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福克I酶切割需要两个特定的DNA位点。

FokI requires two specific DNA sites for cleavage.

作者信息

Vanamee E S, Santagata S, Aggarwal A K

机构信息

Department of Physiology and Biophysics, Mount Sinai School of Medicine, NY 10029, USA.

出版信息

J Mol Biol. 2001 May 25;309(1):69-78. doi: 10.1006/jmbi.2001.4635.

Abstract

FokI is a bipartite restriction endonuclease that recognizes a non-palindromic DNA sequence, and then makes double-stranded cuts outside of that sequence to leave a 5' overhang. Earlier kinetic and crystallographic studies suggested that FokI might function as a dimer. Here, we show, using dynamic light-scattering, gel-filtration and analytical ultracentrifugation, that FokI dimerizes only in the presence of divalent metal ions. Furthermore, analysis of the DNA-bound complex reveals that two copies of the recognition sequence are incorporated into the dimeric complex and that formation of this complex is essential for full activation of cleavage. These results have broad implications for the mechanism by which monomeric type II endonucleases achieve high fidelity.

摘要

FokI是一种二分体限制性内切酶,它识别非回文DNA序列,然后在该序列之外进行双链切割,留下5'端突出。早期的动力学和晶体学研究表明,FokI可能以二聚体形式发挥作用。在这里,我们通过动态光散射、凝胶过滤和分析超速离心表明,FokI仅在二价金属离子存在下才会二聚化。此外,对与DNA结合的复合物的分析表明,识别序列的两个拷贝被纳入二聚体复合物中,并且该复合物的形成对于切割的完全激活至关重要。这些结果对单体II型内切酶实现高保真度的机制具有广泛的意义。

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