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酿酒酵母的Srs2解旋酶对三联体重复发夹结构的快速解旋作用。

Rapid unwinding of triplet repeat hairpins by Srs2 helicase of Saccharomyces cerevisiae.

作者信息

Dhar Alok, Lahue Robert S

机构信息

Eppley Institute for Research in Cancer and Allied Diseases, University of Nebraska Medical Center, Box 986805, Omaha, NE 68198-6805, USA.

出版信息

Nucleic Acids Res. 2008 Jun;36(10):3366-73. doi: 10.1093/nar/gkn225. Epub 2008 Apr 25.

Abstract

Expansions of trinucleotide repeats cause at least 15 heritable human diseases. Single-stranded triplet repeat DNA in vitro forms stable hairpins in a sequence-dependent manner that correlates with expansion risk in vivo. Hairpins are therefore considered likely intermediates during the expansion process. Unwinding of a hairpin by a DNA helicase would help protect against expansions. Yeast Srs2, but not the RecQ homolog Sgs1, blocks expansions in vivo in a manner largely dependent on its helicase function. The current study tested the idea that Srs2 would be faster at unwinding DNA substrates with an extrahelical triplet repeat hairpin embedded in a duplex context. These substrates should mimic the relevant intermediate structure thought to occur in vivo. Srs2 was faster than Sgs1 at unwinding several substrates containing triplet repeat hairpins or another structured loop. In contrast, control substrates with an unstructured loop or a Watson-Crick duplex were unwound equally well by both enzymes. Results with a fluorescently labeled, three-way junction showed that Srs2 unwinding proceeds unabated through extrahelical triplet repeats. In summary, Srs2 maintains its facile unwinding of triplet repeat hairpins embedded within duplex DNA, supporting the genetic evidence that Srs2 is a key helicase in Saccharomyces cerevisiae for preventing expansions.

摘要

三核苷酸重复序列的扩增会导致至少15种可遗传的人类疾病。体外单链三联体重复DNA以序列依赖的方式形成稳定的发夹结构,这与体内的扩增风险相关。因此,发夹被认为可能是扩增过程中的中间产物。DNA解旋酶解开发夹有助于防止扩增。酵母Srs2而非RecQ同源物Sgs1在很大程度上依赖其解旋酶功能在体内阻断扩增。本研究测试了这样一种观点,即Srs2在解开双链环境中嵌入额外螺旋三联体重复发夹的DNA底物时速度更快。这些底物应模拟体内可能出现的相关中间结构。在解开几种含有三联体重复发夹或另一种结构化环的底物时,Srs2比Sgs1更快。相比之下,两种酶对具有非结构化环或沃森-克里克双链体的对照底物的解旋效果相同。对荧光标记的三链连接体的研究结果表明,Srs2的解旋作用在通过额外螺旋三联体重复序列时不会减弱。总之,Srs2能够轻松解开双链DNA中嵌入的三联体重复发夹,这支持了Srs2是酿酒酵母中防止扩增的关键解旋酶的遗传学证据。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/923c/2425488/e445f66c3298/gkn225f1.jpg

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