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一种采用酶扩增技术从未纯化的细胞裂解物中终止特定核糖体RNA的夹心杂交检测方法。

A sandwich hybridization assay employing enzyme amplification for termination of specific ribosomal RNA from unpurified cell lysates.

作者信息

Wicks B, Cook D B, Barer M R, O'Donnell A G, Self C H

机构信息

Department of Microbiology, University of Newcastle upon Tyne, Tyne, NE2 4HH, United Kingdom.

出版信息

Anal Biochem. 1998 Jun 1;259(2):258-64. doi: 10.1006/abio.1998.2643.

Abstract

We have employed the power of the cyclic NAD-based enzyme amplification system to the determination of 16S rRNA. This generally applicable system employs two oligonucleotide probes, one of which is captured on a microtiter well surface and the other labeled with alkaline phosphatase. The detection of very low levels of hybridization of the capture probe is then achieved by the means of the ultrasensitive enzyme-amplified assay system, resulting in a highly sensitive, convenient, and rapid technology which can be directly employed on unpurified samples. We have been able to demonstrate the detection of 20 amol (10(7) molecules) of pure rRNA, and specific signals from as few as 2000 bacterial cells have also been demonstrated. The total procedural time can be short-5 to 18 h-depending on the dynamic range and sensitivity required. RNA target in the range of 10(12)-10(8) molecules can be assayed within 5 h. Extending the substrate incubation time enables between 10(11) and 10(7) molecules to be determined within 18 h. The system has great potential use with respect to studying the distribution and physiological states of cellular organisms.

摘要

我们已将基于环状烟酰胺腺嘌呤二核苷酸(NAD)的酶扩增系统的强大功能应用于16S rRNA的测定。这个普遍适用的系统使用两种寡核苷酸探针,其中一种固定在微量滴定孔表面,另一种用碱性磷酸酶标记。然后,通过超灵敏的酶扩增检测系统实现对捕获探针极低水平杂交的检测,从而产生一种高度灵敏、方便且快速的技术,可直接用于未纯化的样品。我们已经能够检测到20 amol(10⁷个分子)的纯rRNA,并且也已经证明了来自低至2000个细菌细胞的特异性信号。根据所需的动态范围和灵敏度,整个操作过程的时间可以很短,为5至18小时。在5小时内可以检测10¹²至10⁸个分子范围内的RNA靶标。延长底物孵育时间可在18小时内测定10¹¹至10⁷个分子。该系统在研究细胞生物体的分布和生理状态方面具有巨大的潜在用途。

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