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在体外碱基切除DNA修复体系中,HeLa DNA聚合酶α进行的缺口填充DNA合成。

Gap-filling DNA synthesis by HeLa DNA polymerase alpha in an in vitro base excision DNA repair scheme.

作者信息

Mosbaugh D W, Linn S

出版信息

J Biol Chem. 1984 Aug 25;259(16):10247-51.

PMID:6469963
Abstract

The ability of HeLa DNA polymerase alpha to utilize gapped PM2 DNAs for synthesis in a model base excision DNA repair scheme was examined. Partially depurinated PM2 DNA was incised on the 5' side of apurinic sites with HeLa apurinic/apyrimidinic endonuclease II, then the baseless sugar was removed and gaps of defined mean lengths were introduced at these sites by exonucleolytic digestion with HeLa DNase V. Gaps smaller than approximately 15 nucleotides did not serve as efficient primer-templates for DNA polymerase alpha. Gaps with mean lengths of 20-63 nucleotides did support limited DNA synthesis, but such synthesis terminated after the gap was reduced to roughly 15 nucleotides. These products were not substrates for Escherichia coli DNA ligase. In contrast, HeLa DNA polymerase beta utilize as primer-templates all of the gapped DNA substrates tested though it acted more efficiently with the smaller gaps. Moreover, the beta-polymerase was capable of filling these gaps to completion. In the case of the gaps that remained after partial closure by DNA polymerase alpha, DNA polymerase beta incorporated roughly 15 nucleotides and formed a product which was a substrate for DNA ligase. These results suggest that in vivo DNA repair pathways that involve a gap-filling DNA synthesis reaction might utilize DNA polymerase alpha only for larger gaps.

摘要

研究了HeLa DNA聚合酶α在模型碱基切除DNA修复方案中利用缺口PM2 DNA进行合成的能力。用HeLa脱嘌呤/脱嘧啶内切酶II在脱嘌呤位点的5'侧切割部分脱嘌呤的PM2 DNA,然后去除无碱基糖,并通过用HeLa DNA酶V进行外切核酸酶消化在这些位点引入确定平均长度的缺口。小于约15个核苷酸的缺口不能作为DNA聚合酶α的有效引物模板。平均长度为20 - 63个核苷酸的缺口确实支持有限的DNA合成,但这种合成在缺口减少到约15个核苷酸后终止。这些产物不是大肠杆菌DNA连接酶的底物。相比之下,HeLa DNA聚合酶β利用所有测试的缺口DNA底物作为引物模板,尽管它对较小的缺口作用更有效。此外,β聚合酶能够将这些缺口完全填补。在DNA聚合酶α部分封闭后留下的缺口情况下,DNA聚合酶β掺入约15个核苷酸并形成一种产物,该产物是DNA连接酶的底物。这些结果表明,在体内涉及缺口填充DNA合成反应的DNA修复途径可能仅在较大缺口时利用DNA聚合酶α。

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