GB2201248A - Enzyme electrode sensors - Google Patents

Enzyme electrode sensors Download PDF

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Publication number
GB2201248A
GB2201248A GB08804038A GB8804038A GB2201248A GB 2201248 A GB2201248 A GB 2201248A GB 08804038 A GB08804038 A GB 08804038A GB 8804038 A GB8804038 A GB 8804038A GB 2201248 A GB2201248 A GB 2201248A
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sensor
potential
voltage
enzyme
period
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GB8804038D0 (en
GB2201248B (en
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Stephen John Churchouse
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Imperial Chemical Industries Ltd
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Imperial Chemical Industries Ltd
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Priority claimed from GB878704244A external-priority patent/GB8704244D0/en
Priority claimed from GB878709796A external-priority patent/GB8709796D0/en
Application filed by Imperial Chemical Industries Ltd filed Critical Imperial Chemical Industries Ltd
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Publication of GB2201248A publication Critical patent/GB2201248A/en
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    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N27/00Investigating or analysing materials by the use of electric, electrochemical, or magnetic means
    • G01N27/26Investigating or analysing materials by the use of electric, electrochemical, or magnetic means by investigating electrochemical variables; by using electrolysis or electrophoresis
    • G01N27/28Electrolytic cell components
    • G01N27/30Electrodes, e.g. test electrodes; Half-cells
    • G01N27/327Biochemical electrodes, e.g. electrical or mechanical details for in vitro measurements
    • G01N27/3271Amperometric enzyme electrodes for analytes in body fluids, e.g. glucose in blood
    • 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
    • Y10TECHNICAL SUBJECTS COVERED BY FORMER USPC
    • Y10STECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
    • Y10S435/00Chemistry: molecular biology and microbiology
    • Y10S435/817Enzyme or microbe electrode

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  • Health & Medical Sciences (AREA)
  • Chemical & Material Sciences (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Analytical Chemistry (AREA)
  • Molecular Biology (AREA)
  • Chemical Kinetics & Catalysis (AREA)
  • Electrochemistry (AREA)
  • Physics & Mathematics (AREA)
  • Hematology (AREA)
  • Biochemistry (AREA)
  • General Health & Medical Sciences (AREA)
  • General Physics & Mathematics (AREA)
  • Immunology (AREA)
  • Pathology (AREA)
  • Measuring Or Testing Involving Enzymes Or Micro-Organisms (AREA)
  • Apparatus Associated With Microorganisms And Enzymes (AREA)

Description

11 i, 2201248 ENZYME RUCTRODE SEKSORS This Invention relates to enzyme
electrode sensors and in particular to analytical methods using such sensors.
Enzyme electrodes are increasingly used in medicai and other laboratories particularly for the determination of materials such as glucose and urea in specimens of blood-and other physiological fluids. Such electrodes are described in many publications notably an article by Clark-& Lyons (Annals of the-New York Academy of Science, 102, 2945, 1962) and US Patents 3539455 and 3979274 to Clark and Newman respectively. Enzyme electrodes are generally used to determine materials which themselves 4re not electrochemically active but which in the presence of suitable enzymes take part in reactions which produce species which can be readily detected by the electrodes. In enzyme electrodes thelenzymes are frequently located whithin polymeric materials in close proximity to the underlying electrode.- A considerable amount of research has been carried out in order to improve the properties of membranes for use in enzyme electrodes and many membranes for this purpose have been disclosed. An example of a type of membrane which is often used is the laminated membrane disclosed by Newman in US Patent 3979274.- This membrane comprises a first or inner layer of an_-essintially homogenous material, for example cellulose adetate, which can prevent the passage of materials of low molecular weight likelyto interfere with the enzymic. signal, a,close adherent layer of the enzyme itself (with or without such other materials that may be blended with it), and a second layer (in this instance an outer layer) of a porous support film which can prevent the passage of cellular and colloidal elements.
The determination of glucose can be taken as an example of the determination of a material,by an enzyme electrode. In the -presence of the enzyme glucose oxidase the following reaction occurs:- 0 glucose Glucose + 02 is oxidase Gluconic acid + H202.
The hydrogen peroxide produced in this reaction passes through the first layer of a membrane such as that of US Patent 397927.C and can be determined using the electrode. Since the hydrogen peroxide produced is dependent upon the glucose present in a specimen, the glucose concentration can be determined using a suitable calibrated sensor.
To date a number of difficulties have limited the utility of enzyme electrodes and restricted the scale of their use in routine analysis of, e.g. blood samples.
one of these difficulties is the limited linearity of the response of electrodes to analytes such as glucose.or lactate which are substrates for the enzyme catalysed reactions. The response is linear only over a limited range of low concentrations of the analytes and hence the concentrations of the materials to be determined must be low and generally diluted,samples must be used in specimens for analysis using enzyme electrodes. It is not always practicable to make diluted samples for routine analysis outside the laboratory and it would be impossible for invasive monitoring. This difficulty can be alleviated to some extent at least by suitable treatment of the outer layers of enzyme electrode membranes as described in our European Patent Application No. 204468 or by using enzyme membranes comprising polymeric layers of res tricted permeability between the enzymic layers and samples to be analysed as described in our European Patent Application No. 216577.
Another difficulty is the effect of interfering species in the sample under test which can themselves give rise to a signal thereby enhancing the overall signal and causing an electrode to give a reading which is too high. For example when an enzyme-electrode is used to measure glucose in blood the enzyme-mediated signal produced 1 t.
t LA 1 t may beap propriate but the observed signal may be elevated by_,a number of other species in the blood such as ascorbic acid which can give direct electrochemical signals at the-hydrogen-peroxide detecting electrode. The difficulty can be alleviated at least to some extent by use in electrodes of membranes formed from alternative polymeric materials as described in our European Patent Application ITo. 86308918.1. Moreover,,-British Patent Application No. 2,019,580A describes a method of-determining the sugar content of a fluid containing an interfering foreign substance by using an electrocatalytic sugar sensor having a measuring electrode which is alternatively given a static reactivation potential and a static measuring potential, the current flowing being measured during the measuring period, and subsequent.delivery of the interfering foreign substance to the measuring electrode being inhibited by a membrane placed before the measuring electrode such that a diffusion-limiting current is rtgt up in the reactivation phase during oxidation of the foreign substances, wherein measurement of the current is effected after a time delay relative to the beginning of the measuring period.
A further development of enzyme electrodes could make possible the large-scale production of inexpensive instruments having for example disposable electrodes or membranes. This would make it possible for rapid routine measurements of e.g.. glucose in blood, to be made regularly in the home or in doctors' surgerys, health centres and out-patients clinics and would facilitate faster diagnosis of many serious conditions. However, such a development is hindered since, when measurements aremade using enzyme electrodes, problems are experienced due to the length of-time required to obtain a stable signal. With present enzyme electrodes periods of 10 minutes and above are often required before a stable base-line can be established. This is ace eptable if the instrument is a multi-use sensor which is kept active constantly. It is not acceptable for intermittent measurements on a regular basis using non-disposable electrode- membrane sets for multiple measurements.
We have now found that enzyme electrodes can be controlled in a manner such that the period required to establish a stable signal is greatly reduced-thereby providing an improved analytical method using an enzyme electrode. It will be appreciated that wh:rlst the invention of British Patent Application No. 2019580A is directed to the constant cleansing of blocking adsorption products from the electrode surface during use by reactivation of the electrode surface 10 by anodic oxidation whereby to achieve long-term operation, the invention of the present application is directed to reducing the time period required, prior to any analytical measurement, before a sufficiently stable signal is achieved to permit the measurement to be effected.
is According to the present invention we provide an analytical method using a sensor of the enzyme electrode type for determining in a sample the concentration-of an analyte-reactive with an enzyme present on the sensor to produce an electrochemically active spec ies detectable by the sensor, wh ich comprises applying a potential across the sensor to cause in electrical current to flow therethrough, contacting the sensor with the sample thereby causing a change in the current flow and, when a working potentia is applied across the sensor, determining the concentration of the analyte as a function of the change in the current characterised in that at some time before the working potential is applied and the concentration of the analyte is determined a potential significantly in excess of the working potential is applied, whereby to reduce the period required to establish a signal sufficiently stable to permit the determination to be effected.
It will be appreciated that where a time response curve is obtained which Is predictable, it will then be possible to effect the desired determination using known numerical analysis techniques such 21 1 as curve stripping and non-linear optimisation techniques.
Suitably the sensor is contacted with the sample before the applied potential is Increased to the level significantly in excess of the working potential and thereafter is reduced to the working potential for determination of-the concentration of the anilyte. However the potential in excess of the working potential can be applied before the tensor is contacted with the sample.
The present invention is thus particularly directed to rapidly adapting the electrochemical performance of a virgin electrode for use in an analytical method as defined above. Such a virgin electrode will in general have the characteristics, particularly the surface characteristics,of an electrode which_has not been subjected to any substantial electrical activity and which thus does not possess the requisite oxidised surface necessary to achieve a signal sufficiently stable to permit the desired determination to be e fective. In general the electrode will not have been subjected to any electrical activity other than for pre-sale testing. Thus for example in relation tametal electrodes, especially platinum electrodes, the oxidised surface may contain no more than about one molecule of oxygen per 2 molecules of metal especially platinum.
Also according to the present invention we provide a preferred analytical method using a sensor of the enzyme electrode type for determining in a sample the concentration of an analyte reactive with an enzyme present on the sensor to produce an electrochemically active species-detectable by the sensor, which comprises applying a potential across the sensor to cause an -electrical current to flo w therethrough, contacting the sensor with the sample thereby causing a change in the current flow and determining the concentration of the analyte as a function of the change in current- characterised in that after -,the sensor is contacted with the sample the applied potential is reduced to zero and then is significantly increased, before being reduced to a working potential for determination of the concentration of the analyte.
It will be appreciated that the expression "the applied potential is reduced to zero" is intended to include disconnection or 5 shorting of the electrical connections.
1 -Further according to the present invention we provide. control apparatus for a sensor of the enzyme electrode type which comprises an electrical circuit connectable to the sensor-and to a recording means wherein the circuit comprises (a) a programmable constant voltage source (PM), (b) control circuitry for the PCVS, (c) current measurement circuitry (CMC), and (d) a switch which can connect a sensor into the circuit, (a), (b), (c), and (d) being connected together in an appropriate manner in the circuit, characterised in that when connected to the sensor the apparatus can carry out the following programme steps automatically;1 (1) applying a potential to the sensor to cause an electrical current to flow therethrough; (2) significantly increasing the potential after a change in current flow is detected when the sensor has been contacted with a sample containing an analyte to be determined by the sensor; and thereafter (3) reducing the potential to a predetermined working potential and determining the concentration of the analyte; the increase in potential and the period for which the increased potential is applied being such that in use the period required to establish a signalsufficiently stable to permit the determination to be effected, is reduced.
Using the method of the Invention the time required to obtain a stable signal is reduced to a period in the range 20 seconds to 3 minutes in most instances.
f The steps in the preferred method of the invention can be listed as follows:- t (1) applying a voltage to the sensor; (2) (3) is (4) (5) applying the specimen to the sensor; when the control-circuitry detects that the specimen has been applied to the sensor, any previous voltage across the sensor is zeroed (or-the connection may be disconnected or shorted) for a period and then is increased to a level significantly above the intended working voltage for a predetermined period of time-, after the pre-cleterm.ined period reducing the voltage applied to the- sensor to the working voltage; and determining the analytain the specimen, steps (1) and (2) being carried out in either order or simultaneously.
In step (3) of the second method defined above the period for which the voltage Ls zeroed should be short, preferably in the range 1 to 3 seconds. The enzyme electrode sensor_used in the method of the invention will generally have an anode which is a working electrode and a cathode which is-a "pseudo-reference" electrode. These electrodes will usually be formed from inert metals such as platinum and silver upon which unstable oxide layers fo rm and carbon. Between the electrodes and the specimen containing the analyte to be determined is a membrane having within it an enzyme-containing layer. In its most simple form-themembrane in such a sensor consists-of an enzyme- containing layer and a layer - usually formed from a polymeric material - of restricted permeability. The layer of restricted permeability is the outer layer in this simple form of membrane and is directly contacted-by the specimen in the method of the invention for determining an analyte. Preferably however the membrane is a laminated membrane of the type of idhich that disclosed in US Patent 3979274 is an example. Such a membrane, as previously stated, comprises a first or inner layer of material positioned between the enzyme-containing layer and the electrode, the enzyme-containing layer and a second layer of material on the other side of the enzymecontaining layer which second layer is the layer having restricted permeability. The membranes in enzyme electrodes can contain more than two layers of material in addition to the enzyme-containing layer. For instance the second layer is not necessarily the outermost layer of the membrane. There may be a further layer or layers of material, i.e. third, fourth etc. layers, between the second layer and the specimen. often however the second layer will be the outer layer and its outer face will be contacted by the specimen.
is The enzyme present in an enzyme electrode may be located in the membrane in any suitable manner. Preferably in a laminated membrane it is present between the first and second layers of porous material and forms the bond between them. In this situation, and also generally, the enzyme is preferably immobilised by mixing with a material which causes cross-linking to occur. A very suitable material for this purpose is glutaraldehyde; proteins such as albumin and other materials may also be included. In order to facilitate the obtaining of rcpid stable readings from the sensor it is preferred that the enzyme- containing layer is thin, i.e. not more than 5 microns thick. The enzyme to be used in the sensor will depend upon the analyte whose concentration is to be determined. If the analyte is glucose then the enzyme will be for example glucose oxidase. Other enzymes which may be present include uricase and lactate oxidase for determination of uric acid and lactic acid respectively. Enzyme systems comprising two or more enzymes,: may also be present. Enzyme electrodes are described in more detail particularly with regard to the porous materials to be used in the membranes in our co-pending patent applications EP 204468A and 216577A, European Application 86308918.1 and UK Application 8626026.
1 i 1 f f 1 The operation of the method of the invention can be varied in a number of ways but a very suitable series of operations is-as follows. First the enzyme electrode or other sensor and a recording means are connected to the control apparatus then, preferably using the switch, the working And reference (i.e. the pseudo-reference electrode mentioned above) electrodes are connected. No curent is passing and no voltage is applied at this stage. A voltage is then applied, preferably positive at the anode, and the current monitored. This voltagecan be either AC or DC and its magnitude is not critical. For instance it can be the working voltage or a lower voltage., The specimen containing the analyte to be determined Is then applied to the sensor. Alternatively this can be done before the voltage is applied.- 'After a delay to allow for diffusion the wetness on the sensor caused by application of the specimen is detected as a significant change in current., At this point the applied voltage is decreased t8"near zero for a standard length of time followed by an increased-voltage. The,voltage now applied is DC. After a predetermined time period when the layer of oxide on the electrode has been deposited, preferably to the extent which will ultimately be reached at.the working voltage, the applied voltage is reduced to the working voltage. The reading on the recorder should now be sufficiently stable for a meaurement to be made.
In an alternative less-preferred embodiment of the method of the invention the voltage first applied in step (1) is a voltage significantly above the intended working voltage. This voltage is then main tained for a-pre-determined period before being reduced to the working voltage.
The control apparatus can usefully include a device for detecting changes in conductivity or any derived parameter in order to indicate when conducting solution has reached an electrode in the sensor.
1 A preferred working voltage Is in the rang. e 0.4 volts to 1 0.75 volts. The significantly higher voltage is preferably in the range 0. 8 volts to 1.9 volts and is preferably maintained for a period in the range 15 seconds to 1 minute, particularly approximately 30 seconds. Generally shorter pre-determined periods are necessary with higher voltages.
- The invention is illustrated by the accompanying drawing which is a simplified circuit diagram of the control apparatus connected to an enzyme electrode and a chart recorder.
The control apparatus shown in the drawing comprises a programmable constant voltage source (PCYS) 1 with programming input at 2, control circuitry 3 for the PUS, current measurement circuitry (CM0 4 and on/off switch 5.. Chart recorder or data processor 6 and enzyme electrode 7 are connected to the control apparatus. The constant voltage supplied by PCVS 1 passes through CMC 4 to the electrode 7. A signal which is a defined function of the current passing electrode 7 passes to recorder 6 and is monitored by control circuitry 3 which can make interpretation of current passing through 20 the electrode and reacts appropriately.
In operation the sequence of steps is as follows:
(i) Switch 5 is moved into the onposition thereby applying a supply voltage to the circuitry and applying an initial voltage to the working electrode of enzyme electrode 7; (ii) A sample is applied to the outer.face of the membrane on enzyme electrode 7; (M) An increase in current passing through the electrode is detected by the control circuitry 3 when the membrane on enzyme electrode 7 has been wetted; (iv) Control circuitry 3 reprogrammes PUS 1 to give a near zero 35 voltage for a short fixed period of time followed by a voltage 1 - It, - li - significantly above the intended working voltage for a pre-determined period of time; fl (v) After the pre-determined period of time control circuitry 3 -5 again reprogrammes PCVS 1# this time for the working voltage; (vi) -The measurement of the electric current flowing through - enzyme electrode 7 ismade and recorded on chart recorder or data processor 6; and (Vii) The circuit switches off. If a further sample is to be examined the apparatus can be returned to (i) above or, without switching the instrument off in-step (vii), directly to (ii).
is In the above procedure operation of the switch can be automatic or manual.

Claims (11)

CLAIMS 1 6.
1. An analytical method using a sendor of the enzyme electrode type for determining in a sample the concentration of an analyte reactive with an enzyme present on the sensor to produce an electrochemically active species detectable by the sensor,-which comprises applying a potential across the sensor to cause an electrical current to flow therethrough, contacting the sensor with the sample thereby causing a change in the current flow and, when a working potential is applied across the sensor, determining the concentration of the analyte as a function of the change in the current characterised in that at some time before the working potential is applied.and the concentration of the analyte is determined a potential significantly in excess of the working potential is applied, whereby I to reduce the period required to establish a signal sufficiently stable to permit the determination to be effected.
2. An analytical method as claimed in claim 1 wherein, after the sensor is contacted with the sample the applied potential is reduced to zero (as herein defined) and then is significantly increased, before being reduced to a working potential for determination of the concentration of the analyte.
3. An analytical method as claimed in claim 2 wherein the period for which the applied potential is zeroed is in the range 1 to 3 seconds.
4. An analytical method as claimed in any one of the preceding claims wherein the sensor of the enzyme electr ode type is disposable.
5. An anlytical method as claimed in any one of the preceding claims wherein the working.voltage is in the range 0.4 to 0.75 volts.
An analytical method as claimed In any one of the preceding - 4 A 1 t; 9 claims wherein the potential significantly in excess of the working potential Is in the range 0.8 to 1.9 volts and Is maintained for a period in the range 15 seconds to 1 minute.
7. A control apparatus for a sensor of the enzyme electrode type which comprises an electrical circuit connectable to the sensor and to a recording means wherein the circuit comprises (a) a programmable constant voltage source, (b) control circuitry for the programmable constant voltage source, (c) current measurement circuitry, and (d) a switch which can connect a sensor into the circuit, (a), (b), (c) and (d) being connected together in an appropriate manner in the circuit, characterised in that when connected to the sensor the. apparatus can carry out the following programme steps automatically:- _ is (1) applying a potential to the sensor to causean electrical current to flow therethrough; (2) significantly increasing the potential after a change in current flow is detected when the sensor has been contacted with a sample containing an analyte to be determined by the sensor; and thereafter (3) - reducing the potential to a predetermined working potential and determining the concentration of the.-lanalyte; the increase in potential and the period for which the increased potential is applied being such that in use the Period required to establish a signal sufficiently stable to permit the determination to be effected, Is reduced.
8. A control apparatus as defined in claim 7 which, when connected to the sensor, can carry out the following programme steps automatically:- (1) (2) (3) apply a voltage to the sensor; applying the specimen to the sensor; when the control circuitry detects that the specimen has been applied to the- sensor, any previous voltage across the (4) (5) sensor is zeroed (as herein defined) for a period and then is increased to a level significantly above the intended working voltage for a pre- determined period of time; after the pre-determined period reducing the voltage applied to the sensor to. the working voltage; and determining the analyte in the specimen, steps (1) and (2) being carried out in either order or simultaneously.
9. A control apparatus is claimed in claim 8 wherein the ccntrol apparatus is programmed such that the period for which the voltage is zeroed is in the range 1 to 3 seconds.
10. An analytical method using a sensor of the enzyme electrode type for determining in a sample the emcantration of an analyte reactive with an enzyme present cn the sensor to produce an electrochemically active species detectable by the sensor, wtiich analytical method is substantially as hereinbefore described.
11. A control apparatus for a sensor of the enzyme electrode type, which apparatus is substantially as hereinbefore described with reference to the acc=panying drawing.
Published 1988 at The Patent Office, State House, 65171 High Holborn, London W01R 4TF. Further copies may be obtained from The Patent office, Sales Branch, St Mary Cray, Orpington, Kent BR5 3RD. Priuted by Multiplex techniques ltd, St Mary Cray, Kent. Con. 1187.
GB8804038A 1987-02-24 1988-02-22 Enzyme electrode sensors Expired GB2201248B (en)

Applications Claiming Priority (2)

Application Number Priority Date Filing Date Title
GB878704244A GB8704244D0 (en) 1987-02-24 1987-02-24 Sensor control apparatus
GB878709796A GB8709796D0 (en) 1987-04-24 1987-04-24 Controls for enzyme electrode sensors

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GB8804038D0 GB8804038D0 (en) 1988-03-23
GB2201248A true GB2201248A (en) 1988-08-24
GB2201248B GB2201248B (en) 1991-04-17

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JP (1) JPH01219661A (en)
AU (1) AU1212988A (en)
DE (1) DE3805773A1 (en)
FR (1) FR2611272B1 (en)
GB (1) GB2201248B (en)
IT (1) IT1215946B (en)

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IT8819511A0 (en) 1988-02-24
US4935105A (en) 1990-06-19
DE3805773A1 (en) 1988-09-22
GB8804038D0 (en) 1988-03-23
IT1215946B (en) 1990-02-22
GB2201248B (en) 1991-04-17
JPH01219661A (en) 1989-09-01
FR2611272A1 (en) 1988-08-26
FR2611272B1 (en) 1991-01-18

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