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植物碱性亮氨酸拉链蛋白DNA结合特异性的双元决定因素

Bipartite determinants of DNA-binding specificity of plant basic leucine zipper proteins.

作者信息

Niu X, Renshaw-Gegg L, Miller L, Guiltinan M J

机构信息

Pioneer Hi-Bred International, Inc., Johnston, IA 50131, USA.

出版信息

Plant Mol Biol. 1999 Sep;41(1):1-13. doi: 10.1023/a:1006206011502.

Abstract

The basic leucine zipper (bZIP) proteins are one of the largest and most conserved groups of eukaryotic transcription factors/repressors. Two major subgroups among the plant bZIP proteins have been identified as G-box (CCACGTGG) or C-box (TGACGTCA) binding proteins based on their DNA binding specificity and the amino acid sequences of their basic regions. We have investigated how plant bZIP proteins determine their DNA binding specificity by mutation of the basic domain of the G-box-binding protein EmBP-1. Four subregions of the EmBP-1 basic domain that differ from the C-box-binding protein TGA1a were substituted singly or in combination with the corresponding regions of TGA1a. DNA binding experiments with the mutant proteins demonstrated that binding specificity of plant bZIP proteins is determined independently by two regions, the core basic region and the hinge region. These two regions have an additive effect on DNA binding specificity. PCR-assisted binding-site selections using key mutants demonstrated that only G-box and C-box binding specificity can be generated by combinations of amino acids in the basic domains of EmBP-1 and TGA1a. These results suggest that factorial contributions of the amino acid residues in the basic domain combine to determine DNA-binding specificity of bZIP proteins.

摘要

碱性亮氨酸拉链(bZIP)蛋白是真核转录因子/阻遏物中最大且最保守的蛋白家族之一。基于植物bZIP蛋白的DNA结合特异性及其碱性区域的氨基酸序列,已鉴定出其中两个主要亚组为G盒(CCACGTGG)或C盒(TGACGTCA)结合蛋白。我们通过对G盒结合蛋白EmBP-1碱性结构域进行突变,研究了植物bZIP蛋白如何确定其DNA结合特异性。EmBP-1碱性结构域中与C盒结合蛋白TGA1a不同的四个亚区域分别或与TGA1a的相应区域组合进行了替换。对突变蛋白进行的DNA结合实验表明,植物bZIP蛋白的结合特异性由两个区域独立决定,即核心碱性区域和铰链区。这两个区域对DNA结合特异性具有累加效应。使用关键突变体进行的PCR辅助结合位点筛选表明,只有EmBP-1和TGA1a碱性结构域中的氨基酸组合才能产生G盒和C盒结合特异性。这些结果表明,碱性结构域中氨基酸残基的因子贡献共同决定了bZIP蛋白的DNA结合特异性。

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