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一种无需平衡子维持的skn-1次等位基因的分离。

Isolation of a Hypomorphic skn-1 Allele That Does Not Require a Balancer for Maintenance.

作者信息

Tang Lanlan, Dodd William, Choe Keith

机构信息

Department of Biology, University of Florida, Gainesville, Florida 32611.

Department of Biology, University of Florida, Gainesville, Florida 32611

出版信息

G3 (Bethesda). 2015 Dec 29;6(3):551-8. doi: 10.1534/g3.115.023010.

Abstract

In Caenorhabditis elegans, the transcription factor SKN-1 has emerged as a central coordinator of stress responses and longevity, increasing the need for genetic tools to study its regulation and function. However, current loss-of-function alleles cause fully penetrant maternal effect embryonic lethality, and must be maintained with genetic balancers that require careful monitoring and labor intensive strategies to obtain large populations. In this study, we identified a strong, but viable skn-1 hypomorphic allele skn-1(zj15) from a genetic screen for suppressors of wdr-23, a direct regulator of the transcription factor. skn-1(zj15) is a point mutation in an intron that causes mis-splicing of a fraction of mRNA, and strongly reduces wildtype mRNA levels of the two long skn-1a/c variants. The skn-1(zj15) allele reduces detoxification gene expression and stress resistance to levels comparable to skn-1 RNAi, but, unlike RNAi, it is not restricted from some tissues. We also show that skn-1(zj15) is epistatic to canonical upstream regulators, demonstrating its utility for genetic analysis of skn-1 function and regulation in cases where large numbers of worms are needed, a balancer is problematic, diet is varied, or RNAi cannot be used.

摘要

在秀丽隐杆线虫中,转录因子SKN-1已成为应激反应和寿命的核心协调因子,这增加了对研究其调控和功能的遗传工具的需求。然而,目前的功能丧失等位基因会导致完全显性的母体效应胚胎致死,必须通过遗传平衡子来维持,而这需要仔细监测且耗费大量人力才能获得大量群体。在本研究中,我们从对转录因子的直接调节因子wdr-23的抑制子进行的遗传筛选中鉴定出一个强但可存活的skn-1次等位基因skn-1(zj15)。skn-1(zj15)是内含子中的一个点突变,导致一部分mRNA发生错误剪接,并强烈降低了两个长skn-1a/c变体的野生型mRNA水平。skn-1(zj)等位基因将解毒基因表达和应激抗性降低到与skn-1 RNA干扰相当的水平,但与RNA干扰不同的是,它不受某些组织的限制。我们还表明,skn-1(zj15)对典型的上游调节因子是上位性的,这表明在需要大量线虫、平衡子存在问题、饮食多样或无法使用RNA干扰的情况下,它在skn-1功能和调控的遗传分析中具有实用性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/33a1/4777118/9de5792e59de/551f1.jpg

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