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复杂DNA群体的序列非依赖性单引物扩增(SISPA)

Sequence-independent, single-primer amplification (SISPA) of complex DNA populations.

作者信息

Reyes G R, Kim J P

机构信息

Molecular Virology Department, Genelabs Incorporated, Redwood City, CA 94063.

出版信息

Mol Cell Probes. 1991 Dec;5(6):473-81. doi: 10.1016/s0890-8508(05)80020-9.

Abstract

Sequence-Independent, Single-Primer Amplification (SISPA) is a primer initiated technique that requires target sequence modification to achieve the non-selective logarithmic amplification of heterogeneous DNA populations. The method contrasts with the polymerase chain reaction (PCR), and its modified approaches, that have as their objective the amplification of unique or homologous sequences. SISPA requires the directional ligation of an asymmetric linker/primer oligonucleotide onto the target population of blunt ended DNA molecules. The common end sequence allows one strand of the double-stranded linker/primer to be used in repeated rounds of annealing, extension and denaturation in the presence of thermostable Taq DNA polymerase. The linker/primers contain restriction endonuclease sites to facilitate the molecular cloning of as little as 1 pg of starting material after amplification. SISPA is especially useful when the nucleotide sequence of the desired molecule is both unknown and present in limited amounts making its recovery by standard cloning procedures technically difficult. These conditions are present in the initial isolation and cloning of previously uncharacterized viral genomes. The application and quantitation of SISPA is described, together with its utility in the cloning and recovery of low abundance genetic sequences, as illustrated here with the hepatitis C virus.

摘要

序列非依赖单引物扩增(SISPA)是一种引物起始技术,需要对靶序列进行修饰,以实现异质DNA群体的非选择性对数扩增。该方法与以扩增独特或同源序列为目标的聚合酶链反应(PCR)及其改进方法形成对比。SISPA需要将不对称接头/引物寡核苷酸定向连接到平端DNA分子的靶群体上。共同的末端序列允许双链接头/引物的一条链在热稳定的Taq DNA聚合酶存在下用于重复的退火、延伸和变性循环。接头/引物含有限制性内切酶位点,便于在扩增后对低至1 pg的起始材料进行分子克隆。当所需分子的核苷酸序列未知且含量有限,通过标准克隆程序进行回收在技术上困难时,SISPA特别有用。这些情况存在于先前未表征的病毒基因组的初始分离和克隆中。本文描述了SISPA的应用和定量,以及它在低丰度遗传序列克隆和回收中的效用,以丙型肝炎病毒为例进行说明。

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