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黑腹果蝇焦刚毛-弱突变体的转录:在P基因背景下通过RNA剪接消除P因子序列并抑制焦刚毛转录

Transcription of the singed-weak mutation of Drosophila melanogaster: elimination of P-element sequences by RNA splicing and repression of singed transcription in a P genetic background.

作者信息

Paterson Jamie, Simmons Michael J, O'Hare Kevin

机构信息

Division of Cell and Molecular Biology, Faculty of Natural Sciences, Imperial College London, Biochemistry Building, South Kensington Campus, London, SW7 2AZ, UK.

出版信息

Mol Genet Genomics. 2007 Jul;278(1):53-64. doi: 10.1007/s00438-007-0227-z. Epub 2007 Mar 14.

DOI:10.1007/s00438-007-0227-z
PMID:17356852
Abstract

The dysgenesis-induced, hypermutable singed-weak allele has two incomplete P-elements inserted in a head-to-head configuration in the 5' non-coding exon of the singed bristle locus of Drosophila melanogaster. In the presence of P transposase, each element excises to produce single element derivatives, singed-extreme and singed-(+), that have either an extreme bristle or wild-type phenotype, respectively. In an M background, pseudo-wild-type transcripts are made that initiate at the singed promoter, read through the insertions, and are spliced to remove the P-element sequences and part of the 5' exon. The abundance of the pseudo-wild-type RNAs in pupae correlates with the bristle phenotype, being highest in singed-(+) and lowest in singed-extreme. Other RNAs are made that retain the insertions, or are truncated with respect to the downstream coding singed exons and have their 3' ends within the insertions. The mutants are female-fertile in an M background but sterile in a P background where little singed RNA can be detected. Transgenes containing either a complete P-element or an incomplete P-element known as KP impair the fertility of females carrying the singed-weak mutation, suggesting that the proteins encoded by these two widely distributed P-elements may be responsible for inhibiting transcription of singed-weak in a P background.

摘要

由发育异常诱导产生的、高度易变的焦刚毛-弱等位基因,在黑腹果蝇焦刚毛基因座的5'非编码外显子中,有两个以头对头构型插入的不完整P因子。在P转座酶存在的情况下,每个因子切除后产生单因子衍生物,即焦刚毛-极端型和焦刚毛-(+),它们分别具有极端刚毛或野生型表型。在M背景中,会产生假野生型转录本,这些转录本从焦刚毛启动子起始,通读插入序列,并通过剪接去除P因子序列和部分5'外显子。蛹中假野生型RNA的丰度与刚毛表型相关,在焦刚毛-(+)中最高,在焦刚毛-极端型中最低。还产生了其他RNA,它们保留了插入序列,或者相对于下游编码的焦刚毛外显子被截断,并且其3'端位于插入序列内。这些突变体在M背景中雌性可育,但在P背景中不育,在P背景中几乎检测不到焦刚毛RNA。含有完整P因子或称为KP的不完整P因子的转基因会损害携带焦刚毛-弱突变的雌性的生育能力,这表明这两个广泛分布的P因子所编码的蛋白质可能负责在P背景中抑制焦刚毛-弱的转录。

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