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双尾mRNA稳定性的发育调控由3'非翻译区的前43个核苷酸介导。

Developmental regulation of bicoid mRNA stability is mediated by the first 43 nucleotides of the 3' untranslated region.

作者信息

Surdej P, Jacobs-Lorena M

机构信息

Department of Genetics, School of Medicine, Case Western Reserve University, Cleveland, Ohio 44106-4955, USA.

出版信息

Mol Cell Biol. 1998 May;18(5):2892-900. doi: 10.1128/MCB.18.5.2892.

Abstract

During the transition from the maternal to the zygotic developmental program, the expression of genes important for pattern formation or cell cycle regulation changes dramatically. Rapid changes in gene expression are achieved in part through the control of mRNA stability. This report focuses on bicoid, a gene essential for formation of anterior embryonic structures in Drosophila melanogaster. bicoid mRNA is synthesized exclusively during oogenesis. Here, we show that bicoid mRNA stability is regulated. While bicoid mRNA is stable in retained oocytes, in unfertilized eggs, and during the first 2 h of embryogenesis, specific degradation is activated at cellularization of the blastoderm. To identify cis-acting sequences required for bicoid mRNA's regulated stability, fusions between bicoid and genes producing stable mRNAs were introduced into the Drosophila germ line by P-element-mediated transformation. The analysis of the fusion mRNAs identified a bicoid instability element (BIE) contained within a 43-nucleotide sequence immediately following the stop codon. The BIE is sufficient to destabilize the otherwise-stable ribosomal protein A1 mRNA and is separable from the previously identified bicoid mRNA localization signals and from the "nanos response element." Similar mechanisms may regulate a class of developmentally important maternal genes whose mRNA has a temporal profile similar to that of bicoid.

摘要

在从母体发育程序向合子发育程序转变的过程中,对模式形成或细胞周期调控至关重要的基因的表达会发生显著变化。基因表达的快速变化部分是通过对mRNA稳定性的控制来实现的。本报告聚焦于双尾,这是一种对黑腹果蝇胚胎前部结构形成至关重要的基因。双尾mRNA仅在卵子发生过程中合成。在此,我们表明双尾mRNA的稳定性受到调控。虽然双尾mRNA在保留的卵母细胞、未受精卵以及胚胎发育的前2小时内是稳定的,但在胚盘细胞化时会激活特异性降解。为了鉴定双尾mRNA受调控稳定性所需的顺式作用序列,通过P因子介导的转化将双尾与产生稳定mRNA的基因之间的融合体导入果蝇种系。对融合mRNA的分析鉴定出一个位于终止密码子后紧接着的43个核苷酸序列内的双尾不稳定元件(BIE)。该BIE足以使原本稳定的核糖体蛋白A1 mRNA不稳定,并且可与先前鉴定的双尾mRNA定位信号以及“纳米反应元件”分离。类似的机制可能调控一类在发育上重要的母体基因,其mRNA具有与双尾相似的时间分布特征。

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