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首页> 外文期刊>Journal of Molecular Biology >Solution structure of the Arabidopsis thaliana telomeric repeat-binding protein DNA binding domain: A new fold with an additional C-terminal helix
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Solution structure of the Arabidopsis thaliana telomeric repeat-binding protein DNA binding domain: A new fold with an additional C-terminal helix

机译:拟南芥端粒重复结合蛋白DNA结合结构域的溶液结构:具有额外C末端螺旋的新折叠

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The double-stranded telomeric repeat-binding protein (TRP) AtTRP1 is isolated from Arabidopsis thaliana. Using gel retardation assays, we defined the C-terminal 97 amino acid residues, Gln464 to Val560 (AtTRP1(464-560)), as the minimal structured telomeric repeat-binding domain. This region contains a typical Myb DNA-binding motif and a C-terminal extension of 40 amino acid residues. The monomeric AtTRP1464-560 binds to a 13-mer DNA duplex containing a single repeat of an A. thaliana telomeric DNA sequence (GGTTTAG) in a 1: 1 complex, with a K-D similar to 10(-6)-10(-7) M. Nuclear magnetic resonance (NMR) examination revealed that the solution structure of AtTRP1464-560 is a novel four-helix tetrahedron rather than the three-helix bundle structure found in typical Myb motifs and other TRPs. Binding of the 13-mer DNA duplex to AtTRP1464-560 induced significant chemical shift perturbations of protein amide resonances, which suggests that helix 3 (H3) and the flexible loop connecting H3 and H4 are essential for telomeric DNA sequence recognition. Furthermore, similar to that in hTRF1, the N-terminal arm likely contributes to or stabilizes DNA binding. Sequence comparisons suggested that the four-helix structure and the involvement of the loop residues in DNA binding may be features unique to plant TRPs. (c) 2005 Elsevier Ltd. All rights reserved.
机译:从拟南芥中分离出双链端粒重复结合蛋白(TRP)AtTRP1。使用凝胶阻滞分析,我们将C末端的97个氨基酸残基Gln464定义为Val560(AtTRP1(464-560)),作为最小的结构性端粒重复结合结构域。该区域包含典型的Myb DNA结合基序和40个氨基酸残基的C端延伸。单体AtTRP1464-560结合到13-mer DNA双链体上,该双链体以1:1的复合物包含拟南芥端粒DNA序列(GGTTTAG)的单个重复序列,其KD类似于10(-6)-10(-7 M.核磁共振(NMR)检查显示,AtTRP1464-560的溶液结构是新颖的四螺旋四面体,而不是典型Myb图案和其他TRP中发现的三螺旋束结构。 13-mer DNA双链体与AtTRP1464-560的结合引起蛋白质酰胺共振的明显化学位移扰动,这表明螺旋3(H3)和连接H3和H4的柔性环对于端粒DNA序列识别至关重要。此外,类似于hTRF1,N末端臂可能有助于或稳定DNA结合。序列比较表明,四螺旋结构和环残基参与DNA结合可能是植物TRP特有的特征。 (c)2005 Elsevier Ltd.保留所有权利。

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