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反义 PCR:一种简单而强大的巢式单管 PCR 方法。

Antisense PCR: A simple and robust method for performing nested single-tube PCR.

机构信息

Department of Haematology and Genetic Pathology, Flinders University and Medical Centre, Bedford Park, SA, Australia.

出版信息

Anal Biochem. 2011 Feb 15;409(2):176-82. doi: 10.1016/j.ab.2010.10.030. Epub 2010 Oct 30.

Abstract

To overcome the disadvantages of two-round nested PCR, we developed a simple and robust closed single-tube nested PCR method (antisense PCR). The method uses antisense oligonucleotides that carry a 5' tag and that can potentially hybridize to the 3' ends of the outer primers, depending on the annealing temperature. During initial cycles, which are performed at a high annealing temperature, the antisense oligonucleotides do not hybridize and amplification is directed by the outer primers. During later cycles, for which the annealing temperature is decreased, the outer primers hybridize to the antisense oligonucleotides, extend to produce sequences that are mismatched to the amplicon templates, and consequently become inactivated, whereas the inner primers hybridize to the amplicon templates and continue amplification. Antisense quantitative PCR (qPCR) was compared with one-round qPCR for real-time amplification of four PCR targets (BCR, APC, N-RAS, and a rearranged IGH gene). It had equal amplification efficiency but produced much less nonspecific amplification. Antisense PCR enables both endpoint detection and real-time quantification. It can substitute for two-round nested PCRs but may also be applicable to instances of one-round PCR in which nonspecificity is a problem.

摘要

为了克服两轮巢式 PCR 的缺点,我们开发了一种简单而强大的封闭单管巢式 PCR 方法(反义 PCR)。该方法使用带有 5' 标签的反义寡核苷酸,这些寡核苷酸可以根据退火温度潜在地与外引物的 3' 末端杂交。在初始循环中,退火温度较高,反义寡核苷酸不会杂交,扩增由外引物指导。在随后的循环中,退火温度降低,外引物与反义寡核苷酸杂交,延伸产生与扩增模板不匹配的序列,因此失活,而内引物与扩增模板杂交并继续扩增。反义定量 PCR(qPCR)与一轮 qPCR 相比,实时扩增了四个 PCR 靶标(BCR、APC、N-RAS 和重排的 IGH 基因)。它具有相同的扩增效率,但产生的非特异性扩增要少得多。反义 PCR 既可以进行终点检测,也可以进行实时定量。它可以替代两轮巢式 PCR,但也可能适用于存在非特异性问题的一轮 PCR 情况。

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