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编码人类嗜酸性粒细胞主要碱性蛋白前体的互补DNA克隆的分离

Isolation of a complementary DNA clone encoding a precursor to human eosinophil major basic protein.

作者信息

McGrogan M, Simonsen C, Scott R, Griffith J, Ellis N, Kennedy J, Campanelli D, Nathan C, Gabay J

机构信息

Invitron Corporation, Redwood City, California 94063.

出版信息

J Exp Med. 1988 Dec 1;168(6):2295-308. doi: 10.1084/jem.168.6.2295.

Abstract

A 14-kD protein was purified from human PMNs and its NH2-terminal sequence was determined. Comparison of a portion of the NH2-terminal sequence of this protein to the recently reported NH2-terminal sequence of eosinophil major basic protein (MBP) showed them to be identical. To aid further characterization of the structural and functional properties of this molecule, we isolated from an HL-60 cDNA library a single class of cDNA clones whose sequence matched exactly the NH2-terminal amino acid sequence of the 14-kD polypeptide. Northern analysis of HL-60 cells suggests that MBP is constitutively expressed in HL-60 cells and is highly transcribed from a single copy gene. The sequence of the full-length cDNA clones predicts that MBP is synthesized as a 23-kD precursor form (pro-MBP) which is subsequently cleaved to release the mature 14-kD MBP. The putative pro-MBP has a predicted pI of 6.0, but both the charged and the hydrophobic residues are asymmetrically distributed, creating a bipolar molecule. The NH2-terminal half has a predicted pI of 3.7 and is hydrophilic, while the COOH-terminal half (corresponding to mature MBP) has a predicted pI of 11.1 and is hydrophobic.

摘要

从人多形核白细胞中纯化出一种14-kD蛋白,并测定了其氨基末端序列。将该蛋白的部分氨基末端序列与最近报道的嗜酸性粒细胞主要碱性蛋白(MBP)的氨基末端序列进行比较,发现它们是相同的。为了进一步表征该分子的结构和功能特性,我们从HL-60 cDNA文库中分离出一类cDNA克隆,其序列与14-kD多肽的氨基末端氨基酸序列完全匹配。对HL-60细胞的Northern分析表明,MBP在HL-60细胞中组成性表达,并且从单拷贝基因高度转录。全长cDNA克隆的序列预测,MBP以23-kD前体形式(前MBP)合成,随后被切割以释放成熟的14-kD MBP。推测的前MBP的预测等电点为6.0,但带电和疏水残基均不对称分布,形成双极分子。氨基末端一半的预测等电点为3.7,是亲水性的,而羧基末端一半(对应于成熟MBP)的预测等电点为11.1,是疏水性的。

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