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骨连接素启动子。DNA序列分析及与骨细胞转录调控潜在相关的S1核酸酶位点。

Osteonectin promoter. DNA sequence analysis and S1 endonuclease site potentially associated with transcriptional control in bone cells.

作者信息

Young M F, Findlay D M, Dominguez P, Burbelo P D, McQuillan C, Kopp J B, Robey P G, Termine J D

机构信息

Bone Research Branch, National Institute of Dental Research, Bethesda, Maryland 20892.

出版信息

J Biol Chem. 1989 Jan 5;264(1):450-6.

PMID:2535844
Abstract

To understand the basis of osteonectin (SPARC) transcriptional regulation, we have isolated a bovine genomic clone (lambda Og15) encoding exon 1 and 15 kilobase pairs (kb) of flanking DNA. Direct RNA sequencing of the 5' end of the osteonectin message showed it contained a sequence identical to that of a 2.4-kb EcoRI-BamHI fragment located midway in the clone lambda Og15. The results indicate exon 1 is located 10 kb away from exon 2 in the bovine genome. The DNA sequence unit CCTG is repeated five times in exon 1 which is composed exclusively of untranslated sequence. Sequence analysis of the 5'-flanking DNA revealed the presence of many regulatory motifs including a "GC" box with four overlapping SP1 consensus sequences. Immediately downstream from the GC box is a 72-base pair purine-rich stretch composed primarily of direct repeats of the sequence motifs GGGGA and GGA (GAGA box). Digestion of the flanking DNA in vitro with S1 endonuclease showed a site for the enzyme at position -55 which is just 3' to the GAGA box. Chimeric chloramphenicol acetyltransferase constructs were prepared containing the S1-sensitive site and showed substantial transcriptional activity in UMR-106 and fetal and adult human bone cells which are known to be high producers of the protein. The results indicate a potential regulatory activity of the S1 site in osteonectin gene activation.

摘要

为了解骨连接素(SPARC)转录调控的基础,我们分离出了一个牛基因组克隆(λOg15),其编码外显子1及侧翼DNA的15千碱基对(kb)。对骨连接素信使RNA 5'端进行直接RNA测序表明,其包含的一段序列与位于克隆λOg15中间位置的一个2.4 kb EcoRI - BamHI片段的序列相同。结果表明,在牛基因组中,外显子1距离外显子2有10 kb。外显子1中DNA序列单元CCTG重复了5次,该外显子完全由非翻译序列组成。对5'侧翼DNA的序列分析揭示了许多调控基序的存在,包括一个具有四个重叠SP1共有序列的“GC”框。紧接在GC框下游的是一段72个碱基对的富含嘌呤的序列,主要由序列基序GGGGA和GGA(GAGA框)的直接重复组成。用S1核酸内切酶在体外消化侧翼DNA,结果显示该酶在 - 55位置有一个位点,该位点正好位于GAGA框的3'端。制备了包含S1敏感位点的嵌合氯霉素乙酰转移酶构建体,其在UMR - 106细胞以及已知是该蛋白高产细胞的胎儿和成人骨细胞中显示出显著的转录活性。结果表明S1位点在骨连接素基因激活中具有潜在的调控活性。

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