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Preservation of B-cell-associated surface antigens by chemical fixation.

作者信息

Caldwell C W

机构信息

Department of Pathology, Ellis Fischel Cancer Center, University of Missouri School of Medicine, Columbia 65203.

出版信息

Cytometry. 1994 Jul 1;16(3):243-9. doi: 10.1002/cyto.990160308.

Abstract

Usual methods of chemical fixation preclude examination of cells with most monoclonal antibodies due to alteration or destruction of the surface antigen itself. A method of chemical stabilization and preservation of human B-cell-associated surface antigens is described which facilitates retrospective flow cytometric analysis. This method involves pretreatment of the cells with protease enzyme inhibitors, followed by chemical cross-linking of surface proteins with 2% formalin, and finally blockade of non-specific reactive groups with excess glycine. Once prepared, the expression of pertinent cellular antigens is stable on the cell surface for as long as 4 years. Such methodology could conceivably be used for preparation of cells for longitudinal quality control of monoclonal antibodies or archival storage of patient specimens for retrospective flow cytometric analysis.

摘要

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