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DAF-3 信号转导分子母抗素结合 DNA 并抑制秀丽隐杆线虫咽部的基因表达。

The DAF-3 Smad binds DNA and represses gene expression in the Caenorhabditis elegans pharynx.

作者信息

Thatcher J D, Haun C, Okkema P G

机构信息

Department of Biological Sciences (M/C567), University of Illinois at Chicago, Chicago, IL 60607, USA.

出版信息

Development. 1999 Jan;126(1):97-107. doi: 10.1242/dev.126.1.97.

DOI:10.1242/dev.126.1.97
PMID:9834189
Abstract

Gene expression in the pharyngeal muscles of Caenorhabditis elegans is controlled in part by organ-specific signals, which in the myo-2 gene target a short DNA sequence termed the C subelement. To identify genes contributing to these signals, we performed a yeast one-hybrid screen for cDNAs encoding factors that bind the C subelement. One clone recovered was from daf-3, which encodes a Smad most closely related to vertebrate Smad4. We demonstrated that DAF-3 binds C subelement DNA directly and specifically using gel mobility shift and DNase1 protection assays. Mutation of any base in the sequence GTCTG interfered with binding in the gel mobility shift assay, demonstrating that this pentanucleotide is a core recognition sequence for DAF-3 binding. daf-3 is known to promote formation of dauer larvae and this activity is negatively regulated by TGFbeta-like signaling. To determine how daf-3 affects C subelement enhancer activity in vivo, we examined expression a gfp reporter controlled by a concatenated C subelement oligonucleotide in daf-3 mutants and other mutants affecting the TGFbeta-like signaling pathway controlling dauer formation. Our results demonstrate that wild-type daf-3 can repress C subelement enhancer activity during larval development and, like its dauer-promoting activity, daf-3's repressor activity is negatively regulated by TGFbeta-like signaling. We have examined expression of this gfp reporter in dauer larvae and have observed no daf-3-dependent repression of C activity. These results suggest daf-3 directly regulates pharyngeal gene expression during non-dauer development.

摘要

秀丽隐杆线虫咽肌中的基因表达部分受器官特异性信号控制,这些信号在肌动蛋白-2基因中靶向一个称为C亚元件的短DNA序列。为了鉴定对这些信号有贡献的基因,我们进行了酵母单杂交筛选,以寻找编码与C亚元件结合的因子的cDNA。筛选出的一个克隆来自daf-3,它编码一种与脊椎动物Smad4最密切相关的Smad蛋白。我们通过凝胶迁移率变动分析和DNase1保护分析证明,DAF-3直接且特异性地结合C亚元件DNA。序列GTCTG中的任何一个碱基发生突变都会干扰凝胶迁移率变动分析中的结合,这表明这个五核苷酸是DAF-3结合的核心识别序列。已知daf-3促进 dauer 幼虫的形成,并且这种活性受到TGFβ样信号的负调控。为了确定daf-3如何在体内影响C亚元件增强子活性,我们检测了在daf-3突变体和其他影响控制dauer形成的TGFβ样信号通路的突变体中,由串联的C亚元件寡核苷酸控制的gfp报告基因的表达。我们的结果表明,野生型daf-3在幼虫发育过程中可以抑制C亚元件增强子活性,并且与其促进dauer形成的活性一样,daf-3的抑制活性受到TGFβ样信号的负调控。我们检测了这种gfp报告基因在dauer幼虫中的表达,未观察到daf-3依赖的C活性抑制。这些结果表明,daf-3在非dauer发育过程中直接调节咽基因的表达。

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Development. 1999 Jan;126(1):97-107. doi: 10.1242/dev.126.1.97.
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