Qualitative immunochromatographic method and device

5232835
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Inventors

Litman, David J.
Li, Thomas M.
Buelteman, Laura L.
Wong, Emmy T.

Application #

726446

Filed

Jul-8-1991

Published

Aug-3-1993

Current US Class

422/56
422/58
435/7.91
435/7.93
435/970
435/973
435/975
436/501
436/514
436/518
436/805
436/810
436/816

International Classes

G01N 033/543; G01N 033/558

Field of Search

435/7.91 435/7.93 435/970 435/973 435/975 436/501 436/514 436/518 436/805 436/810 436/816 422/56 422/58

Assignee

Syntex (U.S.A.) Inc. (Palo Alto, CA)

Examiners

Saunders; David

Attorney, Agent or Firm

Leitereg; Theodore J.

US Patent References

3992631   Fluorometric syste...
4163779   Test for quantitation...
4207307   Simultaneous imm...
4308028   Device and method...
4540659   Simultaneous calib...
4786594   Enzyme immunoas...
4837395   Single step heterog...
4999285   Chromatographic c...

Referenced by:

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Citation

Cite This Patent

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Abstract
A method for determining the presence of a predetermined minimum detectible amount of one or more analytes in a sample suspected of containing the analyte is disclosed. Each analyte is a member of a specific binding pair ("sbp member") consisting of ligand and its complementary receptor. The method comprises contacting with a test solution containing said sample and predetermined amounts of two or more of a plurality of first sbp members, each respectively analogous to one of said analytes, a contact portion of a piece of bibulous material capable of being traversed in at least one direction by the test solution by capillary migration. The bibulous material contains predetermined amounts of two or more of a plurality of second sbp members, each respectively capable of binding one of the analytes and corresponding first sbp member. The second sbp members are non-diffusively bound to the bibulous material at least between the contact portion and a predetermined site on the piece of bibulous material separated from the contact portion such that in the presence of a predetermined amount of one or more analytes the analogous first sbp member migrates at least to the predetermined site on the piece of bibulous material. Next, at least a portion of the test solution is allowed to traverse the bibulous material by means of capillary migration. The predetermined site is examined for the presence of one or more of the first sbp members, which is usually indicated by the presence of a detectible signal.
 
Claims
What is claimed is:

1. A device for determining the presence at or above a predetermined minimum amount of one or more of a plurality of analytes in a test solution containing predetermined amounts of two or more first sbp members, each respectively analogous to one of said analytes, each analyte being a member of a specific binding pair, said device comprising--

a piece of bibulous material capable of traversal by said test solution in at least one direction by capillary migration, said bibulous material having a contact portion for contacting said test solution and

predetermined amounts of two or more second sbp members, each respectively complementary to one of said analytes, substantially uniformly and non-diffusively bound to said bibulous material, said predetermined amounts of said second sbp members being such that in the presence of at least one of said analytes a first sbp member migrates to a predetermined site on said bibulous material separated from said contact portion, and



Description
BACKGROUND OF THE INVENTION

1. Field of the Invention

The ability to employ naturally occurring receptors or antibodies directed to specific compounds in assaying for the presence of a compound of interest has created a burgeoning immunoassay business. In each of the assays, a homologous pair of specific binding pair ("sbp") members, usually an immunological pair, involving a ligand and a receptor (antiligand) is involved, wherein one of the sbp members is labeled with a label which provides a detectible signal. The immunoassay methodology results in a distribution of the signal label between signal label bound in a complex of the sbp members and unbound signal label. The differentiation between bound and unbound signal label can be as a result of physical separation of bound from unbound signal label or modulation of the detectible signal between bound and unbound signal label.

For the most part, immunoassays have been directed to quantitative determination of a wide variety of compounds of interest in clinical laboratories requiring relatively sophisticated equipment and careful technique. Immunoassays have found less extensive commercial application where sem-quantitative or qualitative results would be acceptable and the determination would involve non-laboratory personnel, such as in a home or a medical practitioner's office. Even in the clinical laboratory, simple and rapid screening tests employing inexperienced personnel could serve to provide substantial economies.
 
  A method for determining the presence of a predetermined minimum detectible amount of one or more analytes in a sample suspected of containing the analyte...  A method and apparatus for the quantitative determination of an analyte in a liquid employs a liquid-permeable solid medium defining a liquid flow path....