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The AAA+ ClpX machine unfolds a keystone subunit to remodel the Mu transpososome

机译:aaa + ClpX机器展开了一个关键的子单元来重塑mu转座体

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摘要

A hyperstable complex of the tetrameric MuA transposase with recombined DNA must be remodeled to allow subsequent DNA replication. ClpX, a AAA+ enzyme, fulfills this function by unfolding one transpososome subunit. Which MuA subunit is extracted, and how complex destabilization relates to establishment of the correct directionality (left to right) of Mu replication, is not known. Here, using altered-specificity MuA proteins/DNA sites, we demonstrate that transpososome destabilization requires preferential ClpX unfolding of either the catalytic-left or catalytic-right subunits, which make extensive intersubunit contacts in the tetramer. In contrast, ClpX recognizes the other two subunits in the tetramer much less efficiently, and their extraction does not substantially destabilize the complex. Thus, ClpX targets the most stable structural components of the complex. Left-end biased Mu replication is not, however, determined by ClpX’s intrinsic subunit preference. The specific targeting of a stabilizing “keystone subunit” within a complex for unfolding is an attractive general mechanism for remodeling by AAA+ enzymes.
机译:必须重塑四聚体MuA转座酶与重组DNA的高稳定复合物,以允许随后的DNA复制。 ClpX,一种AAA +酶,通过展开一个转座子亚基来实现这一功能。未知哪个MuA亚基被提取,以及复杂的去稳定化与建立Mu复制的正确方向(从左到右)有多大关系。在这里,使用改变的特异性MuA蛋白/ DNA位点,我们证明了转座体去稳定化需要左催化左或催化右亚基的优先ClpX折叠,从而使四聚体中广泛的亚基间接触。相比之下,ClpX识别四聚体中其他两个亚基的效率要低得多,并且它们的提取基本上不会破坏复合物的稳定性。因此,ClpX靶向复合物最稳定的结构组分。但是,左端偏向Mu复制不是由ClpX固有的亚基偏好决定的。在复合物中稳定的“基石亚基”的特异性靶向是展开的,是通过AAA +酶重塑的有吸引力的通用机制。

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