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E47-神经分化因子1/β2碱性螺旋-环-螺旋结构域-DNA复合物的晶体结构:异二聚体选择性与DNA识别

Crystal structure of E47-NeuroD1/beta2 bHLH domain-DNA complex: heterodimer selectivity and DNA recognition.

作者信息

Longo Antonella, Guanga Gerald P, Rose Robert B

机构信息

Department of Molecular and Structural Biochemistry, North Carolina State University, 128 Polk Hall, Raleigh, North Carolina 27695-7622, USA.

出版信息

Biochemistry. 2008 Jan 8;47(1):218-29. doi: 10.1021/bi701527r. Epub 2007 Dec 11.

DOI:10.1021/bi701527r
PMID:18069799
Abstract

The ubiquitous class I basic helix-loop-helix (bHLH) factor E47 forms heterodimers with multiple tissue specific class II bHLH proteins to regulate distinct differentiation pathways. In order to define how class I- class II heterodimer partners are selected, we determined the crystal structure of the E47-NeuroD1-bHLH dimer in complex with the insulin promoter E-box sequence. Purification of the bHLH domain of E47-NeuroD1 indicates that E47 heterodimers are stable in solution. The interactions between E47 and NeuroD1 in the heterodimer are comparable to the interactions between E47 monomers in the homodimer, including hydrogen bonding, buried hydrophobic surface, and packing interactions. This is consistent with a model in which E47-NeuroD1 heterodimers are favored due to the instability of NeuroD1 homodimers. Although E47-NeuroD1 is oriented uniquely on the E-box sequence (CATCTG) within the promoter of the insulin gene, no direct contacts are observed with the central base pairs within this E-box sequence. We propose that concerted domain motions allow E47 to form specific base contacts in solution. NeuroD1 is restrained from adopting the same base contacts by an additional phosphate backbone interaction by the neurogenic-specific residue His115. Orienting E47-NeuroD1 on promoters may foster protein-protein contacts essential to initiate transcription.

摘要

普遍存在的I类碱性螺旋-环-螺旋(bHLH)因子E47与多种组织特异性II类bHLH蛋白形成异二聚体,以调节不同的分化途径。为了确定如何选择I类-II类异二聚体伴侣,我们确定了与胰岛素启动子E盒序列结合的E47-NeuroD1-bHLH二聚体的晶体结构。E47-NeuroD1的bHLH结构域的纯化表明E47异二聚体在溶液中是稳定的。异二聚体中E47和NeuroD1之间的相互作用与同二聚体中E47单体之间的相互作用相当,包括氢键、埋藏的疏水表面和堆积相互作用。这与一个模型一致,即由于NeuroD1同二聚体的不稳定性,E47-NeuroD1异二聚体更受青睐。尽管E47-NeuroD1在胰岛素基因启动子内的E盒序列(CATCTG)上有独特的取向,但未观察到与该E盒序列内的中央碱基对有直接接触。我们提出,协同的结构域运动使E47在溶液中形成特定的碱基接触。NeuroD1因神经源性特异性残基His115的额外磷酸主链相互作用而无法形成相同的碱基接触。将E47-NeuroD1定位在启动子上可能促进启动转录所必需的蛋白质-蛋白质接触。

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