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转座元件在秀丽隐杆线虫的生殖系而非体细胞中被激活。

Activation of a transposable element in the germ line but not the soma of Caenorhabditis elegans.

作者信息

Collins J, Saari B, Anderson P

出版信息

Nature. 1987;328(6132):726-8. doi: 10.1038/328726a0.

Abstract

The genetic activity of transposable elements is tightly controlled in many species. Transposons that are relatively quiescent under certain circumstances can excise or transpose at greatly increased rates under other circumstances. For example, 'genomic shock' can activate quiescent maize transposons, 'cytotype' and tissue-specific splicing regulate Drosophila P factors, copy number controls Tn5 transposition in bacteria, and developmental timing affects the production of transposon-like intracisternal A-particles in mouse embryos. The Caenorhabditis elegans transposable element Tc1 is subject to both strain-specific and tissue-specific control. Multiple copies of Tc1 are present in the genome of all C. elegans strains collected from nature. However, these elements are genetically active in only certain isolates. For example, in C. elegans variety Bristol transposition and excision of Tc1 are undetectable, but in variety Bergerac transposition and excision are frequent. Moreover, in variety Bergerac, Tc1 is about 1,000-fold more active in somatic cells than in germ cells. We have investigated the genetic basis for the germ/soma regulation of Tc1 activity. We have isolated mutants that exhibit increased frequencies of Tc1 excision in the germ line. The frequencies of Tc1 excision in the soma are unaltered in these mutants. These mutants also exhibit high frequencies of Tc1 germ-line transposition, and this results in a mutator phenotype. Nearly all mutator-induced mutations are caused by insertion of Tc1.

摘要

在许多物种中,转座元件的基因活性受到严格控制。在某些情况下相对静止的转座子,在其他情况下可以以大幅增加的速率进行切除或转座。例如,“基因组冲击”可激活静止的玉米转座子,“细胞型”和组织特异性剪接调节果蝇P因子,拷贝数控制细菌中的Tn5转座,发育时间影响小鼠胚胎中转座子样核内A颗粒的产生。秀丽隐杆线虫的转座元件Tc1受到菌株特异性和组织特异性的控制。从自然界收集的所有秀丽隐杆线虫菌株的基因组中都存在多个拷贝的Tc1。然而,这些元件仅在某些分离株中具有遗传活性。例如,在布里斯托尔品系的秀丽隐杆线虫中,未检测到Tc1的转座和切除,但在伯杰拉克品系中,转座和切除很频繁。此外,在伯杰拉克品系中,Tc1在体细胞中的活性比在生殖细胞中高约1000倍。我们研究了Tc1活性的生殖系/体细胞调控的遗传基础。我们分离出了在生殖系中Tc1切除频率增加的突变体。在这些突变体中,体细胞中Tc1的切除频率没有改变。这些突变体还表现出Tc1生殖系转座的高频率,这导致了突变体表型。几乎所有由突变体诱导的突变都是由Tc1的插入引起的。

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