Enzyme Electrode

Information

  • Patent Application
  • 20150129425
  • Publication Number
    20150129425
  • Date Filed
    June 25, 2013
    11 years ago
  • Date Published
    May 14, 2015
    9 years ago
Abstract
An enzyme electrode includes an electrode, and a detection layer that is in contact with the electrode and includes an oxidoreductase, a water-soluble conductive polymer, and conductive particles, electrons being transferred between the enzyme and the electrode by direct electron transfer in the detection layer.
Description
TECHNICAL FIELD

The present invention relates to an enzyme electrode.


BACKGROUND ART

There is known an enzyme electrode including an electrode and a detection layer containing an enzyme that is formed on the electrode. The enzyme electrode has a structure that takes electrons generated by an enzyme reaction out of the electrode.


PRIOR ART DOCUMENTS
Patent Document



  • Patent Document 1: Japanese Laid-Open Patent Publication No. 01-075956

  • Patent Document 2: Japanese Laid-Open Patent Publication No. 63-050748

  • Patent Document 3: Japanese Laid-Open Patent Publication No. 10-100306

  • Patent Document 4: Japanese Laid-Open Patent Publication No. 2006-234788



Non Patent Document



  • Non Patent Document 1: Brianna C. Thompson et al., Macromol. Rapid Commun. 2010, 31, 1293-1297

  • Non Patent Document 2: A. Kros et al., Third generation Polyethylenedioxythiophene (PEDOT) based glucose sensor, Symposia Papers Presented Before the Division of Environmental Chemistry, American Chemical Society Anaheim, Calif. Mar. 21-25, 1999

  • Non Patent Document 3: A. Kros et al., Poly(pyrrole) versus poly(3,4-ethylenedioxythiophene): implications for biosensor applications, Sensors and Actuators B 106 (2005) 289-295

  • Non Patent Document 4: C. G. J. Koopal et al., Glucose sensor utilizing polypyrrole incorporated in track-etch membranes as the mediator, Biosensor and Bioelectronics 7 (1992) 461-471



SUMMARY OF THE INVENTION
Problems to be Solved by the Invention

Generally, when an enzyme contained in a detection layer of an enzyme electrode is in an inactive state, the function as an enzyme electrode will be impaired. One of the factors of the inactivation of an enzyme is the inactivation by heat. For example, heat leading to the inactivation may be applied to an enzyme electrode in an environment during storage or transportation. Further, heat may be applied while using an enzyme electrode. It is preferred that an enzyme electrode have good heat resistance in a sense of increasing the life of an enzyme electrode.


One aspect of the present invention is directed to provide an enzyme electrode having improved heat resistance.


Means for Solving the Problems

In order to achieve an object as mentioned above, one aspect of the present invention applies configurations below. Namely, the one aspect of the present invention is an enzyme electrode. The enzyme electrode includes an electrode, and a detection layer that is in contact with the electrode and includes an oxidoreductase, a water-soluble conductive polymer, and conductive particles, wherein electrons are transferred between the enzyme and the electrode by direct electron transfer in the detection layer. For example, the water-soluble conductive polymer is polyaniline sulfonic acid.


In the one aspect of the present invention, the oxidoreductase may have a subunit including cytochrome. The oxidoreductase also may have a domain including cytochrome. Further, as the oxidoreductase, an oligomeric enzyme including at least a catalytic subunit and a subunit including cytochrome may be applied. Moreover, as the oxidoreductase, an enzyme including at least a catalytic domain and a domain including cytochrome may be applied. Each of the catalytic subunit and the catalytic domain may include at least one selected from pyrroloquinoline quinone and flavin adenine dinucleotide.


In the one aspect of the present invention, the conductive particles may include carbon. For example, concentration of the above-described polyaniline sulfonic acid is 0.01 to 2%. A functional group of the above-mentioned polyaniline sulfonic acid may be a hydroxy group or a sulfo group.


Preferably, at least one of the electrode and the detection layer may include conductive particles.


The enzyme electrode in the one aspect of the present invention is characterized in that has an improved heat resistance. One of other aspects of the present invention is a biosensor including an enzyme electrode. The enzyme electrode includes an electrode, and a detection layer that is in contact with the electrode and includes an oxidoreductase, a water-soluble conductive polymer, and conductive particles, wherein electrons are transferred between the enzyme and the electrode by direct electron transfer in the detection layer.


One of other aspects of the present invention is an electronic apparatus. The electronic apparatus includes includes an electrode, and a detection layer that is in contact with the electrode and includes an oxidoreductase, a water-soluble conductive polymer, and conductive particles, wherein electrons are transferred between the enzyme and the electrode by direct electron transfer in the detection layer.


One of other aspects of the present invention is an apparatus including an enzyme electrode, and a feed section that supplies, to a load, a current generated by an enzyme reaction at the enzyme electrode, the enzyme electrode including an electrode and a detection layer that is in contact with the electrode and includes an oxidoreductase, a water-soluble conductive polymer, and conductive particles, wherein electrons are transferred between the enzyme and the electrode by direct electron transfer in the detection layer. Further, the other aspects of the present invention may include an electronic apparatus including the above-described biosensor and an electronic apparatus including the above-described apparatus.


One of the other aspects of the present invention is a method of producing an enzyme electrode, including forming a detection layer on an electrode, the detection layer including an oxidoreductase, a water-soluble conductive polymer, and conductive particles, wherein electrons are transferred between the enzyme and the electrode by direct electron transfer.


One of the other aspects of the present invention is a reagent having improved heat resistance, including an oxidoreductase, a water-soluble conductive polymer, and conductive particles.


Effects of the Invention

According to one aspect of the present invention, an enzyme electrode having improved heat resistance may be provided.





BRIEF DESCRIPTION OF DRAWINGS


FIG. 1 is a schematic view illustrating the structure of an enzyme electrode according to the embodiment.



FIG. 2 is a schematic view illustrating the inside of a detection layer.



FIG. 3 is a graph illustrating the relationship between the temperature and the response current during heat treatment in the case where the time of heat treatment is fixed.



FIG. 4 is a graph illustrating the relationship between the time and the response current in the case where the temperature of heat treatment is fixed, and the time of heat treatment is changed.



FIG. 5 is a graph illustrating the relationship between the concentration of polyaniline sulfonic acid and the heat resistance.



FIG. 6 is a graph illustrating the relationship between the concentration of polyaniline sulfonic acid and the heat resistance.



FIG. 7 is a graph illustrating the results of Test 4 (influence of the concentration of a polymer added to a reagent).



FIG. 8 is a graph illustrating the results of Test 5 (influence of heat treatment time).





DESCRIPTION OF EMBODIMENTS

Hereinafter, an enzyme electrode as an embodiment of the present invention will be described with reference to drawings. The embodiment to be described below is for illustration purposes, and the present invention is not limited to the structure of the following embodiment.


[Structure of Enzyme Electrode]



FIG. 1 is a schematic view illustrating the side surface of an enzyme electrode according to the embodiment. In FIG. 1, an enzyme electrode 10 includes an electrode 1 and a detection layer 2 formed on the surface (upper surface in FIG. 1) of the electrode 1.


<Electrode>


The electrode 1 is formed of a metallic material such as gold (Au), platinum (Pt), silver (Ag), and palladium, or a carbon material such as carbon. The electrode 1 is formed, for example, on an insulating substrate 3 as illustrated in FIG. 1. The insulating substrate 3 is formed of an insulating material such as various resins (plastics) such as a thermoplastic resin, such as polyether imide (PEI), polyethylene terephthalate (PET), and polyethylene (PE), a polyimide resin, and an epoxy resin; glass; ceramics; and paper. Any known material can be applied as an electrode material forming the electrode 1 and a material for the insulating substrate 3. The size and the thickness of the electrode 1 and the insulating substrate 3 can be suitably set. Hereinafter, the combination of the insulating substrate 3 and the electrode 1 may be called a “base material.”


<Detection Layer>



FIG. 2 schematically illustrates the state in the detection layer 2 illustrated in FIG. 1. As illustrated in FIG. 2, the detection layer 2 is in contact with the electrode 1, contains an oxidoreductase 4 (hereinafter may be simply represented by an “enzyme 4”), and a conductive polymer (polyaniline: for example, polyaniline sulfonic acid) 5, and does not contain an electron-transfer mediator.


As illustrated in FIG. 2, in the detection layer 2, the molecule of the enzyme 4 has a structure in which it is intricately entangled with the conductive polymer 5. Electrons generated by an enzyme reaction can be transferred to the electrode 1 directly or through the conductive polymer 5. That is, in the enzyme electrode 10 according to the embodiment, electrons are transferred between the enzyme 4 and the electrode 1 by direct electron transfer in the detection layer 2.


Thus, the enzyme electrode 10 is a direct electron transfer-type enzyme electrode. The “direct electron transfer-type enzyme electrode” is a type of enzyme electrode in which electrons are transferred between an enzyme and an electrode in a way in which electrons generated by an enzyme reaction in a detection layer are directly transferred to the electrode without the involvement of an oxidation-reduction material such as an electron-transfer mediator.


Further, the “direct electron transfer-type enzyme electrode” is distinguished from a type of enzyme electrode in which electrons are transferred to an electrode through a material generated by an enzyme reaction, such as the oxidation of hydrogen peroxide (H2O2) generated by an enzyme reaction on an electrode when glucose oxidase (GOD) is applied as an enzyme.


Note that, it is said that the maximum limit of distance in which direct electron transfer occurs in a physiological reaction system is 10 to 20 Å. In a longer distance than this maximum limit, in the electron exchange in an electrochemical reaction system including an electrode and a biomolecule (enzyme), as well, it will be difficult to detect the electron exchange on the electrode without the involvement of mass transfer (for example, transfer by diffusion) of the enzyme or a mediator.


In the enzyme electrode 10, entanglement of the molecules of the enzyme 4 and the conductive polymer 5 in the detection layer 2 is considered to act so as to mitigate the action exerted on the enzyme 4 (structural change of the enzyme molecules) by the thermal energy from the outside.


Further, in the detection layer 2, the conductive sites of the conductive polymer 5 are located in the vicinity of the electron transfer sites of the enzyme 4 (sites where electrons are transferred in an enzyme reaction), thereby leading to a state where electron transfer between the enzyme 4 and the electrode 1 easily occurs. As an effect of one aspect of the present invention, the enzyme 4 is probably in an environment where it can easily maintain a higher-order structure of the molecules because the enzyme is surrounded by the conductive polymer 5. Further, electrons generated from the enzyme 4 are probably in a state where a plurality of suitable electron transport pathways from the enzyme 4 to the electrode 1 are formed through the conductive sites of the conductive polymer 5. Therefore, as an effect of one aspect of the present invention, even when the action (physical change or change of arrangement) to the enzyme 4 occurs by thermal energy from the outside, the electron transfer from the enzyme 4 to the electrode 1 is probably large or relieved from a sudden disturbance by having secured the plurality of suitable electron transport pathways. Consequently, the enzyme electrode 10 according to the embodiment can have suitable heat resistance.


Further, in the detection layer 2, the influence of heat stress to the enzyme 4 is probably relieved by thermoelectric conversion characteristics by the Seebeck effect of the conductive polymer (conductive polymer 5). Particularly, when polyaniline sulfonic acid is applied as the conductive polymer 5, the polyaniline sulfonic acid provides a higher Seebeck effect because it has a long molecular chain that represents a m-electron conjugated system, has good compatibility (mixing) with the enzyme 4 because it is not water-dispersible but water-soluble, and probably easily structurally entraps the enzyme 4 in the detection layer 2. Therefore, the suppression effect of the influence of heat on the enzyme 4 at least during the preparation of the enzyme electrode 10 is probably improved.


<<Oxidoreductase>>


An oxidoreductase which can be applied as the enzyme 4 can contain cytochrome. Further, the oxidoreductase can contain an electron transfer subunit. As the oxidoreductase having the electron transfer subunit, at least one can be selected, for example, from among glucose dehydrogenase containing cytochrome (CyGDH), pyrroloquinoline quinone glucose dehydrogenase (PQQGDH complex), sorbitol dehydrogenase (Sorbitol DH), D-fructose dehydrogenase (Fructose DH), Glucose-3-Dehydrogenase derived from Agrobacterium tumefasience (Glucose-3-Dehydrogenase) (G3DH from Agrobacterium tumefasience), and cellobiose dehydrogenase. It is preferred to apply a subunit containing cytochrome as the electron transfer subunit. As the oxidoreductase having the subunit containing cytochrome, for example, a fusion protein of CyGDH or PQQGDH as described above with cytochrome can be applied. Further, the oxidoreductase can contain an electron transfer domain. As the oxidoreductase having the electron transfer domain, at least one can be selected, for example, from among cholesterol dehydrogenase (CDH) and quinoheme ethanol dehydrogenase (QHEDH (PQQ Ethanol dh), “QHGDH” (fusion enzyme; GDH with heme domain of QHGDH). As the electron transfer domain, it is preferred to apply a domain containing cytochrome. For example, it is preferred to apply the cytochrome domain of QHEDH as described above.


A fusion protein of PQQGDH with cytochrome illustrating the subunit containing cytochrome as described above and a cytochrome domain of QHGDH illustrating the domain containing cytochrome are disclosed, for example, in International Publication No. WO 2005/030807. Further, the oxidoreductase contains a catalytic subunit, and the catalytic subunit can have an electron transfer subunit. Examples of the catalytic subunit include an α-subunit of the glucose dehydrogenase containing cytochrome. As the oxidoreductase, it is preferred to apply an oligomeric enzyme including at least a catalytic subunit and a subunit containing cytochrome. Further, as the oxidoreductase, it is preferred to apply an enzyme including at least a catalytic domain and a domain containing cytochrome.


Furthermore, the oxidoreductase further contains a catalytic domain, and the catalytic domain can have an electron transfer domain. Examples of the catalytic domain include a flavin domain of cholesterol dehydrogenase.


The catalytic subunit and the catalytic domain as described above each can contain at least one of pyrroloquinoline quinone (PQQ) and flavin adenine dinucleotide (FAD).


<<Polyaniline Sulfonic Acid>>


As the polyaniline sulfonic acid which can be applied as the conductive polymer 5, a polyaniline sulfonic acid having various attributes (for example, water solubility) can be applied. The concentration of polyaniline sulfonic acid 6 is, for example, 0.01 to 5%, preferably 0.01 to 2%. Further, a functional group of polyaniline sulfonic acid is a hydroxy group or a sulfo group.


<<Conductive Particles>>


Although not illustrated, the detection layer 2 of the enzyme electrode 10 can further contain conductive particles. Since the detection layer 2 contains conductive particles, a more suitable electron transfer to an electrode can be expected. Examples of the conductive particles include carbon. Specifically, metal particles such as gold, platinum, silver, and palladium or a higher-order structure formed from carbon can be applied as the conductive particles. The higher-order structure can include particle or fine particle types of carbon such as conductive carbon black, Ketjen Black, carbon nanotube (CNT), and fullerene. At least one of the metals and carbons as described above can be selected as the conductive particles.


Note that the surface of the detection layer 2 may be covered with an outer-layer film made of cellulose acetate (CA) and the like.


[Method for Preparing Enzyme Electrode]

The enzyme electrode 10 as described above is prepared, for example, as follows. Specifically, a metal layer which functions as an electrode 1 is formed on one side of an insulating substrate 3. For example, a metal layer having a desired thickness (for example, about 30 nm) is formed by depositing a metallic material by physical vapor deposition (PVD, for example, sputtering) or chemical vapor deposition (CVD) on one side of an insulating substrate 3 in a film form having a predetermined thickness (for example, about 100 μm). An electrode layer formed of a carbon material can also be formed instead of the metal layer.


Next, a detection layer 2 is formed on an electrode 1. That is, a solution (reagent) containing an oxidoreductase 4 containing cytochrome and polyaniline sulfonic acid as a conductive polymer 5 is prepared. The solution (reagent) is dropped on the surface of the electrode 1. The solution (reagent) is dried and solidified on the electrode 1, thereby providing the enzyme electrode 10 in which the detection layer 2 is formed on the electrode 1.


EXAMPLES

Hereinafter, Examples of the enzyme electrode will be described.


<Test 1>


<<Preparation of Reagent Solution>>

First, two types of reagent solutions according to Example 1 and Comparative Example as described below were prepared.


Example 1



  • Ketjen Black: 0.8%

  • Water-soluble polyaniline (trade name: Aqua-PASS (hereinafter represented by “AQP”)): 0.45%

  • Glucose dehydrogenase containing cytochrome (Cy-GDH): 0.56%

  • Stabilizing agent (sucrose): 0.5%

  • Phosphate buffer (pH 5.8): 16 mM



Note that “%” represents the percent by weight concentration of a reagent contained in the reagent solution.


Comparative Example



  • Ketjen Black: 0.8%

  • Glucose dehydrogenase containing cytochrome (Cy-GDH): 0.56%

  • Stabilizing agent (sucrose): 0.5%

  • Phosphate buffer (pH 5.8): 16 mM



Note that “%” represents the percent by weight concentration of a reagent contained in the reagent solution. Thus, the reagent solution in Comparative Example is a reagent solution in which AQP is removed from the reagent solution in Example 1.


<<Preparation of Enzyme Electrode (Sample)>>


Next, a plurality of insulating substrates in which an electrode (electrode layer) is formed on one side of the substrate by gold vapor deposition (base materials) were prepared. The reagent solutions according to Example 1 and Comparative Example were each dispensed on each of the insulating substrates, and the resulting base materials were dried by allowing them to stand for 30 minutes in a low humidity drying furnace. In this way, enzyme electrodes (samples) according to Example 1 and enzyme electrodes (samples) according to Comparative Example, in which a detection layer was formed by the solidification of a reagent on each of the electrodes, were obtained.


At this time, four types (a total of eight types) of samples were obtained by drying each of the samples of Example 1 and Comparative Example at a furnace temperature of 30° C., 80° C., 100° C., or 120° C. (drying temperature).


<<Measurement of Glucose Concentration>>

Next, a response current value was measured for 100 mg/dl of glucose in the above samples after the heat treatment. In the glucose measurement, the above samples were immersed in a phosphate buffer (pH 7.4) heated to 37° C.; a platinum wire was used for the counter electrode, and a silver/silver chloride electrode was used for the reference electrode; and the applied voltage to the working electrode was set to +0.4 V (vs. Ag/AgCl).


<<Evaluation of Measurement Results>>



FIG. 3 is a graph illustrating the results of Test 1, that is, the relationship between the response current value (μA) and the drying temperature (° C.) for the eight types of samples as described above. In FIG. 3, white bar graphs illustrate the results of the samples according to Example 1, and black bar graphs illustrate the results of the samples according to Comparative Example. Note that the measurement was performed twice using two samples for each type, and the results illustrated in FIG. 3 indicate the average values of the results at the two times of measurement.


According to the test results illustrated in FIG. 3, apparent reduction in response sensitivity was observed with the increase in drying temperature as for the samples to which no AQP was added (Comparative Example), while high response sensitivity was maintained with the increase in drying temperature as for the samples to which AQP was added (Example 1). Thus, it is found that in the samples to which AQP is added, heat resistance of electrode response is largely improved, and improvement in response sensitivity is also achieved.


<Test 2>


Eight types of reagent solutions according to Example 1 and Comparative Example were prepared in the same manner as in Test 1 as described above, and each reagent solution was dispensed on an electrode in the same base material as the base material used in Test 1. Then, the reagent solution was dried in a low humidity drying furnace (at a drying temperature of 100° C.) to obtain an enzyme electrode (sample). However, in Test 2, the drying time (heat treatment time) in the furnace was changed to 10 minutes, 30 minutes, 60 minutes, and 120 minutes to obtain four types (a total of eight types) of enzyme electrodes (samples) for Example 1 and Comparative Example, respectively. Then, the response current values for glucose were measured in the same manner (the measurement techniques and measurement conditions) as in Test 1.



FIG. 4 is a graph illustrating the results of Test 2, that is, the relationship between the response current value (μA) and the drying time (min) for the eight types of samples as described above. In FIG. 4, white bar graphs illustrate the results of the samples according to Example 1, and black bar graphs illustrate the results of the samples according to Comparative Example. Note that the measurement was performed using two samples for each type, and the results illustrated in FIG. 4 indicate the average of the two measurement results.


According to the test results illustrated in FIG. 4, a tendency of significant reduction in response sensitivity was observed with the increase in drying time as for the samples to which no AQP was added (Comparative Example), while a tendency of maintaining suitable response sensitivity was observed irrespective of the change (increase) of drying time as for the samples to which AQP was added (Example 1). Thus, it is found that the samples to which AQP is added can have suitable heat resistance for a long time.


<Test 3>


Next, four types of reagent solutions in which the concentration of AQP was changed were prepared. The concentration (% by weight) of AQP was set to 0 (Comparative Example), 0.20%, 0.45% (Example 1), and 1%. Note that the components in the reagent solutions excluding AQP were prepared with the same contents as in Example 1.


Four types of reagent solutions obtained in this way were each dispensed on an electrode in the same manner as in Test 1 and dried at each drying time of 10 minutes, 30 minutes, 60 minutes, or 120 minutes (drying temperature was set at 100° C. in all cases) to obtain 16 types of enzyme electrodes (samples). Then, the response current value for glucose was measured in the same manner as in Test 1.


<Results of Test 3>



FIG. 5 is a graph illustrating the results of Test 3, that is, the relationship between the drying time (heat treatment time) (minutes) and the response current value (μA) for each sample. In FIG. 5, four bar graphs are illustrated for each heat treatment time. The four bar graphs each represent the response current value (response sensitivity) when the concentration of AQP is 0, 0.20%, 0.45%, or 1%, sequentially from the left.



FIG. 6 is a graph illustrating relative response sensitivity (%) at a heat treatment time of 30 minutes, 60 minutes, or 120 minutes when response sensitivity at a heat treatment time of 10 minutes in Test 3 is defined as 100%. In FIG. 6, four bar graphs are illustrated for each heat treatment time. The four bar graphs each represent the relative response sensitivity when the concentration of AQP is 0, 0.20%, 0.45%, or 1%, sequentially from the left.


Note that in Test 3, the measurement for one type of sample was performed twice using two samples of the same type. The results illustrated in FIG. 5 and FIG. 6 indicate the average values of the results at the two times of measurement.


From the results illustrated in FIG. 5 and FIG. 6, it was observed that when the concentration of AQP was 0 (without addition), the response sensitivity was reduced as the increase of heat treatment time, and the response sensitivity was almost lost at a heat treatment time of 60 minutes and 120 minutes. On the other hand, it was observed that when the concentration of AQP was 0.20%, the response sensitivity at any heat treatment time of 30 minutes, 60 minutes, or 120 minutes was lower than the response sensitivity at a heat treatment time of 10 minutes, but better than the response sensitivity when the concentration of AQP was 0. It was observed that when the concentration of AQP was 0.45%, the response sensitivity at a heat treatment time of 30 minutes, 60 minutes, and 120 minutes was almost the same as or higher than the response sensitivity at a heat treatment time of 10 minutes. It was further observed that when the concentration of AQP was 1%, the response sensitivity at any heat treatment time of 30 minutes, 60 minutes, and 120 minutes was two or more times higher than the response sensitivity at a heat treatment time of 10 minutes. From the above results, the upper limit concentration of polyaniline sulfonic acid in order for an enzyme electrode to obtain suitable heat resistance is 5% or less, preferably 1% or less, when the ease of preparation of the enzyme electrode is taken into consideration. Further, the lower limit concentration for obtaining suitable heat resistance is 0.01% or more, preferably 0.2% or more, more preferably 0.45% or more.


<Test 4>


Next, the results of a test on the influence of the concentration of a conductive polymer added to a reagent solution will be described.


<<Procedure for Preparing Enzyme Electrode (Glucose Sensor)>>


The procedure for preparing a glucose sensor is as follows. Specifically, 0.1 μl of a mixed reagent was dropped on an electrode, allowed to stand for 20 minutes at room temperature, and then dried in an oven for 30 minutes at an oven temperature of 120° C.


[Composition of Mixed Reagent (“%” is the Percent by Weight Concentration)]



  • Carbon black: 4%

  • Aqueous Tween 20 solution: 1.6% (surfactant)

  • Stabilizing agent: 0.5%

  • Phosphate buffer (pH 7.0): 16 mM

  • Aqueous glucose dehydrogenase (GDH) solution: 5.6 mg/ml

  • Aqueous polyaniline sulfonic acid solution (0, 0.01%, 0.05%, 0.1%, 0.2%, 0.4%, 0.75%, 1%, 1.5%, and 2%)

  • Water (H2O)



<<Evaluation Procedure>>

As the electrodes of the glucose sensor prepared as described above, a silver/silver chloride electrode (Ag/AgCl (manufactured by BAS)) was used for the working electrode and the reference electrode, and a platinum (Pt) wire was used for the counter electrode. Such a glucose sensor was used to measure the glucose response current (response sensitivity) by amperometry in a PBS (Phosphate Buffered Saline) solution. Specifically, the applied voltage was set to +0.4 V (vs. Ag/AgCl), and a aqueous 2 M-glucose solution was added so that final concentration might be 100 mg/dL after background current reached a plateau in the PBS solution. A value obtained by subtracting the background current value from a recorded response current value after the addition of the aqueous glucose solution was defined as the response current value of the glucose sensor for the addition of the aqueous glucose solution.


<<Results of Test 4>>



FIG. 7 is a graph illustrating the results of Test 4 obtained by the evaluation procedure as described above. FIG. 7 reveals that, at 120° C., suitable response current values are obtained over a concentration range of 0.1 to 2%. Generally, an enzyme is deactivated in high temperatures. On the other hand, since a suitable response current value is obtained even after the enzyme has passed through a high temperature of 120° C., it is found that the enzyme is properly protected from heat by polyaniline sulfonic acid. Further, it can also be grasped from the results illustrated in FIG. 7 that the concentration range that can be employed as the concentration of polyaniline sulfonic acid is 5% or less, preferably 2% or less, more preferably 1% or less, when the ease of preparation of the enzyme electrode is taken into consideration, and the lower limit concentration for obtaining suitable heat resistance is 0.01% or more, preferably 0.2% or more, more preferably 0.45% or more.


<Test 5>


Next, the results of a test on the influence of heat treatment time of a glucose sensor will be described as Test 5. In Test 5, a plurality of glucose sensors were used, each of the sensors having been prepared by a procedure in which 0.1 μl of a mixed reagent having the composition as described with respect to Test 4 was dropped on the electrode, allowed to stand for 20 minutes at room temperature, and then subjected to heat treatment in an oven for any of a plurality of different drying times (heat treatment time of 10 minutes, 30 minutes, 60 minutes, or 120 minutes) at a predetermined oven temperature (100° C.). The electrode configuration and evaluation procedure of the glucose sensor in Test 5 are the same as in Test 4.



FIG. 8 is a graph illustrating the results of Test 5. FIG. 8 illustrates four graphs indicating the relationship between the polymer concentration and the response current value with respect to four heat treatment times (10 minutes, 30 minutes, 60 minutes, and 120 minutes). It is found that, in every polymer concentration, response current values which can be applied as a glucose sensor are obtained without the influence of heat treatment time. Therefore, it is found that the response sensitivity of the glucose sensor using polyaniline sulfonic acid is not largely influenced (proper heat resistance can be exhibited) even after the sensor is placed under a high temperature for a long time.


OPERATIONS AND EFFECTS OF THE EMBODIMENT

According to the enzyme electrode 10 as described above, suitable heat resistance can be obtained by forming a detection layer 2 containing oxidoreductase 4 and a conductive polymer 5 (for example, polyaniline sulfonic acid) on an electrode 1. Thereby, a reduction or loss in function of an enzyme or a reagent by heat can be suppressed. Thus, the life of the enzyme electrode 10 can be increased because the enzyme electrode 10 exhibits suitable heat resistance during each of the transportation, storage, and use thereof.


Note that the enzyme electrode 10 can be applied, for example, to a biosensor which is applied to glucose measurement as described above, or an electronic apparatus (for example, measuring device). Alternatively, the enzyme electrode 10 can also be applied as a part of an electric power unit that supplies, to a load, current generated by an enzyme reaction (current caused by electrons transferred to an electrode) as electric power through a feed section that connects the electrode and the load. The electronic apparatus can include an electronic apparatus including a biosensor to which the enzyme electrode according to the embodiment is applied and an electronic apparatus including the above device (electric power unit) to which the enzyme electrode according to the embodiment is applied. The components described in the embodiment as described above can be suitably combined.


DESCRIPTION OF THE REFERENCE NUMERALS


1: electrode, 2: detection layer, 3: insulating substrate, 4: enzyme, 5: conductive polymer, 10: enzyme electrode

Claims
  • 1. An enzyme electrode, comprising: an electrode; anda detection layer that is in contact with the electrode and comprises an oxidoreductase, a water-soluble conductive polymer, and conductive particles,
  • 2. The enzyme electrode according to claim 1, wherein the water-soluble conductive polymer is polyaniline sulfonic acid.
  • 3. The enzyme electrode according to claim 1, wherein the oxidoreductase has a subunit containing cytochrome.
  • 4. The enzyme electrode according to claim 1, wherein the oxidoreductase has a domain containing cytochrome.
  • 5. The enzyme electrode according to claim 1, wherein the oxidoreductase is an oligomeric enzyme including at least a catalytic subunit and a subunit containing cytochrome.
  • 6. The enzyme electrode according to claim 1, wherein the oxidoreductase is an enzyme including at least a catalytic domain and a domain containing cytochrome.
  • 7. The enzyme electrode according to claim 5, wherein the catalytic subunit includes at least any one of pyrroloquinoline quinone and flavin adenine dinucleotide.
  • 8. The enzyme electrode according to claim 6, wherein the catalytic domain includes at least any one of pyrroloquinoline quinone and flavin adenine dinucleotide.
  • 9. The enzyme electrode according to claim 1, wherein the conductive particles comprise carbon.
  • 10. The enzyme electrode according to claim 2, wherein the concentration of the polyaniline sulfonic acid is 0.01 to 2%.
  • 11. The enzyme electrode according to claim 2, wherein a functional group of the polyaniline sulfonic acid is a hydroxy group or a sulfo group.
  • 12. The enzyme electrode according to claim 1, wherein the enzyme electrode has an improved heat resistance.
  • 13. A biosensor, comprising: an enzyme electrode, the enzyme electrode including:an electrode; anda detection layer that is in contact with the electrode and includes an oxidoreductase, a water-soluble conductive polymer, and conductive particles,
  • 14. An electronic apparatus comprising the biosensor according to claim 13.
  • 15. An apparatus, comprising: an enzyme electrode; anda feed section configured to supply, to a load, a current generated by an enzyme reaction at the enzyme electrode, the enzyme electrode including an electrode and a detection layer that is in contact with the electrode and comprises an oxidoreductase, a water-soluble conductive polymer, and conductive particles, wherein electrons are transferred between the enzyme and the electrode by direct electron transfer in the detection layer.
  • 16. An electronic apparatus comprising the device according to claim 15.
  • 17. A method for producing an enzyme electrode, comprising: forming a detection layer on an electrode, the detection layer comprising an oxidoreductase, a water-soluble conductive polymer, and conductive particles,
  • 18. A reagent having improved heat resistance, comprising: an oxidoreductase;a water-soluble conductive polymer; andconductive particles.
Priority Claims (1)
Number Date Country Kind
2012-142376 Jun 2012 JP national
PCT Information
Filing Document Filing Date Country Kind
PCT/JP2013/067382 6/25/2013 WO 00