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IS200/IS605 family single-strand transposition: mechanism of IS608 strand transfer

机译:IS200 / IS605家族单链转座:IS608链转移的机制

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Transposase, TnpA, of the IS200/IS605 family member IS608, catalyses single-strand DNA transposition and is dimeric with hybrid catalytic sites composed of an HUH motif from one monomer and a catalytic Y127 present in an α-helix (αD) from the other (trans configuration). αD is attached to the main body by a flexible loop. Although the reactions leading to excision of a transposition intermediate are well characterized, little is known about the dynamic behaviour of the transpososome that drives this process. We provide evidence strongly supporting a strand transfer model involving rotation of both αD helices from the trans to the cis configuration (HUH and Y residues from the same monomer). Studies with TnpA heterodimers suggest that TnpA cleaves DNA in the trans configuration, and that the catalytic tyrosines linked to the 5′-phosphates exchange positions to allow rejoining of the cleaved strands (strand transfer) in the cis configuration. They further imply that, after excision of the transposon junction, TnpA should be reset to a trans configuration before the cleavage required for integration. Analysis also suggests that this mechanism is conserved among members of the IS200/IS605 family.
机译:IS200 / IS605家族成员IS608的转座酶TnpA催化单链DNA转座,并与由一个单体的HUH基序和另一个α-螺旋(αD)中存在的催化Y127组成的杂化催化位点二聚(反式配置)。 αD通过柔性环连接到主体。尽管对导致转座中间体切除的反应进行了很好的表征,但对于驱动该过程的转座体的动态行为知之甚少。我们提供了有力的证据证明链转移模型涉及两个αD螺旋从反式到顺式的旋转(来自同一单体的HUH和Y残基)。用TnpA异二聚体进行的研究表明,TnpA以反式构型切割DNA,并且连接到5'-磷酸的催化酪氨酸交换位置,从而允许以顺式构型重新连接切割的链(链转移)。他们进一步暗示,在转座子连接切除后,TnpA应该在整合所需的切割之前重设为反式构型。分析还表明,该机制在IS200 / IS605系列成员中是保守的。

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