首页> 外文期刊>Protein Science: A Publication of the Protein Society >Structure of the Cdt1 C-terminal domain: conservation of the winged helix fold in replication licensing factors.
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Structure of the Cdt1 C-terminal domain: conservation of the winged helix fold in replication licensing factors.

机译:Cdt1 C末端域的结构:复制许可因子中的翼状螺旋折叠的保守性。

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摘要

In eukaryotic replication licensing, Cdt1 plays a key role by recruiting the MCM2-7 complex onto the origin of chromosome. The C-terminal domain of mouse Cdt1 (mCdt1C), the most conserved region in Cdt1, is essential for licensing and directly interacts with the MCM2-7 complex. We have determined the structures of mCdt1CS (mCdt1C_small; residues 452 to 557) and mCdt1CL (mCdt1C_large; residues 420 to 557) using X-ray crystallography and solution NMR spectroscopy, respectively. While the N-terminal 31 residues of mCdt1CL form a flexible loop with a short helix near the middle, the rest of mCdt1C folds into a winged helix structure. Together with the middle domain of mouse Cdt1 (mCdt1M, residues 172-368), this study reveals that Cdt1 is formed with a tandem repeat of the winged helix domain. The winged helix fold is also conserved in other licensing factors including archaeal ORC and Cdc6, which supports an idea that these replication initiators may have evolved from a common ancestor. Based on the structure of mCdt1C, in conjunction with the biochemical analysis, we propose a binding site for the MCM complex within the mCdt1C.
机译:在真核复制许可中,Cdt1通过将MCM2-7复合物募集到染色体的起源上起关键作用。小鼠Cdt1(mCdt1C)的C末端结构域是Cdt1中最保守的区域,对于许可至关重要,并直接与MCM2-7复合体相互作用。我们分别使用X射线晶体学和溶液NMR光谱法确定了mCdt1CS(mCdt1C_small;残基452至557)和mCdt1CL(mCdt1C_large;残基420至557)的结构。虽然mCdt1CL的N端31个残基形成一个柔性环,中间附近有一个短螺旋,但其余的mCdt1C却折叠成带翼的螺旋结构。连同小鼠Cdt1的中间结构域(mCdt1M,残基172-368)一起,这项研究揭示了Cdt1是由有翼螺旋结构域的串联重复序列形成的。翼状螺旋折叠在其他许可因素(包括古细菌ORC和Cdc6)中也得到保留,这支持了这些复制引发剂可能是从共同祖先进化而来的想法。基于mCdt1C的结构,结合生化分析,我们提出了mCdt1C中MCM复合物的结合位点。

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