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由不依赖核酸内切酶的LINE-1逆转录转座介导的DNA修复。

DNA repair mediated by endonuclease-independent LINE-1 retrotransposition.

作者信息

Morrish Tammy A, Gilbert Nicolas, Myers Jeremy S, Vincent Bethaney J, Stamato Thomas D, Taccioli Guillermo E, Batzer Mark A, Moran John V

机构信息

Department of Human Genetics, University of Michigan Medical School, 1241 E. Catherine Street, Ann Arbor, Michigan 48105-0618, USA.

出版信息

Nat Genet. 2002 Jun;31(2):159-65. doi: 10.1038/ng898. Epub 2002 May 13.

DOI:10.1038/ng898
PMID:12006980
Abstract

Long interspersed elements (LINE-1s) are abundant retrotransposons in mammalian genomes that probably retrotranspose by target site-primed reverse transcription (TPRT). During TPRT, the LINE-1 endonuclease cleaves genomic DNA, freeing a 3' hydroxyl that serves as a primer for reverse transcription of LINE-1 RNA by LINE-1 reverse transcriptase. The nascent LINE-1 cDNA joins to genomic DNA, generating LINE-1 structural hallmarks such as frequent 5' truncations, a 3' poly(A)+ tail and variable-length target site duplications (TSDs). Here we describe a pathway for LINE-1 retrotransposition in Chinese hamster ovary (CHO) cells that acts independently of endonuclease but is dependent upon reverse transcriptase. We show that endonuclease-independent LINE-1 retrotransposition occurs at near-wildtype levels in two mutant cell lines that are deficient in nonhomologous end-joining (NHEJ). Analysis of the pre- and post-integration sites revealed that endonuclease-independent retrotransposition results in unusual structures because the LINE-1s integrate at atypical target sequences, are truncated predominantly at their 3' ends and lack TSDs. Moreover, two of nine endonuclease-independent retrotranspositions contained cDNA fragments at their 3' ends that are probably derived from the reverse transcription of endogenous mRNA. Thus, our results suggest that LINE-1s can integrate into DNA lesions, resulting in retrotransposon-mediated DNA repair in mammalian cells.

摘要

长散在元件(LINE-1s)是哺乳动物基因组中丰富的逆转座子,可能通过靶位点引发的逆转录(TPRT)进行逆转座。在TPRT过程中,LINE-1核酸内切酶切割基因组DNA,释放出一个3'羟基,作为LINE-1逆转录酶逆转录LINE-1 RNA的引物。新生的LINE-1 cDNA与基因组DNA连接,产生LINE-1的结构特征,如频繁的5'端截短、3'端多聚腺苷酸尾巴和可变长度的靶位点重复序列(TSD)。在这里,我们描述了中国仓鼠卵巢(CHO)细胞中LINE-1逆转座的一条途径,该途径独立于核酸内切酶,但依赖于逆转录酶。我们表明,在两个缺乏非同源末端连接(NHEJ)的突变细胞系中,不依赖核酸内切酶的LINE-1逆转座以接近野生型的水平发生。对整合前和整合后位点的分析表明,不依赖核酸内切酶的逆转座会导致异常结构,因为LINE-1s整合在非典型靶序列上,主要在其3'端被截短且缺乏TSD。此外,九个不依赖核酸内切酶的逆转座中有两个在其3'端包含cDNA片段,这些片段可能来源于内源性mRNA的逆转录。因此,我们的结果表明,LINE-1s可以整合到DNA损伤中,导致哺乳动物细胞中逆转座子介导的DNA修复。

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