用于检测DNA-RNA杂交体的酶免疫测定中比色、荧光和酶促扩增底物系统的比较。
Comparison of colorimetric, fluorescent, and enzymatic amplification substrate systems in an enzyme immunoassay for detection of DNA-RNA hybrids.
作者信息
Coutlee F, Viscidi R P, Yolken R H
机构信息
Department of Pediatrics, Johns Hopkins University School of Medicine, Baltimore, Maryland 21205.
出版信息
J Clin Microbiol. 1989 May;27(5):1002-7. doi: 10.1128/jcm.27.5.1002-1007.1989.
Abstract
The monoclonal antibody solution hybridization assay is a novel enzyme immunoassay for detection of RNA with a biotinylated DNA probe. To increase the sensitivity of this test, a fluorescent substrate and an enzymatic amplification cycling system were compared with a conventional colorigenic substrate for alkaline phosphatase. The fluorescent, cycling, and colorigenic substrates detected, respectively, 10, 10, and 100 amol of unbound alkaline phosphatase in 2 h. With a prolonged incubation period of 16.6 h, the conventional substrate measured 10 amol of the enzyme. In the immunoassay for RNA detection, the fluorescence and cycling assays were faster than that using the colorigenic substrate and reached an endpoint sensitivity of 3.2 pg/ml (0.16 pg per assay) of cRNA. However, longer incubation periods (16.6 h) for optimal generation of the colorigenic product led to a comparable level of sensitivity for the conventional substrate.
摘要
单克隆抗体溶液杂交测定法是一种用生物素化DNA探针检测RNA的新型酶免疫测定法。为提高该检测方法的灵敏度,将荧光底物和酶促扩增循环系统与碱性磷酸酶的传统显色底物进行了比较。荧光底物、循环底物和显色底物在2小时内分别检测到10、10和100 amol未结合的碱性磷酸酶。在延长至16.6小时的孵育期后,传统底物检测到10 amol的酶。在RNA检测的免疫测定中,荧光测定法和循环测定法比使用显色底物的方法更快,并且达到了对cRNA的终点灵敏度为3.2 pg/ml(每次测定0.16 pg)。然而,为了使显色产物达到最佳生成效果而延长孵育期(16.6小时)会使传统底物的灵敏度达到相当的水平。
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