ENZYME-IMMUNOASSAY FOR INTACT HUMAN INSULIN IN SERUM OR PLASMA

被引：0

作者：

ANDERSEN, L ^{[1
]}

DINESEN, B ^{[1
]}

JORGENSEN, PN ^{[1
]}

POULSEN, F ^{[1
]}

RODER, ME ^{[1
]}

机构：

[1] STENO DIABET CTR,DK-2820 GENTOFTE,DENMARK

来源：

CLINICAL CHEMISTRY | 1993年 / 39卷 / 04期

关键词：

MONOCLONAL ANTIBODIES; TYPE-II DIABETES; ENZYME IMMUNOASSAY VS RADIOIMMUNOASSAY;

D O I：

暂无

中图分类号：

R446 [实验室诊断]; R-33 [实验医学、医学实验];

学科分类号：

1001 ;

摘要：

We describe an enzyme-linked two-site immunoassay for quantitation of intact insulin in human serum and plasma. The method uses two murine monoclonal antibodies that bind to two different epitopes on the insulin molecule. The immunoassay is specific. Human proinsulin is not bound by the antibodies, and the binding of partially processed proinsulin intermediates is believed to be of minor clinical importance. The relative response of human, bovine, and porcine insulin is 1, 1, and 3, respectively. The assay is sensitive (detection limit 5 pmol/L), accurate (101% recovery with 50 pmol/L insulin added to samples, 95% with 100 pmol/L, and 89% with 300 pmol/L), and fast (results within 3 h), and has a high analytical capacity (done in microtiter plates). The working assay range selected is 5-600 pmol/L, corresponding to a clinically useful range. Because of its specificity, this two-site immunoassay gives results that are lower than those obtained by using a competitive radioimmunoassay, both in normal individuals and in non-insulin-dependent diabetics.

引用

页码：578 / 582

页数：5

共 28 条

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