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牛单核细胞趋化蛋白-2基因的克隆

Cloning of the gene for bovine monocyte chemoattractant protein-2.

作者信息

Wempe F, Hanes J, Scheit K H

机构信息

Laboratory of Genetic Engineering, Slovak Academy of Science, Bratislava, CSFR.

出版信息

DNA Cell Biol. 1994 Jan;13(1):1-8. doi: 10.1089/dna.1994.13.1.

DOI:10.1089/dna.1994.13.1
PMID:8286035
Abstract

Bovine monocyte chemoattractant protein-1 (bovine MCP-1) cDNA has recently been characterized and shown to be highly expressed in bovine seminal vesicles secretory epithelium as well as in phytohemagglutinin (PHA)-stimulated peripheral blood mononuclear leukocytes (PMNLs). In an attempt to isolate the MCP-1 gene, we screened a bovine genomic cosmid library with a MCP-1-specific probe pH42. A positive clone, c11/1, was subjected to restriction analysis and fragments probed with pH42 by southern blotting. pH42-positive fragments were subcloned and sequenced. The sequence revealed three exon-like regions that coded for a protein displaying an identity of 51% with bovine MCP-1. Employing this sequence information from c11/1, the c11/1-specific cDNA was generated from poly(A)+RNA of bovine PMNLs by reverse transcription and a combination of polymerase chain reaction (PCR) methods. The assembled c11/1 cDNA comprised a 5' UTR coding region as well as 3' UTR for the gene product c11/1. Amino acid sequence comparison of the bovine c11/1 gene product with human monocyte chemotactic proteins yielded the highest sequence identity with human MCP-2, and it is assumed that the c11/1 gene product represents the bovine MCP-2. The exon/intron structure of the bovine MCP-2 gene was found to be similar to the human MCP-1 gene. The bovine MCP-2 gene consists of three exons separated by two introns. In the 5'-flanking region of the 3.3-kb gene, a TATA box as well as an AP-1 sequence motif were identified. The bovine MCP-2 is specified by a single-copy gene.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

牛单核细胞趋化蛋白-1(牛MCP-1)的cDNA最近已得到鉴定,显示其在牛精囊分泌上皮以及植物血凝素(PHA)刺激的外周血单个核白细胞(PMNL)中高表达。为了分离MCP-1基因,我们用MCP-1特异性探针pH42筛选了一个牛基因组黏粒文库。一个阳性克隆c11/1接受了限制性分析,并用pH42通过Southern印迹法对片段进行探测。pH42阳性片段被亚克隆并测序。该序列揭示了三个外显子样区域,编码一种与牛MCP-1有51%同一性的蛋白质。利用来自c11/1的这一序列信息,通过逆转录和聚合酶链反应(PCR)方法的组合,从牛PMNL的聚腺苷酸加尾RNA(poly(A)+RNA)中生成了c11/1特异性cDNA。组装好的c11/1 cDNA包含该基因产物c11/1的5'非翻译区编码区以及3'非翻译区。牛c11/1基因产物与人单核细胞趋化蛋白的氨基酸序列比较显示,与人MCP-2的序列同一性最高,据推测c11/1基因产物代表牛MCP-2。发现牛MCP-2基因的外显子/内含子结构与人类MCP-1基因相似。牛MCP-2基因由三个外显子组成,被两个内含子隔开。在这个3.3 kb基因的5'侧翼区域,鉴定出了一个TATA盒以及一个AP-1序列基序。牛MCP-2由一个单拷贝基因编码。(摘要截短至250字)

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