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The structures of mouse and human L1 elements reflect their insertion mechanism

机译:小鼠和人类L1元素的结构反映了它们的插入机制

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摘要

L1 is an abundant, interspersed repeated DNA element of mammalian genomes. It has achieved its high copy number via retrotransposition. Like other non-LTR retrotransposons, L1 insertion into chromosomal DNA apparently occurs by target-site primed reverse transcription, or TPRT. L1 retrotransposition often generates elements with 5' truncations that are flanked by a duplication of the genomic target site (TSD). It is typically assumed that the 5' truncated elements are the consequence of poor processivity of the L1 reverse transcriptase. However, we find that the majority of young L1 elements from both the human and mouse genomes are truncated at sequences that can basepair with the target site. Thus, to whatever extent truncation is a consequence of poor processivity, we suggest that truncation is likely to occur when target site sequence can basepair with L I sequence. This finding supports a model for insertion that occurs by two sequential TPRT reactions, the second of which relies upon the homology between the target site and L1. Because perfect heteroduplex formation is not required for all insertions, a dynamic relationship between the primer, template and enzyme during reverse transcription is inferred. 5' truncation may be a successful evolutionary strategy that is exploited by L1 as a means to escape host suppression of transposition. Copyright (c) 2005 S. Karger AG, Basel.
机译:L1是哺乳动物基因组中丰富的,散布的重复DNA元素。它通过逆转转获得了很高的拷贝数。像其他非LTR反转录转座子一样,L1插入染色体DNA显然是通过靶位引物的逆转录或TPRT发生的。 L1逆转座通常会产生具有5'截短的元素,其侧翼是基因组目标位点(TSD)的重复。通常假定5'截短的元素是L1逆转录酶差的生产力的结果。但是,我们发现,来自人类和小鼠基因组的大多数年轻L1元件都被截短了可以与目标位点碱基配对的序列。因此,无论何种程度的截断都是差的生产力的结果,我们认为当靶位点序列可以与L I序列碱基配对时,截断很可能发生。这一发现支持了由两个连续的TPRT反应产生的插入模型,其中第二个反应依赖于靶位点与L1之间的同源性。由于并非所有插入都需要完美的异源双链体形成,因此可以推断反转录过程中引物,模板和酶之间的动态关系。 5'截短可能是成功的进化策略,被L1用作逃避宿主抑制转座的手段。版权所有(c)2005 S.Karger AG,巴塞尔。

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