Enzyme-labeled immunoassay and device therefor

6221625
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Inventors

Ashihara, Yoshihiro
Isomura, Mitsuo
Sato, Atsuka

Application #

017214

Filed

Feb-2-1998

Published

Apr-24-2001

Current US Class

422/56
422/57
422/58
435/287.1
435/287.2
435/7.71
435/7.9
435/7.91
435/7.92
435/970
436/514
436/518
436/536
436/537
436/538
436/810

International Classes

G01N 033/53

Field of Search

435/7.9 435/7.71 435/7.91 435/7.92 435/287.1 435/287.2 435/970 436/536 436/537 436/538 436/518 436/514 436/810 422/56 422/57 422/58

Assignee

Fujirebio Inc. (Tokyo, JP)

Examiners

Chin; Christopher L.

Attorney, Agent or Firm

Oblon, Spivak, McClelland, Maier & Neustadt, P.C.

US Patent References

4585792   Protective additive t...
4835099   Signal enhanceme...
5296347   Bridge immunoassay

Referenced by:

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Citation

Cite This Patent

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Abstract
An enzyme-labeled immunoassay is performed by the steps of allowing a test sample to react with an enzyme-labeled reagent, allowing a substrate to react with the enzyme to form a signal, and immobilising the enzyme-labeled reagent, with the prevention of a further signal formation from a predetermined time on after the immobilisation of the enzyme-labeled reagent, using an enzyme inhibitor. A device for performing this enzyme-labeled immunoassay includes an absorbent material capable of transporting a developing solution by capillary action, the absorbent material including (a) a developing liquid application zone, (b) an enzyme-labeled reagent zone containing an enzyme-labeled reagent, (c) a sample receiving zone, and (d) an indicator reagent zone capable of immobilising the enzyme-labeled reagent after the reaction of the test sample with the enzyme-labeled reagent in an amount dependent on the assay result, with an enzyme inhibitor being applied to a portion in the absorbent material upstream of the enzyme-labeled reagent zone, which enzyme inhibitor prevents the formation of a signal from a predetermined time on after the enzyme-labeled reagent is immobilised at the indicator reagent zone.
 
Claims
What is claimed is:

1. An enzyme-labeled immunoassay comprising the steps of:

providing an absorbent material capable of transporting a developing solution by capillary action,

applying a test sample containing an analyte to the absorbent material,

allowing the analyte to react with an enzyme-labeled reagent, the reaction being allowed in the absorbent material,

immobilizing the reacted enzyme-labeled reagent,

allowing a substrate to react with the immobilized enzyme to form a signal, wherein, by the formation of the signal or no formation of the signal, a presence or absence of the analyte is detected,

preventing a further signal formation from a predetermined time on after the immobilization of the enzyme-labeled reagent, using an enzyme inhibitor transported in the absorbent material, and



Description
BACKGROUND OF THE INVENTION

1. Field of the Invention

The present invention relates to an enzyme-labeled immunoassay comprising the steps of allowing a test sample to react with an enzyme-labeled reagent, allowing a substrate to react with the enzyme to form a signal, and immobilising the enzyme-labeled reagent, with the prevention of a further signal formation from a pre- determined time on after the immobilisation of the enzyme-labeled reagent, using an enzyme inhibitor. The present invention also relates to a device for performing this enzyme-labeled immunoassay.

2. Discussion of Background

Recently immunoassays using an enzyme as a labeling material and a device comprising an absorbent material capable of transporting an enzyme-labeled reagent by capillary action, using a developing solution, are known as convenient and simple assays for the detection of analyte substances in biological fluids, and medicinal substances in test samples, utilizing immunoreactions (refer to, for example, Japanese Laid-Open Patent Application 61-145459, European Patent 186,799, Japanese Laid-Open Patent Application 63-501595, U.S. Patent 5,604,110 and European Patent 225,054). When using a test strip comprising such a device, for example, a test sample containing an analyte is allowed to react with an enzyme-labeled reagent, a substrate is then allowed to react with the enzyme to form a signal, and immobilising the enzyme-labeled reagent reacted with the test sample, using an immunoreactive substance in an indicator reagent zone, and in a predetermined period of time after the reaction of the test sample and the enzyme-labeled reagent, the degree of the formation of the signal, such as the coloring degree of the indicator reagent zone, is measured or evaluated, whereby the amount of the analyte contained in the test sample is assayed.
 
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