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MN的克隆与鉴定,MN是一种人类肿瘤相关蛋白,具有与碳酸酐酶同源的结构域和一个假定的螺旋-环-螺旋DNA结合片段。

Cloning and characterization of MN, a human tumor-associated protein with a domain homologous to carbonic anhydrase and a putative helix-loop-helix DNA binding segment.

作者信息

Pastorek J, Pastoreková S, Callebaut I, Mornon J P, Zelník V, Opavský R, Zat'ovicová M, Liao S, Portetelle D, Stanbridge E J

机构信息

Institute of Virology, Slovak Academy of Sciences, Bratislava.

出版信息

Oncogene. 1994 Oct;9(10):2877-88.

PMID:8084592
Abstract

MN is a transmembrane glycoprotein that has been detected in HeLa cells and in some human carcinomas. The expression of MN protein in HeLa cells is regulated by cell density. In HeLa x fibroblast cell hybrids its expression correlates with tumorigenicity. Using a specific monoclonal antibody we have identified a cDNA clone coding for MN. Analysis of the deduced amino acid sequence revealed strong structural homology between the central region of the MN protein and carbonic anhydrases (CA). MN sequence retains the conserved zinc-binding site as well as the enzyme's active center. In accord with these findings, MN protein from HeLa cells was found to bind zinc and to have carbonic anhydrase activity. The N-terminal region of MN shares some similarity with DNA binding proteins of the helix-loop-helix (HLH) family, and the protein was found to have affinity for DNA by DNA-cellulose chromatography. The region between the CA-like domain and the putative HLH domain is rich in imperfect repeats of serine, proline, glycine and acidic residues with few hydrophobic amino acids, resembling thus an activation region of transcription factors. The fact that MN protein is detectable in several types of human carcinomas, but not in corresponding non-cancerous tissues, suggests its possible role in neoplasia. In addition, the analysis of biological consequences of MN expression of NIH3T3 cells provides the evidence in favour of MN protein involvement in control of cell proliferation and transformation.

摘要

MN是一种跨膜糖蛋白,已在HeLa细胞和一些人类癌组织中被检测到。HeLa细胞中MN蛋白的表达受细胞密度调节。在HeLa与成纤维细胞的杂种细胞中,其表达与致瘤性相关。利用一种特异性单克隆抗体,我们鉴定出了一个编码MN的cDNA克隆。对推导的氨基酸序列的分析显示,MN蛋白的中央区域与碳酸酐酶(CA)之间存在很强的结构同源性。MN序列保留了保守的锌结合位点以及该酶的活性中心。与这些发现一致的是,发现来自HeLa细胞的MN蛋白能结合锌并具有碳酸酐酶活性。MN的N端区域与螺旋-环-螺旋(HLH)家族的DNA结合蛋白有一些相似性,并且通过DNA-纤维素层析发现该蛋白对DNA有亲和力。类CA结构域和假定的HLH结构域之间的区域富含丝氨酸、脯氨酸、甘氨酸和酸性残基的不完全重复序列,疏水性氨基酸很少,因此类似于转录因子的激活区域。MN蛋白在几种类型的人类癌组织中可检测到,但在相应的非癌组织中未检测到,这一事实表明其在肿瘤形成中可能发挥作用。此外,对NIH3T3细胞中MN表达的生物学后果的分析提供了证据,支持MN蛋白参与细胞增殖和转化的调控。

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