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Last Updated: April 25, 2024

Claims for Patent: 5,310,647


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Summary for Patent: 5,310,647
Title: Detection and measurement of destructive and polymer forming enzymes by colloidal flocculation
Abstract:The change between a dispersed state and a flocculated state of a colloidal agent (e.g. Congo Rubin, colloidal gold) is used to provide sensitive visual detection and optionally assay of enzyme in a sample. The test cell includes a substrate for the enzyme, and, depending on the action of the enzyme, polymer which protects the colloid from electrolyte-induced flocculation is either formed or destroyed by the test reaction. In a test for a hydrolytic enzyme (e.g. a protease) the colloid loses protection and flocculates. In a test for a polymer-forming enzyme, the colloid gains protection and is prevented from flocculating by added electrolyte, or alternatively, depending on the polymer\'s behavior, becomes more sensitive to the flocculating action of the added electrolyte. The measurement may be quantitated using an instrumental monitor. The test uses a natural substrate for the enzyme to be assayed (e.g., gelatin for the gelatinase class of enzymes) and may achieve rapid speed. The test may be performed using a biologically-derived sample for diagnostically relevant purposes, e.g. to detect an enzyme indicative of periodontal disease. A kit for performing the test is also disclosed.
Inventor(s): Kerschensteiner; Daniel A. (Chester County, PA)
Assignee: Cherrystone Corporation (Wayne, PA)
Application Number:07/861,654
Patent Claims:1. A method for detecting gelatinase in a sample comprising:

preparing a sol by adding a colloidal protector selected from the gorup consisting of IgM, IgA, IgG, gelatin, casein, elastin, collagen, fibrin and bovine serum albumin (BSA), to colloidal gold to form a protected sol and by further adding a sensitizing amount of sodium chloride to said protected sol where said sensitizing amount is more than the amount required to flocculate said colloidal gold in the absence of the protection provided by said colloidal protector but is less than the amount required to flocculate said colloidal gold in the presence of said colloidal protector; and

exposing said sol to said sample to flocculate said colloidal gold from a dispersed state to a visually observable flocculated state when gelatinase is present in the sample to thereby visually detect said gelatinase in said sample.

2. The method of claim 1 wherein said exposing step comprises hydrolytically cleaving molecules of said colloidal protector by said gelatinase to expose said colloidal gold to said sensitizing amount of sodium chloride.

3. The method of claim 1 wherein the ratio of said colloidal protector to said colloidal gold is varied to change detection limits for the presence of said gelatinase.

4. The method of claim 1 wherein said colloidal protector is specific to said gelatinase.

5. A method of detecting gelatinase in a sample comprising:

adding gelatin to colloidal gold to form a protected sol;

adding a sensitizing amount of sodium chloride to said protected sol where said sensitizing amount is more than the amount required to flocculate said colloidal gold in the absence of the protection provided by said gelatin but is less than the amount required to flocculate said colloidal gold in the presence of said gelatin; and

contacting said protected sol with said gelatinase to hydrolytically cleave molecules of said gelatin to unprotect said protected sol whereby said colloidal gold in said unprotected sol is flocculated from a dispersed state to a visually observable flocculated state.

6. The method of claim 5 wherein said gelatinase is a destructive enzyme responsible for an active periodontal disease obtained from a saliva, gingival crevicular fluid or a subgingival plaque specimen.

7. A method of detecting collagenase responsible for an active periodontal disease obtained from a saliva, gingival crevicular fluid or a subgingival plaque specimen comprising:

adding a colloidal protector selected from the group consisting of gelatin and collagen to colloidal gold to form a protected sol;

adding a sensitizing amount of sodium chloride to said protected sol where said sensitizing amount is more than the amount required to flocculate said colloidal gold in the absence of the protection provided by said colloidal protector but is less than the amount required to flocculate said colloidal gold in the presence of said colloidal protector; and

contacting said protected sol with said collagenase to hydrolytically cleave molecules of said colloidal protector to unprotect said protected sol whereby said colloidal gold in said unprotected sol is flocculated from a dispersed state to a visually observable flocculated state.

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