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染色体结构与基因表达的关系。

Relation of chromosome structure and gene expression.

作者信息

Mirkovitch J, Gasser S M, Laemmli U K

机构信息

Department of Molecular Biology, University of Geneva, Switzerland.

出版信息

Philos Trans R Soc Lond B Biol Sci. 1987 Dec 15;317(1187):563-74. doi: 10.1098/rstb.1987.0081.

Abstract

We have been able to map specific DNA fragments at the bases of chromatin loops with the help of a novel extraction procedure by using lithium-3',5'-diiodosalicylate. One such scaffold-attached region (SAR) is found in the non-transcribed spacer in each repeat of the histone gene cluster, on a 657 base pair (b.p.) restriction fragment. Exonuclease III digestion has localized two protein-binding domains on the SAR of the histone cluster. Each covers approximately 200 b.p. and they are separated by a nuclease-accessible region of about 100 b.p. These domains are rich in sequences closely related to the topoisomerase II cleavage consensus. We have studied the scaffold association of three developmentally regulated genes of Drosophila melanogaster: alcohol dehydrogenase (Adh), the homoeotic gene fushi tarazu (ftz) and Sgs-4, a gene encoding one of the glue proteins secreted by third-instar larvae. We find regions attached to the nuclear scaffold (SARS) both 5' and 3' of all three genes, defining small domains ranging from 4.5 to 13 kilobases. In the case of Adh, a gene with two promoters, we find two upstream and two downstream SARS. Those 5' of the gene co-map with regulatory regions for the adult and the larval transcripts, respectively. For Sgs-4, the 5' SAR covers 866 b.p. immediately upstream of the transcript, and encompasses the 200 b.p. regulatory region defined by two deletion mutants that produce little or no Sgs-4 protein. In ftz the 5' SAR is found 4.8 kilobases upstream of the start of transcription within a 2.5 kilobase element required for a high level of ftz expression in the early embryo. Sequence analysis of five upstream SARS reveals clusters of sequences closely related to the cleavage consensus of topoisomerase II. In addition, they contain multiple copies of two sequence motifs: a specific 10 b.p. A-rich sequence, and another 10 b.p. T-rich stretch. In conclusion, the intimate association of the SAR with the upstream/enhancer elements, the presence of clustered sequences highly homologous to the topoisomerase II cleavage consensus, and the localization of topoisomerase II in the scaffold, suggest a structure-function relation between chromosome organization and gene expression.

摘要

借助一种使用3',5'-二碘水杨酸锂的新型提取方法,我们已能够在染色质环基部定位特定的DNA片段。在组蛋白基因簇的每个重复序列的非转录间隔区中,在一个657碱基对(bp)的限制性片段上发现了一个这样的支架附着区域(SAR)。核酸外切酶III消化已将两个蛋白质结合结构域定位在组蛋白簇的SAR上。每个结构域覆盖约200 bp,它们被一个约100 bp的核酸酶可及区域隔开。这些结构域富含与拓扑异构酶II切割共有序列密切相关的序列。我们研究了果蝇的三个发育调控基因的支架关联:乙醇脱氢酶(Adh)、同源异型基因分节基因(ftz)和Sgs-4,Sgs-4是一个编码三龄幼虫分泌的一种胶蛋白的基因。我们在所有三个基因的5'和3'端都发现了附着于核支架(SARS)的区域,定义了范围从4.5到13千碱基的小结构域。就具有两个启动子的Adh基因而言,我们发现了两个上游和两个下游SARS。该基因5'端的那些区域分别与成虫和幼虫转录本的调控区域共定位。对于Sgs-4,5' SAR覆盖转录本上游紧邻的866 bp,并包含由两个产生很少或不产生Sgs-蛋白的缺失突变体所定义的200 bp调控区域。在ftz中,5' SAR位于转录起始点上游4.8千碱基处,在早期胚胎中高水平ftz表达所需的一个2.5千碱基元件内。对五个上游SARS的序列分析揭示了与拓扑异构酶II切割共有序列密切相关的序列簇。此外,它们包含两个序列基序的多个拷贝:一个特定的10 bp富含A的序列和另一个10 bp富含T的片段。总之,SAR与上游/增强子元件的紧密关联、与拓扑异构酶II切割共有序列高度同源的成簇序列的存在以及拓扑异构酶II在支架中的定位,表明染色体组织与基因表达之间存在结构 - 功能关系。

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