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Last Updated: April 18, 2024

Claims for Patent: 4,774,174

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Summary for Patent: 4,774,174

Title:	Solid phase system for ligand assay
Abstract:	A method for conducting a ligand assay in an inert porous medium wherein a binding material is immunologically immobilized within the medium, which includes the steps of immunologically immobilizing a binding material within a finite zone of the medium, applying an analyte to the zone containing the immobilized binding material, applying a labeled indicator to the zone which becomes immobilized within the zone in an amount which can be correlated to the amount of analyte in the zone, applying a solvent to substantially the center of the zone to chromatographically separate the unbound labeled indicator from the zone, and measuring the amount of labeled indicator remaining in the zone.
Inventor(s):	Giegel; Joseph L. (Miami, FL), Brotherton; Mary M. (Miami, FL)
Assignee:	Baxter Travenol Laboratories, Inc. (Deerfield, IL)
Application Number:	06/719,656
Patent Claims:	1. A competitive method for conducting a solid phase enzyme immunoassay of a fluid sample within the interstices of a solid, inert proous medium, said fluid sample containing an unknown level of analyte, the method comprising: a. providing a binding material which has been immobilized within a finite zone of the interstices of the solid, inert porous medium, said binding material being capable of immunological reaction with said analyte from among the constitutents of the fluid sample; b. applying, under binding conditions, to substantially the center of said finite zone, containing said immobilized binding material, a fluid sample containing the analyte for which said binding material is specific, said analyte being applied as a solution so as to permit diffusion thereof within the interstices of a reaction zone of the porous medium; c. applying an enzyme-labeled indicator to substantially the center of said reaction zone, under conditions which allow said indicator and said analyte to compete for binding sites on said immobilized binding material, said indicator, which comprises an enzyme conjugated to a ligand, being immunochemically bound to said immobilized binding material in an amount which can be correlated to the amount of analyte in said reaction zone; d. applying an eluting solvent to substantially the center of said reaction zone, the quantity of eluting solvent being sufficient to effect radial chromatographic separation, within said porous medium, of unbound enzyme-labeled indicator from bound enzyme-labeled indicator within said reaction zone; e. contacting said bound enzyme-labeled indicator within said reaction zone, with a substrate for the enzyme portion of said indicator; and f. observing the extent to which the bound enzyme-labeled indicator is present within a delimited area of said reaction zone by measurement of the level of chromophore or fluorophore produced by the action of the bound enzyme-labeled indicator on said substrate, said delimited area of said reaction zone being essentially free of unbound indicator. 2. The enzyme immunoassay of claim 1, wherein the fluid sample and enzyme-labeled indicator are applied to the porous medium at the same time. 3. The enzyme immunoassay of claim 1, wherein the analyte is immunoglobulin G, the binding material is an anti-human immunoglobulin G and the enzyme-labeled indicator comprises an enzyme conjugated to anti-human immunoglobulin G. 4. The enzyme immunoassay of claim 1, wherein the enzyme-labeled indicator is anti-human immunoglobin G and the label is an enzyme selected from the group consisting of E. coli alkaline phosphatase, beta galactosidase and horse radish peroxidase. 5. The enzyme immunoassay of claim 1, wherein the analyte is hepatitis surface antigen (HB.sub.s Ag), the binding material is anti-HB.sub.s Ag, and the enzymelabeled indicator is enzyme-labeled anti-HB.sub.s Ag. 6. The enzyme immunoassay of claim 1, wherein the assay is a competitive enzyme immunoassay for digoxin in a biological fluid; the binding material is digoxin antibody; the labeled indicator is digoxin labeled with alkaline phosphatase enzyme; and the eluting solvent is a buffered medium in which labeled indicator can dissolve. 7. In an analytical method for conducting a solid phase enzyme immunoassay of a fluid sample by immunological differentiation of complex molecules in such fluid by contacting such fluid, containing an unknown level of analyte, and an enzyme-labeled indicator with an immobilized binding material within a reaction zone of a porous medium under conditions favoring immunochemical interaction of said binding material with the analyte and the enzyme-labeled indicator, whereby the analyte of interest of said fluid and the enzyme-labeled indicator compete for available sites on said binding material, said enzyme-labeled indicator comprising an enzyme conjugated to a ligand, applying a wash fluid to said porous medium to remove unreacted enzyme-labeled indicator from said medium, and measuring the amount of enzyme-labeled indicator immunochemically bound to the binding material within the porous medium, the improvement comprising: a. applying, to substantially the center of a reaction zone, within an inert porous medium, a stream of eluting solvent, the quantity of said eluting solvent applied to said reaction being sufficient to effect radial separation, within said inert porous medium, of unbound enzyme-labeled indicator from bound enzyme-labeled indicator within said reaction zone; and b. contacting said bound enzyme-labeled indicator, within said reaction zone, with a substrate for the enzyme portion of said indicator; and c. observing the extent to which the bound enzyme-labeled indicator is present within a delimited area of said reaction zone by measurement of the level of chromophore or fluorophore produced by the action of the bound enzyme-labeled indicator on said substrate, said delimited area of said reaction zone being essentially free of unbound indicator. 8. A sandwich method for conducting an enzyme immunoassay of a fluid sample within the interstices of a solid, inert porous medium, said fluid sample containing an unknown level of analyte, the method comprising: a. providing a binding material which has been immobilized within a finite zone of a solid, inert porous medium, said binding material being capable of immunological reaction with said analyte from among the constituents of the fluid sample; b. applying, under binding conditions, to substantially the center of said finite zone containing said immobilized binding materials, a fluid sample containing the analyte for which the said binding material is specific, said analyte being applied as a solution so as to permit diffusion thereof within a reaction zone of the solid, porous medium containing the immobilized binding material, whereby substantially all of said analyte is bound to the binding material; c. applying an enzyme-labeled indicator to substantially the center of said reaction zone, under conditions which allow said labeled indicator to become immunochemically bound to said analyte in a manner which can be correlated to the amount of analyte in the reaction zone, said indicator comprising an enzyme conjugated to a ligand; d. applying, to substantially the center of said reaction zone, a stream of eluting solvent, the quantity of eluting solvent being sufficient to effect radial separation, within said porous medium, of unbound enzyme-labeled indicator from the indicator which is bound within said reaction zone; and e. contacting said bound enzyme-labeled indicator, within said reaction zone, with a substrate for the enzyme of said indicator; and f. observing the extent to which the bound enzyme-labeled indicator is present within a delimited area of said reaction zone by measurement of the level of chromophore or fluorophore produced by the action of the bound enzyme-labeled indicator on said substrate, said delimited area of said reaction zone being essentially free of unbound indicator. 9. In an analytical method for a solid phase enzyme immunoassay of a fluid sample by immunological differentiation of complex molecules in such fluid by contacting such fluid, containing an unknown level of analyte, with an immobilized binding material within a reaction zone of a porous medium under conditions favoring immunochemical interaction of said binding material with the analyte, whereby the analyte of interest of said fluid is immunochemically bound to the binding material, contacting the analyte with an enzyme-labeled indicator under conditions favoring immunochemical interaction of said indicator with the analyte, said indicator comprising an enzyme conjugated to a ligand, applying a wash fluid to said porous medium to remove unreacted enzyme-labeled indicator from said medium and measuring the amount of enzyme-labeled indicator which is immunochemically bound to the analyte, the improvement comprising: a. applying, to substantially the center of a reaction zone within an inert, porous medium, a stream of eluting solvent, the quantity of solvent applied to said reaction zone being sufficient to effect radial separation within said porous medium, of unbound enzyme-labeled indicator from bound enzyme-labeled indicator within said reaction zone; and b. contacting said bound enzyme-labeled indicator, within said reaction zone, with a substrate for the enzyme of said indicator; and c. observing the extent to which the bound enzyme-labeled indicator is present within a delimited area of said reaction zone by measurement of the level of chromophore or fluorophore produced by the action of the bound enzyme-labeled indicator on said substrate, said delimited area of said reaction zone being essentially free of unbound labeled indicator. 10. The method of claim 9, wherein the fluid sample and enzyme-labeled indicator are combined in advance of contact with the immobilized binding material. 11. The method of claim 9, wherein the fluid sample is contacted with the immobilized binding material in advance of contact of the enzyme-labeled indicator with the fluid sample.

Details for Patent 4,774,174

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Applicant	Tradename	Biologic Ingredient	Dosage Form	BLA	Approval Date	Patent No.	Expiredate
Csl Behring Ag	CARIMUNE, CARIMUNE NF, PANGLOBULIN, SANDOGLOBULIN	immune globulin intravenous (human)	For Injection	102367	07/27/2000	⤷ Try a Trial	2001-01-23
Csl Behring Ag	PRIVIGEN	immune globulin intravenous (human), 10% liquid	Injection	125201	07/26/2007	⤷ Try a Trial	2001-01-23
Csl Behring Ag	PRIVIGEN	immune globulin intravenous (human), 10% liquid	Injection	125201	10/02/2009	⤷ Try a Trial	2001-01-23
Csl Behring Ag	PRIVIGEN	immune globulin intravenous (human), 10% liquid	Injection	125201	02/07/2013	⤷ Try a Trial	2001-01-23
Bio Products Laboratory	GAMMAPLEX	immune globulin intravenous (human)	Injection	125329	09/17/2009	⤷ Try a Trial	2001-01-23
Bio Products Laboratory	GAMMAPLEX	immune globulin intravenous (human)	Injection	125329	02/06/2017	⤷ Try a Trial	2001-01-23
Csl Behring Ag	HIZENTRA	immune globulin subcutaneous (human), 20% liquid	Injection	125350	03/04/2010	⤷ Try a Trial	2001-01-23
>Applicant	>Tradename	>Biologic Ingredient	>Dosage Form	>BLA	>Approval Date	>Patent No.	>Expiredate

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