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白血病相关MLL组蛋白甲基转移酶的非甲基化CpG结合CXXC结构域的溶液结构

Solution structure of the nonmethyl-CpG-binding CXXC domain of the leukaemia-associated MLL histone methyltransferase.

作者信息

Allen Mark D, Grummitt Charles G, Hilcenko Christine, Min Sandra Young, Tonkin Louise M, Johnson Christopher M, Freund Stefan M, Bycroft Mark, Warren Alan J

机构信息

Centre for Protein Engineering, Cambridge, UK.

出版信息

EMBO J. 2006 Oct 4;25(19):4503-12. doi: 10.1038/sj.emboj.7601340. Epub 2006 Sep 21.

Abstract

Methylation of CpG dinucleotides is the major epigenetic modification of mammalian genomes, critical for regulating chromatin structure and gene activity. The mixed-lineage leukaemia (MLL) CXXC domain selectively binds nonmethyl-CpG DNA, and is required for transformation by MLL fusion proteins that commonly arise from recurrent chromosomal translocations in infant and secondary treatment-related acute leukaemias. To elucidate the molecular basis of nonmethyl-CpG DNA recognition, we determined the structure of the human MLL CXXC domain by multidimensional NMR spectroscopy. The CXXC domain has a novel fold in which two zinc ions are each coordinated tetrahedrally by four conserved cysteine ligands provided by two CGXCXXC motifs and two distal cysteine residues. We have identified the CXXC domain DNA binding interface by means of chemical shift perturbation analysis, cross-saturation transfer and site-directed mutagenesis. In particular, we have shown that residues in an extended surface loop are in close contact with the DNA. These data provide a template for the design of specifically targeted therapeutics for poor prognosis MLL-associated leukaemias.

摘要

CpG二核苷酸的甲基化是哺乳动物基因组主要的表观遗传修饰,对调控染色质结构和基因活性至关重要。混合系白血病(MLL)CXXC结构域选择性结合非甲基化的CpG DNA,是MLL融合蛋白转化所必需的,这些融合蛋白通常源自婴儿期复发性染色体易位以及继发性治疗相关急性白血病。为阐明非甲基化CpG DNA识别的分子基础,我们通过多维核磁共振光谱法测定了人MLL CXXC结构域的结构。CXXC结构域具有一种新颖的折叠方式,其中两个锌离子分别由两个CGXCXXC基序和两个远端半胱氨酸残基提供的四个保守半胱氨酸配体进行四面体配位。我们通过化学位移扰动分析、交叉饱和转移和定点诱变确定了CXXC结构域的DNA结合界面。特别是,我们已经表明,一个延伸表面环中的残基与DNA紧密接触。这些数据为设计针对预后不良的MLL相关白血病的特异性靶向治疗药物提供了模板。

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