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不育的芬兰约克郡公猪在KPL2基因内携带一个全长的LINE-1反转录转座子。

Infertile Finnish Yorkshire boars carry a full-length LINE-1 retrotransposon within the KPL2 gene.

作者信息

Sironen Anu, Vilkki Johanna, Bendixen Christian, Thomsen Bo

机构信息

Food and Biotechnology, Animal Genomics, MTT Agrifood Research Finland, 31600, Jokioinen, Finland.

出版信息

Mol Genet Genomics. 2007 Oct;278(4):385-91. doi: 10.1007/s00438-007-0256-7. Epub 2007 Jul 4.

DOI:10.1007/s00438-007-0256-7
PMID:17610085
Abstract

The KPL2 gene is expressed predominantly in cells with cilia or flagella. We have previously demonstrated that a large intronic insertion in KPL2 is associated with immotile sperm cells and infertility in the domesticated pig (Sus scrofa). To fully characterize the structure of the mutation, we have now cloned and sequenced the insertion. The data identified the presence of a long interspersed nuclear element-1 (LINE-1) encoding all activities required for retrotransposition, including a 5'-untranslated region (UTR) with an internal RNA polymerase II promoter, two open reading frames (ORF1 and ORF2) separated by an intergenic region and a 3' UTR containing a polyadenylation signal. Characterization of the junctions between the LINE-1 and the genomic target revealed the presence of direct repeats of 14 bp at both ends, showing that integration occurred by target-primed reverse transcription. Furthermore, sequence analysis suggested that the aberrant splicing pattern of KPL2 transcripts induced by the LINE-1 element is caused by interference with putative intronic splice signals and activation of a cryptic splice site. These data demonstrate that integration of a transposition-competent L1 element into KPL2 is responsible for the defective spermatozoa, which accentuates the role of mobile DNA elements as insertional mutagens in mammalian genomes.

摘要

KPL2基因主要在具有纤毛或鞭毛的细胞中表达。我们之前已经证明,KPL2基因中的一个大的内含子插入与家猪(Sus scrofa)的精子活动力缺乏和不育有关。为了全面表征该突变的结构,我们现在克隆并测序了该插入片段。数据确定了一个长散在核元件1(LINE-1)的存在,它编码逆转录转座所需的所有活性,包括一个带有内部RNA聚合酶II启动子的5'非翻译区(UTR)、两个由基因间隔区隔开的开放阅读框(ORF1和ORF2)以及一个包含多聚腺苷酸化信号的3'UTR。对LINE-1与基因组靶点之间连接点的表征揭示了两端存在14bp的直接重复序列,表明整合是通过靶标引发的逆转录发生的。此外,序列分析表明,由LINE-1元件诱导的KPL2转录本异常剪接模式是由对假定的内含子剪接信号的干扰和一个隐蔽剪接位点的激活引起的。这些数据表明,一个具有转座能力的L1元件整合到KPL2基因中是精子缺陷的原因,这突出了移动DNA元件作为哺乳动物基因组中插入诱变剂的作用。

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