DE10221435B4 - Enzyme electrode arrangement, a method for the production thereof and a biosensor arrangement comprising this enzyme electrode arrangement - Google Patents

Abstract

Enzyme electrode assembly comprising in the following order
a substrate with a surface roughness in the range from 20 nm to 10 μm, a metal electrode,
an ultra thin semipermeable membrane with a thickness in the range of 10 to 100 nm and
at least one enzyme membrane.

Description

The The present invention relates to an enzyme electrode assembly comprising a substrate with a surface roughness in the range from 20 nm to 10 μm, a metal electrode with an ultra-thin semipermeable membrane a thickness in the range from 10 to 100 nm and at least one enzyme membrane, a process for their preparation and this enzyme electrode arrangement comprehensive biosensor arrangement.

The Detection of biomolecules is for many applications in the researching pharmaceutical industry and in the clinical diagnostics of central importance. Usually done this evidence about a so-called affinity reaction, at the complementary Bind analytes specifically to each other. Basically there is the problem that the analyte to be detected only in the smallest concentrations in one Test approach available stands. Mostly is the sensitivity today's measuring systems too low to directly detect these low concentrations of an analyte. One therefore uses amplification systems that carry the biological signal so indirectly reinforce that the lower detection limit of the measuring apparatus preferably far exceeded becomes.

affinity sensors are special biosensors that detect any type of biomolecular from highly specific affinity partners use, such as Antibody-antigen, Nucleic acid complementary nucleic acid or Receptor ligand. Bio and affinity sensors generally settle composed of two components: the biological component for the specific Detection of an analyte and the detector component, the transducer (i.e. signal or transducer), who capture this biomolecular recognition reaction and convert it into an evaluable one Implement signal. The selective biological components (e.g. nucleic acids, Enzymes, antibodies, antigens or microorganisms) are immobilized in close proximity to the transducer and can today be characterized by a wide range of measuring principles prove. The choice of transducer depends on the reaction the biological component and the resulting changes. A number of transducers are described in the prior art, who work according to different principles. common are transducers on electrochemical, electrical or optical Base.

Sensitivity and specificity of the biomolecular Mark detection - next to other parameters such as reproducibility, manufacturing costs, manageability - the quality and practicality of the Sensors. The specificity of the biosensor is largely determined by the biological component. A specific bioactive material is used to find the one you are looking for Substance under an abundance others - also more similar - to find out. The chemical reactions taking place influence physical ones Parameters, for example the electrical potential. The basic values or their changes are converted into an electrical output signal by the transducer and then electronically amplified. Thus the biological component of the sensor, e.g. an enzyme a receptor or an antibody, the substance to be analyzed - and essentially only this - and generates a signal whose intensity is the concentration of the bound Corresponds to the substance. For example, in the case of enzymes, an electrical one Signal caused by the formation of a reaction product and be recorded with an electrode. In the case of an enzyme sensor for glucose the electrode is usually with a thin one Covered membrane containing immobilized glucose oxidase (GOD). The enzyme molecules are enclosed, for example, in gelatin or polyurethane. The membrane is only for molecules certain size permeable. Out a mixture of amino acids, The enzyme converts proteins, fats, glucose and other sugars GOD just turns the glucose around using oxygen. It is formed Gluconolactone and hydrogen peroxide. The immobilized enzyme can not be washed out of the membrane, rather it is up to to the natural Aging reusable. The smaller molecules like glucose, hydrogen peroxide and oxygen, on the other hand, easily escape from the one to be analyzed solution into and out of the enzyme membrane. That with the enzyme reaction Forming hydrogen peroxide gives as an electrode active substance two electrons per molecule to the electrode. The electrons generated in this reaction are then delivered to the electrode of the biosensor. Thereby a micro current is generated. Simultaneously with the reaction of the glucose with the enzyme GOD is sometimes used in a bioinactive field Background current measured by interfering substances in the blood sample can arise. With the interfering substances can it be e.g. to medicines, vitamins or metabolites in act in high concentrations, which also cause a microcurrent can. The net current calculated in this way is a measure of the amount of glucose in e.g. a blood sample and can be proportional to the blood glucose concentration can be converted.

The reproducible, easy-to-use and stable immobilization of the biological components still presents difficulties. To achieve a fast response time and a reliable measured value, for example, a thin immobilizate layer and a high immobilization to achieve high storage and functional stability to strive for enzyme activity. However, relatively unstable systems are obtained by adsorption on corresponding support surfaces, including a metal electrode layer. The problems associated with this occur even more intensely in planar systems or carriers, insofar as an essentially mechanical sandwich structure for sensor production can no longer be used there. If cracks in the individual membrane layers are formed in such sandwich-type biosensors due to the loss of mechanical cohesion, the measured values obtained are falsified, for example, by the above-mentioned interfering substances to such an extent that even the previously mentioned differential measuring arrangements with a bioinactive field can no longer compensate them.

DE 42 08 186 A1 describes a sandwich membrane for biosensors, whereby a biomaterial layer is provided, which is delimited from the sensor with a gas-selective layer and which is covered with a microstructured layer facing the measurement solution, the permeability of which is inhomogeneous for different substrates / cosubstrates, with the gas-selective layer Layer and the biomaterial layer or on the side facing the measurement solution of the microstructured layer, if necessary, dialysis layers. JP 031 30 656 A describes an electrode based on a laminate film. DE 41 28 569 C1 describes a method for producing a semi-permeable polymer layer which is deposited in situ on an electrically conductive substrate. The polymer layers formed by electrochemical polymerization are composed of polyoxyphenylene or polyoxynaphthalene chains which carry ion-exchangeable and ion-conductive groups on the aromatic groups. These polymer layers are suitable as a semipermeable membrane in an electrode / membrane unit, as a selective phase or as a component of a selective phase for potentiometric or amperometric sensors. DE 689 13 144 T2 inter alia describes a biosensor which comprises an electrode with an enzyme immobilized thereon and, in the order given, an electroplated metal layer on the electrode surface which contains the enzyme and a mediator for electron transfer, and a layer of an electropolymerized substance which contains the enzyme and the Contains intermediaries for electron transfer. JP 020 87 056 A describes an enzyme sensor wherein a film having an enzyme such as glucokinase fixed is laminated on a surface of a conductive film. JP 020 99 850 A. describes the immobilization of a mediator in a highly conductive polymer film formed on an electrode substrate together with an enzyme.

DE 100 25 174 A1 describes an electrode made of a composite, the surface of which has a microroughness, biomolecules being bound to the surface.

Consequently is the object of the present invention, a stable To provide an enzyme electrode arrangement or a biosensor in sandwich construction, which) measurements quickly and with high precision without the occurrence of Interference effects should enable continued use and thus a reliable Generate signal amplification of biological binding reactions should. This should be done without covalent coupling, usually in a membrane immobilized biological components can be realized.

This Task is characterized by those characterized in the independent claims embodiments solved.

In particular, an enzyme electrode arrangement is provided, comprising in the following order at least one substrate with a surface roughness in the range from 20 nm to 10 μm, measured by AFM measurement,
a metal electrode,
an ultra-thin semipermeable membrane with a thickness in the range from 10 to 100 nm, and
at least one enzyme membrane.

The Figures show:

1 shows a schematic top view ( 1a ) a section of an exemplary biosensor arrangement according to the present invention and a cross-sectional view along the line AB ( 1b ).

2 shows a schematic cross section ( 2a ) an exemplary biosensor arrangement according to the present invention in connection with a flow cell and a corresponding top view thereof ( 2 B ).

3 shows schematically a cross-sectional view of the layer structure of an enzyme electrode arrangement according to the invention and below an enlarged section thereof.

The material of the substrate is not subject to any specific limitation as long as it is capable of forming a surface roughness in the range from 20 nm to 10 μm and is generally suitable as a substrate for a biosensor. The substrate is preferably made of an organic polymer selected from the group consisting of polyacrylate, polyimide, polyester and polycarbonate ho mo and copolymers thereof. Alternatively, substrates based on inorganic materials such as porous silicon or etched glass can be used. The substrates used preferably have thicknesses in the range from 0.01 to 5 mm.

The Metal electrode can be made from any of those commonly used in biosensors materials used, such as platinum or gold. The layer thickness of the metal electrode is so thin that that she capable is to adhere to the surface roughness structure to adapt the micro-rough substrate. In particular, the metal electrode layer thin enough designed, at least part of the surface roughness of the used according to the invention Substrate on its surface to receive or take over. Usually has the metal electrode in the context of the enzyme electrode arrangement according to the invention Layer thickness in the range of 50 to 250 nm.

According to the sandwich construction of the enzyme electrode arrangement according to the invention, an ultra-thin semipermeable membrane or an anti-interference membrane is arranged on the metal electrode. In the context of the present invention, this is understood to mean a membrane which has a sufficient porosity that molecules such as H ₂ O ₂ or O ₂ or those of a similar size diffuse through and can contact the metal electrode surface. The entry of substances such as ascorbic acid, uric acid, pracetamol and gentisic acid as a metabolite of acetylsalicylic acid, which each have a molecular weight greater than 100 daltons and, if they could reach the metal electrode, would be oxidized, which would produce a "wrong" signal, is prevented, however, by the ultra-thin semipermeable membrane, which is preferably constructed from an organic polymer material which is electropolymerized from organic monomers selected from (i) diamino, (ii) dihydroxy or (iii) both amino and hydroxy substituted aromatic hydrocarbons and mixtures thereof, the organic monomers preferably being 1,2-diaminobenzene, 1,3-diaminobenzene, 2,3-diaminonaphthalene, 1,5-diaminonaphthalene, 1,8-diaminonaphthalene, 5-amino -1-naphthol or resorcinol selected.

On The semipermeable membrane has a conventional enzyme membrane. There is preferably at least one enzyme from the group in this membrane of the oxidases immobilized. The oxidases can be selected from the group consisting of lactate oxidase, galactose oxidase, L-2-hydroxy acid oxidase, Glucose oxidase, glycolate oxidase, hexose oxidase, L-gulonolactone oxidase, L-sorbose oxidase, pyridoxol-4-oxidase and alcohol oxidase.

By starting from the micro-rough substrate via the metal electrode and the semipermeable membrane is transferred to the lower surface side of the enzyme membrane Roughness structure is within the sandwich composite of the enzyme electrode arrangement according to the invention mechanical self-cohesion in a simple way, So that the enzyme electrode arrangement according to the invention Measurements of corresponding analytes quickly and with high precision without the occurrence of interference effects with continued use, this being particularly advantageous without covalent coupling the usual biological components immobilized in a membrane becomes. This is the decrease in time of the Anti-interference effect, as is the case with the use of smooth Substrates, counteracted.

In addition can on the enzyme membrane to further improve the measurement accuracy a diffusion-inhibiting membrane, for example a pHEMA membrane, and / or a catalase membrane is arranged to prevent or reduce interference become.

• (a) Bereitstellen eines Substrats mit einer Oberflächenrauhigkeit im Bereich von 20 nm bis 10 μm,
• (b) Aufbringen einer Metallelektrodenschicht auf dem Substrat in einer Schichtdicke, die ausreichend dünn ausgelegt ist, sich an die Oberflächenrauhigkeitsstruktur des Substrats anzupassen,
• (c) Aufbringen einer semipermeablen Membran in einer Dicke im Bereich von 10 bis 100 nm und
• (d) Aufbringen von mindestens einer Enzymmembran.

The present invention further relates to a method for producing an enzyme electrode arrangement, comprising the steps:

• (a) providing a substrate with a surface roughness in the range from 20 nm to 10 μm,
• (b) applying a metal electrode layer on the substrate in a layer thickness that is designed to be sufficiently thin to adapt to the surface roughness structure of the substrate,
• (c) applying a semipermeable membrane with a thickness in the range from 10 to 100 nm and
• (d) applying at least one enzyme membrane.

The generation of the surface roughness in the substrate can be achieved, in particular, by providing a pretreated metallic or ceramic master and subsequent replica molding by applying a corresponding liquid or thermally softenable polymer precursor or polymer to the master and subsequent hardening or cooling, or also by thermal embossing in the polymer precursor or the polymer is made with the provision of the substrate with a surface roughness in the range from 20 nm to 10 μm. The master can provide a corresponding micro-rough surface, which functions as a negative form in the context of replica molding, for example by micro-milling, photolithographic etching zen, sandblasting, mechanical stamping or galvanic roughening. If the substrate has been embossed into the master in this way, the substrate is then separated from the master by either mechanically separating it or by dissolving the master, for example, by an etching process.

A further embodiment regarding the generation of the surface roughness of the substrate consists in etching the substrate. So can for example glass surfaces exposed to hydrofluoric acid vapors in a known manner become. Furthermore, for example, polyimide can be used in the prior art usually for this used acid mixtures etched become.

The Application of the metal electrode layer in step (b), in particular a platinum or gold electrode, for example using a vacuum deposition process, for example PVD or CVD processes can be carried out. The metal electrode is applied in a layer thickness that is adapted is the surface roughness structure of the micro-rough substrate. The layer thickness of the metal electrode layer is chosen so that at least part of the surface roughness of the substrate used according to the invention is retained or taken over becomes. Usually has the metal electrode in the context of the enzyme electrode arrangement according to the invention Layer thickness in the range of 50 to 250 nm.

Preferably in step (c) the semipermeable membrane is electropolymerized of organic monomers selected from diamino or dihydroxy substituted Benzenes or naphthalenes and mixtures thereof, in more usual Way applied. The application can, for example, by electropolymerization by means of cyclic variation of the potential in a solution for example, neutral phosphate buffer.

The Application of the membrane solutions to form the enzyme membrane and optionally one or more other membrane, such as a diffusion-inhibiting Membrane or a catalase membrane, can be made using conventional techniques, such as. Dispense or spin / dip coating. As part of of the method according to the invention is usually first a photoreactive membrane precursor solution applied, which for Networking afterwards UV light irradiation in an oxygen-free atmosphere, e.g. Argon atmosphere, is exposed. The enzyme membrane solutions preferably contain at least one enzyme from the group of oxidases. The oxidases can from the group consisting of lactate oxidase, galactose oxidase, L-2-hydroxy acid oxidase, Glucose oxidase, glycolate oxidase, hexose oxidase, L-gulonolactone oxidase, L-sorbose oxidase, Pyridoxol-4-oxidase and alcohol oxidase can be selected. A typical membrane precursor solution contains pHEMA as a polymeric binder, HEMA (hydroxyethyl acrylate) as a reactive Monomer, TEGDMA (tetraethylene glycol dimethacrylate) as crosslinking agent, Polyethylene glycol as a plasticizer and a photoinitiator such as. ω, ω'-dimethoxy-ω-phenylacetophenone and water. After loosening the above components and filtration become the desired ones Enzymes added to the precursor solution.

Preferably become such enzymes on the enzyme electrode arrangement according to the invention immobilized in a cross-linked pHEMA membrane.

When proteins, such as enzymes, are immobilized in polymers by means of their polymerization or crosslinking, which is triggered by free radicals which are generated in particular by photolysis with UV light, proteins which have sulfhydryl (-SH) groups arise have on their surface, such as glucose oxidase, the problem that such SH groups consume free radicals to such an extent that the polymerization or crosslinking is substantially inhibited. However, this can be avoided according to the invention in that the composition for producing an enzyme membrane is admixed with a molecular quinoid agent which is capable of abstracting a hydrogen atom from the -SH groups under UV light irradiation. This not only prevents the consumption of other radicals by -SH groups, but also supports the polymerization or crosslinking to be carried out to provide the enzyme membrane through the intermediate sulfur radical. Such molecular quinoid agents which can be used are unsubstituted or substituted benzoquinones, anthraquinones or naphthoquinones and their derivatives or a mixture of one or more thereof. As derivatives, for example, their imine, oxime, cyanimine and / or dicyanomide compounds, such as 1,4-benzoquinone dioxime, 1,4-benzoquinone diimine, tetracyano-p-quinodimethane and N, N'-dicyanoquinone diimine, can be used. An unsubstituted or substituted, ortho- or para-benzoquinone is preferably used as the quinoid agent in the electrode formulation according to the invention. In addition to straight-chain or branched-chain (C ₁ -C ₆ ) alkyl, (C ₃ -C ₇ ) cycloalkyl, (C ₁ -C ₆ ) alkoxy and (C ₁ -C ₆ ) thioether, the substituents can also be one or more, identical or different, electron-withdrawing groups, preferably selected from fluorine, chlorine, bromine, nitro, cyano and sulfonate. Examples of such quinoid agents are chloranil, duroquinone and p-benzoquinone.

Preferably the membrane solutions are applied using dispensing technology, whereby a cannula, from which is dispensed, if necessary provided with a hydrophobic coating can be, whereby both the stability of the dispensing process and its reproducibility is also increased. Applying the then active membranes by means of dispensing technology Cheap, if instead of a single, correspondingly large electrode, a large number smaller electrodes according to the present Invention provided for realizing the desired signal strength become.

On the present application further relates to the use the enzyme electrode arrangement according to the invention in a biosensor arrangement. Such a biosensor arrangement can in addition to the enzyme electrode arrangement according to the invention, in which the metal electrode acts as a working electrode, for example further an Ag / AgCl electrode as a reference electrode and / or a differential measuring electrode or "dummy electrode" for elimination of side effects over Include differential measurement. The reference electrode is preferably and / or differential measuring electrode arranged on the same micro-rough substrate material as for the enzyme electrode arrangement according to the invention provided, i.e. the reference electrode and / or the differential measuring electrode are spatially predetermined Neighborhood to the invention, the Enzyme membrane arrangement having an enzyme membrane arranged.

to Isolation of the biosensor arrangement and simultaneous generation of Wells for receiving the enzyme membrane or the reference electrode and / or the differential measuring electrode can on the biosensor arrangement according to the invention a 25 to 200 μm thick layer of a photostructurable material, e.g. Vacrel 8120, distributed by DuPont. Arranging such Layer also on the back of the substrate as a carrier the biosensor arrangement according to the invention can compensate for the occurrence of mechanical stress, which otherwise lead to bending could and also allows use within the scope of the present invention also very thin Substrate materials.

to Provision of an outside enclosing the desired measuring room Seal or a spacer can also use a 25 to 200 μm thick photostructurable material can be provided. Further can use a double-sided adhesive structured film to connect Sensor and an upper part are provided, such an adhesive film at the same time as a spacer and seal for forming a measuring chamber with the sensor electrodes. As the upper part of such measuring chambers a structured stainless steel foil can be provided, such a stainless steel foil both for sealing the Measuring chamber as well as for deriving the current of the sensors.

In 1 is a schematic plan view of such an exemplary biosensor arrangement according to the present invention, in which an enzyme electrode according to the invention ( 1 ), a dummy electrode ( 2 ) and an Ag / AgCl reference electrode ( 3 ) spaced apart on a chip surface ( 6 ), such as a polyimide film, are arranged. The reference symbols ( 4 ) respectively. ( 5 ) stand for corresponding contact surfaces (contact pads) or metal surfaces such as the metal electrode layer. Electrical wiring (not shown) is arranged on the contact pads and usually leads to one or more conventional measuring devices. 1b shows schematically a cross-sectional view along the line AB. On the substrate ( 7 ) are next to an enzyme electrode that consists of the metal electrode layer ( 5 ), the semipermeable membrane ( 15 ), the enzyme membrane ( 11 ), a diffusion-inhibiting membrane ( 12 ) and a catalase membrane ( 13 ) is constructed, a dummy electrode with a dummy membrane or differential sensor membrane ( 10 ) instead of the enzyme membrane and an Ag / AgCl electrode (reference symbol ( 8th ) respectively. ( 9 ) stand for Ag or AgCl). The electrodes ( 1 ), ( 2 ) and ( 3 ) and the contact surfaces are in openings in the on the substrate ( 7 ) arranged insulation layer ( 14 ), which is usually a photostructured dry resist film, arranged or embedded.

2 shows a schematic cross section ( 2a ) an exemplary biosensor arrangement according to the present invention in connection with a flow cell and a corresponding top view thereof ( 2 B ). The flow cell is exposed to the outside by a second layer of dry resist ( 16 ) completed. Alternatively, a structured film that is adhesive on both sides can be provided for this. A structured stainless steel foil ( 17 ) arranged. The reference symbols ( 18 ) and ( 19 ) stand for a liquid inlet or liquid outlet.

In 3 is shown schematically in a cross-sectional view of the layer or sandwich structure of an enzyme electrode arrangement according to the invention and an enlarged section thereof. On a micro-rough substrate according to the invention ( 7 ) is a metal electrode ( 5 ) arranged in a layer thickness which is designed so thin that the metal electrode adapts to the surface roughness structure of the substrate. There is an ultra-thin semipermeable membrane on the metal electrode layer ( 15 ) arranged on wel an enzyme membrane ( 11 ) is applied.

The The present invention is explained in more detail by the following example.

example

To produce a biosensor arrangement according to the present invention, the corresponding copper layer is first removed from a commercially available polyimide film (Pyralux AP, DuPont) by etching with 20% by weight Na ₂ S ₂ O ₈ , whereby a polyimide substrate with a micro-rough surface was obtained. A commercially available photoresist layer (Tenmaster TM 100, DuPont) was then applied to the micro-rough substrate produced in this way and structured correspondingly photolithographically to form predetermined zones or contact areas, for example for applying the analyte.

Then was to form a metal electrode layer a 100 nm thick platinum layer in the Vacuum evaporated. To avoid surface contamination of the so formed Pt metal electrode layer in the subsequent process steps can optionally a 100 nm thick titanium layer on the Pt layer be deposited. After peeling the previously applied resist layer remains a structured one Metal layer on the polyimide substrate.

to Compensation for shrinkage and for insulation purposes were on the top and bottom of the thus structured polyimide substrate dry resist layers (Vacrel 8120, DuPont) arranged and again structured accordingly photolithographically.

To removal of the titanium layer by conventional etching was done on the substrate an Ag / AgCl reference electrode by electroplating one Silver layer and subsequent galvanically converting part of it into silver chloride 0.1 M KCl arranged.

it closed itself the application of a semi-permeable membrane by electropolymerization a solution of 3 mM 1.3 diaminobenzene in neutral phosphate buffer using cyclic Variation of the potential over 6pm.

A glucose oxidase-containing membrane based on the following composition was then applied:
1 part by volume of a solution C + 1 part by volume of a solution B + 6 parts by volume of a solution A, solutions A, B and C having the following compositions:

Solution A: 24% by weight pHEMA, 12% by weight HEMA, 3% by weight TEGDMA, 1% by weight ω, ω'-dimethoxy-ω-phenylacetophenone, 36% by weight PEG400 and 24% by weight. % H ₂ O;

Solution B: 0.2% by weight of benzoquinone and 1% by weight of N-methyldiethanolamine in PEG 400;

Solution C: 25% by weight glucose oxidase lyophilisate in water

Then was a membrane on a dummy "electrode applied, which had been additionally arranged on the substrate, this "dummy" membrane having the following composition based (1 part by volume of water + 1 part by volume of solution B + 6 parts by volume of the above solution A).

In order to slow the flow of material through diffusion, a diffusion-inhibiting membrane based on the following composition was additionally applied to the enzyme membrane formed above:
18 wt% pHEMA, 18 wt% HEMA, 3 wt% TEGDMA, 1 wt% ω, ω'-dimethoxy-ω-phenylacetophenone, 36 wt% PEG400 and 24 wt% H ₂ O

Finally, a catalase membrane was applied in order to prevent the sensor from responding transversely and to minimize the dependence of the sensor sensitivity on the speed of movement of the solution. The catalase membrane was based on the following composition:
1 part by volume of a solution D + 1 part by volume of glycerol + 6 parts by volume of a solution A, the solution A having the above composition and the solution D being composed as follows:

1

enzyme electrode

2

Dummy electrode

3

Ag / AgCl reference electrode

4

contact surfaces

5

metal surfaces

6

chip area

7

micro Rough substratum

8th

silver

9

silver chloride

10

Difference sensor membrane ( "Dummy membrane")

11

enzyme membrane

12

diffusion-resistant Membrane, e.g. pHEMA membrane

13

Catalase membrane

14

insulation layer

15

semipermeable membrane

16

Further Dry resist layer or structured film that is adhesive on both sides

17

structured stainless steel foil

18

liquid inlet

19

liquid outlet

Claims (21)

An enzyme electrode assembly comprising the following sequence a substrate with a surface roughness in the range of 20 nm to 10 μm, a metal electrode, using an ultra thin semipermeable membrane a thickness in the range of 10 to 100 nm and at least one Enzyme membrane. The enzyme electrode assembly of claim 1, wherein the An organic polymer substrate selected from the group consisting of made of polyacrylate, polyimide, polyester and polycarbonate homo- and Copolymers thereof. Enzyme electrode arrangement according to claim 1 or 2, wherein the metal electrode has a layer thickness in the range of 50 to 250 nm. The enzyme electrode assembly according to claim 3, wherein the , Metal electrode is a platinum electrode or gold electrode. Enzyme electrode arrangement according to one of claims 1 to 4, the semi-permeable membrane made of an organic polymer material is built up by electropolymerization of organic monomers, selected from (i) diamino, (ii) dihydroxy or (iii) both amino and hydroxy-substituted aromatic hydrocarbons and mixtures of which has been formed. The enzyme electrode assembly according to claim 5, wherein the organic monomers from 1,2-diaminobenzene, 1,3-diaminobenzene, 2,3-diaminonaphthalene, 1,5-diaminonaphthalene, 1,8-diaminonaphthalene, 5-amino-1-naphthol and resorcinol Enzyme electrode arrangement according to one of claims 1 to 6, wherein the enzyme membrane at least one enzyme from the group of Oxidases includes. The enzyme electrode assembly of claim 7, wherein the Oxidases from the group consisting of lactate oxidase, galactose oxidase, L-2-hydroxy-acid, Glucose oxidase, glycolate oxidase, hexose oxidase, L-gulonolactone oxidase, L-sorbose oxidase, pyridoxol-4-oxidase and alcohol oxidase. Enzyme electrode arrangement according to one of claims 1 to 8, with a diffusion-inhibiting membrane on the enzyme membrane, preferably a pHEMA membrane, and / or a catalase membrane arranged to reduce interference is or are. Method of making an enzyme electrode assembly according to one of the claims 1 to 9, comprising the steps: (a) Providing a substrate with a surface roughness in the range from 10 nm to 10 μm, (B) Applying a metal electrode layer on the substrate, (C) Application of a semipermeable membrane with a thickness in the area from 10 to 100 nm, and (d) applying at least one Enzyme membrane. The method of claim 10, wherein before step (a) generating the surface roughness in the substrate by providing a pretreated metallic or ceramic masters and subsequent replica molding Applying a liquid polymer precursor on the master and hardships of the polymer precursor while providing the substrate with a surface roughness in the range from 20 nm to 10 μm he follows. The method of claim 11, wherein the master is by Micro milling, photolithographic etching, sandblasting, mechanical embossing or galvanic roughening is pretreated. The method of claim 10, wherein before step (a) generating the surface roughness in the substrate by removing the metal layer in a metal-polymer laminate film by means of etching he follows. A method according to any one of claims 11 to 13, wherein the application the metal electrode layer in step (b) by means of a vacuum deposition process he follows. A method according to any one of claims 11 to 14, wherein in step (c) the semipermeable membrane by electropolymerization of organic Monomers selected from (i) diamino, (ii) dihydroxy or (iii) both amino and hydroxy-substituted aromatic hydrocarbons and mixtures of which is applied. A method according to any one of claims 11 to 15, wherein in step (d) the application of at least one enzyme membrane takes place by means of dispensing technology. The method of claim 16, wherein a photoreactive membrane precursor solution is first applied, which is then used for crosslinking exposed to UV light in an oxygen-free atmosphere. Use of the enzyme electrode arrangement according to one of claims 1 to 9 in a biosensor arrangement. Biosensor arrangement, comprising an enzyme electrode arrangement according to one of the claims 1 to 9. The biosensor arrangement according to claim 19, further comprising an Ag / AgCl electrode as a reference electrode and / or a differential measuring electrode for elimination of side effects over Differential measurement. Use of a molecular quinoid agent for Production of an enzyme membrane, in which at least one enzyme is immobilized becomes.