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负责叶酸受体α和β差异配体结合的不同氨基酸的完整图谱。

Complete mapping of divergent amino acids responsible for differential ligand binding of folate receptors alpha and beta.

作者信息

Maziarz K M, Monaco H L, Shen F, Ratnam M

机构信息

Department of Biochemistry and Molecular Biology, Medical College of Ohio, Toledo, Ohio 43614-5804, USA.

出版信息

J Biol Chem. 1999 Apr 16;274(16):11086-91. doi: 10.1074/jbc.274.16.11086.

DOI:10.1074/jbc.274.16.11086
PMID:10196192
Abstract

The folate receptor (FR) type alpha may be distinguished from FR-beta by its higher affinity for the circulating folate coenzyme, (6S)-5-methyltetrahydrofolate (5-CH3H4folate), and its opposite stereospecificity for reduced folate coenzymes. Previous studies showed that a single leucine to alanine substitution at position 49 of the mature protein sequence is responsible for the functional divergence of FR-beta (Shen, F., Zheng, X., Wang, H., and Ratnam, M. (1997) Biochemistry 36, 6157-6163); however, the results also indicated that the minimum requirement for conversion of FR-beta to the functional equivalent of FR-alpha should include amino acid substitution(s) downstream of residue 92 in addition to mutation of L49A. To pinpoint those residues, chimeric FR-betaL49A/FR-alpha constructs including progressively shorter segments of FR-alpha downstream of position 92 as well as selected point mutants were studied. Simultaneous substitution of Leu-49, Phe-104, and Gly-166 in FR-beta with the corresponding FR-alpha residues Ala, Val, and Glu, respectively, reconstituted the ligand binding characteristics of FR-alpha. The results also exclude a role for other residues in FR-alpha in determining its functional divergence. A homology model of FR-alpha based on the three-dimensional structure of the chicken riboflavin-binding protein is used to show the position of residues 49, 104, and 166 in relation to the hydrophobic cleft corresponding to the riboflavin-binding pocket.

摘要

α型叶酸受体(FR)与β型叶酸受体的区别在于,它对循环叶酸辅酶(6S)-5-甲基四氢叶酸(5-CH3H4folate)具有更高的亲和力,并且对还原型叶酸辅酶具有相反的立体特异性。先前的研究表明,成熟蛋白序列第49位的单个亮氨酸到丙氨酸的取代是FR-β功能差异的原因(Shen, F., Zheng, X., Wang, H., and Ratnam, M. (1997) Biochemistry 36, 6157-6163);然而,结果还表明,将FR-β转化为功能等同于FR-α的最低要求除了L49A突变外,还应包括92位残基下游的氨基酸取代。为了确定这些残基,研究了嵌合的FR-βL49A/FR-α构建体,包括92位下游逐渐缩短的FR-α片段以及选定的点突变体。将FR-β中的Leu-49、Phe-104和Gly-166分别同时替换为相应的FR-α残基Ala、Val和Glu,可重建FR-α的配体结合特性。结果还排除了FR-α中其他残基在决定其功能差异方面的作用。基于鸡核黄素结合蛋白三维结构的FR-α同源模型用于显示残基49、104和166相对于对应于核黄素结合口袋的疏水裂缝的位置。

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