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一项基因筛选鉴定出果蝇中类固醇触发的程序性细胞死亡的新调控因子。

A genetic screen identifies new regulators of steroid-triggered programmed cell death in Drosophila.

作者信息

Wang Lei, Evans Janelle, Andrews Hillary K, Beckstead Robert B, Thummel Carl S, Bashirullah Arash

机构信息

Department of Human Genetics, University of Utah School of Medicine, Salt Lake City, Utah 84112-5330, USA.

出版信息

Genetics. 2008 Sep;180(1):269-81. doi: 10.1534/genetics.108.092478. Epub 2008 Aug 30.

Abstract

The steroid hormone ecdysone triggers the rapid and massive destruction of larval tissues through transcriptional cascades that culminate in rpr and hid expression and caspase activation. Here we describe the use of genetic screens to further our understanding of this steroid-triggered programmed cell death response. Pupal lethal mutants were screened for specific defects in larval salivary gland destruction. A pilot screen using existing P-element collections resulted in the identification of mutations in known cell death regulators, E74 and hid, as well as multiple alleles in CBP (nejire) and dTrf2. A large-scale EMS mutagenesis screen on the third chromosome resulted in the recovery of 48 mutants. These include seven multiallelic complementation groups, at least five of which do not map to regions or genes previously associated with cell death. Five mutants display defects in the transcriptional induction of rpr and hid, and all display a penetrant block in caspase activation. Three were mapped to specific genes: CG5146, which encodes a protein of unknown function, Med24, which encodes a component of the RNA polymerase II mediator complex, and CG7998, which encodes a putative mitochondrial malate dehydrogenase. These genetic screens provide new directions for understanding the regulation of programmed cell death during development.

摘要

类固醇激素蜕皮激素通过转录级联反应引发幼虫组织的快速大量破坏,最终导致rpr和hid表达以及半胱天冬酶激活。在此,我们描述了利用遗传筛选来进一步了解这种类固醇触发的程序性细胞死亡反应。对蛹期致死突变体进行筛选,以寻找幼虫唾液腺破坏中的特定缺陷。使用现有的P因子文库进行的初步筛选,鉴定出已知细胞死亡调节因子E74和hid中的突变,以及CBP(nejire)和dTrf2中的多个等位基因。在第三条染色体上进行的大规模EMS诱变筛选,获得了48个突变体。其中包括七个多等位基因互补群,其中至少五个并不定位于先前与细胞死亡相关的区域或基因。五个突变体在rpr和hid的转录诱导中表现出缺陷,并且都在半胱天冬酶激活中表现出明显的阻断。三个突变体被定位到特定基因:CG5146,编码一种功能未知的蛋白质;Med24,编码RNA聚合酶II中介复合物的一个组分;CG7998,编码一种假定的线粒体苹果酸脱氢酶。这些遗传筛选为理解发育过程中程序性细胞死亡的调控提供了新的方向。

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