Arneson Nona, Hughes Simon, Houlston Richard, Done Susan
CSH Protoc. 2008 Jan 1;2008:pdb.prot4921. doi: 10.1101/pdb.prot4921.
INTRODUCTIONPCR-based whole-genome amplification (WGA) has the goal of generating microgram quantities of genome-representative DNA from picogram or nanogram amounts of starting material. This amplification should introduce little, or ideally no, representational bias. In contrast to other techniques for WGA, PCR-based methods are generally less affected by DNA quality and are more applicable to DNA extracted from various sources (fixed and fresh tissues). Primer extension preamplification PCR (PEP-PCR), in contrast to degenerate oligonucleotide primed PCR (DOP-PCR), uses totally degenerate 15-mer PCR primers. An additional difference is that in PEP-PCR, the number of potential priming sites is orders of magnitude larger. The effectiveness of PEP-PCR has been increased by several alterations. The improved PEP (I-PEP) PCR approach, described in this protocol, uses a DNA polymerase cocktail that includes Taq DNA polymerase (to carry out the primer extension as in a traditional PCR) and a proofreading DNA polymerase (to provide 3'-to-5'-exonuclease activity, excising misincorporated nucleotides that slow the progression of Taq DNA polymerase). The result is far more efficient WGA, with increased fidelity due to the removal of the misincorporated nucleotides. Similar to DOP-PCR, PEP-PCR generates a smear of DNA fragments that are visible on an agarose gel.
引言
基于聚合酶链反应(PCR)的全基因组扩增(WGA)旨在从皮克或纳克量的起始材料中生成微克量的基因组代表性DNA。这种扩增应引入很少的代表性偏差,理想情况下不引入偏差。与其他WGA技术相比,基于PCR的方法通常受DNA质量的影响较小,更适用于从各种来源(固定组织和新鲜组织)提取的DNA。与简并寡核苷酸引物PCR(DOP-PCR)不同,引物延伸预扩增PCR(PEP-PCR)使用完全简并的15聚体PCR引物。另一个区别是,在PEP-PCR中,潜在的引物结合位点数量要多几个数量级。通过几种改进提高了PEP-PCR的有效性。本方案中描述的改进型PEP(I-PEP)PCR方法使用了一种DNA聚合酶混合物,其中包括Taq DNA聚合酶(用于像传统PCR那样进行引物延伸)和一种校正DNA聚合酶(用于提供3'至5'核酸外切酶活性,切除错误掺入的核苷酸,这些核苷酸会减缓Taq DNA聚合酶的进展)。结果是WGA效率大大提高,由于错误掺入的核苷酸被去除,保真度也有所提高。与DOP-PCR类似,PEP-PCR会产生在琼脂糖凝胶上可见的DNA片段拖尾现象。
