Method and apparatus for analyte detection using an electrochemical biosensor
阅读说明:本技术 用于采用电化学生物传感器进行分析物检测的方法和设备 (Method and apparatus for analyte detection using an electrochemical biosensor ) 是由 S·M·奥贾 B·费尔德曼 于 2018-06-29 设计创作,主要内容包括:本发明涉及一种用于利用具有工作电极的传感器感测分析物的方法,该方法包括向工作电极提供分析物特异性酶和氧化还原介体,向所述分析物提供所述工作电极,使源自与所述分析物特异性酶和所述氧化还原介体反应的所述分析物的电荷累积达设定的时间段,在所述设定的时间段之后将所述工作电极连接至电路,和测量来自所累积的电荷的信号。(The invention relates to a method for sensing an analyte with a sensor having a working electrode, the method comprising providing an analyte-specific enzyme and a redox mediator to the working electrode, providing the working electrode to the analyte, accumulating charge derived from the analyte reacting with the analyte-specific enzyme and the redox mediator for a set period of time, connecting the working electrode to an electrical circuit after the set period of time, and measuring a signal from the accumulated charge.)
1. A method for sensing an analyte with a sensor comprising a working electrode, the method comprising:
providing an analyte-specific enzyme and a redox mediator to the working electrode;
providing the working electrode to the analyte;
accumulating charge derived from the analyte reacted with the analyte-specific enzyme and the redox mediator for a set period of time;
connecting the working electrode to an electrical circuit after the set period of time; and
a signal from the accumulated charge is measured.
2. The method of claim 1, wherein prior to providing the working electrode to the analyte, the method further comprises connecting the working electrode to the electrical circuit, and prior to providing the working electrode to the analyte, the method further comprises disconnecting the working electrode from the electrical circuit.
3. The method of claim 1, wherein the working electrode is connected to the electrical circuit prior to providing the working electrode to the analyte, the method further comprising disconnecting the working electrode from the electrical circuit prior to providing the working electrode to the analyte.
4. The method of claim 1, wherein the sensor is an enzymatic electrochemical biosensor.
5. The method of claim 1, wherein the redox mediator is an immobilized redox polymer.
6. The method of claim 1, wherein the analyte is selected from the group consisting of cortisol, glucose, lactic acid, 3-hydroxybutyrate, alcohols, pyruvate, glutamate, theophylline, and creatinine.
7. The method of claim 1, wherein the analyte-specific enzyme is selected from the group consisting of Nicotinamide Adenine Dinucleotide (NAD) -dependent dehydrogenase, Flavin Adenine Dinucleotide (FAD) -dependent oxidase, and Flavin Mononucleotide (FMN) -dependent oxidase.
8. The method of claim 1, wherein the analyte-specific enzyme is selected from the group consisting of 11 β -hydroxysteroid dehydrogenase type 2 (11 β -HSD-2), glucose oxidase, NAD-glucose dehydrogenase, FAD-glucose dehydrogenase, lactate oxidase, NAD-lactate dehydrogenase, NAD-alcohol dehydrogenase, pyruvate oxidase, NAD-glutamate dehydrogenase, and xanthine oxidase.
9. The method of claim 1, wherein the concentration of the analyte is as low as 4.7 nanomolar.
10. The method of claim 1, wherein the measuring a signal from the accumulated charge comprises measuring a peak height of the signal and/or measuring a peak area of the signal.
11. The method of claim 10, further comprising calibrating the measured peak heights to provide a concentration of the analyte.
12. The method of claim 10, further comprising calibrating the measured peak areas to provide a concentration of the analyte.
13. The method of claim 1, wherein the measuring a signal from accumulated charge comprises recording the signal at a sampling rate of 0.1 to 0.5 hertz (Hz) and/or filtering the signal at a frequency of 0.032 to 3.2 hertz (Hz).
14. The method of claim 1, wherein the working electrode comprises a sensing element comprising the analyte-specific enzyme and the redox mediator.
15. The method of claim 14, wherein the sensing element further comprises a carbon nanotube.
16. A method for sensing an analyte with a sensor comprising a working electrode comprising an analyte-specific enzyme and a redox mediator, the method comprising:
providing the working electrode to the analyte;
accumulating charge derived from the analyte reacted with the analyte-specific enzyme and the redox mediator; and
measuring a signal from the accumulated charge by measuring a peak height of the signal and/or measuring a peak area of the signal.
17. A system for sensing an analyte, the system comprising:
a working electrode;
a sensing element disposed on the working electrode, the sensing element comprising an analyte-specific enzyme and a redox mediator, the sensing element configured to accumulate charge derived from the analyte reacted with the analyte-specific enzyme for a set period of time; and
a circuit configured to connect with the working electrode after the set period of time and measure a signal from the accumulated charge.
18. The system of claim 17, further comprising an outer membrane covering at least the sensing element.
19. The system of claim 17, wherein the analyte-specific enzyme is selected from the group consisting of Nicotinamide Adenine Dinucleotide (NAD) -dependent dehydrogenase, Flavin Adenine Dinucleotide (FAD) -dependent oxidase, and Flavin Mononucleotide (FMN) -dependent oxidase.
20. The system of claim 17, wherein the analyte-specific enzyme is selected from the group consisting of 11 β -hydroxysteroid dehydrogenase type 2 (11 β -HSD-2), glucose oxidase, NAD-glucose dehydrogenase, FAD-glucose dehydrogenase, lactate oxidase, NAD-lactate dehydrogenase, NAD-alcohol dehydrogenase, pyruvate oxidase, NAD-glutamate dehydrogenase, and xanthine oxidase.
Technical Field
Embodiments of the present invention relate to analyte sensing using an electrochemical enzyme biosensor. For example, embodiments of the present invention relate to a method and an enzyme biosensor that allow for the detection of low concentrations of an analyte by allowing the analyte to accumulate on the biosensor.
Background
Enzyme biosensors have been developed and used, which utilize an enzyme associated with a transducer as a biorecognition element for a target analyte. Although many different signal conversion methods have been used, electrochemical methods are most commonly used. Electrochemical biosensors allow direct conversion of biological events (e.g., analyte detection) into electrical signals, eliminating the need for complex instrumentation, thereby providing desirable features to electrochemical biosensors in terms of size, cost, and portability. In electrochemical techniques for signal conversion, amperometry (amperometry) is often used. In amperometric measurements, the working electrode of the sensor is held at a constant potential (voltage) while measuring the current flowing through the sensor. Such sensors are designed such that the current depends on the analyte concentration.
An example of an enzymatic biosensor that utilizes amperometry is a continuous glucose sensor, which is a wearable in-vivo device designed to provide frequent blood glucose concentration measurements to a user. These devices use a glucose oxidoreductase, such as glucose oxidase (GOx), immobilized on the working electrode as a glucose sensing element. Electrons are first transferred from glucose to the enzyme via enzymatic oxidation and then through a redox mediator (e.g., oxygen (O)2) Or osmium (Os) -containing redox polymers) to the working electrode. While amperometry has proven useful for measuring analytes such as glucose present at relatively high physiological concentrations, equal to or above 5 millimolar (mM), it may not be suitable for measuring analytes present at lower concentrations.
Disclosure of Invention
Aspects of embodiments of the invention are directed to detection of low concentrations (e.g., equal to or less than 5mM, 1 nanomolar (nM) to 5mM, or 4.7nM to 5mM) of analyte by allowing accumulation of analyte on the enzyme biosensor.
In some embodiments of the invention, a method for sensing an analyte with a sensor having a working electrode, wherein the method comprises: providing an analyte-specific enzyme and a redox mediator to the working electrode, providing the working electrode to the analyte, accumulating charge derived from the analyte reacting with the analyte-specific enzyme and the redox mediator for a set period of time, connecting the working electrode to an electrical circuit after the set period of time, and measuring a signal from the accumulated charge.
In some embodiments of the invention, the method comprises connecting the working electrode to the electrical circuit prior to providing the working electrode to the analyte, and disconnecting the working electrode from the electrical circuit prior to providing the working electrode to the analyte.
In some embodiments of the invention, the working electrode is connected to the electrical circuit prior to providing the working electrode to the analyte, and the method comprises disconnecting the working electrode from the electrical circuit prior to providing the working electrode to the analyte.
In some embodiments of the invention, the sensor is an enzymatic electrochemical biosensor.
In some embodiments of the invention, the redox mediator is an immobilized redox polymer.
In some embodiments of the invention, the immobilized redox polymer comprises a redox species (redox species) selected from osmium (Os), ruthenium (Ru), iron (Fe), or cobalt (Co) containing polymers and a polymer selected from poly (vinylpyridine), poly (thiophene), poly (aniline), poly (pyrrole), or poly (acetylene).
In some embodiments of the invention, the immobilized redox polymer is an Os-containing poly (vinylpyridine).
In some embodiments of the invention, the analyte is selected from cortisol, glucose, lactic acid, 3-hydroxybutyrate, alcohol, pyruvate, glutamate, theophylline or creatinine.
In some embodiments of the invention, the analyte-specific enzyme is a Nicotinamide Adenine Dinucleotide (NAD) -dependent dehydrogenase, a Flavin Adenine Dinucleotide (FAD) -dependent oxidase, and/or a Flavin Mononucleotide (FMN) -dependent oxidase.
In some embodiments of the invention, the analyte-specific enzyme is selected from 11 β -hydroxysteroid dehydrogenase type 2 (11 β -HSD-2), glucose oxidase, NAD-glucose dehydrogenase, FAD-glucose dehydrogenase, lactate oxidase, NAD-lactate dehydrogenase, NAD-alcohol dehydrogenase, pyruvate oxidase, NAD-glutamate dehydrogenase, or xanthine oxidase.
In some embodiments of the invention, the accumulated charge comprises accumulated electrons.
In some embodiments of the invention, the sensor is placed subcutaneously in the body of a subject.
In some embodiments of the invention, the concentration of the analyte is as low as 4.7 nanomolar (nM).
In some embodiments of the invention, the set period of time ranges from 60 seconds to 30 minutes. In some embodiments, the set period of time ranges from 120 seconds to 30 minutes. In some embodiments, the set period of time ranges from 120 seconds to 10 minutes.
In some embodiments of the invention, the sensor comprises an outer membrane. In some embodiments, the outer membrane is a flux limiting membrane. In some embodiments, the outer membrane is an analyte permeable membrane.
In some embodiments of the invention, the measuring the signal from the accumulated charge comprises measuring a peak height of the signal and/or measuring a peak area of the signal.
In some embodiments, the method further comprises calibrating the measured peak heights to provide the concentration of the analyte.
In some embodiments, the method further comprises calibrating the measured peak areas to provide the concentration of the analyte.
In some implementations, the measuring the signal from the accumulated charge includes recording the signal at a sampling rate of 0.1 to 0.5 hertz (Hz) and/or filtering the signal at a frequency of 0.032 to 3.2 hertz (Hz).
In some embodiments of the invention, the working electrode comprises a sensing element comprising the analyte-specific enzyme and the redox mediator. In some embodiments, the sensing element further comprises a carbon nanotube.
In some embodiments, a method for sensing an analyte with a sensor comprising a working electrode comprising an analyte-specific enzyme and a redox mediator, the method comprising: providing the working electrode to the analyte; accumulating charge derived from the analyte reacted with the analyte-specific enzyme and the redox mediator; and measuring a signal from the accumulated charge by measuring a peak height of the signal and/or measuring a peak area of the signal.
In some embodiments of the present invention, a system for sensing an analyte includes a working electrode, a sensing element disposed on the working electrode, the sensing element including an analyte-specific enzyme and a redox mediator, the sensing element configured to accumulate a charge derived from the analyte reacted with the analyte-specific enzyme for a set period of time, and a circuit configured to connect to the working electrode after the set period of time and measure a signal from the accumulated charge.
Drawings
Fig. 1 is a flow chart describing a method for accumulation mode sensing according to an embodiment of the present invention, including
Fig. 2 shows a schematic diagram of an electrode arrangement for accumulation mode sensing according to an embodiment of the invention, in which the working electrode is at a potential (voltage) sufficient to drive the redox reaction of the analyte under steady state conditions when the circuit is connected as shown in the left panel, and the working electrode is electrically disconnected from the circuit when the circuit is disconnected as shown in the right panel, so that electrons originating from the analyte can be stored in the redox polymer until the working electrode is reconnected to the circuit and the stored charge can be measured.
Fig. 3A shows several quantitative parameters of expected current versus (vers, vs.) time signal and accumulation mode sensing (as shown, accumulation time, peak area, and peak height when the circuit is open, respectively) according to an embodiment of the invention.
FIG. 3B shows the use of a redox polymer (Os) with osmium, according to an embodiment of the present invention3+) Schematic representation of the redox reaction that co-immobilized oxidase (AOx) undergoes during cumulative mode sensing of oxidizable analyte (analyte a) (as shown when the circuit is open as described for "open circuit").
Fig. 3C shows a trace of current versus (vs.) time obtained using an exemplary glucose sensor (at +40mV, shown in hatched lines) for cumulative mode sensing of 2 μ Μ glucose (shown in white), and 5 different cumulative times were measured, according to an embodiment of the invention.
Fig. 3D shows a calibration curve of amperometry and cumulative mode signal measured by peak height or peak area of the accumulation time as shown in fig. 3C, in accordance with an embodiment of the present invention.
Fig. 4A shows a trace of representative current versus (vs.) time for a calibration experiment using cumulative mode sensing and an exemplary glucose sensor at +40mV, as shown by the hatched lines, and a 60 second cumulative time (when the circuit is open as shown in white) for each detection, according to an embodiment of the invention.
Fig. 4B shows a comparison of a calibration curve derived from amperometry and the cumulative mode signal measured by the sensing experiment shown in fig. 4A, in accordance with an embodiment of the present invention.
Fig. 5 shows calibration curves for amperometric and accumulation mode sensing (peak height and peak area) at blood glucose concentrations of 0, 50, 100, 200, and 500 μ M at 1 (diamond), 2 (triangle), 5 (square), and 10 (circle) minute accumulation times as shown, where each calibration curve represents the average response of four sensors, according to an embodiment of the invention.
FIG. 6A shows a graph of potential versus time signal for a model glucose sensor obtained using an open-circuit potentiometry to sense glucose at various nanomolar (nM) concentrations as shown, in accordance with an embodiment of the present invention.
Fig. 6B shows a calibration curve (slope versus glucose concentration (nM)) for the graphical data of fig. 6A, in accordance with an embodiment of the present invention.
FIG. 6C shows a graph of potential versus time signal for a model glucose sensor obtained using an open-circuit potentiometry to sense glucose at various nM concentrations as shown, in accordance with an embodiment of the invention.
Fig. 6D shows a calibration curve (slope versus glucose concentration (nM)) for the graphical data of fig. 6C, in accordance with an embodiment of the present invention.
Fig. 6E shows a composite calibration curve for a model glucose sensor (filled circle data points, n-8) and a control sensor (open circle data points, n-4) using an open circuit potentiometry for in vitro glucose sensing, according to an embodiment of the present invention.
Fig. 6F shows an enlarged view of the calibration curve of fig. 6E for 0 to 200nM glucose, in accordance with an embodiment of the present invention.
FIG. 6G shows a graph of potential versus time signals for a model glucose sensor for sensing various nM concentrations of glucose as shown, using an open circuit potentiometric approach with a model glucose sensor as the working electrode and a control sensor (with redox polymer but without glucose oxidase) as the reference electrode, according to an embodiment of the invention.
Fig. 6H shows a calibration curve (slope versus glucose concentration (nM)) for the graphical data of fig. 6G, in accordance with an embodiment of the present invention.
Fig. 7 shows a comparison of cumulative mode signal shapes at different filtering frequencies according to an embodiment of the present invention, where the solid line shows 3.2Hz and the dashed line shows 0.032 Hz.
Figure 8A shows photomicrographs of two deposited glucose sensing reagents with (right panel) and without (left panel) carbon nanotube CNTs, according to an embodiment of the invention.
FIG. 8B shows calibration curves for amperometric and accumulation mode detection (peak height and peak area) with different filtering frequencies (0.032Hz shown in circles and 3.2Hz shown in triangles) and sensing agents with and without CNTs, according to an embodiment of the invention.
Fig. 9A shows a cumulative mode signal obtained from a representative glucose sensor during a calibration experiment using glucose concentrations of 0 to 200nM, with a 30 minute cumulative time per detection, with signal filtered at 3.2Hz, and CNT added to the sensing reagent, according to an embodiment of the invention.
Fig. 9B shows a calibration curve with a corresponding linear fit derived from the amperometric and cumulative mode signals measured for the sensing experiment shown in fig. 8A, each signal being the average of 8 sensors minus the background, the error bars representing the standard deviation, and the bottom of the graph is an enlarged graph showing glucose concentrations from 0 to 50nM, in accordance with an embodiment of the invention.
Fig. 10A shows the cumulative mode signal for a representative glucose sensor under background conditions ([ glucose ] ═ 0) with atmospheric open (bold line) and oxygen scavenging (thin line) buffer solutions, according to an embodiment of the invention.
Fig. 10B shows an overview of the background amperometric and cumulative mode signals from the experiment shown in fig. 10A, where the signals are averages (averages) of 4 sensors, and the oxygen scavenging data are shown as filled circles and the atmospheric data are shown as open circles, according to an embodiment of the present invention.
Fig. 11 shows calibration curves obtained for amperometric and accumulation mode sensing (peak height and peak area) during sensing experiments with glucose concentrations of 0 to 200 μ Μ, according to an embodiment of the invention, where the linear lines are shown as linear best fit lines obtained from 0 to 200nM concentrations and predicted from higher concentrations, each signal being an average of 8 sensors.
FIG. 12 shows a schematic diagram of an analyte sensor according to an embodiment of the invention.
FIG. 13 is a cross-sectional view depicting a portion of an analyte sensor compatible with one or more embodiments of the present invention.
FIG. 14A illustrates a plan view of an implantable analyte sensor compatible with one or more embodiments of the invention.
FIG. 14B is a cross-sectional view depicting a portion of any analyte sensor having a membrane compatible with one or more embodiments of the present invention.
FIG. 14C shows a close-up view of a sensing layer, working electrode, and substrate with an overlying outer membrane, according to an embodiment of the invention.
FIG. 14D is a schematic diagram depicting a redox reaction of an analyte with an analyte-specific enzyme and a redox mediator on a working electrode, according to an embodiment of the invention.
Fig. 15 is a block diagram of an embodiment of an analyte monitoring system according to an embodiment of the present invention.
Fig. 16 is a block diagram of an embodiment of a reader device of the analyte monitoring system of fig. 15, according to an embodiment of the present invention.
Fig. 17 is a block diagram of an embodiment of a sensor control device of the analyte monitoring system of fig. 15, according to an embodiment of the present invention.
Detailed Description
Embodiments of the present invention provide an electrochemical measurement method for measuring low nanomolar concentrations of analytes in vitro and in vivo using an electrochemical sensor. Embodiments of the invention include electrochemical sensors, such as enzyme biosensors modified to measure low nanomolar concentrations of analytes.
Where a range of values is provided, it is understood that each intervening value, to the tenth of the unit of the lower limit unless the context clearly dictates otherwise, between the upper and lower limit of that range is also expressly disclosed. Each smaller range between any stated value or intervening value in a stated range and any other stated value or intervening value in a stated range is encompassed within the invention. The upper and lower limits of these smaller ranges may independently be included in the range or excluded in the range, and each range where either, neither or both limits are included in the smaller ranges is also encompassed within the invention, subject to any specifically excluded limit in the stated range. Where the stated range includes one or both of the limits, ranges excluding either or both of those included limits are also included in the invention.
As used herein, the terms "substantially," "about," and similar terms are used as terms of approximation and not as terms of degree, and are intended to account for inherent deviations in measured or calculated values that would be recognized by one of ordinary skill in the art.
In the description disclosed herein, it is also to be understood that a term in the singular includes its plural counterpart and a term in the plural also includes its singular counterpart, unless implicitly or explicitly understood or stated otherwise. For example only, reference to "a" or "the" analyte "includes a single analyte as well as a combination and/or mixture of two or more different analytes, reference to" a "or" the "concentration value" includes a single concentration value as well as two or more concentration values, and so forth, unless implicitly or explicitly understood or otherwise stated. Additionally, it should also be understood that for any given component described herein, any listed possible candidates or alternatives for that component may generally be used individually or in combination with each other, unless implicitly or explicitly understood or stated otherwise. Additionally, it should also be understood that any list of such candidates or alternatives is only illustrative and not limiting, unless implicitly or explicitly understood or otherwise stated.
As used herein, the term "measuring/measuring" may encompass the meaning of the respective one of the terms "determining/measuring" and "calculating/calculating".
As used herein, an "electrochemical sensor" is a device configured to detect the presence and/or measure the level of an analyte in a sample by electrochemical oxidation and reduction reactions on the sensor. These reactions are converted into an electrical signal that can be correlated to the amount, concentration, or level of analyte in the sample.
As used herein, a "working electrode" is an electrode at which an analyte (or a second compound, the level of which depends on the level of the analyte) is electro-oxidized or electro-reduced with or without the action of an electron transfer agent.
As used herein, "counter electrode" refers to an electrode paired with a working electrode, and the current through the "counter electrode" is equal in magnitude but opposite in sign to the current through the working electrode. In the context of embodiments of the present invention, unless explicitly indicated otherwise, the term "counter electrode" includes a) a counter electrode and b) a counter electrode (i.e., a counter/reference electrode) that also serves as a reference electrode.
As used herein, unless otherwise specifically indicated, the term "reference electrode" includes a) a reference electrode and b) a reference electrode (i.e., counter/reference electrode) that also serves as a counter electrode.
As used herein, "electrolysis" refers to the electro-oxidation or electro-reduction of a compound, either directly at an electrode or via one or more electron transfer agents.
As used herein, a component is "immobilized" within a sensor, for example, when the component is captured on or covalently, ionically, or coordinately bound to a constituent component of the sensor and/or on a polymer or sol-gel matrix or immobile membrane.
As used herein, an "electron transfer agent" is a compound that carries electrons between an analyte and a working electrode, either directly or in coordination with other electron transfer agents. An example of an electron transfer agent is a redox mediator.
As used herein, a "redox mediator" is an electron transfer agent used to carry electrons between an analyte, an enzyme that reduces the analyte, or oxidizes the analyte, and an electrode, either directly or via one or more additional electron transfer agents. Redox mediators comprising a polymeric backbone may also be referred to as "redox polymers".
As used herein, the term "precursor polymer" refers to the starting polymer prior to attachment of various modifying groups to form a modified polymer.
As used herein, a "sensing layer" is a component of a sensor that includes a constituent that facilitates electrolysis of an analyte. The sensing layer can include constituents such as an electron transfer agent (e.g., a redox mediator or redox polymer), a catalyst that catalyzes a reaction of the analyte to produce a response at the working electrode (e.g., an analyte-specific enzyme), or both an electron transfer agent and a catalyst. In some embodiments of the invention, the sensor comprises a sensing layer non-leachably disposed near or on the working electrode.
As used herein, a "sensing element" is an application or region of an analyte-specific enzyme disposed with a sensing layer. Thereby, the sensing element is able to interact with the analyte. The sensing layer may have more than one sensing element that constitutes an analyte detection region disposed on the working electrode. In some embodiments, the sensing element includes an analyte-specific enzyme and an electron transfer agent (e.g., a redox mediator). In some embodiments, the sensing element comprises an analyte-specific enzyme, an electron transfer agent, and a cross-linking agent.
As used herein, a "non-leachable" or "non-releasable" compound or a "non-leachable disposed" compound is meant to define a compound that is attached to the sensor such that it does not substantially diffuse away from the sensing layer of the working electrode during use of the sensor (e.g., during implantation of the sensor in a patient or measurement of a sample).
As used herein, a "crosslinker" is a molecule comprising at least two reactive groups capable of linking at least two molecules together or linking at least two moieties of the same molecule together. The linkage of at least two molecules is referred to as intermolecular crosslinking, while the linkage of at least two portions of the same molecule is referred to as intramolecular crosslinking. Crosslinkers having more than two reactive groups may be capable of simultaneously performing intermolecular and intramolecular crosslinking.
The "membrane solution" is a solution containing all necessary components for crosslinking and forming a membrane, and includes a modified polymer containing a heterocyclic nitrogen group, a crosslinking agent, and a buffer or an alcohol-buffer mixed solvent.
As used herein, "biological fluid" is any bodily fluid or bodily fluid derivative in which an analyte can be measured, such as blood, interstitial fluid, plasma, dermal fluid, sweat, and tear fluid.
As used herein, "accumulation mode sensing" refers to the accumulation of electrons resulting from oxidation of an analyte, which occurs at or on a sensing element that is not connected to a working electrode of an electrical circuit, thereby producing an accumulation of electrons.
Accumulation mode sensing
Referring to the method flow diagram of fig. 1, some embodiments of the invention include a method for obtaining a signal from an analyte using a sensor comprising a working electrode and another electrode (e.g., a counter and/or reference electrode), wherein the working electrode is provided with or modified by a catalyst (e.g., an analyte-specific enzyme) and an electron transfer agent (e.g., a redox mediator) (10). The analyte-specific enzyme and redox mediator modified region of the working electrode may be referred to as the sensing element or sensing layer of the working electrode. As shown in fig. 1, the analyte is provided (15) to a working electrode that has been provided with an analyte-specific enzyme (e.g., analyte-specific enzyme modification). In the presence of the analyte, the modified working electrode oxidizes the analyte and measures the amount of oxidation as the amount of charge resulting from the reaction. As long as the working electrode is not connected to another electrode, charge from the redox reaction will continue to accumulate on the working electrode (20). For low concentrations of analytes in the body (e.g., cortisol), accumulating charge (electrons) for a set period of time allows the low concentration analyte to produce a signal output that is easy to measure and quantify compared to other known methods. After charge accumulation for a set period of time (e.g., up to 120 seconds, up to 3 minutes, up to 5 minutes, up to 10 minutes, up to 15 minutes, up to 20 minutes, up to 25 minutes, or up to 30 minutes), the working electrode is connected (25) to at least one other electrode (e.g., a counter electrode and/or a reference electrode) to form an electrical circuit. Once the circuit is completed, the electrons accumulated on the working electrode are released as an electrical signal, the magnitude of which is measured (30) and correlated to the amount of analyte present at the working electrode. Thus, low concentrations (e.g., nanomolar amounts as low as 4.7 nM) of analyte can be readily detected and measured according to the method of embodiments of the present invention depicted in
Referring to fig. 2, an example of a three electrode arrangement with a working
Referring to fig. 3A and 3B, one example of an electrochemical enzyme biosensor is depicted in a conceptual overview of the accumulation mode. In this example, sensing of analyte (a) relies on the redox enzyme (AOx) being electrically "linked" to the working electrode of the sensor through the redox polymer. In conventional amperometric sensing, the potential (voltage) at which the electrodes are exposed causes the analyte to react at a constant rate, which is proportional to the analyte concentration. As shown in FIG. 3B, for the analyte oxidation reaction (A to A)+) Electrons will flow at a constant rate from the analyte (A) to the analyte-specific enzyme (AOx) to the redox polymer (e.g., Os)3+) To the working electrode, resulting in a steady state current as shown in figure 3A. If the working electrode is disconnected from the circuit, the flow of electrons from the redox polymer to the working electrode will stop, resulting in no current flowing through the circuit. However, the analyte will still undergo enzymatic oxidation, leading to reduction of the redox polymer (Os)3+To Os2+). This results from electrons (e) from the analyte-) Reduced form of redox polymers (Os) stored in redox polymers2+) Accumulate over time (as Os)2+By "cloud" of (c). When in useWhen the working electrode is reconnected to the circuit so that it is at its initial potential (voltage), the accumulated reduced form of redox polymer will be oxidized, resulting in a large current spike (spike) as shown in fig. 3A. Subsequently, when the redox system reaches steady state again, the current will decay back to the original ampere current. This two-step process forms the basis for accumulation mode sensing: one is that the working electrode of the sensor is disconnected from or not connected to the circuit for a set period of time (also referred to as an accumulation time) to enable charge from the analyte to "accumulate" in the redox polymer, and the second is that the working electrode of the sensor is connected to the circuit after the accumulation time to discharge and measure the accumulated charge as a spike.
Referring to fig. 3C and 3D, an example of cumulative mode sensing is shown with a developed glucose sensor consisting of a glucose-specific sensing reagent deposited on a screen printed carbon electrode. The glucose sensing reagent consists of glucose oxidase crosslinked with an Os-redox polymer. The reagent has proven useful in glucose biofuel cells and self-powered and potentiostat-powered continuous glucose sensors. See, e.g., Mao et al, J.Am.chem.Soc.2003,125: 4951-4957; mano et al, J.Am.chem.Soc.2003,125: 6588-; liu et al, anal. chem.2012,84: 3403-; feldman et al, Diabetes technol. ther.2003,5: 769-; hoss et al, J.Diabetes Sci.Technol.2013,7: 1210-; and Hoss et al, j. diabetes sci. technol.2014,8:89-94, all of which are incorporated herein by reference in their entirety. In some embodiments of the invention, the method of accumulation mode sensing may be used to increase the sensitivity of electrochemical measurements. For the experiments shown in fig. 3C and 3D, the glucose sensor was placed in a solution of 2 μ M glucose and 100mM Phosphate Buffered Saline (PBS), and several cumulative mode measurements were made while monitoring the sensor current. For each measurement, the sensor was first placed at a voltage of +40mV to drive steady-state glucose oxidation, then the working electrode was left electrically off for a set period of time (accumulation time) to allow charge accumulation, and then the working electrode was reconnected to measure the accumulated charge. As shown, the magnitude of the oxidation current spike increases with increasing integration time. Thus, by simply increasing the integration time (e.g., up to 30 seconds, 60 seconds, or up to 120 seconds), the sensitivity of measurements using the glucose sensor and glucose concentration is increased. In fig. 3D, the amperometric signal measured as the steady-state sensor current and the peak height and peak area of the current spike measured in fig. 3C are plotted against the accumulated time. As shown, the ampere current is independent of the integration time and remains constant. However, both the height and the area of the current spike show a linear dependence on the accumulation time, which highlights the advantage of accumulation mode sensing over traditional amperometry. That is, the sensitivity of the sensor can be adjusted by changing parameters in the measurement technique that can be easily adjusted, such as the time period for which charge is accumulated.
According to an embodiment of the invention, the accumulation mode sensing method provides a signal over a range of analyte concentrations. Fig. 4A and 4B show examples of calibration experiments using an exemplary glucose sensor to measure glucose concentrations up to 100 μ M. As shown, each test takes an accumulation time of 60 seconds. Fig. 4A shows the current versus time trace obtained from this experiment. As shown, the magnitude of both the steady state amperometric current and the accumulation mode current peak increases with increasing glucose concentration. Fig. 4B shows a graph of peak height and peak area of amperometric current and current spikes as a function of glucose concentration, wherein all three signals show a linear dependence on analyte concentration. Thus, the results show that the accumulation mode sensing, whether using peak height or peak area measurements, results in a linear calibration curve and thus it can be sensed with increased sensitivity in a manner similar to conventional amperometry. Therefore, since the peak height obtained from the accumulation mode sensing is measured in units of current, the sensitivity of the measurement method can be quantitatively compared with that of the amperometric method. For example, the sensitivity of the measurement method may be accomplished by comparing the slopes of the calibration curves (such as the slopes shown in fig. 4B). By comparison, amperometry has a sensitivity of 0.44nA/μ M, while accumulation mode sensing (with peak height measurements) has a sensitivity of 1.69nA/μ M. Thus, the accumulation mode sensing according to embodiments of the present invention increases the sensitivity of electrochemical measurements by about 4 times with an accumulation time of 60 seconds, compared to amperometry.
Furthermore, since both peak height and peak area provide the same results and sensitivity, in some embodiments of the invention, the means of measuring the resulting current signal of the working electrode comprises calculating the peak height and/or peak area.
In some embodiments of the invention, cumulative mode sensing is performed with a sensor having an outer membrane. Since electrochemical sensors often coat an outer membrane (e.g., a polymeric membrane) to provide stability to the sensing agent, bulk transport limitations, biocompatibility, and/or to prevent electrode fouling, polymer-coated sensors have been tested to ensure that cumulative mode sensing performs as expected. Referring to fig. 5, exemplary glucose sensors coated with flux limiting polymeric outer membranes were used to obtain calibration curves by amperometric and accumulation mode sensing at glucose concentrations of 0, 50, 100, 200, and 500 μ M. As shown by the data points in fig. 5, four consecutive measurements were made at each glucose concentration using different integration times of 1,2,5, and 10 minutes, respectively.
As shown in fig. 5, both amperometric (left panel) and accumulation mode measurements (middle and right panels) produced a linear response to analyte concentration. As expected, the sensitivity of the sensor is independent of the integration time using amperometry (left panel of fig. 5). However, with accumulation mode sensing (middle and right panels of fig. 5), the sensitivity of the sensor increases with increasing accumulation time. Due to the flux limiting adventitia, the sensitivity of the sensor using amperometric and accumulation modes is much less than that of the sensor without the adventitia. This is expected because the outer membrane limits diffusion of the analyte to the sensing reagent. However, as shown in fig. 5, when a polymer outer film is added to the sensor, the accumulation mode sensing performs as expected and gives another example of how to adjust the sensitivity of the sensor by changing the accumulation time. Furthermore, it should be noted that using a set period of time greater than 10 minutes for charge accumulation sensed in an accumulation mode with a continuously monitoring sensor may negatively impact the time resolution of the sensor. Thus, in some embodiments of the invention, accumulation mode sensing is implemented with a sensor having an outer membrane, wherein a set period of time for charge accumulation is up to 10 minutes.
It is further noted that while an outer membrane (such as a flux limiting outer membrane) may not be required to prevent electrode fouling when measuring low concentrations of analytes, the outer membrane may provide a biocompatible interface with the in vivo environment and/or provide stability to the underlying sensing layer including electron transfer agents and/or analyte specific enzymes. For accumulation mode sensing, where an outer membrane is employed, the set time period for accumulated charge may be increased to allow for oxidation of the total analyte concentration. In some embodiments of the invention, a method of accumulation mode sensing with a sensor having an outer membrane includes increasing a set period of time for accumulating charge to up to 1 minute, up to 2 minutes, up to 3 minutes, up to 4 minutes, up to 5 minutes, up to 6 minutes, up to 7 minutes, up to 8 minutes, up to 9 minutes, or up to 10 minutes in order to allow complete reaction of all analytes present at a working electrode. In some embodiments of the invention, a method of accumulation mode sensing with a sensor having an outer membrane includes increasing a set time period for accumulating charge from 10 minutes to 30 minutes.
Alternatively, in some embodiments of the invention, the outer membrane may be made of a material with high permeability, whereby the permeable membrane allows for stability, bulk transport limitations, and/or biocompatibility while not impairing the rate at which the analyte reaches the sensing layer of the working electrode. Non-limiting examples of high permeability membrane materials include poly (vinylpyridine) crosslinked with high molecular weight (MW ≧ 400g/mol) poly (ethylene glycol) diglycidyl ether, derivatized poly (vinylpyridine) crosslinked with high molecular weight (MW ≧ 400g/mol) poly (ethylene glycol) diglycidyl ether, poly (vinyl alcohol), poly (acrylic acid), and poly (methacrylic acid).
Referring to fig. 6A-6B, an electrochemical glucose sensor is used in an in vitro experiment to measure (e.g., sense) glucose concentrations in the range of 0 to 1000 nanomolar (nM) glucose. In this embodiment, the working electrode of the sensor comprises glucose oxidase enzyme crosslinked with an Os-based redox polymer deposited and immobilized on a screen printed carbon electrode. The experiment was performed as disclosed herein (as in example 8). Additionally, a screen printed carbon counter electrode and an Ag/AgCl reference electrode were used. Before each measurement, the working electrode was held at +40mV against (vs.) Ag/AgCl for 3 minutes, after which time point the open circuit potential of the electrode was measured for 3 minutes. The graph in fig. 6A shows the resulting potential versus time trace for the glucose concentrations shown (from 0 to 100nM glucose). Thus, as shown, higher glucose concentrations result in greater magnitude potential drift rates. In some embodiments of the invention, the drift rate is calculated as the slope of the trace of potential versus time. Fig. 6B is a calibration curve showing the drift rate (calculated as the slope from 30 to 180 seconds) versus glucose concentration. As shown in fig. 6B, the potential drift rate shows a linear dependence on the glucose concentration.
Referring to FIGS. 6C-6D, the same electrochemical glucose sensor used in the experiments of FIGS. 6A-6B was used in vitro experiments to measure glucose concentrations ranging from 0 to 750nM, including glucose concentrations below 100nM (e.g., 10nM, 25nM, and 50nM) glucose. The graph in fig. 6C shows a trace illustrating the resulting potential of glucose concentration versus time. Thus, as shown in fig. 6D, the drift rate plotted for this experiment remains linear as low as 10nM glucose. The above correlation is further illustrated in fig. 6E, which shows a calibration curve obtained by testing 8 individual glucose sensors. In addition, a control sensor that did not contain glucose oxidase (but still had Os redox polymer) was also tested in this experiment. As shown in fig. 6E and 6F, the drift rate of the control sensor, represented by open circles, showed no dependence on glucose concentration.
According to some embodiments of the invention, the methods disclosed herein may be used to reduce background signal (e.g., signal when [ analyte ] ═ 0). Referring to fig. 6G to 6H, experiments were performed using the glucose sensor used in the experiment shown in fig. 6A as the working electrode. In addition, a control sensor that did not contain glucose oxidase but still had Os redox polymer was used as a reference electrode in the open circuit potential measurement. With this configuration, the amount of measurement signal that is not from glucose oxidation can be minimized. For example, when a control sensor without glucose oxidase is used as a reference electrode, the background signal (the slope of the trace of potential versus time when the glucose concentration is zero) is approximately zero. The resulting intercept of the calibration curve shown in fig. 6H is two orders of magnitude smaller than the intercept of the calibration curve obtained using the Ag/AgCl reference electrode shown in fig. 6F. Thus, the method and system of the present invention, including the use of a glucose oxidase-free control sensor as a reference electrode during open circuit potential measurement, is an effective method for reducing signal background.
In some embodiments of the invention, the signal generated by the redox reaction of the analyte at the sensing layer of the working electrode may be adjusted or modified to enhance the signal output for any given sensor and/or analyte concentration. In some embodiments of the invention, the signal is enhanced by modifying the frequency of the recording current signal. For example, referring to FIG. 7, to maximize the peak height measured during the cumulative detected current spikes, the signal may be recorded at a faster sampling rate (e.g., 0.1Hz) and filtered at a higher frequency (e.g., 3.2Hz) than the sampling rate of 0.5Hz and the frequency of the 0.03Hz filter used in the cumulative mode sensing experiments disclosed herein and shown in FIGS. 3A-3D, 4A-4B, and 5. As shown in fig. 7, at higher frequencies of 3.2Hz, the detected peaks are sharper, resulting in greater peak heights. Thus, in some embodiments of the invention, the accumulation mode sensing method includes increasing the frequency filter to 3.2Hz to maximize the signal amplitude. Note that at frequencies above 3.2Hz, the signal to noise ratio is too large to make an accurate measurement using either amperometric or cumulative peak measurements.
In some embodiments of the invention, Carbon Nanotubes (CNTs) are added to the sensing element of the working electrode. For example, CNTs are added to a sensing reagent that includes a redox mediator and an analyte-specific enzyme and applied to a working electrode. Referring to fig. 8A, CNTs are added to the sensing reagent in the micrograph on the right, and CNTs are not added in the micrograph on the left. Accumulation mode sensing is measured with and without CNTs. As shown in fig. 8B, with the addition of CNT in the sensing element on the working electrode, the cumulative mode current spike has a larger peak height.
In some embodiments of the invention, accumulation mode sensing includes using a sensor with a 30 minute accumulation time (e.g., a set time period for accumulated charge), a 3.2Hz signal frequency filter, and adding Carbon Nanotubes (CNTs) to the sensing element on the working electrode. Fig. 9A shows the cumulative mode signal obtained for a representative glucose sensor at a cumulative time of 30 minutes at glucose concentrations of 0 to 200nM in the presence of CNTs, and the signal was filtered at 3.2 Hz. Thus, as shown in the signal calibration curve of fig. 9B, the accumulation mode sensing according to embodiments of the invention provides increased sensitivity to low concentrations of analyte compared to amperometry. As shown, using a 30 minute integration time, the integration mode sensing using peak height measurement provides a 800-fold improvement in sensitivity over the amperometric method. Cumulative mode sensing using peak area measurements is more than adequate in terms of detection limit, which yields a lower limit of detection (LOD) of 4.7 ± 1.4nM, a 25-fold improvement over amperometry. Although the linear range for accumulation mode sensing is more limited than for amperometry, it should be noted that this range can be shifted to higher concentrations by using shorter accumulation times.
Sensor for accumulation mode sensing
The sensors described herein may be in vivo sensors or in vitro sensors (i.e., discrete monitoring test strips). Such sensors may be formed on a substrate, such as a substantially planar substrate. In certain embodiments, the sensor is a wire, e.g., a portion of the working electrode wire to which one or more other electrodes are connected (e.g., on top, including wrapped around). The sensor may also comprise at least one counter electrode (or counter/reference electrode) and/or at least one reference electrode or at least one reference/counter electrode.
Fig. 12 schematically depicts an embodiment of an
The
Fig. 13 shows a cross-sectional view of an embodiment of an
Still referring to fig. 13,
A first insulating layer 505 (such as a first dielectric layer in some embodiments) may be disposed or layered on at least a portion of the first conductive layer 508, and further, a second conductive layer 511 may be disposed or layered on top of at least a portion of the first insulating layer (or dielectric layer) 505. As shown in fig. 13, the second conductive layer 511 in combination with a second
A second insulating layer 506 (e.g., a second dielectric layer in some embodiments) can be disposed or layered over at least a portion of the second conductive layer 511. In addition, a third conductive layer 513 may be disposed on at least a portion of the second insulating
In any or all embodiments, some or all of the
Referring now to fig. 14A, another embodiment of an analyte sensor according to one or more embodiments of the invention is shown and represents a variation of
Additionally, in one or more embodiments, sensing region 920 may include a reference electrode, a counter electrode, or a counter-reference electrode, such as those shown in fig. 13 and 14B. Alternative electrode configurations may be used without departing from the scope of the invention.
Referring to fig. 13, 14A and 14B, it is noted that sensors (or sensing regions) 500, 920 include a sensing function at the distal portion of their respective sensor tails. As described above, this location may allow for enhanced contact with a deeper location (e.g., subcutaneous space) beneath the wearer's skin where the wearer's interstitial fluid is more readily accessible, possibly allowing for easier access to (e.g., concentration of) the analyte of interest being measured. That is, placing the sensing region deep enough within the wearer's skin to allow accurate measurements of a particular analyte, while placing the sensing region closer to the skin surface may not be sufficient to properly determine the concentration or other characteristic of the desired analyte.
Referring to fig. 13 and 14B-14D, one or more embodiments of the invention include a working
Fig. 14C also shows sensing element 322 disposed on at least a portion of working
In some embodiments of the invention, any suitably configured sensing element 322 may be disposed on working
In some embodiments of the invention, referring to fig. 14B,
FIG. 14C depicts a close-up view of the
Analyte-specific enzymes and electron transfer agents (redox mediators)
In some embodiments of the invention, the sensors of the invention are not capable of directly measuring an analyte. That is, the electrodes on the sensor cannot directly interact with the analyte. Thus, analytes are detected by enzyme proteins that are capable of direct interaction with analyte molecules. However, since the redox active sites of some enzymes (such as glucose oxidase) are buried deep within the enzyme protein structure, they cannot directly exchange electrons with the electrode. Thus, in order to transfer electrons between the redox active site of the enzyme and the electrode, an electron transfer agent (i.e., redox mediator) is employed. Since the immobilized molecules are capable of transferring electrons, the immobilization of the electron transfer agent and the analyte-specific enzyme on the sensing layer forms a so-called "wire", and is thus "electrically wired". The analyte-specific enzyme is also referred to as a "tethered enzyme". Linked enzymes are disclosed, for example, in Greg et al (U.S. Pat. No.5,262,035), Say et al (U.S. Pat. No.6,134,461), and Hoss et al (U.S. Pat. publication No.2012/0150005), all of which are incorporated herein by reference in their entirety. In some embodiments, the analyte-specific enzyme is crosslinked with an electron transfer agent.
In some embodiments of the invention, an electron transfer agent (e.g., a redox mediator) is an electroreductive and electrooxidative ion or molecule having a redox potential (voltage) that is several hundred millivolts higher or lower than the redox potential (voltage) of a Standard Calomel Electrode (SCE). In some embodiments, the electron transfer agent is no longer reduced at greater than about-150 mV and no longer oxidized at greater than about +400mV relative to SCE. Examples of suitable redox mediators in the form of redox polymers are disclosed, for example, in Mao et al (U.S. Pat. No.6,605,200), the entire contents of which are incorporated herein by reference.
According to an embodiment of the present invention, referring to fig. 14D, an
In some embodiments of the invention, the electron transfer agent used in accumulation mode sensing comprises a redox species selected from osmium, ruthenium, iron, or cobalt coupled to a polymer selected from poly (vinylpyridine), poly (thiophene), poly (aniline), poly (pyrrole), or poly (acetylene). In some embodiments, the electron transfer agent is an osmium (Os) -containing poly (vinylpyridine) redox polymer of formula I.
In some embodiments of the invention, the electron transfer agent may be organic, organometallic, or inorganic. Examples of organic redox species are quinones and species having a quinoid structure in their oxidized state, such as nile blue and indoxyl. Some quinones and partially oxidized hydroquinones (quinhydrones) react with functional groups of proteins (e.g., thiol groups of cysteine, amine groups of lysine and arginine, and phenol groups of tyrosine), which makes these redox species unsuitable for some sensors of the invention because of the presence of interfering proteins in analyte-containing liquids. It should be noted that most substituted quinones and molecules with quinoid structures are less reactive with proteins. In some embodiments, the tetra-substituted quinone has carbon atoms at the 1,2, 3, and 4 positions.
Electron transfer agents suitable for use in accumulation mode sensing methods according to embodiments of the invention have a structure or charge that prevents or substantially reduces diffusion loss of the electron transfer agent during a period of sample analysis. In some embodiments of the invention, the electron transfer agent comprises a redox species bound to a polymer capable of being immobilized onto the sensing layer of the working electrode. The binding between the redox species and the polymer may be covalent, coordinated or ionic. Useful electron transfer agents and methods for their preparation are described in U.S. Pat. Nos. 5,264,104, 5,356,786, 5,262,035 and 5,320,725, all of which are incorporated herein by reference in their entirety. Although any organic or organometallic redox species can be bound to the polymer and used as an electron transfer agent, in some embodiments of the invention, the redox mediator is a transition metal compound or complex. In some embodiments, the transition metal compound or complex comprises an osmium, ruthenium, iron, and cobalt compound or complex. It will be appreciated that many of the redox mediator species described herein (e.g., without a polymeric component) may be used as an electron transfer agent in a carrier fluid or sensing layer of a sensor where leaching of the electron transfer agent is acceptable.
One class of non-releasable polymeric electron transfer agents comprises redox species covalently bound in a polymeric composition. An example of such a mediator is poly (vinylferrocene).
Another class of non-releasable electron transfer agents comprises ionically-bound redox species. Typically, such mediators comprise a charged polymer coupled to an oppositely charged redox species. Examples of such mediators include negatively charged polymers (such as nafion (dupont)) coupled to positively charged redox species (such as polypyridyl cations coupled to osmium, ruthenium, iron or cobalt). Another example of an ion binding mediator is a positively charged polymer (such as quaternized poly (4-vinylpyridine) or poly (1-vinylimidazole)) coupled to a negatively charged redox species (such as ferricyanide or ferrocyanide). In some embodiments of the invention, the bound redox species is a highly charged redox species bound into an oppositely charged redox polymer.
In some embodiments of the invention, suitable non-releasable electron transfer agents include redox species that are coordinately bound to a polymer. For example, a mediator formed by coordinating an osmium or
In some embodiments of the invention, the electron transfer agent is an osmium transition metal complex having one or more ligands, each ligand having a nitrogen-containing heterocycle, such as 2, 2' -bipyridine, 1, 10-phenanthroline, or a derivative thereof. Further, in some embodiments, the electron transfer agent has one or more ligands covalently incorporated into the polymer, each ligand having at least one nitrogen-containing heterocycle, such as pyridine, imidazole, or derivatives thereof. These preferred electron transfer agents rapidly exchange electrons between each other and the working electrode so that the complex can be rapidly oxidized and reduced.
In some embodiments of the invention, the electron transfer agent comprises (a) a polymer or copolymer having pyridine or imidazole functionality, and (b) an osmium cation complexed with two ligands, each ligand comprising 2, 2' -bipyridine, 1, 10-phenanthroline, or a derivative thereof, the two ligands not necessarily being the same. In some embodiments, the derivatives of 2,2 '-bipyridine used to complex with the osmium cation are 4, 4' -dimethyl-2, 2 '-bipyridine and mono-, di-, and polyalkoxy-2, 2' -bipyridines, such as with 4,4 '-dimethoxy-2, 2' -bipyridine. In some embodiments, the derivatives of 1, 10-phenanthroline used to complex with the osmium cation are 4, 7-dimethyl-1, 10-phenanthroline and mono-, di-and polyalkoxy-1, 10-phenanthrolines, such as 4, 7-dimethoxy-1, 10-phenanthroline. In some embodiments of the invention, polymers useful for complexing with osmium cations include polymers and copolymers of poly (1-vinylimidazole) (referred to as "PVI") and poly (4-vinylpyridine) (referred to as "PVP"). Suitable copolymer substituents of poly (1-vinylimidazole) include acrylonitrile, acrylamide, and substituted or quaternized N-vinylimidazoles. In some embodiments, the electron transfer agent comprises osmium complexed to a polymer or copolymer of poly (1-vinylimidazole).
According to an embodiment of the invention, the electron transfer agent has an oxidation-reduction potential (voltage) in the range of-100 mV to about +150mV relative to a Standard Calomel Electrode (SCE). More particularly, the potential (voltage) of the electron transfer agent ranges from-100 mV to +150mV, and in some embodiments, the potential (voltage) ranges from-50 mV to +50 mV. In other embodiments of the invention, the electron transfer agent has osmium, ruthenium, iron, or cobalt redox centers, and a redox potential (voltage) in the range of +50mV to-150 mV relative to SCE.
Examples of analyte-specific enzymes
In some embodiments, the analyte-specific enzyme is selected from glucose oxidase, NAD-glucose dehydrogenase, and FAD-glucose dehydrogenase for oxidizing glucose, in some embodiments, the analyte-specific enzyme is lactate oxidase or NAD-lactate dehydrogenase for oxidizing lactate.
One of ordinary skill in the art will appreciate that any Nicotinamide Adenine Dinucleotide (NAD) or flavin oxidase can be coupled or immobilized to the sensing layer of the working electrode in order to oxidize its corresponding analyte substrate.
Examples of the NAD-dependent enzymes include (-) -borneol dehydrogenase, (+) -dehydro-ketol dehydrogenase, (+) -dehydro-geraniol-2-ketol dehydrogenase, (3S,4R) -3-ketoxykinase, NAD-2-phospho dehydrogenase, NAD-2-ketoxykinase, NAD-2-pyruvate dehydrogenase, NAD-2-ketoxykinase, NAD-2-pyruvate dehydrogenase, NAD-2-pyruvate dehydrogenase, 2-ketoxykinase, NAD-2-phospho-2-ketoreductase, NAD-2-pyruvate dehydrogenase, NAD-2-dihydrofolate-pyruvate dehydrogenase, NAD-2-dihydrofolate-dehydrogenase, NAD-2-dihydrofolate-dehydrogenase, NAD-2-dehydrogenase, NADH-2-dehydrogenase, NAD-2-dihydrofolate-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NAD-2-dehydrogenase, NADH-2-dehydrogenase, NAD-dihydrofolate-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NADH-2-dihydrofolate-2-dihydrofolate-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dihydrofolate-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-dihydrofolate-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NADH-2-dihydrofolate-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dihydrofolate-2-dihydrofolate-dehydrogenase, NADH-dihydrofolate-2-dihydrofolate-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NADH-dihydrofolate-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-dihydrofolate-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-dihydrofolate-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dihydrofolate-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NAD-2-dehydrogenase, NAD-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dihydrofolate-dehydrogenase, NADH-dihydrofolate-2-dihydrofolate-2-dehydrogenase, NADH-2-dihydrofolate-2-dihydrofolate-2-dihydrofolate-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NAD-2-dehydrogenase, NADH-dehydrogenase, NAD-2-dihydrofolate-2-dehydrogenase, NAD-2-dehydrogenase, NAD-2-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NADH-dihydrofolate, NADH-dehydrogenase, NADH-dihydrofolate-2-dehydrogenase, NAD-2-dehydrogenase, NADH-dihydrofolate-dehydrogenase, NADH-2-dehydrogenase, NADH-dihydrofolate, NADH-dehydrogenase, NADH-2-dihydrofolate, NADH-2-dihydrofolate-dehydrogenase, NADH-dihydrofolate-dehydrogenase, NAD-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dihydrofolate-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-dihydrofolate, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2-dehydrogenase, NADH-2.
In some embodiments of the invention, the analyte-specific enzymes include flavin oxidases such as Flavin Adenine Dinucleotide (FAD) -dependent oxidase or Flavin Mononucleotide (FMN) -dependent oxidase FAD-dependent or FMN-dependent oxidases examples of FAD-dependent or FMN-dependent oxidases include (R) -6-hydroxycinnamic oxidase, (S) -2-hydroxy-oxidase, (S) -6-hydroxycinnamic oxidase, 2-enoate (enoate) reductase, 2-methyl-branched-enoyl-CoA reductase, 2-nitropropane dioxygenase, 2, 4-dichlorophenol 6-monooxygenase, 2, 6-dihydroxypyridine 3-monogluconate, 3-iso-nitropropane oxidase, 3-hydroxy-2-methylpyridine carboxylate dioxygenase, 3-hydroxybenzoic acid 4-monooxygenase, 3-hydroxybenzoic acid 6-monooxygenase, 3-hydroxybenzoate monooxygenase, 4-aminobenzoate dehydrogenase, 4-cresol dehydrogenase (hydroxymandelate), 4-hydroxybenzoate 1-dehydrogenase, 4-hydroxybenzoate dehydrogenase, 4-pyruvate-1-pyruvate dehydrogenase, 4-pyruvate dehydrogenase, NADH-pyruvate dehydrogenase, 2-pyruvate-dehydrogenase, 2-pyruvate-2-pyruvate-dehydrogenase, 2-pyruvate-dehydrogenase, 3-pyruvate-dehydrogenase, 3-pyruvate-dehydrogenase, 3-pyruvate-dehydrogenase, 3-pyruvate-dehydrogenase, 3-pyruvate-dehydrogenase, 3-pyruvate-dehydrogenase, 3-pyruvate-dehydrogenase, 3-pyruvate-4-pyruvate-dehydrogenase, 3-pyruvate-dehydrogenase, 3-pyruvate-reductase, 3-pyruvate.
Sensor film
In some embodiments of the invention, referring to fig. 13 and 14B-14D,
In some embodiments of the invention, the membrane is composed of two components: a hydrophilic (hydrophilic) polymer and a crosslinking agent. The cross-linking agent links the polymer molecules together and anchors them to the sensing layer of the sensor. For an analyte (such as glucose) at a concentration of about 5mM in vivo, a flux limiting membrane must be used to prevent electrode fouling. Examples of flux limiting sensor membranes are disclosed, for example, in U.S. patent No.6,932,894 to Mao et al, which is incorporated herein by reference in its entirety.
For lower concentrations of analyte, the flux limiting membrane may be used with increased accumulation times, for example, up to 30 minutes. Alternatively, for lower concentrations of analyte, a high permeability membrane may be used in order to maintain the natural flow of analyte to the sensing layer, while also having a membrane to increase the biocompatibility of the sensor. For example, the hydrophilic membrane surface does not stimulate (aggregate) the immune system of the human body, thereby reducing the risk of inflammation and other responses that may impair sensor performance.
Analyte monitoring system
Accordingly, embodiments include analyte monitoring devices and systems that include an analyte sensor for in vivo detection of an analyte in a bodily fluid, at least a portion of which may be disposed beneath a skin surface of a user. Analyte monitoring systems are disclosed in Say et al (U.S. Pat. No.6,134,461) and Hoss et al (U.S. patent application publication No.2012/0150005), both of which are incorporated herein by reference in their entirety. Embodiments of the present invention include fully implantable analyte sensors and analyte sensors in which only a portion of the sensor is placed under the skin while a portion of the sensor remains above the skin, wherein the portion of the sensor remaining above the skin is used, for example, to interface with a sensor control unit (which may include a transmitter), a receiver/display unit, a transceiver, a processor, and the like. The sensor, for example, may be placed subcutaneously in the body of the user for continuously or periodically monitoring the analyte level in the interstitial fluid of the user. For purposes of this description, continuous monitoring and periodic monitoring are used interchangeably unless otherwise noted. The sensor response may be correlated and/or converted to an analyte level in blood or other fluid. In some embodiments, an analyte sensor may be placed in contact with interstitial fluid to detect an analyte level, which may be used to infer the analyte level in the blood stream of a user. The analyte sensor may be inserted into a vein, artery, or other body part containing a fluid. In some embodiments, the analyte sensor may be configured to monitor analyte levels for a period of time, which may be a few seconds, minutes, hours, days, weeks to months, or longer.
In some embodiments of the invention, the analyte sensor is capable of detecting the analyte in vivo for 1 hour or more, for example, several hours or more, such as several days or more, such as three days or more, such as five days or more, such as seven days or more, such as weeks or more, or a month or more. Future analyte levels may be predicted based on the obtained information, such as the current analyte level at time t0, the rate of change of the analyte, and the like. The predictive alarm may notify the user of a predicted analyte level that may require attention before the user's analyte level reaches the predicted future analyte level. This provides the user with the opportunity to take corrective action.
Fig. 15 illustrates a data monitoring and management system, such as, for example, an
Analytes that can be monitored include, but are not limited to, glucose, lactate, 3-hydroxybutyrate, cortisol, alcohol, pyruvate, glutamate, theophylline, acetylcholine, amylase, bilirubin, cholesterol, chorionic gonadotropin, glycosylated hemoglobin (HbA1c), creatine kinase (e.g., CK-MB), creatine, creatinine, DNA, fructosamine, glucose derivatives, glutamine, growth hormones, 3-hydroxybutyrate, ketones, ketone bodies, peroxides, prostate specific antigen, prothrombin, RNA, thyroid stimulating hormone, and troponin. Analytes that may also be monitored also include drugs such as, for example, antibiotics (e.g., gentamicin, vancomycin, and the like), digitoxin, digoxin, drugs of abuse, theophylline, and warfarin. In some embodiments, more than one analyte is monitored, which may be monitored at the same or different times.
The
Also shown in fig. 15 is an optional
In the embodiment of the
In some embodiments, the
In certain embodiments, the
In operation, in certain embodiments, the
Referring again to fig. 15, the
The
In certain embodiments, a
In further embodiments, the
A sensor for measuring low nanomolar concentrations of an analyte as disclosed herein, such as an enzyme biosensor, can be used in an in vivo monitoring system that can be placed in a user, such as a human subject, to contact the user's bodily fluid and sense the levels of one or more analytes contained therein. The in vivo monitoring system may include one or more reader devices that receive sensed analyte data from the sensor control apparatus. These reader devices may process and/or display sensed analyte data or sensor data to a user in a variety of forms.
Referring to fig. 16, in some embodiments, the
The
Fig. 16 is a block diagram of an exemplary embodiment of a
As shown in fig. 16, the communication processor 202 may interface with the
Referring also to fig. 16, the
Memory 210 may be shared by one or more of the various functional units present within
The power source 216 may include one or more batteries, which may be rechargeable or single-use disposable batteries. The
The
The combination device may function as part of a closed loop system (e.g., an artificial pancreas system that is operable without requiring user intervention) or a semi-closed loop system (e.g., an insulin loop system that is operable with little user intervention, such as confirming a change in dosage). For example, the analyte level of diabetes may be monitored by the sensor control device 102 in a repeated automated manner, and then the sensor control device 102 may transmit the monitored analyte level to the
Fig. 17 is a block diagram illustrating one exemplary embodiment of a sensor control device 102 having an analyte sensor 104 and sensor electronics 250 (including analyte monitoring circuitry), the
The memory 253 is also included within the ASIC 251, and may be shared by various functional units present within the ASIC 251, or may be distributed between two or more of them. The memory 253 may be a separate chip. The memory 253 is persistent and can be volatile and/or nonvolatile memory. In this embodiment, the ASIC 251 is connected to a power supply 260 (which may be a button cell battery or the like). AFE 252 interfaces with in vivo analyte sensor 104 and receives measurement data therefrom and outputs the data in digital form to processor 256, which processor 256, in turn, may process in any suitable manner in some embodiments. This data is then provided to communication circuitry 258 for transmission to
Information may be transferred from the sensor control device 102 to a second device (e.g., the reader device 120) upon activation of the sensor control device 102 or the
Different types and/or forms and/or amounts of information may be transmitted as part of each communication, including, but not limited to, one or more of current sensor measurements (e.g., newly obtained analyte level information corresponding in time to the time at which the reading began), a rate of change of the metric measured over a predetermined period of time, a rate of change of the metric (acceleration of the rate of change), or historical metric information corresponding to metric information obtained prior to a given reading and stored in a memory of the sensor control device 102.
Some or all of the real-time, historical, rate of change (e.g., acceleration or deceleration) information may be sent to the
The following examples are provided for illustrative purposes only and do not limit the scope or content of the present application.
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