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编码人SPH结合因子的cDNA的分子克隆,SPH结合因子是一种保守蛋白,可与U6小核RNA基因启动子的增强子样区域结合。

Molecular cloning of a cDNA encoding human SPH-binding factor, a conserved protein that binds to the enhancer-like region of the U6 small nuclear RNA gene promoter.

作者信息

Rincon J C, Engler S K, Hargrove B W, Kunkel G R

机构信息

Department of Biochemistry and Biophysics, Texas A&M University, College Station, TX 77843-2128, USA.

出版信息

Nucleic Acids Res. 1998 Nov 1;26(21):4846-52. doi: 10.1093/nar/26.21.4846.

Abstract

Many vertebrate small nuclear RNA gene promoters contain an SPH motif in their distal control regions that can confer transcriptional stimulation by RNA polymerase II or RNA polymerase III. Using the human U6 gene SPH motif as a probe, we isolated a cDNA encoding human SPH-binding factor (hSBF) from a HeLa cell expression library. The coding region of hSBF is almost identical to ZNF143, a 626 amino acid, seven zinc finger protein of previously unknown function. Furthermore, the predicted amino acid sequence of hSBF is highly homologous to Xenopus laevis and mouse Staf proteins, that bind to SPH motifs and stimulate transcription of selenocysteine tRNA gene promoters. Recombinant hSBF expressed in vitro or from Escherichia coli bound specifically to the human U6 gene SPH motif as shown by DNase I footprinting and electrophoretic mobility shift assays using various mutant SPH sites as competitors. Antibodies prepared against recombinant hSBF inhibited assembly of native SBF-DNA complexes. Immunodepleted HeLa S100 transcription extract no longer supported elevated levels of transcription by RNA polymerase III from a U6 promoter containing an SPH motif, whereas addition of recombinant hSBF protein to the immunodepleted extract reconstituted stimulated transcription.

摘要

许多脊椎动物小核RNA基因启动子在其远端控制区域含有一个SPH基序,该基序可赋予RNA聚合酶II或RNA聚合酶III转录刺激作用。我们以人U6基因的SPH基序为探针,从HeLa细胞表达文库中分离出一个编码人SPH结合因子(hSBF)的cDNA。hSBF的编码区与ZNF143几乎相同,ZNF143是一种626个氨基酸的、具有七个锌指的蛋白质,其功能此前未知。此外,hSBF的预测氨基酸序列与非洲爪蟾和小鼠的Staf蛋白高度同源,这些蛋白可结合SPH基序并刺激硒代半胱氨酸tRNA基因启动子的转录。如使用各种突变的SPH位点作为竞争者进行的DNase I足迹分析和电泳迁移率变动分析所示,体外表达或从大肠杆菌表达的重组hSBF特异性结合人U6基因的SPH基序。针对重组hSBF制备的抗体抑制天然SBF-DNA复合物的组装。免疫耗尽的HeLa S100转录提取物不再支持来自含有SPH基序的U6启动子的RNA聚合酶III的高水平转录,而向免疫耗尽的提取物中添加重组hSBF蛋白可重建刺激的转录。

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