Apparatus and method for measuring concentration of an analyte in whole blood samples

What is claimed is: 1. A method for measuring a concentration of an analyte in a bio-sample, the method comprising: a step of introducing a liquid bio-sample into a sample cell in which an oxidation/reduction enzyme capable of catalyzing an oxidation/reduction reaction of the analyte and an electron transfer mediator are fixed and a working electrode and a counter electrode are provided; a step of obtaining a first induced current by applying a constant DC voltage to the working electrode to start the oxidation/reduction reaction of the analyte and proceed with an electron transfer reaction; a step of obtaining a second induced current by applying a Λ-step ladder-type perturbation potential after applying the constant DC voltage, wherein the step of obtaining the second induced current is subsequent to the step of obtaining the first induced current; a step of calculating a predetermined feature from two or more characteristic points from the first induced current or the second induced current; and a step of calculating a concentration of the analyte using a calibration equation formed of at least one feature function so as to minimize an effect of at least one hindering material in the bio-sample, wherein the at least one feature function comprises a function using the first induced current obtained from the constant DC voltage and a function using the second induced current obtained from the Λ-step ladder-type perturbation potential, wherein the Λ-step ladder-type perturbation potential is characterized by a height (V step ) of each step, an application time (t step ) for each step, a difference (V center ) between a middle voltage and the constant DC voltage in an entire range of variations, a difference (V peak ) between a middle voltage and a peak voltage, and a time difference (t cycle ) between a peak voltage of an entire step ladder-type wave and a peak voltage of an adjacent next step ladder-type wave, wherein the constant DC voltage and the Λ-step ladder-type perturbation potential are applied to the working electrode through a same digital-to-analog converter circuit linked with a microcontroller, and wherein a characteristic point, having different linearity with respect to the analyte and the hindering material, is selected from the first or second induced current, wherein a feature is formed of the characteristic point, and wherein a calibration equation is formed of the feature. 2. The method for measuring a concentration of an analyte in a bio-sample of claim 1 , wherein the second induced current is obtained within 0.1 to 1 second after the first induced current is obtained. 3. The method for measuring a concentration of an analyte in a bio-sample of claim 1 , wherein the feature is formed of the characteristic point by using one of second induced currents near peak and valley voltages of a specific step ladder type, curvature of a curved line formed of induced currents of each step of the Λ-step ladder-type perturbation potential, a difference between a current value of a peak and a current value of a valley of the Λ-step ladder-type perturbation potential, induced currents in the middle of ups and downs of the Λ-step ladder-type perturbation potential, induced currents at a starting point and an ending point of each step ladder-type perturbation potential cycle, and an average value of induced currents obtained from the Λ-step ladder-type perturbation potential, and values which can be obtained by expressing the current values obtained therefrom by four fundamental arithmetic operations and mathematical functions including an exponential function, a logarithmic function, and a trigonometric function are used. 4. The method for measuring a concentration of an analyte in a bio-sample of claim 1 , wherein the calibration equation formed of at least one feature function is obtained by applying multivariable regression analysis to the at least one feature function as a linear mixture of the at least one feature function, and the calibration equation varies depending on a material of the working and counter electrodes, an arrangement of the working and counter electrodes, a shape of a flow path, and a characteristic of a reagent to be used. 5. The method for measuring a concentration of an analyte in a bio-sample of claim 4 , wherein the analyte is one of glucose, β-hydroxybutyric acid, cholesterol, triglyceride, lactate, pyruvate, alcohol, bilirubin, uric acid, phenylketonuria, creatine, creatinine, glucose-6-phosphate dehydrogenase, NAD(P)H, and a ketone body. 6. The method for measuring a concentration of an analyte in a bio-sample of claim 4 , wherein the oxidation/reduction enzyme is one of a glucose oxidase (GOx), a glucose dehydrogenase (GDH), a glutamate oxidase, a glutamate dehydrogenase, a cholesterol oxidase, a cholesterol esterase, a lactate oxidase, an ascorbic acid oxidase, an alcohol oxidase, an alcohol dehydrogenase, a bilirubin oxidase, and a ketone body dehydrogenase. 7. The method for measuring a concentration of an analyte in a bio-sample of claim 1 , wherein the electron transfer mediator which can be used together with the oxidation/reduction enzyme is one of ferrocene, ruthenium hexamine(III) chloride, potassium ferricyanide, 1,10-phenanthroline-5,6-dione, and bipyridine, or an osmium complex including phenanthroline as a ligand, 2,6-dimethyl-1,4-benzoquinone, 2,5-dichloro-1,4-benzoquinone, 3,7-diamino-5-phenothiaziniumthionine, 1-methoxy-5-methylphenazinium methylsulfate, methylene blue, and toluidine blue. 8. The method for measuring a concentration of an analyte in a bio-sample of claim 1 , wherein the constant DC voltage having a voltage range of 0 to 800 mV is consecutively or intermittently applied for 1 second or more to less than 1 minute, and the first induced current is measured one time or several times while the constant DC voltage is applied. 9. The method for measuring a concentration of an analyte in a bio-sample of claim 1 , wherein a height (V step ) of a step of the Λ-step ladder-type potential is 0.5 to 20 mV, a duration time (t step ) of the step is 0.001 to 0.1 second, a difference (V center ) between a middle voltage and a constant voltage of the step A step ladder-type potential is −150 to 150 mV, a difference (V peak ) between the middle voltage and a peak or valley voltage of the Λ-step ladder-type potential is 5 to 150 mV, and a cycle of the Λ-step ladder-type potential or a time difference (t cycle ) between a peak and an adjacent next peak is in a range of 0.01 to 1 second. 10. The method for measuring a concentration of an analyte in a bio-sample of claim 1 , wherein: the at least one feature function further comprises a function using a temperature value measured by a measuring apparatus, and a function which can be obtained by expressing measured current values by four fundamental arithmetic operations and mathematical functions including an exponential function, a logarithmic function, and a trigonometric function. 11. The method for measuring a concentration of an analyte in a bio-sample of claim 1 , wherein the calibration equation formed of at least one feature function is one of glucose=E j □ c j f j (i), glucose=E j □ c j f j (i,T), and ketone body=E j □ c j f j (i), wherein i denotes one or more current values which can be obtained from the first induced current and the second induced current, c denotes a constant, j denotes a number, and T denotes temperature values that are independently measured.