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A comprehensive approach to expression of L1 loci

机译:L1基因座表达的综合方法

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摘要

L1 elements represent the only currently active, autonomous retrotransposon in the human genome, and they make major contributions to human genetic instability. The vast majority of the 500 000 L1 elements in the genome are defective, and only a relatively few can contribute to the retrotransposition process. However, there is currently no comprehensive approach to identify the specific loci that are actively transcribed separate from the excess of L1-related sequences that are co-transcribed within genes. We have developed RNA-Seq procedures, as well as a 1200 bp 5' RACE product coupled with PACBio sequencing that can identify the specific L1 loci that contribute most of the L1-related RNA reads. At least 99% of L1-related sequences found in RNA do not arise from the L1 promoter, instead representing pieces of L1 incorporated in other cellular RNAs. In any given cell type a relatively few active L1 loci contribute to the `authentic' L1 transcripts that arise from the L1 promoter, with significantly different loci seen expressed in different tissues.
机译:L1元素代表人类基因组中唯一目前活跃的自主逆转录,对人类遗传不稳定进行了重大贡献。基因组中的500 000 L1元素的绝大多数是有缺陷的,并且只有相对较少的可能导致反向转移过程。然而,目前没有综合方法来识别与在基因内共转录的过量的L1相关序列分开的具体轨迹。我们已经开发了RNA-SEQ程序,以及1200bp 5'种族产品,与PACBIO测序相结合,可识别有贡献大多数L1相关RNA读数的特定L1基因座。从L1启动子出现至少99%的RNA相关序列,而不是表示掺入其他细胞RNA中的L1的片。在任何给定的细胞类型中,相对较少的活性L1基因座有助于从L1启动子产生的`真正的L1转录物,其在不同组织中表达的显着不同的基因座。

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