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用于灵敏检测临床人类免疫缺陷病毒分离株的聚腺苷酸连接的非同位素微量滴定板逆转录酶测定法。

Poly A-linked non-isotopic microtiter plate reverse transcriptase assay for sensitive detection of clinical human immunodeficiency virus isolates.

作者信息

Suzuki K, Saito T, Kondo M, Osanai M, Watanabe S, Kano T, Kano K, Imai M

机构信息

Biomedical Research Center, Olympus Optical Co. Ltd., Tokyo, Japan.

出版信息

J Virol Methods. 1995 Nov;55(3):347-56. doi: 10.1016/0166-0934(95)00073-5.

Abstract

A colorimetric reverse transcriptase assay (cRT assay) was developed for quantitative detection of HIV-1. In this format, reverse transcriptase incorporates biotin-labeled dUTP onto oligo-dT primers hybridized to poly A templates. The templates are covalently bound to the surface of microtiter wells. The amount of incorporated biotin-labeled dUTP is measured by binding horseradish peroxidase conjugated streptavidin, washing away unbound peroxidase, adding colorimetric substrate and then reading with a standard colorimetric reader. The sensitivity of the assay is very good. As little as 3 x 10(5) molecules of recombinant HIV-RT can be detected after 20 h of reaction time. Direct comparison using 3 cultured clinical isolates indicates that this level of detection is equivalent to the commercially available p24 antigen capture assay and the HIV-RNA assay based on branched DNA signal amplification. Other retroviruses, such as HIV-2 and feline immunodeficiency virus (FIV), can also be detected in this format. This non-isotopic assay is easy to perform and could provide a convenient and quantitative method for HIV study by monitoring reverse transcriptase, an essential activity in the infection process.

摘要

开发了一种用于定量检测HIV-1的比色逆转录酶测定法(cRT测定法)。在这种方法中,逆转录酶将生物素标记的dUTP掺入与聚A模板杂交的寡聚dT引物上。模板共价结合到微量滴定孔的表面。通过结合辣根过氧化物酶偶联的链霉亲和素、洗去未结合的过氧化物酶、加入比色底物,然后用标准比色读数仪读取,来测量掺入的生物素标记的dUTP的量。该测定法的灵敏度非常好。反应20小时后,低至3×10⁵个重组HIV-RT分子都能被检测到。使用3种培养的临床分离株进行直接比较表明,这种检测水平等同于市售的p24抗原捕获测定法和基于分支DNA信号放大的HIV-RNA测定法。其他逆转录病毒,如HIV-2和猫免疫缺陷病毒(FIV),也可以用这种方法检测。这种非同位素测定法易于操作,通过监测逆转录酶(感染过程中的一种基本活性),可为HIV研究提供一种方便的定量方法。

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