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编码人血清甘露糖结合蛋白的基因的结构与进化起源

Structure and evolutionary origin of the gene encoding a human serum mannose-binding protein.

作者信息

Taylor M E, Brickell P M, Craig R K, Summerfield J A

机构信息

Department of Medicine, St. Mary's Hospital Medical School, London, U.K.

出版信息

Biochem J. 1989 Sep 15;262(3):763-71. doi: 10.1042/bj2620763.

Abstract

The N-terminal sequence of the major human serum mannose-binding protein (MBP1) was shown to be identical at all positions determined with the amino acid sequence predicted from a cDNA clone of a human liver MBP mRNA. An oligonucleotide corresponding to part of the sequence of this cDNA clone was used to isolate a cosmid genomic clone containing a homologous gene. The intron/exon structure of this gene was found to closely resemble that of the gene encoding a rat liver MBP (MBP A). The nucleotide sequence of the exons differed in several places from that of the human cDNA clone published by Ezekowitz, Day & Herman [(1988) J. Exp. Med. 167, 1034-1046]. The MBP molecule comprises a signal peptide, a cysteine-rich domain, a collagen-like domain, a 'neck' region and a carbohydrate-binding domain. Each domain is encoded by a separate exon. This genomic organization lends support to the hypothesis that the gene arose during evolution by a process of exon shuffling. Several consensus sequences that may be involved in controlling the expression of human serum MBP have been identified in the promoter region of the gene. The consensus sequences are consistent with the suggestion that this mammalian serum lectin is regulated as an acute-phase protein synthesized by the liver.

摘要

主要人血清甘露糖结合蛋白(MBP1)的N端序列在所有已确定的位置上都与从人肝脏MBP mRNA的cDNA克隆预测的氨基酸序列相同。一个与该cDNA克隆部分序列相对应的寡核苷酸被用于分离一个包含同源基因的黏粒基因组克隆。发现该基因的内含子/外显子结构与编码大鼠肝脏MBP(MBP A)的基因非常相似。外显子的核苷酸序列在几个位置上与Ezekowitz、Day和Herman发表的人cDNA克隆([1988] J. Exp. Med. 167, 1034 - 1046)不同。MBP分子包含一个信号肽、一个富含半胱氨酸的结构域、一个胶原样结构域、一个“颈部”区域和一个碳水化合物结合结构域。每个结构域由一个单独的外显子编码。这种基因组组织为该基因在进化过程中通过外显子重排过程产生的假说提供了支持。在该基因的启动子区域已鉴定出几个可能参与控制人血清MBP表达的共有序列。这些共有序列与该哺乳动物血清凝集素作为肝脏合成的急性期蛋白受到调节的观点一致。

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