes at least one block copolymer, the synthetic polymer material also includes at least one polymer or copolymer. In another particularly preferred 25 embodiment, the synthetic polymer material includes at least one stabilizing polymer. BRIEF DESCRIPTION OF THE DRAWINGS Figure 1 illustrates a fuel cell in accordance with the present invention. 30 Figure 2 is a schematic representation of the transfer of electrons and protons in an anode compartment of a fuel cell in one embodiment of the present invention.
WO 03/054995 PCT/US2/25148 10 Figure 3a illustrates an anode and cathode disposed on opposite sides of a dielectric barrier. Figure 3b illustrates, in cross section, an arrangement of a dielectric barrier, an anode, a cathode and a biocompatible 5 membrane in accordance with the present invention. Figure 3c shows schematically a view of a fuel cell including the barrier, anode, cathode and membrane of Figure 3b. Figure 3d is a second embodiment of a membrane in accordance with the present invention illustrated schematically 10 as disposed within perforations contained in a dielectric substrate. Figure 3e is a second embodiment of a membrane in accordance with the present invention illustrated schematically as disposed within perforations contained in a dielectric 15 substrate. Figure 4a is a cross-sectional view of an aperture having a beveled edge and a biocompatible membrane Figure 4b is a cross-sectional view of an aperture having a beveled edge and a biocompatible membrane 20 Figure 4c is a cross-sectional view of an aperture having a beveled edge and a biocompatible membrane DETAILED DESCRIPTION Biocompatible membranes in accordance with the present invention can be formed from any synthetic polymer material 25 that, when associated with one or more polypeptides as described herein, meet the objectives of the present invention. Synthetic polymer materials can include polymers, copolymers and block copolymers and mixtures of same. These can be bound, crosslinked, functionalized or otherwise associated 30 with one another. "Functionalized" means that the polymers, copolymers and/or block copolymers have been modified with end groups that are selected to perform a specific function, whether WO 03/054995 PCT/US02/25148 11 that be polymerization (crosslinking of blocks, for example), anchoring to a particular surface chemistry (use of, for example, certain sulfur linkages), facilitated electron transport via covalently linking an electron carrier or electron 5 transfer mediator, and the like known to the art. Typically, these end groups are not considered a constituent of the polymer or block itself and are often added at the end of or after synthesis. Synthetic polymer materials are generally present on the finished membrane (the membrane in condition for use) in an 10 amount of at least about 50% by weight of the finished membrane, more typically at least about 60% by weight of the finished membrane and often between about 70 and about as much as 99% by weight thereof. A portion of the total amount of the synthetic polymer material may be a stabilizing polymer, generally up to 15 about a third, by weight based on the weight of the total synthetic polymer material in the finished biocompatible membrane. The biocompatible membranes of the invention are preferably produced from one or more block copolymers such as A-B, A-B-A or 20 A-B-C block copolymers, with or without other synthetic polymer materials such as polymers or copolymers, and with or without additives. One suitable block copolymer is described in a series of articles by Corinne Nardin, Wolfgang Meier and others. Angew 25 Chem Int. Ed. 39: 4599-4602, 2000; Langmuir 16: 1035-1041, 2000; Langmuir 16: 7708-7712, 2000. The functionalized poly(2 methyloxazoline)-block-poly (dimethylsiloxane)-block-poly(2 methyloxazoline) triblock copolymer described is as follows: WO 03/054995 PCT/US02/25148 12 0 0 O N EtO-nP Si Si-nPrO--Et- C F Y O NH C In the above chemical formula, the average x value is 68, and the average y value is 15. This is an A-B-A block copolymer in which the "C" recited in the formula does not necessarily 5 equate with the "C" designation of an A-B-C block copolymer. The polymer illustrated above can provide relatively large membranes that can incorporate functional proteins. The methacrylate moieties at the ends of the polymer molecules allow for free-radical mediated crosslinking after incorporating 10 protein to add greater mechanical stability. Biocompatible membranes such as this, particularly those that are nonionic, have greater stability to higher voltage differences between the anode and cathode. The functionalized poly(2-methyloxazoline)-block 15 poly(dimethylsiloxane)-block-poly(2-methyloxazoline)triblock copolymer discussed above is one example of a synthetic polymer material that can be used. Other exemplary block copolymers include, without limitation: Amphiphilic block copolymers [The triblock copolymer shells of the vesicles can be regarded as a 20 mimetic of biological membranes although they are 2 to 3 times thicker than a conventional lipid bilayer. Nevertheless, they can serve as a matrix for membrane-integral proteins. Surprisingly, the proteins remain functional despite the extreme thickness of the membranes and even after polymerization of the WO 03/054995 PCT/USO2/25148 13 reactive triblock copolymers.]; Triblock copolyampholytes from 5-(N,N-dimethylamino)isoprene, styrene, and methacrylic acid [Bieringer et al., Eur. Phys. J.E. 5:5-12, 2001. Among such polymers are Ai1 4 S6 3
A
2 3 , Ai 3 1
S
2 3
A
4 6, Ai4 2
S
23
A
3 s, Ai56S 2 3 A21, Ai 57
SIA
3 2 ] ; 5 Styrene-ethylene/butylene-styrene triblock copolymer [(KRATON) G 1650, a 29% styrene, 8000 solution viscosity (25 wt-% polymer), 100% triblock styrene-ethylene/butylene-styrene (S-EB-S) block copolymer; (KRATON) G 1652, a 29% styrene, 1350 solution viscosity (25 wt-% polymer), 100% triblock S-EB-S block 10 copolymer; (KRATON) G 1657, a 4200 solution viscosity (25 wt-% polymer), 35% diblock S-EB-S block copolymer; all available from the Shell Chemical Company. The preferred block copolymers are of the styrene-ethylene/propylene (S-EP) types and are commercially available under the tradenames (KRATON) G 1726, a 15 28% styrene, 200 solution viscosity (25 wt-% polymer), 70% diblock S-EB-S block copolymer; (KRATON) G-1701X a 37% styrene,>50,000 solution viscosity, 100% diblock S-EP block copolymer; and (KRATON) G-1702X, a 28% styrene,>50,000 solution viscosity, 100% diblock S-EP block copolmyer also available from 20 the Shell Chemical Company, Houston, Texas, USA]; Siloxane triblock copolymer [Nitrile containing siloxane block copolymers were developed as stabilizers for siloxane magnetic fluids. The siloxane magnetic fluids have been recently proposed as internal tamponades for retinal detachment surgery. PDMS-b 25 PCPMS-b-PDMSs (PDMS = polydimethylsiloxane, PCPMS = poly(3 cyanopropylmethyl-cyclosiloxane) were successfully prepared through kinetically controlled polymerization of hexamethylcyclotrisiloxane initiated by lithium silanolate endcapped PCPMS macroinitiators. The macroinitiators were 30 prepared by equilibrating mixtures of 3 cyanopropylmethylcyclosiloxanes (DxCN) and dilithium diphenylsilanediolate (DLDPS). DxCNs were synthesized by WO 03/054995 PCT/USO2/25148 14 hydrolysis of 3-cyanopropylmethyldichlorosilane, followed by cyclization and equilibration of the resultant hydrolysates. DLDPS was prepared by deprotonation of diphenylsilanediol with diphenylmethyllithium. It was found that mixtures of DxCN and 5 DLDPS could be equilibrated at 100 0 C within 5-10 hours. By controlling the DxCN-to-DLDPS ratio, macroinitiators of different molecular weights could be obtained. The major cyclics in the macroinitiator equilibrate are tetramer (8.6 + 0.7 wt%), pentamer (6.3 + 0.8 wt%) and hexamer (2.1 ± 0.5 wt%). 2.5k-2.5k 10 2.5k, 4k-4k-4k, and 8k-8k-8k triblock copolymers were prepared and characterized. These triblock copolymers are transparent, microphase separated and highly viscous liquids. It was found that these triblock copolymers can stabilize nanometer gamma Fe203 and cobalt particles in octamethylcyclotetrasiloxane or 15 hexane. Hence PDMS-b-PCPMS -b-PDMSs represent a class of promising steric stabilizers for silicone magnetic fluids.]; DEO-CPPO-CPEO triblock copolymer; PEO-PDMS-PEO triblock copolymer [Polyethylene oxide (PEO) is soluble in the aqueous phase, while the poly-dimethyl siloxane (PDMS) is soluble in oil 20 phase]; PLA-PEG-PLA triblock copolymer; Poly(styrene-b butadiene-b-styrene) triblock copolymer [Commonly used thermoplastic elastomers, includes Styrolux from BASF, Ludwigshafen, Germany]; Poly(ethylene oxide)/poly(propylene oxide) triblock copolymer films [Pluronic F127, Pluronic P105, 25 or Pluronic L44 from BASF, Ludwigshafen, Germany]; Poly(ethylene glycol)-poly(propylene glycol) triblock copolymer; PDMS-PCPMS PDMS (polydimethylsiloxane-polycyanopropylmethylsiloxane) triblock copolymer [A series of epoxy and vinyl endcapped polysiloxane triblock copolymers with systematically varied 30 molecular weights were synthesized via anionic polymerization using LiOH as an initiator. The nitrile groups on the central copolymer block are thought to adsorb onto the particle WO 03/054995 PCT/USO2/25148 15 surfaces, while the PDMS endblocks protrude into the reaction medium.]; Azo-functional styrene-butadiene-HEMA triblock copolymer, Amphiphilic triblock copolymer carrying polymerizable end groups; Syndiotactic polymethylmethacrylate (sPMMA) 5 polybutadiene (PBD)- sPMMA triblock copolymer, Tertiary amine methacrylate triblock [AB diblock copolymer which can form both micelles (B block in the core) and reverse micelles (A block in the core) in water at 20 0 C.]; Biodegradable PLGA-b-PEO-b-PLGA triblock copolymer; Polyactide-b-polyisoprene-b-polyactide 10 triblock copolymer; PEO-PPO-PEO triblock copolymer [Same as Pluronic from BASF]; Poly(isoprene-block-styrene-block dimethylsiloxane) triblock copolymer; Poly(ethylene oxide) block-polystyrene-block-poly(ethylene oxide) triblock copolymer; Poly(ethylene oxide)-poly(THF)-poly(ethylene oxide) triblock 15 copolymer; Ethylene oxide triblock; Poly E-caprolactone [Birmingham Polymers]; Poly(DL-lactide-co-glycolide) [Birmingham Polymers]; Poly(DL-lactide) [Birmingham Polymers]; Poly(L lactide) [Birmingham Polymers]; Poly(glycolide) [Birmingham Polymers]; Poly(DL-lactide-co-caprolactone) [Birmingham 20 Polymers]; Styrene-Isoprene-styrene triblock copolymer [Japan Synthetic Rubber Co., MW= 140kg/mol, Block ratio of PS/PI= 15/85]; PEO/PPO triblock copolymer; PMMA-b-PIB-b-PMMA [linear triblock TPE]; PLGA-block-PEO-block-PLGA triblock copolymer [Sulfonated styrene/ethylene-butylene/styrene (S-SEBS) TBC 25 polymer proton conducting membrane. Available as Protolyte A700 from Dais Analytic, Odessa FL]; Poly(l-lactide)-block poly(ethylene oxide)-block-poly(l-lactide) triblock copolymer; Poly-ester-ester-ester triblock copolymer; PLA/PEO/PLA triblock copolymer [The synthesis of the triblock copolymers will be 30 prepared by ring-opening polymerization of DL-lactide or e caprolactone in the presence of poly(ethylene glycol), using non-toxic Zn metal or calcium hydride as co-initiator instead of WO 03/054995 PCT/USO2/25148 16 the stannous octoate. The composition of the copolymers will be varied by adjusting the polyester/polyether ratio.]; PCC/PEO/PCC triblock copolymer [The above polymers can be used in mixtures of two or more. For example, in two polymer mixtures measured 5 in weight percent of the first polymer, such mixtures can comprise 20-25%, 25-30%, 30-35%, 35-40%, 40-45% or 45-50%.]; Poly(t-butyl acrylate-b-methyl methacrylate-b-t-butyl acrylate) [Polymer Source, Inc., Dorval, Quebec, Canada]; Poly(t-butyl acrylate-b-styrene-b-t-butyl acrylate) [Polymer Source, Inc.]; 10 Poly(t-butyl methacrylate-b-t-butyl acrylate-b-t-butyl methacrylate) [Polymer Source, Inc.]; Poly(t-butyl methacrylate b-methyl methacrylate-b-t-butyl methacrylate) [Polymer Source, Inc.]; Poly(t-butyl methacrylate-b-styrene-b-t-butyl methacrylate) [Polymer Source, Inc.]; Poly(methyl methacrylate 15 b-butadiene(1,4 addition)-b-methyl methacrylate) [Polymer Source, Inc.]; Poly(methyl methacrylate-b-n-butyl acrylate-b methyl methacrylate) [Polymer Source, Inc.]; Poly(methyl methacrylate-b-t-butyl acrylate-b-methyl methacrylate) [Polymer Source, Inc.]; Poly(methyl methacrylate-b-t-butyl methacrylate 20 b-methyl methacrylate) [Polymer Source, Inc.]; Poly(methyl methacrylate-b-dimethylsiloxane-b-methyl methacrylate) [Polymer Source, Inc.]; Poly(methyl methacrylate-b-styrene-b-methyl methacrylate) [Polymer Source, Inc.]; Poly(methyl methacrylate b-2-vinyl pyridine-b-methyl methacrylate) [Polymer Source, 25 Inc.]; Poly(butadiene(1,2 addition)-b-styrene-b-butadiene(l,2 addition)) [Polymer Source, Inc.]; Poly(butadiene(1,4 addition) b-styrene-b-butadiene(1,4 addition)) [Polymer Source, Inc.]; Poly(ethylene oxide-b-propylene oxide-b-ethylene oxide) [Polymer Source, Inc.]; Poly(ethylene oxide-b-styrene-b-ethylene oxide) 30 [Polymer Source, Inc.]; Poly(lactide-b-ethylene oxide-b-lactide) [Polymer Source, Inc.]; Poly(lactone-b-ethylene oxide-b-lactone) [Polymer Source, Inc.]; a, w-Diacrylonyl Terminated WO 03/054995 PCT/US02/25148 17 poly(lactide-b-ethylene oxide-b-lactide) [Polymer Source, Inc.]; Poly(styrene-b-acrylic acid-b-styrene) [Polymer Source, Inc.]; Poly(styrene-b-butadiene (1,4 addition) -b-styrene) [Polymer Source, Inc.]; Poly(styrene-b-butylene-b-styrene) [Polymer 5 Source, Inc.]; Poly(styrene-b-n-butyl acrylate-b-styrene) [Polymer Source, Inc.]; Poly(styrene-b-t-butyl acrylate-b styrene) [Polymer Source, Inc.]; Poly(styrene-b-ethyl acrylate b-styrene) [Polymer Source, Inc.]; Poly(styrene-b-ethylene-b styrene) [Polymer Source, Inc.]; Poly(styrene-b-isoprene-b 10 styrene) [Polymer Source, Inc.]; Poly(styrene-b-ethylene oxide b-styrene) [Polymer Source, Inc.]; Poly(2-vinyl pyridine-b-t butyl acrylate-b-2-vinyl pyridine) [Polymer Source, Inc.]; Poly(2-vinyl pyridine-b-butadiene(1,2 addition)-b-2-vinyl pyridine) [Polymer Source, Inc.]; Poly(2-vinyl pyridine-b 15 styrene-b-2-vinyl pyridine) [Polymer Source, Inc.]; Poly(4-vinyl pyridine-b-t-butyl acrylate-b-4-vinyl pyridine) [Polymer Source, Inc.]; Poly(4-vinyl pyridine-b-methyl methacrylate-b-4-vinyl pyridine) [Polymer Source, Inc.]; Poly(4-vinyl pyridine-b styrene-b-4-vinyl pyridine) [Polymer Source, Inc.]; 20 Poly(butadiene-b-styrene-b-methyl methacrylate) [Polymer Source, Inc.]; Poly(styrene-b-acrylic acid-b-methyl methacrylate) [Polymer Source, Inc.]; Poly(styrene-b-butadiene-b-methyl methacrylate) [Polymer Source, Inc.]; Poly(styrene-b-butadiene b-2-vinyl pyridine) [Polymer Source, Inc.]; Poly(styrene-b 25 butadiene-b-4-vinyl pyridine) [Polymer Source, Inc.]; Poly(styrene-b-t-butyl methacrylate-b-2-vinyl pyridine) [Polymer Source, Inc.]; Poly(styrene-b-t-butyl methacrylate-b-4-vinyl pyridine) [Polymer Source, Inc.]; Poly(styrene-b-isoprene-b glycidyl methacrylate) [Polymer Source, Inc.]; Poly(styrene-b-a 30 methyl styrene-b-t-butyl acrylate) [Polymer Source, Inc.]; Poly(styrene-b-a-methyl styrene-b-methyl methacrylate) [Polymer Source, Inc.]; Poly(styrene-b-2-vinyl pyridine-b-ethylene oxide) WO 03/054995 PCT/USO2/25148 18 [Polymer Source, Inc.]; Poly(styrene-b-2-vinyl pyridine-b-4 vinyl pyridine) [Polymer Source, Inc.]. The above block copolymers can be used alone or in mixtures of two or more in the same or different classes. For example, 5 in mixtures of two block copolymers measured in weight percent of the first polymer, such mixtures can comprise 10-15%, 15-20%, 20-25%, 25-30%, 30-35%, 35-40%, 40-45% or 45-50%. Where three polymers are used, the first can comprise 10-15%, 15-20%, 20 25%, 25-30%, 30-35%, 35-40%, 40-45% or 45-50% of the whole of 10 the polymer components, and the second can 10-15%, 15-20%, 20 25%, 25-30%, 30-35%, 35-40%, 40-45% or 45-50% of the remainder. Stated another way, the amount of each block copolymer in a mixture can vary considerably with the nature and number of the block copolymers used and the desired properties to be obtained. 15 However, generally, each block copolymer of a mixture in accordance with the present invention will be present in an amount of at least about 10% based on weight of total polymers in the membrane or solution. These same general ranges would apply to membranes produced from one or more polymers, 20 copolymers and/or mixtures with block copolymers. There may also be instances where a single polymer, copolymer or block copolymer may be "doped" with a small amount of a distinct polymer, copolymer or block copolymer, even as little as 1.0% by weight of the membrane to adjust the membrane's specific 25 properties. Embodiments of the invention include, without limitation, A-B, A-B-A or A-B-C block copolymers. The average molecular weight for triblock copolymers of A (or C) is, for example, 1,000 to 15,000 daltons, and the average molecular weight of B 30 is 1,000 to 20,000 daltons. More preferably, block A and/or C will have an average molecular weight of about 2,000-10,000 WO 03/054995 PCT/USO2/25148 19 Daltons and block B will have an average molecular weight of about 2,000-10,000 daltons. If a diblock copolymer is used, the average molecular weight for A is between about 1,000 to 20,000 Daltons, more 5 preferably, about 2,000-15,000 Daltons. The average molecular weight of B is between about 1,000 to 20,000 Daltons, more preferably about 2,000 to 15,000 Daltons. Preferably, the block copolymer will have a hydrophobic/hydrophilic balance that is selected to (i) provide 10 a solid at the anticipated operating and storage temperature and (ii) promote the formation of biomembrane-like structures rather than micelles. More preferably, the hydrophobic content (or block) shall exceed the hydrophilic content (or block). Thus, at least one block of the diblock or triblock copolymers is 15 preferably hydrophobic. While wettable membranes are possible, preferably the content of hydrophobic and hydrophilic synthetic polymeric materials will render the membrane sparingly wettable. As described above, in one preferred embodiment of the present invention, there is provided a biocompatible membrane 20 produced using a mixture of synthetic polymer materials. Such mixtures can be a mixture of two or more block copolymers that are identical but for the molecular weight of their respective blocks. For example, a biocompatible membrane can be produced using a mixture of two block copolymers, both of which are 25 poly(2-methloxazoline)-polydimethylsiloxane-poly(2 methloxazoline), one of which having an average molecular weight of 2kD-5kD-2kD and the other 3kD-7kD-3kD and the ratio of the first block copolymer to the second is about 67% to 33% of the total synthetic polymer material used w/w. This, of course 30 means that the majority block copolymer's first block has a molecular weight of about 2 thousand Daltons, the second block has a molecular weight of 5 thousand Daltons and the third block WO 03/054995 PCT/US02/25148 20 has a molecular weight of 2 thousand Daltons. The minority block copolymer has blocks of about 3 thousand, 7 thousand and 3 thousand Daltons respectively. Of course, two or more entirely different block copolymers 5 can be used and mixtures of different block copolymers and identical block copolymers that differ only in the size of their respective blocks are also contemplated. But mixtures are not limited to block copolymers. Polymers and copolymers can be used, alone, in combination, 10 and in combination with block copolymers in accordance with the present invention to produce biocompatible membranes having the properties described herein. Polymers and copolymers useful are preferably solid at room temperature (25 0 C). They can be dissolved in solvents or solvent systems that can accommodate 15 any other synthetic polymer material used, any additive used, and the polypeptide used. Polymers and copolymers useful in producing biocompatible membranes can include, without limitation polystyrenes, polyalkyl and polydialkyl siloxanes such as polydimethylsiloxane, polyacrylates such as 20 polymethylmethacrylate, polyalkenes such as polybutadiene, polyalkylenes and polyalkylene glycols, sulfonated polystyrene, polydienes, polyoxiranes, poly(vinyl pyridines), polyolefins, polyolefin/alkylene vinyl alcohol copolymers, ethylene propylene copolymers, ethylene-butene-propylene copolymers, ethyl vinyl 25 alcohol copolymers, perfluorinated sulfonic acids, vinyl halogen polymers and copolymers such as copolymers of vinyl chloride and acrylonitrile, methacrylic/ethylene copolymers and other soluble but generally hydrophobic polymers and copolymers all in a molecular weight of between about 5,000 and about 500,000. 30 Particularly preferred polymers include: Poly(n-butyl acrylate); Poly(t-butyl acrylate); Poly(ethyl acrylate); Poly(2 ethyl hexyl acrylate); Poly(hydroxy propyl acrylate); WO 03/054995 PCT/USO2/25148 21 Poly(methyl acrylate); Poly(n-butyl methacrylate); Poly(s-butyl methacrylate); Poly(t-butyl methacrylate); Poly(ethyl methacrylate) ; Poly(glycidyl methacrylate); Poly(2 hydroxypropyl methacrylate); Poly(methyl methacrylate) ; Poly(n 5 nonyl methacrylate); Poly(octadecyl methacrylate); Polybutadiene (1,4-addition); Polybutadiene (1,2-addition); Polyisoprene (1,4 addition); Polyisoprene (1,2-addition and 1,4 addition); Polyethylene; Poly(dimethyl siloxane); Poly(ethyl methyl siloxane); Poly(phenyl methyl siloxane); Polypropylene; 10 Poly (propylene oxide); Poly(4-acetoxy styrene); Poly(4-bromo styrene); Poly(4-t-butyl styrene); Poly(4-chloro styrene); Poly(4-hydroxyl styrene); Poly(a-methyl styrene); Poly(4-methyl styrene); Poly(4-methoxy styrene); Polystyrene; Isotactic Polystyrene; Syndiotactic Polystyrene; Poly(2-vinyl pyridine); 15 Poly(4-vinyl pyridine); Poly(2,6-dimethyl-p-phenylene oxide); Poly(3-(hexafluoro-2-hydroxypropyl)-styrene); Polyisobutylene; Poly(9-vinyl anthracene); Poly(4-vinyl benzoic acid); Poly(4 vinyl benzoic acid sodium salt) ; Poly(vinyl benzyl chloride); Poly(3(4)-vinyl benzyl tetrahydrofurfuryl ether); Poly(N-vinyl 20 carbazole); Poly(2-vinyl naphthalene) and Poly(9-vinyl phenanthrene). Since polymers and copolymers are generally synthetic polymer materials, they may be used in the same amounts described previously for block copolymers and mixtures. In a particularly preferred aspect of the present 25 invention, the biocompatible membrane includes a synthetic polymer material, preferably at least one block copolymer (most preferably one that is, at least in part, amphiphilic) and a synthetic polymer material that can stabilize the biocompatible membrane. It has been discovered that certain polymers, most 30 notably, hydrophilic polymers and copolymers capable of forming a plurality of hydrogen-bonds ("hydrogen bonding rich") can stabilize the membrane. In the context of stabilizing polymers, WO 03/054995 PCT/USO2/25148 22 the term "polymer" includes monomers, polymers and copolymers. "Hydrophilic" in this context means that the stabilizing polymer will dissolve or be solubilized in water or water miscible solvents. Without wishing to be bound to any particular theory 5 of operation, it is believed that the use of such polymers can assist in functionally integrating polypeptides into the biocompatible membrane's structure. A stabilizing polymer imparts to a biocompatible membrane greater operating life and/or greater resistance to mechanical failure when compared to 10 an identical biocompatible membrane produced without the stabilizing polymer when exposed to the same conditions. A stabilized biocompatible membrane wherein the synthetic polymer material includes a stabilizing polymer, used in a fuel cell, for example, can have an increased operating life of at least 15 about 10%, more preferably at least about 50%, most preferably at least about 100%. Particularly preferred polymers capable of stabilizing the polypeptides in the biocompatible membranes of the present invention include: dextrans, polyalkylene glycols, polyalkylene 20 oxides, polyacrylamides, and polyalkyleneamines. These stabilized polymers (again including copolymers) have an average molecular weight which is generally lower than polymers and copolymers used as synthetic polymer materials. Their molecular weight generally ranges from about 1,000 daltons to about 15,000 25 daltons. Particularly preferred polymers capable of stabilizing biocompatible membranes include, without limitation, polyethylene glycol having an average molecular weight of between about 2,000 and about 10,000, polyethylene oxide having an average molecular weight of between about 2,000 and about 30 10,000, poly acrylamide having an average molecular weight of between about 5,000 and 15,000 daltons. Other stabilizing polymers include: polypropylene, Poly(n-butyl acrylate); WO 03/054995 PCT/US02/25148 23 Poly(t-butyl acrylate); Poly(ethyl acrylate); Poly(2-ethyl hexyl acrylate); Poly(hydroxy propyl acrylate); Poly(methyl acrylate); Poly(n-butyl methacrylate); Poly(s-butyl methacrylate); Poly(t butyl methacrylate); Poly(ethyl methacrylate) ; Poly(glycidyl 5 methacrylate); Poly(2-hydroxypropyl methacrylate); Poly(methyl methacrylate); Poly(n-nonyl methacrylate); and Poly(octadecyl methacrylate). The amount of stabilizing polymer(s) used in the biocompatible membranes is not critical so long as some 10 measurable improvement in properties is realized and the functionality of the biocompatible membrane is not unduly hampered. Some trade of functionality and longevity is to be expected. However, generally, the amount of stabilizing polymer used, as a function of the total amount of synthetic polymer 15 material found in the finished biocompatible membrane (by weight) is generally not more than one-third, and typically 30% by weight or less. Preferably, the amount used is between 5 and about 30%, more preferably between about 5 and about 15% by weight of the synthetic polymer material in the finished 20 membrane is used. In addition to one or more polymers, copolymers and/or block copolymers, and/or stabilized polymers, the synthetic polymer material of the invention can include at least one additive. Additives can include crosslinking agents and lipids, 25 fatty acids, sterols and other natural biological membrane components and their synthetic analogs. These are generally added to the synthetic polymer material when in solution. These additives, if present at all, generally would be found in an amount of between about 0.50% and about 30%, preferably between 30 about 1.0% and about 15%, based on the weight of the synthetic polymer material.
WO 03/054995 PCT/USO2/25148 24 Where the biocompatible membrane incorporates cross-linking moieties, procedures useful for polymerization include chemical polymerization with radical-forming or propagating agents and polymerization via photochemical radical generation with or 5 without further radical propagating agents. Parameters can be adjusted depending on such conditions as the membrane material, the size of biocompatible membrane segments, the structure of the support, and the like. Care should be taken to minimize the damage to the polypeptide. One particularly useful method 10 involves using peroxide at a neutral pH, followed by acidification. Examples of useful polypeptides that can be associated with a synthetic polymer material, so as to form a biocompatible membrane in accordance with the present invention, and that can 15 participate in one or both of the oxidation/reduction and transmembrane transport functions (molecules, atoms, protons, electrons) include, for example, NADH dehydrogenase ("complex I") (e.g., from E. coli. Tran et al., "Requirement for the proton pumping NADH dehydrogenase I of Escherichia coli in 20 respiration of NADH to fumarate and its bioenergetic implications," Eur. J. Biochem. 244: 155, 1997), NADPH transhydrogenase, proton ATPase, and cytochrome oxidase and its various forms. Further polypeptides include: glucose oxidase (using NADH, available from several sources, including number of 25 types of this enzyme available from Sigma Chemical), glucose-6 phosphate dehydrogenase (NADPH, Boehringer Mannheim, Indianapolis, IN), 6-phosphogluconate dehydrogenase (NADPH, Boehringer Mannheim), malate dehydrogenase (NADH, Boehringer Mannheim), glyceraldehyde-3-phosphate dehydrogenase (NADH, 30 Sigma, Boehringer Mannheim), isocitrate dehydrogenase (NADH, Boehringer Mannheim; NADPH, Sigma), c-ketoglutarate dehydrogenase complex (NADH, Sigma) and proton-translocating WO 03/054995 PCT/US02/25148 25 pyrophosphates. Also included are succinate:quinone oxidoreductase, also referred to as "Complex II," "A structural model for the membrane-integral domain of succinate:quinone oxidoreductases" Hagerhall, C. and Hederstedt, L., FEBS Letters 5 389; 25-31 (1996) and "Purification, crystallisation and preliminary crystallographic studies of succinate:ubiquinone oxidoreductase from Escherichia coli." Tornroth, S., et al., Biochim. Biophys. Acta 1553; 171-176 (2002), heterodisulfide reductases, F(420)H(2) dehydrogenase, (Baumer et al., "The 10 F420H2 dehydrogenase from Methanosarcina mazei is a Redox-driven proton pump closely related to NADH dehydrogenases." 275 J. Biol. Chem. 17968 (2000)) or a formate hydrogenlyase (Andrews, et al., A 12-cistron Escherichia coli operon (hyf) encoding a putative proton-translocating formate hydrogenlyase system." 143 15 Microbiology 3633 (1997)), Nicotinamide nucleotide transhydrogenases: "Nicotinamide nucleotide transhydrogenase: a model for utilization of substrate binding energy for proton translocation." Hatefi, Y. and Yamaguchi, M., Faseb J., 10; 444 452 (1996), Proline Dehydrogenase: "Proline Dehydrogenase from 20 Escherichia coli K2." Graham, S., et al., J. Biol. Chem. 259; 2656-2661 (1984), and Cytochromes including, without limitation, cytochrome C oxidase (crystallized with either undecyl-o-D maltoside or cyclohexyl-hexyl-3-D-maltoside), Cytochrome bc 1 : "Ubiquinone at Center N is responsible for triphasic reduction 25 of cytochrome bc, complex." Snyder, C.H., and Trumpower, B.L., J. Biol. Chem. 274; 31209-16 (1999), Cytochrome bo 3 : "Oxygen reaction and proton uptake in helix VIII mutants of cytochrome bo 3 ." Svensson, M., et al., Biochemistry 34; 5252-58 (1995), "Thermodynamics of electron transfer in Escherichia coli 30 cytochrome bo 3 ." Schultz, B.E., and Chan, S.I., Proc. Natl. Acad. Sci. USA 95; 11643-48 (1998), and Cytochrome d: "Reconstitution of the Membrane-bound, ubiquinone-dependent pyruvate oxidase WO 03/054995 PCT/US02/25148 26 respiratory chain of Escherichia coli with the cytochrome d terminal oxidase." Koland, J.G., et al., Biochemistry 23; 445 453 (1984), Joost and Thorens, "The extended GLUT-family of sugar/polyol transport facilitators: nomenclature, sequence 5 characteristics, and potential function of its novel members (review)" 18 Mol. Membr. Biol. 247-56 (2001), and selective channel proteins including those disclosed in Goldin, A.L., "Evolution of voltage-gated Na(+) channels." J. Exp. Biol. 205; 575-84 (2002), Choe, S., "Potassium channel structures." Nat. 10 Rev. Neurosci. 3;115-21 (2002), Dimroth, P., "Bacterial sodium ion-coupled energetics." Antonie Van Leeuwenhoek 65; 381-95 (1994), and Park, J.H. and Saier, M.H.Jr., "Phylogenetic, structural and functional characteristics of the Na-K-Cl cotransporter family." J. Membr. Biol. 149; 161-8 (1996). All 15 of the foregoing are hereby incorporated by reference. Methods of isolating such an NADH dehydrogenase enzyme are described in detail, for example, in Braun et al., Biochemistry 37: 1861 1867, 1998; and Bergsma et al., "Purification and characterization of NADH dehydrogenase from Bacillus subtilis," 20 Eur. J. Biochem. 128: 151-157, 1982. As described by Spehr et al., Biochemistry 38:16261-16267, 1999, the complex I NADH dehydrogenase (or, NADH:ubiquinone oxidoreductase), which is expressed from a operon, can be overexpressed in E. coli by substituting a T7 promoter in the operon to provide useful 25 quantities for use in the invention. Complex I can be isolated from over-expressing E. coli by the method described by Spehr et al. using solubilization with dodecyl maltoside. Complex I can be handled such that NADH dehydrogenase activity is eliminated or greatly reduced. As described in 30 B6ttcher et al., "A Novel, Enzymatically Active Conformation of the Escherichia coli NADH:Ubiquinone Oxidoreductase (Complex I)," web published as accepted for publication at www.jbc.org, WO 03/054995 PCT/US02/25148 27 2002 (Manuscript M112357200), in high salt or high pH solution Complex I changes conformation such that proton transport is uncoupled from NADH dehydrogenase activity, creating DH form. Applicants have used these conditions and combinations of these 5 conditions to show that the fuel cell of the invention can operate without NADH dehydrogenase activity in the anode/cathode barrier. Such conditions include anolyte or anode salt concentrations of 200 mM to 2M, and pH of 8.0 or above. Transporter activity is believed to function against a 10 countering [Hi ] gradient, due to the charge imbalance between the anode and cathode sides. Proton transporter activity of the DH form has been confirmed from the maintenance of current generation in fuel cells in which biocompatible membranes gated by this form provided the only avenue to relieve charge 15 imbalance. (Note that with complex I reverse transport of protons has been further controlled against by using conditions on the cathode side that maintain the NADH dehydrogenase coupling of any inversely oriented complex I -thereby blocking reverse transport due to lack of NADH substrate.) 20 It will be recognized that the source of any enzyme used in the invention can be a thermophilic organism providing a more temperature stabile enzyme. For example, complex I can be isolated from Aquifex aeolicus in a form that operates optimally at 90 oC, as described in Scheide et al., FEBS Letters 512: 80 25 84, 2002 (describing a preliminary isolation using the type of detergent extraction used elsewhere for complex I). Additionally, it is contemplated that genetically modified polypeptides, such as modified enzymes, can be used. One commonly applied technique for genetically modifying an enzyme 30 is to use recombinant tools (e.g., exonucleases) to delete N terminal, C-terminal or internal sequence. These deletion products are created and tested systematically using ordinary WO 03/054995 PCT/US02/25148 28 experimentation. As is often the case, significant portions of the gene product can be found to have little effect on the commercial function of interest. More focused deletions and substitutions can increase stability, operating temperature, 5 catalytic rate and/or solvent compatibility providing enzymes that can be used in the invention. Of course it is possible to use mixtures of various polypeptides described herein as may be desirable. The amount of polypeptide used will vary with the type of 10 polypeptide used, the nature and function of the biocompatible membrane, the environment in which it will be used, etc. The amount of polypeptide may be important to certain applications such as fuel cells where, in general, the higher the concentration of polypeptide per square centimeter of surface 15 area, the higher the rate of proton transfer per unit area (in terms of current). In general, however, as long as some polypeptide is present and functional, and as long as the amount of polypeptide used does not prevent membrane formation or render the membrane unstable, then any amount of polypeptide is 20 possible. Generally, the amount of polypeptide will be at least about 0.01%, more preferably about 5%, even more preferably 10%, and still more preferably at least about 20% and most preferably 30% or more by weight based on the final weight of the biocompatible membrane. The amount of polypeptide to solvent 25 can be as low as 0.001% w/v and as high as 50.0% w/v. Preferably, the concentration is from about 0.5% to about 5.0% w/v. More preferably the concentration is from about 1.0% to about 3.0% w/v. Suitable solubilizing and/or stabilizing agents such as 30 cosolvents, detergents and the like may also be needed, particularly in connection with the polypeptide solution. Solubilizing detergents are commonly found at the 0.01% to 1.0% WO 03/054995 PCT/US2/25148 29 concentration level, and more preferably up to about 0.5% is contemplated. Such detergents include ionic detergents: Sodium dodecyl sulfate, Sodium N-dodecyl sarcosinate, N-dodecyl Beta-D glucopyranoside, Octyl-Beta-D-glucopyranoside, dodecyl 5 maltoside, decyl, undecyl, tetradecyl-maltoside (in general, an alkyl chain of about 8 carbons or more bonded to a sugar as a general form of an ionic detergent) octyl-beta-D-glucoside and polyoxytheylane (9) dodecyl-ether, C 12
E
9 , as well as non-ionic detergents, such as triton X-100, or Nonidet P-40. Also useful 10 are certain polymers, typically diblock copolymers which exhibit surfactant properties, such as BASF's Pluronic series, or Disperplast (BYK-Chemie). The solvent used in producing the synthetic polymer material solution is preferably selected to be miscible with 15 both the water used (the polypeptide solution often includes water) and at least one of the synthetic polymer materials (polymer, copolymer and/or block copolymer). However, as described above, it is possible to form membranes using solvents or mixtures which are not water miscible. Note that while the 20 use of solvents to produce solutions is preferred, the term "solution" as used herein generally encompasses suspensions as well. When a block copolymer is used, the solvent should solubilize these synthetic polymer materials. While the 25 synthetic polymer material may be relatively sparingly soluble in the solvent (less than 5% w/v), it is preferably more soluble than 5% w/v and generally, solubility is at least 5 to 10% w/v, preferably greater than 10% w/v synthetic polymer material to solvent. 30 Appropriate solvents may include, without limitation, low molecular weight aliphatic alcohols and diols of between 1 and 12 carbons such as methanol, ethanol, 2-propanol, isopropanol, WO 03/054995 PCT/US2/25148 30 1-propanol, aryl alcohols such as phenols, benzyl alcohols, low molecular weight aldehydes and ketones such as acetone, methyl ethyl ketone, cyclic compounds such as benzene, cyclohexane, toluene and tetrahydrofuran, halogenated solvents such as 5 dichloromethane and chloroform, and common solvent materials such as 1,4-dioxane, normal alkanes (C 2
-C
12 ) and water. Solvent mixtures are also possible as long as the mixture has the appropriate miscibility, rate of evaporation and the other criteria described for individual solvents. (Solvent components 10 that have any tendency to form protein-destructive contaminants such as peroxides can be used as long as they can be appropriately purified and handled.) Solvent typically comprises 30% v/v or more of the polypeptide/synthetic polymer material solution, preferably 20% v/v or more, and usefully 10% 15 v/v or more. If the membranes are to include "other materials" such as detergents, lipids (e.g. cardiolipin), sterols (e.g. cholesterol) or buffers and/or salts, those too would be added prior to formation of the membrane and they would be present in 20 an amount of between about 0.01 and about 30%, preferably between about .01 and about 15% based on the weight of the finished biocompatible membrane. Other materials, as opposed to additives, are most often mixed with the polypeptide solutions, not the synthetic polymer solutions. 25 Biocompatible membranes in accordance with the present invention can be produced using any one of a number of conventional techniques used in the production of membranes from synthetic polymer materials and even lipid bilayers, as long as the resulting biocompatible membranes are useful as described 30 herein. One method of forming a biocompatible membrane, which is preferred for use with block copolymer-based membrane, is as follows: WO 03/054995 PCT/US02/25148 31 1. Form a solution or suspension of synthetic polymer material in a solvent or mixed solvent system. The solution or suspension can be a mixture of two or more block copolymers, although it may contain one or more polymers and/or copolymers. 5 The solution or suspension preferably contains 1 to 90% w/v synthetic polymer material, more preferably 2 to 70%, or yet more preferably 3 to 20% w/v. Seven % w/v is particularly preferred. 2. One or more polypeptides (typically with solubilizing 10 detergent) are placed in solution or suspension, either separately or by being added to the existing polymer solution or suspension. Where the solvent used to solubilize the synthetic polymer materials is the same, or of similar characteristics and solubility to that which can solubilize the polypeptide, it is 15 usually more convenient to add the polypeptide to the polymer solution or suspension directly. Otherwise, the two or more solutions or suspensions containing the synthetic polymer materials and the polypeptide must be mixed, possibly with an additional cosolvent or solubilizer. Most often, the solvent 20 used for the polypeptide is aqueous. Mixing of these solutions and/or suspensions is often a relatively simple matter and can be accomplished by hand or with automated mixing tools. Heating or cooling may also be useful in membrane formation depending on the solvents and polymers 25 used. In general, rapidly evaporating solvents tend to form membranes better with cooling while extremely slowly evaporating solvents would most likely benefit from a slight degree of heating. One can examine the boiling point of solvents used to select those with the most favorable characteristics provided 30 they are appropriate for the polymer used. One must, of course, however consider also the need to incorporate the polypeptide into the solvent polymer mixture, which can be a nontrivial WO 03/054995 PCT/USO2/25148 32 matter. It is possible, for example, to mix 5 microliters of a detergent solubilized Complex I (0.15 % w/v dodecyl maltoside) having 10 mg/ml of Complex I into 95 microliters of a mixture of a 3.2% w/v polystyrene-polybutadiene-polystyrene triblock 5 copolymer (a completely hydrophobic triblock Sold under the trademark STYROLUX 3G55, Lot No. 7453064P, available from BASF in a 50/50 mixture of acetone and hexane and to deposit same in a manner that will allow for membrane formation. In this case, the final mixture included about 5% v/v of water, and 0.75% w/w 10 Complex I relative to the weight of the synthetic polymer material. Generally, the solutions are sufficiently stable at room temperature to be useful for at least about 30 minutes, provided that the solvents do not evaporate during that time. They also can be stored overnight, or longer, generally under 15 refrigerated conditions. 3. A volume of the final solution or suspension including both the polypeptide(s) and the synthetic polymer materials is formed into a membrane and allowed to at least partially dry, thereby removing at least a portion of the solvent. It is 20 possible to completely dry some of the membranes produced in accordance with the invention or to substantially dry same. By substantially dry it is meant that there may be some residual solvent, up to about 15%, which is often retained even if left out at room temperature for several hours. 25 In a particularly preferred embodiment, substantially all of the weight of the finished membrane will be either polypeptide or synthetic polymer material. In this case, the amount of synthetic polymer material, including additives and stabilizing polymers ranges from about 70% to about 99% by 30 weight of the finished membrane. However, it may be desirable to have an even greater polypeptide content or it may be necessary to retain some solvent, so the amount of synthetic WO 03/054995 PCT/US02/25148 33 polymer material may be reduced accordingly. Generally, however, at least about 50% by weight of the finished biocompatible membrane will be synthetic polymer material. When the synthetic polymer material is a mixture that includes a 5 block copolymer and a polymer or copolymer, other than a stabilizing polymer, the block copolymer can be present in an amount of at least about 35% by weight of the biocompatible membrane. Up to about 30% by weight of the biocompatible membrane can be "additives" and "other materials" (collectively) 10 as defined herein. More preferably the amount of additives and other materials is up to about 15% by weight of the biocompatible membrane. Up to about 30% by weight of the synthetic polymer material can be stabilizing polymer. Generally the stabilizing polymer will be present in an amount 15 of between about 5 and about 20% of the weight of the synthetic polymer material used. Identifying which solvents are particularly useful in accordance with the present invention and which combination of polymers and polypeptides and solvents should be used depends on 20 a number of factors, some of which have already been discussed in terms of miscibility, evaporation and the like. The polymer and protein constituents must be able to be completely dissolved in the solvent or solvent mixture. Evaporation rate must be sufficiently long to allow one time to produce a membrane. 25 However, the amount of time should not be so long as to render manufacturing impractical. While apolar solvents may be useful, generally more apolar solvents may not be useful in certain circumstances as ionic or hydroxyl components of the polymer may be poorly soluble in completely apolar solvents. Thus one may 30 be able to dissolve a highly rigid, hydrophobic component such as polystyrene and be unable to simultaneously dissolve a highly ionic component such as an acrylic acid. However, with polymers WO 03/054995 PCT/US02/25148 34 of completely hydrophobic character, then apolar solvents are preferred. The solvents should generally be, in part, nonaqueous as the polymer should be at least in part nonwater dissolvable. And while water-miscibility is most desired for 5 membrane protein reconstitution, it is not a rigidly limiting factor. Thus, preferably, all solvents are nonaqueous. The solvent for the polypeptide and stabilizing polymers, however, is predominantly water or at least water miscible. Preferred methods of forming biocompatible membranes 10 including both at least one synthetic polymer material and a stabilizing polymer include the step of making an appropriate solution of block copolymer and, usually separately stabilizing polymer and polypeptide. As described elsewhere, the polypeptide may include one or more detergents or surfactants 15 and is typically in an aqueous solution. Once the appropriate solutions are made and mixed, membranes can be made by any of the techniques disclosed herein or known to the art including, for example, coating a perforated dielectric substrate with the solution followed by at least partial evaporation of solvents. 20 Such evaporation can be facilitated in a vacuum. One method of forming a biocompatible membrane, including a hydrogen-bonding rich stabilizing polymer, is as follows: 1. A solution or suspension of Protolyte A700 block copolymer in a solvent as supplied is diluted with an equal 25 volume of ethanol (5% water w/v). The solution contains about 5% w/v of block copolymer. 2. Separately, an aqueous solution or suspension of the stabilizing agent is made by mixing 943 mg of polyethylene glycol (PEG) 8000 to produce a solution having a concentration 30 of about 2.3% w/v. The concentration of the stabilizing agent in solution is near the saturation limit.
WO 03/054995 PCT/USO2/25148 35 3. Next, 4 microliters of a solution including 10 mg/ml of E. coli derived Complex I along with 0.15% w/v of dodecyl maltoside is added to 6 microliters of the PEG solution and mixed them to generate a solution or suspension. 5 4. The 10 microliters of the solution is then mixed with 10 microliters of the solution including the block copolymer. 5. A small volume (e.g., 4 microliters) resulting solution is dropped onto the apertures of a subset of apertures (holes drilled through the support) of a perforated substrate of 1 mil 10 (25.4 microns) thick KAPTON, a brand of polyimide, having apertures that are 100 micrometers in diameter and 1 mil deep. 6. The solution is allowed to air dry in a hood thereby removing the solvent. 7. Steps 5 and 6 are repeated as needed to cover all 15 apertures. The above-described method of introducing polypeptide to a solution containing a stabilizing polymer prior to mixing with non-aqueous solvent(s) in the presence of block copolymers is believed to stabilize the function of polypeptides used in the 20 biocompatible membrane. However, the polymer and block copolymer could also be mixed and the resulting solution mixed with a generally aqueous polypeptide solution. Optionally one would check each aperture to ensure membrane formation, or check at least a statistically relevant number of apertures 25 microscopically. If apertures do not contain a membrane, repair holes using additional solution and a micropipette-scaled pipetting device. It typically requires only a very small volume of solution to repair such holes. The membranes can be completely or substantially completely dried in a vacuum 30 apparatus, or desiccator. Membranes so formed may be stored dried in vacuum or desiccated, if desired.
WO 03/054995 PCT/US02/25148 36 Where the biocompatible membrane incorporates cross-linking moieties, such as methacrylates, and will be used in a fuel cell, the following procedure can be used: Prepare biocompatible membrane in a support that will form 5 the cathode/anode barrier. Assemble a cell with biocompatible membrane on anode/cathode barrier support, electrodes and buffers only. Connect the two electrodes to a high load, such as approximately 150 kilo-Ohms. 10 Add hydrogen peroxide to cathode side to initiate cross linking process, for example such that the concentration of the peroxide will be 1% by volume. Let fuel cell stand under load for a period of time, for example 1 hour (±10%). 15 Adjust pH of the cathode side to below pH 5 to stop the crosslinking. Parameters can be adjusted depending on such conditions as the membrane material, the size of biocompatible membrane, the thickness of the biocompatible membrane, the structure of the 20 support, and the like. Once the polypeptide/synthetic polymer material solution has been produced, it can be formed into a membrane. Biocompatible membranes in accordance with the present invention can be free standing membranes. Such membranes can be formed by 25 pouring the solution into a pan or onto a sheet such that they achieve the desired thickness. Once the solution has been dried and the solvent dried off, the dry membrane may be removed from the pan or peeled from the backing layer. Suitable antitack agents may be used to assist in this process. Biocompatible 30 membranes can be formed against a solid material, such as by coating onto glass, carbon that is surface modified to increase hydrophobicity, or a polymer (such as polyvinyl acetate, PDMS, WO 03/054995 PCT/US02/25148 37 Kapton®, a perfluorinated polymer, PVDF, PEEK, polyester, or UHMWPE, polypropylene or polysulfone). Polymers such as PDMS provide an excellent support that can be used to establish openings on which biocompatible membranes can be formed. 5 The membrane may then be cut or shaped as needed or used as is. Furthermore, to facilitate use of the membrane, it may be attached physically or through some sort of fastening device or adhesive to a holder if desired. This can be conceptualized as stretching a canvas over a frame prior to painting a picture 10 when the frame is the support and the membrane is the canvas. Alternatively, the membrane may be formed with such a structure. A suitable analogy would be taking a child's bubble wand, used for blowing bubbles, and dipping it into a solution of soap and water. A film of soap and water forms across the opening of the 15 wand. The structural material used at the periphery allows the film to be handled and manipulated and provides rigidity and strength. It also helps provide the desired shape of the film. The same sort of process can be employed using a physical structure and the membrane forming solutions of the present 20 invention. In one preferred embodiment in accordance with the present invention, a biocompatible membrane may be disposed and/or formed within or across apertures of various perforated substrates including preferably dielectric substrates. 25 "Perforated substrates" means that it has at least one hole, aperture (synonymous with hole as used herein) or pore into which, or over which, a biocompatible membrane could be disposed. For example, Figure 3b shows an embodiment of a membrane construction useful in a fuel cell. A perforated 30 substrate 42, which defines various perforations 49, has its surfaces metalized to form a perforated anode 44 and a perforated cathode 45. Note also that perforated substrate 42 WO 03/054995 PCT/US02/25148 38 can be a porous substrate without, for example, drilled holes. In such instances, perforations 49 are to be understood as being pores. A biocompatible membrane 61 in accordance with the present invention is formed across the apertures or 5 perforations 49 of perforated substrate 42, and is attached directly to the surface of the anode. Biocompatible membrane 61 can also be disposed within the perforation and flush with anode 44 or can be attached to or adjacent cathode 45. Two membranes 61 can be provided, one, for example, disposed across the anode 10 as illustrated and one within the perforation 49 of the substrate 42, flush with anode 45, etc. (not shown). The membranes 61 may be the same or different in terms of the synthetic polymer materials used, the polypeptides used or both. Indeed, a plurality of such membrane 61 and indeed, layers of 15 biocompatible membrane 61 can be used in conjunction with other types of membranes, diffusive barriers and the like. While the foregoing has been explained in the context of Figure 3b, it is equally applicable to other constructions and, in particular, any type of fuel cell construction. Biocompatible membrane 61 20 can include one or more polypeptides 62 and 63 as illustrated. Coating methods which can be used to form electrodes (44, 45) on a substrate include a first coating or lamination of conductor, followed by plating, sputtering or using another coating procedure to coat with titanium or a noble conductor 25 such as gold or platinum. Another method is directly sputtering an attachment layer, such as chromium or titanium onto the support, followed by plating, sputtering or other coating procedure to attach a noble conductor. The outer metal layer can be favorably treated to increase its hydrophobicity, such as 30 with dodecane-thiol. Supports or substrates with high natural surface charge densities, such as Kapton and Teflon, are in some embodiments WO 03/054995 PCT/USO2/25148 39 preferred. As noted above, these can be used to form the anode/cathode barrier without the use of surface electrodes. Substrate 42 is often preferably dielectric. The perforations or pores 49 and metallized surfaces (anode 5 44 and cathode 45 (for embodiments that use so-located electrodes)) of the substrate 42 can be constructed, for example, with masking and etching techniques of photolithography well known in the art. Perforations can also be formed, for example, by punching, drilling, laser drilling, stretching, and 10 the like. Alternatively, the metallized surfaces (electrodes) can be formed for example by (1) thin film deposition through a mask, (2) applying a blanket coat of metallization by thin film then photo-defining, selectively etching a pattern into the metallization, or (3) photo-defining the metallization pattern 15 directly without etching using a metal impregnated resist (DuPont Fodel process, Drozdyk et al., "Photopatternable Conductor Tapes for PDP Applications," Society for Information Display 1999 Digest, 1044-1047; Nebe et al., US Patent 5,049,480). In one embodiment, the perforated or porous 20 substrate is a film. For example, the dielectric can be a porous film that is rendered non-permeable outside the "perforations" by the metallizations. The surfaces of the metal layers can be modified with other metals, for instance by electroplating. Such electroplatings are, for example, with 25 titanium, gold, silver, platinum, palladium, mixtures thereof, or the like. In addition to metallized surfaces, the electrodes can be formed by other appropriate conductive materials, which materials can be surface modified. For example, the electrodes can be formed of carbon (graphite), including graphite fiber, 30 which can be applied to the dielectric substrate by, for example, electron beam evaporation, chemical vapor deposition or pyrolysis. Surfaces to be metallized can be solvent cleaned and WO 03/054995 PCT/USO2/25148 40 oxygen plasma etched. Useful means of forming hydrophilic electrodes are described for example in Surampudi, US Patent 5,773,162, Surampudi, US Patent 5,599,638, Narayanan, US Patent 5,945,231, Kindler, US Patent 5,992,008, Surampudi, 5 WO 96/12317, Surampudi, WO 97/21256 and Narayanan, WO 99/16137. Biocompatible membranes used in the invention are optionally stabilized against a solid support. One method for accomplishing such stabilization uses sulfur-mediated linkages of lipid-related molecules to glue, tether or bond metal 10 surfaces or surfaces of another solid support to biocompatible membranes. For example, a porous support can be coated with a sacrificial or removable filler layer, and the coated surface smoothed by, for example, polishing. Such a porous support can include any of the proton-conductive polymeric membranes 15 discussed, typically so long as the proton-conductive polymeric membrane can be smoothed following coating, and is stable to the processing described below. One useful porous support is glass frit. The smoothed surface is then coated (with prior cleaning as necessary) with metal, such as with a first layer of chrome 20 and an overcoat of gold. The sacrificial material is then removed, such as by dissolution, taking with it the metallization over the pores but leaving a metallized surface surrounding the pores. The sacrificial layer can comprise photoresist, paraffin, cellulose resins (such as ethyl 25 cellulose), and the like. The tether or glue comprises alkyl thiol, alkyl disulfides, thiolipids and the like adapted to tether a biocompatible membrane as illustrated if Figures 7A and 7B. Such tethers are described for example in Lang et al., Langmuir 10: 197-210, 30 1994. Additional tethers of this type are described in Lang et al., US Patent 5,756,355 and Hui et al., US Patent 5,919,576.
WO 03/054995 PCT/US02/25148 41 Figure 3d includes a similar arrangement. However, unlike Figure 3b, where biocompatible membrane 61 is actually attached to the metalized surface of anode 44, in Figure 3d, membrane 61 is formed within aperture 49 in perforated substrate 42, such 5 that it does not necessarily contact either anode 44 or cathode 45. Note that these figures are not to scale and that the membrane may be thicker or thinner than the electrode and may be thicker or thinner than the perforated substrate 42. Note also that in Figure 3b, biocompatible membrane 61 is not disposed 10 between the anode 44 and cathode 45. However, biocompatible membrane 61 is disposed between anode 44 and cathode 45 in Figure 3d. In each of Figures 3b and 3d, the combination of the substrate 42 and biocompatible membrane 61 (along with the anode 44 in Figure 3b) form a structure that can also be referred to 15 as a barrier. Figure 3e illustrates a preferred embodiment for fuel cells. In this figure, the arrangement of the membrane 61 and the perforated substrate 42 (a substrate containing pores, perforations or apertures) is as described previously in 20 connection with Figure 3d. However, the cathode and anode are spaced apart from the perforated substrate. They can be plate electrodes, but they are not plated onto the surface, or even in contact with substrate 42 or membrane 61. In this case, the membrane 61 and substrate 42 are the barrier. 25 The biocompatible membrane can be formed across the pores, perforations or apertures 49 and enzyme incorporated therein by, for example, the methods described in detail in Niki et al., US Patent 4,541,908 (annealing cytochrome C to an electrode) and Persson et al., J. Electroanalytical Chem. 292: 115, 1990. Such 30 methods can comprise the steps of: making an appropriate solution of polypeptide and synthetic polymer material as previously discussed, the perforated substrate 49 preferably a WO 03/054995 PCT/USO2/25148 42 dielectric substrate is dipped into the solution to form the enzyme-containing biocompatible membranes. Sonication or detergent dilution may be required to facilitate enzyme incorporation into a biocompatible membrane. See, for example, 5 Singer, Biochemical Pharmacology 31: 527-534, 1982; Madden, "Current concepts in membrane protein reconstitution," Chem. Phys. Lipids 40: 207-222, 1986; Montal et al., "Functional reassembly of membrane proteins in planar lipid bilayers," Quart. Rev. Biophys. 14: 1-79, 1981; Helenius et al., 10 "Asymmetric and symmetric membrane reconstitution by detergent elimination," Eur. J. Biochem. 116: 27-31, 1981; Volumes on biomembranes (e.g., Fleischer and Packer (eds.)), in Methods in Enzymology series, Academic Press. Alternatively, a thin partition made (preferably but not 15 necessarily) of a hydrophobic material such as Teflon with a small aperture has a small amount of amphiphile introduced. The coated aperture is immersed in a dilute electrolyte solution upon which the droplet will thin and spontaneously self-orient spanning the aperture. Biocompatible membranes of substantial 20 area have been prepared using this general technique. Two common methods for formation of the biocompatible membranes themselves are the Langmuir-Blodgett technique and the injection technique. The Langmuir-Blodgett technique involves the use of a 25 Langmuir-Blodgett trough with a partition, such as a Teflon TM polymer partition at the center. The trough is filled with aqueous solution. The aperture of the polymer partition is placed above the water level. The polypeptide and synthetic polymer material containing solution is spread over the surface 30 and the polymer partition is lowered slowly into the aqueous solution forming a biocompatible membrane over the aperture. The injection method is similar except the polymer partition is WO 03/054995 PCT/USO2/25148 43 kept fixed. In this method the aqueous phase is filled to just under the aperture, the solution is introduced over the surface and then the liquid level is raised over the partition by injecting additional electrolyte solution from underneath. 5 Another method for forming biocompatible membranes is using the technique of self-assembly. This is a variation from the above two described techniques and was in fact the first technique to be successfully employed to fabricate synthetic lipid membranes. The technique involves the preparation of a 10 membrane forming solution as described above. A drop of the solution is introduced into a perforated substrate 42, often a hydrophobic substrate. The substrate 42 is then immersed in a dilute aqueous electrolyte solution whereupon the droplet will spontaneously thin and orient. The remaining material migrates 15 to the perimeter of the layer where it forms a reservoir called the Plateau-Gibbs border. The thickness of substrate 42, be it a perforated substrate having apertures or a porous material, is for example between about 15 micrometer (gm) to about 5 millimeters, preferably from 20 about 15 to about 1,000 micrometers, and more preferably, from about 15 micrometer to about 30 micrometers. The width of the perforations or pores is, for example, from about 1 micrometer to about 1,500 micrometers, more preferably about 20 to about 200 micrometers, and even more preferably, about G60 to about 140 25 micrometers. About 100 micrometers is particularly preferred. Preferably, perforations or pores comprise in excess of about 30% of the area of any area of the dielectric substrate involved in transport between the chambers, such as from about 50 to about 75% of the area. 30 In certain preferred embodiments, the substrate is glass or a polymer (such as polyvinyl acetate, polydimethylsiloxane (PDMS), Kapton® (polyimide film, Dupont de Nemours, Wilmington, WO 03/054995 PCT/USO2/25148 44 DE), a perfluorinated polymer (such as Teflon, from DuPont de Nemours, Wilmington, DE), polyvinylidene fluoride (PVDF, e.g., a semi-crystalline polymer containing approximately 59% fluorine sold as Kynar T M by Atofina, Philadelphia, PA), PEEK (defined 5 below), polyester, UHMWPE (described below), polypropylene or polysulfone), soda lime glass or borosilicate glass, or any of the foregoing coated with metal. The metal can be used to anchor biocompatible membrane (such as a monolayer or bilayer of amphiphilic molecules). The metal coating can be receded from 10 any junctions in which they provide too likely an electrically conductive pathway for a short between the anode and cathode compartments. In a particularly preferred aspect of the present invention, perforated substrate 42 is made of a dielectric material. 15 The polypeptide 62 can be immobilized in the biocompatible membrane with the appropriate orientation to allow access of the catalytic site for the oxidative reaction to the anode compartment and asymmetric pumping of protons. However, if the polypeptide is not asymmetrically oriented, the reverse oriented 20 polypeptide is not detrimental for a variety of reasons depending on the context. First, the charge imbalance created by the fuel cell on the anode side drives proton transport to the cathode side even against a proton concentration gradient. In situations where the pumping is tied to the use of a reduced 25 electron carrier, the reverse pumping has no such carrier since the electron carrier is substantially isolated in the anode compartment 41. (By "substantially isolated" those of ordinary skill will recognize sufficiently isolated to allow the fuel cell to operate.) 30 In one embodiment, as shown in Figures 4a to 4c, the biocompatible membrane 61 contains cross-linking moieties and is formed across an aperture with beveled edges to the substrate WO 03/054995 PCT/USO2/25148 45 42. The degree of beveling can be any degree that increases the stability of the biocompatible membrane. Where the cross-linked block copolymer is relatively less rigid, greater beveling can be used to increase stability, while a lesser amount of beveling 5 can be appropriate for more rigid cross-linked block copolymer. As illustrated, numerous beveling shapes can contribute to increasing stability. In another alternate embodiment in accordance with the present invention, the solution containing the polypeptide and 10 the synthetic polymer material can be laid across a surface of a porous supporting material, rather than a perforated material as illustrated in Figure 3b. Once protons, for example, were pumped across the membrane, they could migrate through the pores of the supporting barrier material. 15 Whether a substrate is perforated or porous, it is not necessary that a membrane be formed across its entire surface. For example, while it may be convenient to form a membrane across the entire surface of a perforated substrate, it may be preferred merely to selectively introduce a solution containing 20 polypeptide and synthetic polymer material into the perforations or merely across the perforations. The thickness of the biocompatible membrane in accordance with the present invention can be adjusted by known techniques such as controlling the volume introduced to a particular size 25 pore, perforation, pan or tray, etc. The thickness of the membrane will be dictated largely by its composition and function. A membrane intended to include a transmembrane proton transporting complex such as complex I must be thick enough to provide sufficient support and orientation to the enzyme 30 complex. It should not, however, be so thick as to prevent effective transportation of the proton across the membrane. For an aperture or perforation of about 100 microns in diameter in WO 03/054995 PCT/USO2/25148 46 an array of about 100 apertures and a solution including complex I in an amount of about 4 microliters in a copolymer solution containing about 7% w/v of the poly(2-methyloxazoline)-block poly(dimethylsiloxane)-block-poly(2-methyloxazoline)-triblock 5 copolymer described in one of the previously identified Meier et al. articles, a membrane of suitable thickness can be obtained. The thickness of the membrane can vary widely depending upon its needed longevity, its function, etc. Membranes that are designed to transport protons for example are 10 often thinner than membranes to which are attached an enzyme which can oxidize something. However, in general, the membranes will range from between about 10 nanometers to 100 micrometers or even thicker. Indeed, biocompatible membranes useful for transporting protons in a fuel cell have been successful at 15 thicknesses of 10 nanometers up to 10 micrometers. Again, thicker membranes are possible. In certain embodiments of the present invention, particularly useful in the creation of fuel cells, the biocompatible membranes of the present invention are capable of 20 transporting protons against a pH gradient. This concept will be discussed further herein. However, conceptually, on the cathode side of the biocompatible membrane, the pH of any medium, electrolyte or the like is acidic while on the anode side of the membrane, the pH is basic. This is opposite of what 25 is found in most fuel cells. Generally, such conditions would favor the transfer of protons from the proton rich acidic side to the relatively proton poor basic side. The use of membranes in accordance with the present invention can, however, pump upstream from the proton poor side to the proton rich side. 30 This highlights another aspect of the present invention which can be particularly useful. The membranes of the present invention can also be active and functional despite relatively WO 03/054995 PCT/USO2/25148 47 large variations in pH conditions on opposite sides thereof. For example, membranes in accordance with the present invention can catalyze proton transfer where the pH in an anode compartment is at least 0.5 pH units higher than the pH in the 5 cathode compartment. In many fuel cells, the pH in the anode compartment is lower than the pH found in the cathode compartment due to the greater concentration of protons. However, fuel cells produced in accordance with the present invention do not need to rely on 10 proton concentration differences to drive protons across the membrane by diffusion. This can be a particularly important advantage because the species used as electron carriers and/or electron transfer mediators often work more efficiently in relatively alkaline pH. Fuel oxidation reactions may also be 15 more efficient under such pH conditions. The pH differential, based on the electrolytes used, etc. may not need to be adjusted during the useful life of a fuel cell. Alternatively, a buffering system can be added, and additional buffer added as needed, to the anode and/or cathode compartment during 20 operation. Preferably, the anode compartment will have a pH that is at least about 1 pH unit higher than the pH in the cathode compartment, more preferably 2 pH units higher. In a particularly preferred embodiment, the pH of the anode compartment is 8 or higher and the pH in a cathode compartment 25 is 5 or lower. See Example No. 59. Another aspect of the present invention is a fuel cell produced using a biocompatible membrane as described herein. Without limitation to other appropriate definitions known in the art, a fuel cell is a device that generates electrical energy by 30 the chemical conversion of a fuel. The specific type of fuel cell, in terms of the type of fuel used, the type of electron transporting species (electron carriers, soluble enzymes, WO 03/054995 PCT/USO2/25148 48 transfer mediators and the like) or electrolytes used, the types of electrodes used and the like are subject to wide variation and all are contemplated so long as they are capable of meeting the appropriate criteria. For example, the systems used must be 5 compatible with the biocompatible membrane. If they are, for example, corrosive to the membrane, then the life of the fuel cell may be unusually short (less than 8 hours useful life). If the materials used cause sufficient instability, then that too may be reason why particular fuel, for example, may not be 10 useful in accordance with the invention. Particularly preferred are fuel cells which are small and light enough to be used in portable electronic devices such as computers, PDAs, cell phones, beepers, personal entertainment systems, PlayStation 2, Game Boy, portable DVD players, power tools, toys, stereo 15 equipment, radios, cameras and video recorders, digital recorders and cameras, flashlights, cars, trucks, boats, planes, etc. The fuel cells are preferably "green," which is to say that they can be disposed of readily because they do not contain corrosive or dangerous chemicals, either as fuels or waste. In 20 addition, these fuel cells may be refillable (adding additional fuel, etc.) or may be single use/disposable. As illustrated in Figure 1, a fuel cell in accordance with the present invention can include an anode compartment 1 having an anode 4 and a cathode compartment 3 having a cathode 5. The 25 assembly also includes a dielectric perforated or porous substrate 2. The fuel cell also includes at least one biocompatible membrane 61 as previously described (not shown in Figure 1). The anode 4 has an electrical lead or contact 6 and the cathode 5 has an electrical lead or contact 7 which can be 30 electrically linked, or linked in an electrical circuit through a load or resistance so as to place them in electrical contact. The biocompatible membrane 61 can be disposed within the anode WO 03/054995 PCT/USO2/25148 49 compartment, as is the case in Figure 3b, within the cathode compartment or between the anode and cathode compartments as shown in Figures 3d and 3e. The biocompatible membrane is also disposed between the anode and cathode in Figures 3d and 3e and 5 can be thought of as defining the boundary between the anode compartment and the cathode compartment in that illustration. The fuel cell normally includes electrical contacts which allow a circuit to be formed between the two electrodes. Anodes and cathodes can be made of any electrically conductive material 10 which is otherwise generally unreactive with the elements of the fuel cell. The anode and cathode are preferably made of metals or carbon as previously described. The size and shape of the anode and cathode can be made to fit the necessary dimensions of a fuel cell and allow for passage of various chemical species. 15 Figure 3c illustrates a fuel cell produced in accordance with the present invention comprising a cell housing 51 and a perforated substrate 42 including within its perforations a biocompatible membrane as described herein 61. The anode and cathode are plated onto the substrate as previously described 20 and are not individually shown. However, as shown in Figure 3c, the anode contact 54 and the cathode contact 55 are attached to the relevant electrodes within the fuel cell. If an electrode is used as part of the support system for a biocompatible membrane, as illustrated in Figure 3b, then the 25 electrode must have sufficient perforations or other means of providing access to allow molecules, atoms, protons or electrons to flow therethrough. When the fuel cell has a configuration similar to Figure 3e, however, it is possible that the electrodes be completely solid. However, it still may be 30 desirable to have fuel or other components of a fuel cell able to pass through and around the electrode and therefore, it is possible to provide perforations in any event.
WO 03/054995 PCT/US2/25148 50 The biocompatible membrane useful in the fuel cell according to the present invention has already been discussed. The biocompatible membrane preferably will facilitate the passage of current in an amount that is greater than that which 5 would result from the use of the same membrane without the polypeptide. More preferably, the biocompatible membrane will facilitate the flow of at least about 10 milliamps/cm 2 , more preferably at least about 50 milliamps/cm 2 , and most preferably at least about 100 milliamps/cm 2 . In the simplest embodiment, the 10 biocompatible membrane is itself free standing and able to support itself or to be supported by a peripheral structure and is disposed across an aperture or is disposed between an anode and cathode. It is also important in this instance that the biocompatible membrane itself be dielectric and that it prevent 15 the free flow of certain components between the anode and cathode compartments such as catholyte, electrolyte, cathode fuel, analyte anode fuel, other ions, etc. The next least complicated embodiment would involve the use of a similar biocompatible membrane, but one that is either 20 incapable of preventing the complete intermixing of the necessary species or which is not dielectric. In such an instance, an additional barrier may be necessary. Such barriers can be made of the same materials used to produce the substrate 42 described earlier or, in the alternative, as illustrated in 25 Figures 3d and 3e, the membrane can be disposed either in or covering perforations or pores in a substrate 42. Materials useful for the substrate and the methods of preparing same have already been discussed. The anode electrode can be coated with an electron transfer 30 mediator such as an organometallic compound which functions as a substitute electron recipient for the biological substrate of the redox enzyme. Similarly, the biocompatible membrane of the WO 03/054995 PCT/USO2/25148 51 embodiment of Fig. 3 or structures adjacent to the biocompatible membrane can incorporate such electron transfer mediators, or the electron transfer mediator can be more generally available in the anode chamber. Such organometallic compounds can 5 include, without limitation, dicyclopentadienyliron (C 1 oH 10 Fe, ferrocene, available along with analogs that can be substituted, from Aldrich, Milwaukee, WI), platinum on carbon, and palladium on carbon. Further examples include ferredoxin molecules of appropriate oxidation/reduction potential, such as the 10 ferredoxin formed of rubredoxin and other ferredoxins available from Sigma Chemical. Other electron transfer mediators include organic compounds such as quinone and related compounds. Still further electron transfer mediators are methylviologen, ethylviologen or benzylviologen (CAS 1102-19-8; 1,1' 15 bis(phenylmethyl)-4,4'-bipyridinium, N,N'-y,y'-dipyridylium), and any listed below in the definition of electron transfer mediator. The anode electrode (as opposed to the biocompatible membrane) can be impregnated with an enzyme, which can be 20 applied before or after the electron transfer mediator. One way to assure the association of the enzyme with the electrode is simply to incubate a solution of the enzyme with electrode for sufficient time to allow associations between the electrode and the enzyme, such as Van der Waals associations, to mature. 25 Alternatively, a first binding moiety, such as biotin or its binding complement avidin/streptavidin, can be attached to the electrode and the enzyme bound to the first binding moiety through an attached molecule of the binding complement. Additional methods of attaching enzyme to electrodes or other 30 materials, and additional electron transfer mediators are described in Willner and Katz, Angew. Chem. Int. Ed. 39:1181 1218, 2000. The anode chamber can include enzymes adjacent to WO 03/054995 PCT/US02/25148 52 or associated with the anode electrode, or separate therefrom. For example, a redox enzyme can be attached to the anode chamber side of a polymer forming a proton conductive anode/cathode barrier, with a layer of conductive material on the anode side 5 providing the anode electrode. In some embodiments of the invention, it is anticipated that the electron carrier will be effective to transfer electrons to the anode electrode in the absence of the redox enzyme. Some embodiments of the invention can, in addition, use a 10 traditional form of anode/cathode barrier: a polymeric membrane selected for it ability to passively conduct protons in conjunction with the biocompatible membrane of the invention. The former anode/cathode barrier is useful since it is effective to pump against a proton gradient. 15 Dual membranes can be disposed across and/or within the perforations or pores of an anode/cathode barrier or can be placed between the anode and cathode compartments. These membranes can be of the traditional composition or biocompatible membranes. One context in which such dual membranes are 20 observed are those in which the pores are of relatively narrow diameter. Another context is one in which the anode cathode barrier is formed of sandwiched materials such that separate junctions between differing materials nucleate the formation of separate biocompatible membranes across the pore. 25 Without limitation to theory, it is believed that the second, more cathode proximate biocompatible membrane, operates to some degree passively, as the pumping from the first biocompatible membrane creates a high proton concentration, driving passive transport to the cathode compartment. Thus, to 30 the extent the cathode compartment contains peroxide that could prospectively damage the transport protein, the active transport WO 03/054995 PCT/USO2/25148 53 function can be damaged, while the second biocompatible membrane insulates the first from higher concentrations of the peroxide. In one embodiment, the dual membrane benefit is obtained with one or more biocompatible membranes, the first of which (at 5 the anode side) incorporates the polypeptide and a proton conductive polymeric membrane fitted at the cathode chamber side to limit peroxide transit towards the biocompatible membranes. Again, an intermediate zone between the biocompatible membrane(s) and the proton-conductive polymeric membrane gains a 10 high proton concentration due to active transport, driving further transit along a concentration gradient into the cathode compartment. In one embodiment, the substrate in which the pores are formed is a sandwich of dielectric Kapton, and conductive Kapton 15 (conductive through the presence of incorporated graphite). The conductive Kapton can form the anode electrode, or be appropriately metallized to form the anode electrode. The three layers are relatively hydrophilic, relatively hydrophobic, then relatively hydrophilic. 20 Figure 2 shows a schematic block diagram representation of one embodiment of the anode side of a fuel cell in accordance with the present invention. The anode compartment contains the fuel. Fuel is an organic molecule that is depleted in accordance with the present invention and consumed. However, 25 its consumption generates protons and electrons. Preferred fuels in accordance with the present invention are compounds that are, or can be transformed into, single carbon compounds. Preferred amongst these is methanol. However, fuels can include, without limitation, oxidizable sugars and sugar 30 alcohols, alcohols, organic acids such as pyruvates, succinates, etc., fatty acids, lactic acids, citric acid, etc., amino acids and short polypeptides, aldehydes, ketones, etc. The fuel in WO 03/054995 PCT/US02/25148 54 this embodiment is first acted upon by soluble enzymes that, in the case of methanol, can be an alcohol dehydrogenase. As will be seen below, other dehydrogenases such as aldehyde dehydrogenase and formate dehydrogenase can also be used or can 5 be used in conjunction with one another. These soluble enzymes are capable of acting upon the fuel to generate electrons and protons. Soluble enzymes are preferably present in a range of between about 0.001 to about 25,000 units, more preferably about 10 0.1 units to about 12,500 units, and most preferably from about 1 unit to about 12,5000 units. Units, in this context, refers to the specific activity of the soluble enzyme and one unit of activity is the amount required to convert 1 micromole of fuel (or enzyme substitution in other contexts) per minute at 25 0 C. 15 "Soluble enzymes" is a bit of a misnomer as these compounds need neither be soluble nor enzymes. These compounds may be suspended or emulsified and/or immobilized on beads or some other solid support. It really does not matter as long as they are functional, can act upon the fuel, and allow electron 20 carriers and/or transfer mediators to carry protons to the biocompatible membrane and electrons to the anode. The protons and electrons are transferred by the coordinated action of the soluble enzymes on the fuel to an electron carrier also referred to as a cofactor. One such 25 electron carrier is NAD+/NADH. Electron carriers can include, without limitation, reduced nicotinamide adenine dinucleotide (denoted NADH; oxidized form denoted NAD or NAD*), reduced nicotinamide adenine dinucleotide phosphate (denoted NADPH; oxidized form denoted NADP or NADP*), reduced nicotinamide 30 mononucleotide (NMNH; oxidized form NMN), reduced flavin adenine dinucleotide (FADH2; oxidized form FAD), reduced flavin mononucleotide (FMNH 2 ; oxidized form FMN), reduced coenzyme A, WO 03/054995 PCT/US02/25148 55 and the like. Electron carriers include proteins with incorporated electron-donating prosthetic groups, such as coenzyme A, protoporphyrin IX, vitamin B12, and the like. All of the above are believed to carry both the electrons and 5 protons that can be generated by the action of the soluble enzymes on the fuel. However, not all electron carriers will convey protons. It will be recognized that C 1 compounds comprising carbon oxygen and hydrogen are electron carriers. However, these are also fuels. Also within the definition of 10 electron carrier are electron transfer mediators, as specified below. Electron carriers, when present, generally are provided in concentrations of between about 1 microMolar to about 2 Molar, more preferably about 10 microMolar to about 1 Molar, and most preferably about 100 microMolar to about 500 milliMolar. 15 Under the influence of the soluble enzymes, protons and electrons, NAD+ is converted to NADH. From this point, electrons and/or protons can be handed off and traded between a number of additional cofactors and/or transfer mediators. An electron transfer mediator is a composition which facilitates 20 transfer of electrons released from an electron carrier to another molecule, typically an electrode or another electron transfer mediator with an equal or lower reduction potential. Examples, in addition to those previously identified, include phenazine methosulfate (PMS), pyrroloquinoline quinone (PQQ, 25 also called methoxatin), Hydroquinone, methoxyphenol, ethoxyphenol, or other typical quinone molecules, methyl viologen, l,1-dibenzyl-4,4'-dipyridinium dichloride (benzyl viologen), N,N,N-,N'-tetramethylphenylenediamine (TMPD) and dicyclopentadienyliron (C1OH1OFe, ferrocene). Electron transfer 30 mediators, when present, generally are provided in concentrations of between about 1 microMolar to abut 2 Molar, more preferably between about 10 microMolar and about 2 Molar, WO 03/054995 PCT/USO2/25148 56 and even more preferably between but 100 microMolar and about 2 Molar. For simplicity, however, and as illustrated in Figure 2, the reduced cofactor or electron carrier can next interact with 5 the polypeptides, in this case, the dehydrogenase function of Complex I embedded in a biocompatible membrane in accordance with the present invention. The Complex I liberates protons from the NADH molecule, as well as electrons. The electrons might flow directly to the anode. However, more often, they are 10 taken up by a transfer mediator, which then transports the electrons to the anode. NADH dehydrogenase Complex I is an interesting polypeptide in that it also can participate in transporting protons across the biocompatible membrane. What is particularly interesting, 15 however, is that the protons transferred are not necessarily the protons liberated by the action of the dehydrogenase portion of Complex I. Therefore, to be most successful, a fuel cell in accordance with this particular aspect of the invention will contain additional proton species in the anode compartment. The 20 proton transporting function of the Complex I is illustrated in Figure 2, as the redox function. When the transfer mediator gives up its electrons to the anode, it has been oxidized, allowing it to be capable of obtaining additional electrons liberated by oxidizing other 25 electron carriers. Oxidized cofactor (NAD+) is also now ready to receive protons and electrons under the influence of fuel and the soluble enzymes. The reactions just described occur at the anode electrode and in the anode compartment and can be exemplified chemically as follows. 30 H20 + NADH - NAD + HO + + 2e (3) This reaction can be fed by the following reactions: WO 03/054995 PCT/USO2/25148 57 ADH
CH
3 OH+NAD+ 1 HCHO+H + NADH (4) ALD HCHO + H 2 0 + NAD > HCO 2 H + H + + NADH (5) FDH
HCO
2 H + NAD + 1 0 CO 2 + H + + NADH (6) Total: CH OH+ HO0 +3 NAD - CO2 +3H+3NADH (7) Thus, the reactions and the electron-generating reaction sum as follows: 3NADH I > 3NAD + 3H + 6e- (3*)
CH
3
OH+H
2 0 +3NAD+ I CO 2 +3H + 3NADH (8) 10 Total:
CH
3 OH + H 2 0 C 2 0 + 6H + + 6e- (9) The soluble enzymes that can be used to generate a reduced electron carrier (such as NADH as illustrated above) from an organic molecule such as methanol can start with a form of 15 alcohol dehydrogenase (ADH). Suitable ADH enzymes are described for example in Ammendola et al., "Thermostable NAD(+)-dependent alcohol dehydrogenase from Sulfolobus solfataricus: gene and protein sequence determination and relationship to other alcohol dehydrogenases," Biochemistry 31: 12514-23, 1992; Cannio et 20 al., "Cloning and overexpression in Escherichia coli of the genes encoding NAD-dependent alcohol dehydrogenase from two Sulfolobus species," J. Bacteriol. 178: 301-5, 1996; Saliola et al., "Two genes encoding putative mitochondrial alcohol dehydrogenases are present in the yeast Kluyveromyces lactis," 25 Yeast 7: 391-400, 1991; and Young et al., "Isolation and DNA WO 03/054995 PCT/USO2/25148 58 sequence of ADH3, a nuclear gene encoding the mitochondrial isozyme of alcohol dehydrogenase in Saccharomyces cerevisiae," Mol. Cell Biol. 5: 3024-34, 1985. If the resulting formaldehyde is oxidized, an aldehyde dehydrogenase (ALD) is used. Suitable 5 ALD enzymes are described for example in Peng et al., "cDNA cloning and characterization of a rice aldehyde dehydrogenase induced by incompatible blast fungus," GeneBank Accession AF323586; Sakano et al., "Arabidopsis thaliana [thale cress] aldehyde dehydrogenase (NAD+)-like protein" GeneBank Accession 10 AF327426. If the further resulting formic acid is oxidized, a formate dehydrogenase (FDH) is used. Suitable FDH enzymes are described for example in Colas des Francs-Small, et al., "Identification of a major soluble protein in mitochondria from nonphotosynthetic tissues as NAD-dependent formate dehydrogenase 15 [from potato]," Plant Physiol. 102(4): 1171-1177, 1993; Hourton-Cabassa, "Evidence for multiple copies of formate dehydrogenase genes in plants: isolation of three potato fdh genes, fdhl, fdh2, and fdh3," Plant Physiol. 117: 719-719, 1998. For reasons discussed below, it can be useful to use 20 soluble enzymes that are adapted to use or otherwise can accommodate quinone-based electron carriers. Such enzymes are, for example, described in: Pommier et al., "A second phenazine methosulphate-linked formate dehydrogenase isoenzyme in Escherichia coli," Biochim Biophys Acta. 1107(2):305-13, 1992. 25 ("The diversity of reactions involving formate dehydrogenases is apparent in the structures of electron acceptors which include pyridine nucleotides, 5-deazaflavin, quinones, and ferredoxin"); Ferry, J.G. "Formate dehydrogenase" FEMS Microbiol. Rev. 7(3 4):377-82, 1990. (formaldehyde dehydrogenase with quinone 30 activity); Klein et al., "A novel dye-linked formaldehyde dehydrogenase with some properties indicating the presence of a protein-bound redox-active quinone cofactor" Biochem J. 301 ( Pt WO 03/054995 PCT/USO2/25148 59 1):289-95, 1994. (representative of a number of articles on dehydrogenases with bound quinone cofactors) ; Goodwin et al., "The biochemistry, physiology and genetics of PQQ and PQQ containing enzymes" Adv. Microb. Physiol. 40:1-80, 1998. (on 5 alcohol dehydrogenases that utilize quinones); Maskos et al., "Mechanism of p-nitrosophenol reduction catalyzed by horse liver and human pi-alcohol dehydrogenase (ADH)" J. Biol. Chem. 269(50):31579-84, 1994 (example of mediator-catalyzed transfer of electrons from NADH to an electrode following NADH reduction 10 by an enzyme); and Pandey, "Tetracyanoquinodimethane-mediated flow injection analysis electrochemical sensor for NADH coupled with dehydrogenase enzymes" Anal. Biochem. 221(2):392-6, 1994. The corresponding reaction at the cathode in the cathode compartment can be any reaction that consumes the produced 15 electrons with a useful redox potential. Using oxygen, for example, the reaction can be: 2H 3 0 + + 1/2 02 + 2e- 3H 2 0 (2) Using reaction 2, the catholyte solution (an electrolyte used in the cathode compartment) can be buffered to account for 20 the consumption of hydrogen ions, hydrogen ion donating compounds can be supplied during operation of the fuel cell, or more preferably, the barrier between the anode and cathode compartments is sufficiently effective to deliver the neutralizing hydrogen ions (hydrogen ion or proton). 25 In one embodiment, the corresponding reaction at the cathode is:
H
2 0 2 + 2H+ + 2e <- 2H20 (10) The cathode reactions result in a net production of water, which, if significant, can be dealt with by, for example, 30 providing for space for overflow liquid, or providing for vapor phase exhaust. A number of electron acceptor molecules are WO 03/054995 PCT/US02/25148 60 often solids at operating temperatures or solutes in a carrier liquid, in which case the cathode chamber should be adapted to carry such non-gaseous material. Where, as possibly the case with hydrogen peroxide as the 5 electron acceptor molecule, the electron acceptor molecule can damage the polypeptides of the biocompatible membrane and any other species in the anode chamber, and a scavenger for such electron acceptor molecules can be used in the fuel cell to prevent peroxide or damaging electron acceptor molecules from 10 entering the anode chamber. Such a scavenger can be, for example, the enzyme catalase (2H 2 0 2 TM 2H 2 0 + 02), especially where conditions at the anode electrode are not effective to catalyze electron transfer to 02. Alternatively, the scavenger can be any noble metal, such as gold or platinum. Such a 15 scavenger, where an enzyme, can be covalently linked to a solid support material. Alternatively, a barrier between the anode chamber and the cathode chamber is provided and has at most limited permeability to hydrogen peroxide. Solid oxidants, such as calcium peroxide, potassium 20 perchlorite (KC10 4 ) or potassium permanganate (KMnO 4 ), can be used as the electron acceptor. The fuel cell operates within a temperature range appropriate for the operation of the redox enzyme or proton transporter. This temperature range typically varies with the 25 stability of the enzyme, and the source of the enzyme. To increase the appropriate temperature range, one can select the appropriate redox enzyme from a thermophilic organism, such as a microorganism isolated from a volcanic vent or hot spring. Additionally genetically modified enzymes can be used. 30 Nonetheless, preferred temperatures of operation of at least the first electrode are about 80 0 C or less, preferably 60 0 C or less.
WO 03/054995 PCT/US02/25148 61 Preferred fuel cells in accordance with the present invention include an anode compartment, a cathode compartment, an anode and a cathode, as well as a biocompatible membrane described herein including a polypeptide capable of 5 participating in the transfer of protons from one side of the membrane to the other. At least one of an electron transfer mediator and an electrode carrier are also found in the anode compartment. The fuel cells of the present invention can preferably generate at least about 10 milliwatts/cm 2 , more 10 preferably at least about 50 milliwatts/cm 2 and most preferably at least about 100 milliwatts/cm 2 over its useful life (there will be some diminished output toward the end of its life). The fuel cell will preferably generate such power density until its fuel ultimately runs out (unless they are refillable), but 15 generally at least eight hours, preferably one week, more preferably a month and most preferably six months or more. EXAMPLES Example No. 1 A solution useful for producing a biocompatible membrane in 20 accordance with the present invention was produced as follows: 7% w/v (70 mg) of a block copolymer (poly (2-methyloxazoline) polydimethyl siloxane-poly(2-methyl(oxazoline) having an average molecular weight of 2KD-5KD-2KD was dissolved in an 95%v/v / 5%v/v ethanol/water solvent mixture with stirring using a 25 magnetic stirrer. Six microliters of this solution was removed and mixed with four microliters of a solution containing 0.015% w/v dodecyl maltoside, 40 micrograms of Complex I (10 mg/ml) in water. This is then mixed. The resulting solution contains 4.2% w/v polymer, 55% EtOH v/v, 45% H 2 0 v/v, 0.06% w/v dodecyl 30 maltoside and protein/polymer ratio is 6% w/w. Example No. 2 WO 03/054995 PCT/USO2/25148 62 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as described in Example No. 1 with the following changes: less polypeptide solution was used so as to provide a final solution 5 including 0.015% w/v dodecyl maltoside and 1.5% w/w polypeptide relative to synthetic polymer materials. Example No. 3 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as 10 described in Example No. 1 with the following changes: less polypeptide solution was used so as to provide a final solution including 0.03% w/v dodecyl maltoside and the final solution contained 3.0% w/w polypeptide relative to synthetic polymer materials. 15 Example No. 4 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as described in Example No. 1 with the following changes: less polypeptide solution was used so as to provide a final solution 20 including 0.045w/v dodecyl maltoside and the final solution contained 4.5% w/w polypeptide relative to synthetic polymer materials. Example No. 5 A solution useful for producing a biocompatible membrane in 25 accordance with the present invention was prepared generally as described in Example No. 1 with the following changes: less polypeptide solution was used so as to provide a final solution including 0.0075w/v dodecyl maltoside and the final solution contained 0.75% w/w polypeptide relative to synthetic polymer 30 materials. Example No. 6 WO 03/054995 PCT/USO2/25148 63 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as described in Example No. 5 with the following changes: the synthetic polymer material was originally present in a solution 5 of 5.0% w/v. Sufficient polypeptide solution of the type described in Example 1 was added so as to produce a final solution including 0.0075% w/v dodecyl maltoside and 0.75% w/w polypeptide relative to synthetic polymer materials. Example No. 7 10 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally of the type described in Example No. 6 with the following changes: sufficient polypeptide solution as described in Example 1 was included so as to produce a final solution including 0.015% w/v 15 dodecyl maltoside and the final solution contained 1.5% w/w polypeptide relative to synthetic polymer materials. Example No. 8 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally of 20 the type described in Example No. 6 with the following changes: sufficient polypeptide solution as described in Example 1 was included so as to produce a final solution including 0.03% w/v dodecyl maltoside and the final solution contained 3% w/w polypeptide relative to synthetic polymer materials. 25 Example No. 9 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally of the type described in Example No. 6 with the following changes: sufficient polypeptide solution as described in Example 1 was 30 included so as to produce a final solution including 0.045% w/v dodecyl maltoside and the final solution contained 4.5% w/w polypeptide relative to synthetic polymer materials.
WO 03/054995 PCT/US02/25148 64 Example No. 10 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally of the type described in Example No. 6 with the following changes: 5 sufficient polypeptide solution as described in Example 1 was included so as to produce a final solution including 0.06% w/v dodecyl maltoside and the final solution contained 6.0% w/w polypeptide relative to synthetic polymer materials. Examples Nos. 11-15 10 Solutions useful for producing a biocompatible membrane in accordance with the present invention were prepared generally as described in Example Nos. 1-5 respectively except that the amount of the synthetic polymer material used in each solution was originally 10% w/v. When 6 microliters of that solution was 15 mixed with sufficient polypeptide solution of the type described in Example 1 a final solution was produced including .06, 0.15, .03, .045 and .0075% w/v dodecyl maltoside and 6.0, 1.5, 3.0, 4.5 and 0.75% w/w polypeptide relative to synthetic polymer materials, respectively. 20 Example No. 16 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as described in Example No. 3, however, the solvent used to dissolve the synthetic polymer material included ethanol, 25% 25 methanol v/v and the amount of water indicated in Example No. 3. Sufficient polypeptide solution was used so as to provide a final solution including 0.03% w/v dodecyl maltoside and 3.0% w/w polypeptide relative to synthetic polymer materials. Example No. 17 30 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as described in Example No. 2, however, the solvent used to WO 03/054995 PCT/US02/25148 65 dissolve the synthetic polymer material included 47.5% v/v ethanol, 2.5% v/v water, 25% v/v Tetrahydrofuran ("THF"), 25% v/v dichloromethane. Sufficient polypeptide solution was used so as to provide a final solution including 0.015.% w/v dodecyl 5 maltoside and 1.5% w/w polypeptide relative to synthetic polymer materials. Example No. 18 A solution useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally 10 as described in Example No. 6, however, the solvent used to dissolve the synthetic polymer material included 9.5% v/v ethanol, 0.5% v/v water, 40% v/v acetone, and 40% v/v hexane. Examples Nos. 19-24 Solutions useful for producing a biocompatible membrane in 15 accordance with the present invention were prepared generally as described in Example Nos. 11-15 above, however, the final concentration of dodecyl maltoside was 0.15% w/v. Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in 20 Example No. 4 above, however, the balance of the surfactant used in the polypeptide solution is dodecyl P-D-glucopyranoside and the final concentration of the surfactants is 0.15% w/v. Example No. 26 A solution useful for producing a biocompatible membrane in 25 accordance with the present invention was prepared generally as described in Example No. 9 above, however, the surfactant used in the polypeptide solution included a mixture of a polymeric surfactant sold under the trademark PLURONIC L101, lot WPDX-522B from BASF, Ludwigshafen Germany and the same concentration of 30 dodecyl maltoside specified in Example No. 9. The polymeric surfactant was diluted to 0.1%v/v of its supplied concentration in the final solution.
WO 03/054995 PCT/US02/25148 66 Example No. 27 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as described in Example No. 2 above, however the surfactant used in 5 the polypeptide solution included a mixture of a polymeric surfactant sold under the trademark DISPERPLAST, lot no. 31J022 from BYK Chemie, Wallingford CT and the same concentration of dodecyl maltoside specified in Example No. 2. The polymeric surfactant was diluted to 0.135%v/v of the supplied 10 concentration in the final solution. Examples Nos. 28-32 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Example Nos. 6-10 respectively, however, the 15 synthetic polymer material used can be a poly(2 methyloxazoline)-polydimethylsiloxane-poly(2-methyloxazoline) (5% w/v) having an average molecular weight of 3kD-7kD-3kD. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final 20 solution is produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 33-38 25 Solutions useful for producing a biocompatible membrane in accordance with the present invention were prepared generally as described in Example Nos. 1-5 respectively, however, the synthetic polymer material used was a mixture of two block copolymers, both of which were poly(2-methyloxazoline) 30 polydimethylsiloxane-poly(2-methyloxazoline), (total 7% w/v) one of which having an average molecular weight of 2kD-5kD-2kD and the other lkD-2kD-lkD and the ratio of the first block copolymer WO 03/054995 PCT/USO2/25148 67 to the second was about 67% to 33% of the total polymer used w/w. When 6 microliters of that solution was mixed with sufficient polypeptide solution of the type described in Example 1 a final solution was produced including 0.06, 0.015, 0.030, 5 0.045 and 0.0075% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 39-43 Solutions useful for producing a biocompatible membrane in 10 accordance with the present invention can be prepared generally as described in Example Nos. 11-15 respectively, however, the synthetic polymer material used can be a mixture of two block copolymers, both of which are poly(2-methyloxazoline) polydimethylsiloxane-poly(2-methyloxazoline), (10% w/v) one of 15 which having an average molecular weight of lkD-2kD-lkD and the other 3kD-7kD-3kD and the ratio of the first block copolymer to the second being about 33% to 67% of the total polymer used w/w. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final 20 solution is produced including 0.075, 0.15, 0.30, 0.45 and 0.60% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 44-48 25 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 6-10 respectively, however, the synthetic polymer material used can be a mixture of two block copolymers, both of which are poly(2-methyloxazoline) 30 polydimethylsiloxane-poly(2-methyloxazoline), (5% w/v) one of which having an average molecular weight of 2kD-5kD-2kD and the other 3kD-7kD-3kD and the ratio of the first block copolymer to WO 03/054995 PCT/USO2/25148 68 the second being about 33% to 67% of the total polymer used w/w. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final solution is produced including 0.0075, 0.015, 0.030, 0.045 and 5 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 49-53 Solutions useful for producing a biocompatible membrane in 10 accordance with the present invention can be prepared generally as described in Example Nos. 1-5 respectively, however, the synthetic polymer material used can be a mixture of two block copolymers, both of which are poly(2-methyloxazoline) polydimethylsiloxane-poly(2-methyloxazoline), (7% w/v) one of 15 which having an average molecular weight of 2kD-5kD-2kD and the other 3kD-7kD-3kD and the ratio of the first block copolymer to the second being about 67% to 33% of the total polymer used w/w. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final 20 solution is produced including 0.06, 0.015, 0.030, 0.045 and 0.0075% w/v dodecyl maltoside and 6.0, 1.5, 3.0, 4.5 and .025% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 54-58 25 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 1-5 respectively, however, the synthetic polymer used can be a mixture of poly(2 methyloxazoline)-polydimethylsiloxane- poly(2-methyloxazoline) 30 (7% w/v) having an average molecular weight of 2kD-5kD-2kD in a solvent of 95% ethanol, 5% water mixed with a solution of 23.5% w/v polyethyleneglycol with an average molecular weight of WO 03/054995 PCT/US02/25148 69 approximately 3,300 Daltons in water in the proportion of 85% triblock copolymer solution, 15% polyethyleneglycol solution v/v. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 5 1 a final solution is produced including 0.06, 0.015, 0.030, 0.045 and 0.0075% w/v dodecyl maltoside and 6.0, 1.5, 3.0, 4.5 and .75% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 59-63 10 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as described in Example No. 12, however, the synthetic polymer used was a mixture of 10% w/v of poly(2-methyloxazoline) polydimethylsiloxane- poly(2-methyloxazoline) having an average 15 molecular weight of 2kD-5kD-2kD in a solvent of 95% ethanol, 5% water mixed with a solution of 23.5% w/v polyethyleneglycol with an average molecular weight of approximately 8,000 Daltons in water in the proportion of 85% triblock copolymer solution, 15% polyethyleneglycol solution v/v. When 6 microliters of that 20 solution was mixed with sufficient polypeptide solution of the type described in Example 1 a final solution was produced including 0.15% w/v dodecyl maltoside and 1.5% w/w polypeptide relative to synthetic polymer materials. Similar solutions can be made using the procedures of examples 11 and 13-15. 25 Examples Nos. 64-68 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 28-32 respectively, however, the synthetic polymer used can be a mixture of 5% w/v of poly(2 30 methyloxazoline)-polydimethylsiloxane- poly(2-methyloxazoline) having an average molecular weight of 3kD-7kD-3kD in a solvent of 95% ethanol, 5% water mixed with a solution of 23.5% w/v WO 03/054995 PCT/US02/25148 70 polyethyleneglycol with an average molecular weight of approximately 3,300 Daltons in water in the proportion of 85% triblock copolymer solution, 15% polyethyleneglycol solution v/v. When 6 microliters of that solution is mixed with 5 sufficient polypeptide solution of the type described in Example 1 a final solution is produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer materials respectively. 10 Examples Nos. 69-73 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 1-5 respectively, however, the synthetic polymer used can be a mixture of 7% w/v of poly(2 15 methyloxazoline)-polydimethylsiloxane- poly(2-methyloxazoline) having an average molecular weight of 3kD-7kD-3kD in a solvent of 95% ethanol, 5% water mixed with a solution of 23.5% w/v polyethyleneglycol with an average molecular weight of approximately 8,000 Daltons in water in the proportion of 85% 20 triblock copolymer solution, 15% polyethyleneglycol solution v/v. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final solution is produced including 0.060, 0.015, 0.030, 0.045 and 0.0075% w/v dodecyl maltoside and 6.0, 1.5, 3.0, 4.5 25 and 0.75% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 74-78 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally 30 as described in Examples Nos. 6-10 respectively, however the synthetic polymer used can be a mixture of 5% w/v of poly(2 methyloxazoline)-polydimethylsiloxane- poly(2-methyloxazoline) WO 03/054995 PCT/US02/25148 71 having an average molecular weight of 2kD-5kD-2kD in a solvent of 50%v/v acetone, 50%v/v heptane mixed with a solution of 5% w/v polystyrene of about 250,000 in molecular weight in 50%v/v acetone, 50%v/v octane in the proportion of 80%v/v block 5 copolymer, 20% v/v polystyrene. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final solution is produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide 10 relative to synthetic polymer materials respectively. Examples Nos. 79-83 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 1-5 respectively, however, the 15 synthetic polymer used can be a mixture of 7% w/v of poly(2 methyloxazoline)-polydimethylsiloxane- poly(2-methyloxazoline) having an average molecular weight of 2kD-5kD-2kD in a solvent of 95% ethanol, 5% water mixed with a solution of 5% w/v of polymethylmethacrylate-polydimethylsiloxane 20 polymethylmethacrylate having an average molecular weight of 4kD-8kD-4kD in a solvent of 50%v/v THF, 50%v/v dichloromethane in the proportion of 66%v/v to 33%v/v, respectively. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final 25 solution is produced including 0.06, 0.015, 0.030, 0.045 and 0.0075% w/v dodecyl maltoside and 6.0, 1.5, 3.0, 4.5 and 0.075% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 84-88 30 Solutions useful for producing a biocompatible membrane in accordance with the present invention were prepared generally as described in Examples Nos. 11-15 respectively, however, the WO 03/054995 PCT/US02/25148 72 synthetic polymer material used was 10% w/v of sulfonated styrene/ethylene-butylene/sulfonated styrene, supplied as Protolyte® A700, lot number LC-29/60-011 by Dais Analytic, Odessa, FL in solvent as supplied, diluted 50%v/v with ethanol 5 containing 5%v/v water. When 6 microliters of that solution was mixed with sufficient polypeptide solution of the type described in Example 1 a final solution was produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic 10 polymer materials respectively. Example No. 89 A solution useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Example No. 84 however, the solvent used to 15 dilute the synthetic polymer material can include 50% v/v Tetrahydrofuran ("THF"), 50% v/v dichloromethane. Examples Nos. 90-94 Solutions useful for producing a biocompatible membrane in accordance with the present invention were prepared generally as 20 described in Examples Nos. 84-88 above, however, the final concentration of dodecyl maltoside was 0.15% w/v. Example No. 95 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally 25 as described in Example No. 85 above, however, the surfactant used in the polypeptide solution can include a mixture of dodecyl -D-glucopyranoside and dodecyl maltoside and the final concentration of the surfactants is 0.15% w/v. Example No. 96 30 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as described in Example No. 87 above, however, the surfactant used WO 03/054995 PCT/USO2/25148 73 in the polypeptide solution included a mixture of a polymeric surfactant sold under the trademark PLURONIC L101, lot WPDX-522B from BASF, Ludwigshafen Germany and the same concentration of dodecyl maltoside specified in Example No. 87. The polymeric 5 surfactant was diluted to 0.1%v/v of its supplied concentration in the final solution. Example No. 97 A solution useful for producing a biocompatible membrane in accordance with the present invention was prepared generally as 10 described in Example No. 88 above, however, the surfactant used in the polypeptide solution included a mixture of a polymeric surfactant sold under the trademark DISPERPLAST, lot no. 31J022 from BYK Chemie, Wallingford CT and the same concentration of dodecyl maltoside specified in Example No. 88. The final 15 concentration of the polymeric surfactant was diluted to 0.135%v/v of the supplied concentration in the final solution. Examples No. 98-102 Solutions useful for producing a biocompatible membrane in accordance with the present invention were prepared generally as 20 described in Examples Nos. 84-88 respectively, however, the synthetic polymer material used was a mixture of two block copolymers, one of which was 10% w/v of sulfonated styrene/ethylene-butylene/sulfonated styrene, supplied as Protolyte® A700, lot number LC-29/60-011 by Dais Analytic, 25 Odessa, FL in solvent as supplied, diluted 50%v/v with ethanol containing 5%v/v water, the other of which was 5% w/v of poly(2-methyloxazoline)-polydimethylsiloxane-poly(2 methyloxazoline) having an average molecular weight of 2kD-5kD 2kD and the ratio of the first block copolymer to the second was 30 about 67% to 33% of the total polymer used w/w. When 6 microliters of that solution was mixed with sufficient polypeptide solution as described in Example 1 a final solution WO 03/054995 PCT/US02/25148 74 was produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer materials respectively. 5 Examples Nos. 103-107 Solutions useful for producing a biocompatible membrane in accordance with the present invention were prepared generally as described in Examples Nos. 84-88 respectively, however, the synthetic polymer material used was a mixture of two block 10 copolymers, one of which was 10% w/v of sulfonated styrene/ethylene-butylene/sulfonated styrene, supplied as Protolyte® A700, lot number LC-29/60-011 by Dais Analytic, Odessa, FL in solvent as supplied, diluted 50%v/v with ethanol containing 5%v/v water, the other of which was 5% w/v of 15 poly(2-methyloxazoline)-polydimethylsiloxane-poly(2 methyloxazoline) having an average molecular weight of 2kD-5kD 2kD and the ratio of the first block copolymer to the second was about 33% to 67% of the total polymer used w/w. When 6 microliters of that solution was mixed with sufficient 20 polypeptide solution as described in Example 1 a final solution was produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer materials respectively. 25 Examples Nos. 108-112 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 103-107 respectively, however, the synthetic polymer material used can be a mixture of two block 30 copolymers, one of which is 10% w/v of sulfonated styrene/ethylene-butylene/sulfonated styrene, supplied as Protolyte® A700, lot number LC-29/60-011 by Dais Analytic, WO 03/054995 PCT/USO2/25148 75 Odessa, FL in solvent as supplied, diluted 50%v/v with ethanol containing 5%v/v water, the other of which is 5% w/v of polymethylmethacrylate-polydimethylsiloxane polymethylmethacrylate having an average molecular weight of 5 4kD-8kD-4kD in a solvent mixture of 50%v/v THF, 50% v/v dichloromethane, the ratio of the first block copolymer to the second being about 67% to 33% of the total polymer used w/w. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final 10 solution is produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 113-117 15 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 103-107 respectively, however, the synthetic polymer material used can be a mixture of two block copolymers, one of which is 10% w/v of sulfonated 20 styrene/ethylene-butylene/sulfonated styrene, supplied as Protolyte® A700, lot number LC-29/60-011 by Dais Analytic, Odessa, FL in solvent as supplied, diluted 50%v/v with ethanol containing 5%v/v water, the other of which is 5% w/v of polymethylmethacrylate-polydimethylsiloxane 25 polymethylmethacrylate having an average molecular weight of 4kD-8kD-4kD in a solvent mixture of 50%v/v THF, 50% v/v dichloromethane, the ratio of the first block copolymer to the second being about 33% to 67% of the total polymer used w/w. When 6 microliters of that solution is mixed with sufficient 30 polypeptide solution of the type described in Example 1 a final solution is produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% WO 03/054995 PCT/US2/25148 76 w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 118-122 Solutions useful for producing a biocompatible membrane in 5 accordance with the present invention were prepared generally as described in Examples Nos. 84-88 respectively, however, the synthetic polymer material used was a mixture of 10% w/v of sulfonated styrene/ethylene-butylene/sulfonated styrene, supplied as Protolyte® A700, lot number LC-29/60-011 by Dais 10 Analytic, Odessa, FL in solvent as supplied, diluted 50%v/v with ethanol containing 5%v/v water mixed with a solution of 23.5% w/v polyethyleneglycol with an average molecular weight of approximately 3,300 Daltons in water in the proportion of 85% triblock copolymer solution, 15% polyethyleneglycol solution 15 v/v. When 6 microliters of that solution was mixed with sufficient polypeptide solution of the type described in Example 1 a final solution was produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer materials 20 respectively. Examples Nos. 123-127 Solutions useful for producing a biocompatible membrane in accordance with the present invention were prepared generally as described in Examples Nos. 84-88 respectively, however, the 25 synthetic polymer material used was a mixture of 10% w/v of sulfonated styrene/ethylene-butylene/sulfonated styrene, supplied as Protolyte® A700, lot number LC-29/60-011 by Dais Analytic, Odessa, FL in solvent as supplied, diluted 50%v/v with ethanol containing 5%v/v water mixed with a solution of 23.5% 30 w/v polyethyleneglycol with an average molecular weight of approximately 8,000 Daltons in water in the proportion of 85% triblock copolymer solution, 15% polyethyleneglycol solution WO 03/054995 PCT/USO2/25148 77 v/v. When 6 microliters of that solution was mixed with sufficient polypeptide solution of the type described in Example 1 a final solution was produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 5 and 6.0% w/w polypeptide relative to synthetic polymer materials respectively. Examples Nos. 128-132 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally 10 as described in Examples Nos. 6-10 respectively, however, the synthetic polymer material used can be 5% w/v of polymethylmethacrylate-polydimethylsiloxane polymethylmethacrylate having an average molecular weight of 4kD-8kD-4kD in a solvent mixture of 50%v/v THF, 50% v/v 15 dichloromethane. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final solution is produced including 0.0075, 0.015, 0.030, 0.045 and 0.060% w/v dodecyl maltoside and 0.75, 1.5, 3.0, 4.5 and 6.0% w/w polypeptide relative to synthetic polymer 20 materials respectively. Examples Nos. 133-134 Solutions useful for producing a biocompatible membrane in accordance with the present invention were prepared generally as described in Examples Nos. 6 and 7 respectively, however, the 25 synthetic polymer material used was 3.2% w/v of polystyrene polybutadiene-polystyrene, supplied as Stryolux® 3G55, lot 7453064P by BASF, Ludwigshafen Germany in a 50%/50%v/v mixture of acetone and hexane. When 6 microliters of that solution was mixed with sufficient polypeptide solution of the type described 30 in Example 1 a final solution was produced including 0.0075 and 0.015% w/v dodecyl maltoside and 0.75 and 1.5% w/w polypeptide relative to synthetic polymer materials respectively.
WO 03/054995 PCT/USO2/25148 78 Examples Nos. 135-136 Solutions useful for producing a biocompatible membrane in accordance with the present invention were prepared generally as described in Examples Nos. 6 and 7 respectively, however, the 5 synthetic polymer material used was 3.2% w/v of polystyrene polybutadiene-polystyrene, supplied as Stryolux® 3G55, lot 7453064P by BASF, Ludwigshafen Germany in a 50%/50%v/v mixture of acetone and heptane. When 6 microliters of that solution was mixed with sufficient polypeptide solution of the type described 10 in Example 1 a final solution was produced including 0.0075 and 0.015% w/v dodecyl maltoside and 0.75 and 1.5% w/w polypeptide relative to synthetic polymer materials respectively. Example Nos. 137-138 Solutions useful for producing a biocompatible membrane in 15 accordance with the present invention were prepared generally as described in Examples Nos. 135 and 136 respectively, however, the synthetic polymer material used was 5% w/v of polystyrene polybutadiene-polystyrene, supplied as Stryolux® 3G55, lot 7453064P by BASF, Ludwigshafen Germany in a 50%/50%v/v mixture 20 of acetone and heptane. When 6 microliters of that solution was mixed with sufficient polypeptide solution of the type described in Example 1 a final solution was produced including 0.0075 and 0.015% w/v dodecyl maltoside and 0.75 and 1.5% w/w polypeptide relative to synthetic polymer materials respectively. 25 Examples Nos. 139-141 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 6-8 respectively, however, the synthetic polymer material used can be a mixture of 5% w/v of 30 polystyrene-polybutadiene-polystyrene, supplied as Stryolux® 3G55, lot 7453064P by BASF, Ludwigshafen Germany in a 50%/50%v/v mixture of acetone and hexane and 5% w/v poly(2- WO 03/054995 PCT/US02/25148 79 methyloxazoline)-polydimethylsiloxane-poly(2-methyloxazoline) having an average molecular weight of 2kD-5kD-2kD in the same solvent in the proportion of about 80%v/v to 20% v/v, respectively. When 6 microliters of that solution is mixed with 5 sufficient polypeptide solution of the type described in Example 1 a final solution is produced including 0.0075, 0.015, and 0.030% w/v dodecyl maltoside and 0.75, 1.5 and 3.0% w/w polypeptide relative to synthetic polymer materials respectively. 10 Examples Nos. 142-145 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 139-141 respectively, however, the synthetic polymer material used can be a mixture of 5% w/v of 15 polystyrene-polybutadiene-polystyrene, supplied as Stryolux® 3G55, lot 7453064P by BASF, Ludwigshafen Germany in a 50%/50%v/v mixture of acetone and hexane and 5% w/v poly(2 methyloxazoline)-polydimethylsiloxane-poly(2-methyloxazoline) having an average molecular weight of 3kD-7kD-3kD in the same 20 solvent in the proportion of about 80%v/v to 20% v/v, respectively. When 6 microliters of that solution is mixed with sufficient polypeptide solution of the type described in Example 1 a final solution is produced including 0.0075, 0.015, and 0.030% w/v dodecyl maltoside and 0.75, 1.5 and 3.0% w/w 25 polypeptide relative to synthetic polymer materials respectively. Examples Nos. 146-290 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally 30 as described in Examples Nos. 1-145, respectively, however, the polypeptide solution mixed with the synthetic polymer can be a solution of 10mg/ml of Succinate:ubiquinone oxidoreductase WO 03/054995 PCT/US2/25148 80 (Complex II) in water which also can include 0.15% Thesit (polyoxyethylene(9)dodecyl ether, C 12
E
9 ) available from Roche, Indianapolis, IN. This surfactant replaces, in general, the dodecyl maltoside in examples 1-145 in similar concentration. 5 Examples Nos. 291-435 Solutions useful for producing a biocompatible membrane in accordance with the present invention can be prepared generally as described in Examples Nos. 1-145, respectively, however, the polypeptide solution used to dilute the synthetic polymer can be 10 a solution of 10mg/ml of Nicotinamide Nucleotide Transhydrogenase in water which also can include 0.15% Triton X 100. This surfactant replaces, in general, the dodecyl maltoside in examples 1-145 in similar concentration. Furthermore, in examples 1-145 which include dodecyl -D 15 glucopyranoside, this detergent can be substituted with Nonidet P-40 in similar concentration. Example 436 Membranes are formed on a dielectric perforated support. The support is made of KAPTON available from DuPont (1 mil 20 thick) and is laser-drilled with apertures of 100 micrometers in diameter and 1 mil deep. The array of apertures can have a density as high as 1,700 apertures/cm 2 . A biocompatible membrane is formed across the apertures using the PEG 8000/PROTOLYTE A700 membrane described in detail previously. The resulting final 25 solution containing the block copolymer, stabilizing polymer and polypeptide is then deposited onto the substrate in a manner that completely covered the apertures, dropwise by pipet, 4 microliters at a time. The solvent was allowed to evaporate at room temperature under a hood. The membrane-support assembly 30 was stored in a vacuum chamber prior to use. A test device, in this case a fuel cell, was constructed from DELRAN plastic. The membrane-support assembly produced as WO 03/054995 PCT/US02/25148 81 described above was sealed in place within the fuel cell with rubber gaskets to form two chambers, an anode compartment and a cathode compartment. The anode and cathode compartments were then filled (20 ml in each) with an aqueous electrolyte (IM TMA 5 formate pH 10 in the anode compartment and 100 mM TMA-sulfate, pH 2.0, containing 1% hydrogen peroxide in the cathode compartment). A titanium foil anode was connected in parallel to an electronically varied load. A computer with an analog/digital board was used to measure current and voltage output. The 10 circuit was completed by wiring these elements to a graphite cathode electrode in the cathode compartment. The titanium foil anode was immersed in the anolyte. Also contained in the anode compartment was 5% v/v methanol as fuel, 12.5mM NAD+ was used as electron carrier, lM hydroquinone was 15 used as electron transfer mediator, yeast alcohol dehydrogenase (5,000 units), aldehyde dehydrogenase (10 units) and formate dehydrogenase (100 units) were used as soluble enzymes. Current and voltage were produced consistent with the function of Complex I embedded in the biocompatible membrane in 20 translocating protons from the anode compartment to the cathode compartment, even against the proton concentration gradient. Peak current density was 158 mA/cm 2 . The membrane was stable for approximately 3 days. By comparison, in another cell formed using the same 25 components and concentrations as above, with the exception that the membrane-forming solution did not include PEG 8000, the peak current density was similar. However, the membrane integrity was limited to 10-12 hours. Membrane failure was assessed via visible flow of the mediator into the cathode compartment. 30 In the absence of Complex I in the membrane, the Protolyte block copolymer nonetheless forms membranes which are modestly permeable to protons. The use of such membranes formed without WO 03/054995 PCT/US02/25148 82 Complex I in a fuel cell, constructed similarly to those above, with the exception that 300 mM PMS was present in the anode as the electron transfer mediator instead of hydroxyquinone, produced maximally 4mA/cm 2 for only a matter of approximately 5 5 minutes before decreasing in output rapidly. INDUSTRIAL APPLICABILITY The invention relates to the industries that produce and use membranes including, without limitation, the fuel cell industry. The invention is also applicable to the industries 10 that use fuel cells such as the automotive and electronic industries. Although the invention herein has been described with reference to particular embodiments, it is to be understood that these embodiments are merely illustrative of the principles and 15 applications of the present invention. It is therefore to be understood that numerous modifications may be made to the illustrative embodiments and that other arrangements may be devised without departing from the spirit and scope of the present invention as defined by the appended claims. 20

Claims (44)

1. A stabilized biocompatible membrane comprising: at least one layer of a synthetic polymer material having a first side and a second side and at least one polypeptide associated 5 therewith, said polypeptide capable of participating in a chemical reaction, participating in the transporting of molecules, atoms, protons or electrons from said first side of said at least one layer to said second side of said at least one layer, or participating in the formation of molecular structures 10 that facilitate such reactions or transport, and wherein said synthetic polymer material includes at least one stabilizing polymer.
2. The biocompatible membrane of claim 1 wherein said at least one polypeptide can participate in transporting protons 15 from said first side of said at least one layer to said second side of said at least one layer.
3. The biocompatible membrane of claim 2 wherein said at least one polypeptide can participate in transporting protons from said first side of said at least one layer to said second 20 side of said at least one layer and can facilitate the passage of current across said layer to a degree at least greater than that which would using an identical biocompatible membrane without said polypeptide.
4. The biocompatible membrane of claim 3 wherein said at 25 least one polypeptide can participate in transporting protons from said first side of said at least one layer to said second side of said at least one layer so as to be capable of providing at least about 10 picoamps/cm 2 of current density.
5. The biocompatible membrane of claim 4 wherein said at 30 least one polypeptide can participate in transporting protons from said first side of said at least one layer to said second WO 03/054995 PCT/USO2/25148 84 side of said at least one layer so as to be capable of providing at least about 10 milliamps/cm 2 of current density.
6. The biocompatible membrane of claim 1 wherein said at least one polypeptide is embedded in said at least one layer. 5
7. The biocompatible membrane of claim 1 wherein said at least one polypeptide is present in an amount of at least about 0.01% by weight of said biocompatible membrane.
8. The biocompatible membrane of claim 7 wherein said at least one polypeptide is present in an amount of at least about 10 5% by weight of said biocompatible membrane.
9. The biocompatible membrane of claim 8 wherein said at least one polypeptide is present in an amount of at least about 10% by weight of said biocompatible membrane.
10. The biocompatible membrane of claim 1 wherein said 15 synthetic polymer material includes at least one block copolymer
11. The biocompatible membrane of claim 10 wherein said at least one block copolymer has a hydrophobic content that exceeds its hydrophilic content.
12. The biocompatible membrane of claim 10 wherein said at 20 least one block copolymer has at least one block having an average molecular weight of between about 1,000 and 15,000 daltons.
13. The biocompatible membrane of claim 12 wherein said at least one block copolymer has at least a second block having an 25 average molecular weight of between about 1,000 and 20,000 daltons.
14. The biocompatible membrane of claim 1 wherein said synthetic polymer material is provided in an amount of at least about 50% by weight based on weight of said biocompatible 30 membrane.
15. The biocompatible membrane of claim 14 wherein said synthetic polymer material is provided in an amount of at least WO 03/054995 PCT/US02/25148 85 about 50% to about 99% by weight based on weight of said biocompatible membrane.
16. The biocompatible membrane of claim 1, wherein said synthetic polymer material includes a mixture of a plurality of 5 block copolymers.
17. The biocompatible membrane of claim 1 wherein said at least one polypeptide can participate in a redox reaction.
18. The biocompatible membrane of claim 1 wherein said at least one polypeptide has the ability to participate in a redox 10 reaction or the transporting of molecules, atoms, protons or electrons from said first side of said at least one layer to said second side of said at least one layer.
19. The biocompatible membrane of claim 18 wherein said at least one polypeptide has both the ability to participate in a 15 redox reaction and the transporting of molecules, atoms, protons or electrons from said first side of said at least one layer to said second side of said at least one layer.
20. The biocompatible membrane of claim 1 wherein said at least one stabilizing polymer is a polymer capable of forming a 20 plurality of hydrogen bonds.
21. The biocompatible membrane of claim 1 wherein said at least one stabilizing polymer is provided in an amount of up to about 30% based on the weight of said synthetic polymer material. 25
22. The biocompatible membrane of claim 21 wherein said at least one stabilizing polymer is provided in an amount of between about 5 and about 20% based on the weight of the synthetic polymer material.
23. The biocompatible membrane of claim 1 wherein said at 30 least one stabilizing polymer is hydrophilic.
24. A biocompatible membrane comprising: at least one layer of a synthetic polymer material having a first side and a WO 03/054995 PCT/USO2/25148 86 second side, said synthetic polymer material being present in an amount of at least about 5% by weight based on weight of the finished membrane and at least one polypeptide embedded therein and being present in an amount of at least about 10% by weight 5 of said biocompatible membrane, said polypeptide having the ability to participate in a redox reaction or in the transporting of protons from said first side of said at least one layer to said second side of said at least one layer and being capable of providing at least about 10 milliamps/cm 2 of 10 current density, and wherein said synthetic polymer material includes at least one stabilizing polymer.
25. A fuel cell comprising: an anode compartment including an anode; a cathode compartment including a cathode; and disposed within said anode compartment, within said cathode 15 compartment, or between said anode compartment and said cathode compartment, at least one stabilized biocompatible membrane having at least one layer of a synthetic polymer material which includes an anode side and a cathode side and at least one polypeptide associated therewith, said polypeptide capable of 20 participating in a chemical reaction, participating in the transporting of protons from said anode side of said at least one layer to said cathode side of said at least one layer or participating in the formation of molecular structures that facilitate such reactions or transport, and wherein said 25 synthetic polymer material includes at least one stabilizing polymer
26. The fuel cell of claim 25 wherein, when said anode and said cathode are placed into electrical contact though a circuit, 10 milliwatts/cm 2 are generated. 30
27. The fuel cell of claim 26 wherein, when said anode and said cathode are placed into electrical contact though a circuit, 50 milliwatts/cm 2 are generated. WO 03/054995 PCT/USO2/25148 87
28. The fuel cell of claim 27 wherein, when said anode and said cathode are placed into electrical contact though a circuit, 100 milliwatts/cm 2 are generated.
29. The fuel cell of claim 25, further comprising: at 5 least one electron carrier within said anode compartment.
30. The fuel cell of claim 25, further comprising: at least one second polypeptide within said anode compartment capable of liberating protons or electrons from an electron carrier. 10
31. The fuel cell of claim 25, further comprising: at least one transfer mediator within said anode compartment capable of transferring electrons to said anode.
32. The fuel cell of claim 25, wherein said at least one biocompatible membrane is disposed between said anode and said 15 cathode.
33. The fuel cell of claim 25, further comprising: a dielectric material disposed between said anode and said cathode that will permit the flow of protons from said anode compartment to said cathode compartment. 20
34. The fuel cell of claim 25, further comprising a first electron transfer mediator disposed in said anode compartment is capable of receiving at least one electron from an electron carrier disposed in said anode compartment and transferring said at least one electron to a second electron carrier, a second 25 electron transfer mediator or said anode.
35. The fuel cell of claim 25, further comprising at least one fuel disposed within said anode compartment.
36. The fuel cell assembly of claim 35, wherein said fuel is an organic compound. 30
37. The fuel cell of claim 25, wherein said polypeptide has the ability to participate in a redox reaction or in the WO 03/054995 PCT/US02/25148 88 transporting of protons from said anode side of said at least one layer to said cathode side of said at least one layer.
38. The fuel cell of claim 37, wherein said polypeptide has the ability to participate in both a redox reaction and in 5 the transporting of protons from said anode side of said at least one layer to said cathode side of said at least one layer.
39. A solution useful for producing a biocompatible membrane comprising: at least one synthetic polymer material, said synthetic polymer material being present in an amount of 10 between about 1 and about 30% w/v, at least one stabilizing polymer present in an amount of up to about 30% by weight of the weight of said synthetic polymer material, at least one polypeptide, in an amount of between at least about 0.001 and about 10.0% w/v said polypeptide capable of participating in a 15 chemical reaction, participating in the transporting molecules, atoms, protons or electrons or participating in the formation of molecular structures that facilitate such reactions or transport, in a solvent system including both organic solvents and water. 20
40. The solution of claim 39 further comprising: at least one detergent in an amount of between about 0.01 and about 1.0% v/v.
41. The solution of claim 39, wherein said at least one polypeptide has the ability to participate in a redox reaction 25 or the transporting of protons.
42. The solution of claim 41, wherein said at least one polypeptide has both the ability to participate in a redox reaction and the transporting of protons.
43. The solution of claim 41, wherein said at least one 30 polypeptide has the ability to participate in transporting of protons. WO 03/054995 PCT/USO2/25148 89
44. The solution of claim 39, wherein said synthetic polymer material includes at least one block copolymer.
AU2002331014A 2001-12-11 2002-08-08 Stabilized biocompatible membranes of block copolymers and fuel cells produced therewith Abandoned AU2002331014A1 (en)

Applications Claiming Priority (21)

Application Number Priority Date Filing Date Title
US33911701P 2001-12-11 2001-12-11
US60/339,117 2001-12-11
US35736702P 2002-02-15 2002-02-15
US35748102P 2002-02-15 2002-02-15
US60/357,481 2002-02-15
US60/357,367 2002-02-15
AU2002303344 2002-04-15
US10/123,008 US20030087141A1 (en) 2001-04-13 2002-04-15 Dual membrane fuel cell
US10/123,021 US20030198858A1 (en) 2001-04-13 2002-04-15 Enzymatic fuel cell with membrane bound redox enzyme
US10/123,021 2002-04-15
US10/123,008 2002-04-15
PCT/US2002/011719 WO2002086999A1 (en) 2001-04-13 2002-04-15 Enzymatic fuel cell
US10/123,022 2002-04-15
US10/123,020 US20030087144A1 (en) 2001-04-13 2002-04-15 Enzymatic fuel cell with fixed dehydrogenase enzyme
US10/123,039 2002-04-15
US10/123,020 2002-04-15
US10/123,022 US20030198859A1 (en) 2002-04-15 2002-04-15 Enzymatic fuel cell
US10/123,039 US20030129469A1 (en) 2001-04-13 2002-04-15 Fuel cell with fuel concentrate metering
US10/213,477 2002-08-07
US10/213,477 US20030049511A1 (en) 2001-04-13 2002-08-07 Stabilized biocompatible membranes of block copolymers and fuel cells produced therewith
PCT/US2002/025148 WO2003054995A1 (en) 2001-12-11 2002-08-08 Stabilized biocompatible membranes of block copolymers and fuel cells produced therewith

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