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非洲爪蟾原肠胚特异性肌动蛋白基因胚胎转录激活的序列要求。

Sequence requirements for embryonic transcriptional activation of a gastrula-specific actin gene in Xenopus laevis.

作者信息

Brennan S M

机构信息

Department of Anatomy, University of Connecticut School of Medicine, Farmington 06032.

出版信息

Mol Reprod Dev. 1991 Dec;30(4):293-303. doi: 10.1002/mrd.1080300403.

DOI:10.1002/mrd.1080300403
PMID:1751033
Abstract

Cytoskeletal actin genes undergo developmentally timed transcriptional activation at the gastrula stage of embryonic development in the amphibian Xenopus laevis. To study the regulation of this process, a molecularly marked cloned actin gene has been introduced into living embryos by microinjection, and levels of its transcripts (which are distinct from endogenous actin message) have been measured by RNase protection. In vitro mutagenesis of the marked gene, followed by microinjection and transcriptional analysis of various mutants, has been used to search for gene sequences that participate in accurate transcriptional initiation and developmental control. Deletion mutants containing only 90 nucleotides of upstream sequence undergo correct developmental regulation, while deletion to -33 prevents normal activation of the gene. In the presence of sufficient upstream sequence, an actin-globin fusion gene, containing only 564 nucleotides downstream of the actin gene transcription startsite, is correctly activated. Taken together, these results imply that all sequences necessary for correct temporal regulation reside between -90 and +564 nucleotides, with respect to the transcriptional start site of the actin gene. They further suggest that developmental activation of actin gene transcription may involve either (1) interaction of non-DNA binding proteins with basal transcription factors, or (2) the concerted action of ubiquitous promoter-binding factors and factors that interact with downstream regulatory regions.

摘要

在两栖动物非洲爪蟾胚胎发育的原肠胚阶段,细胞骨架肌动蛋白基因经历了发育定时的转录激活。为了研究这一过程的调控机制,通过显微注射将一个分子标记的克隆肌动蛋白基因导入活胚胎中,并通过核糖核酸酶保护法测量其转录本水平(与内源性肌动蛋白信息不同)。对标记基因进行体外诱变,随后对各种突变体进行显微注射和转录分析,以寻找参与精确转录起始和发育控制的基因序列。仅包含90个核苷酸上游序列的缺失突变体能够进行正确的发育调控,而缺失至-33则会阻止基因的正常激活。在存在足够上游序列的情况下,一个仅在肌动蛋白基因转录起始位点下游包含564个核苷酸的肌动蛋白-珠蛋白融合基因被正确激活。综上所述,这些结果表明,相对于肌动蛋白基因的转录起始位点,正确的时间调控所需的所有序列都位于-90至+564个核苷酸之间。它们进一步表明,肌动蛋白基因转录的发育激活可能涉及(1)非DNA结合蛋白与基础转录因子的相互作用,或(2)普遍存在的启动子结合因子与与下游调控区域相互作用的因子的协同作用。

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