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在单链 DNA 结合蛋白 (SSB) 的存在下,分枝杆菌解旋酶-核酸酶 AdnAB 对双链断裂进行解旋和切除。

Double strand break unwinding and resection by the mycobacterial helicase-nuclease AdnAB in the presence of single strand DNA-binding protein (SSB).

机构信息

Sloan-Kettering Institute, New York, New York 10065, USA.

出版信息

J Biol Chem. 2010 Nov 5;285(45):34319-29. doi: 10.1074/jbc.M110.162925. Epub 2010 Aug 23.

Abstract

Mycobacterial AdnAB is a heterodimeric DNA helicase-nuclease and 3' to 5' DNA translocase implicated in the repair of double strand breaks (DSBs). The AdnA and AdnB subunits are each composed of an N-terminal motor domain and a C-terminal nuclease domain. Inclusion of mycobacterial single strand DNA-binding protein (SSB) in reactions containing linear plasmid dsDNA allowed us to study the AdnAB helicase under conditions in which the unwound single strands are coated by SSB and thereby prevented from reannealing or promoting ongoing ATP hydrolysis. We found that the AdnAB motor catalyzed processive unwinding of 2.7-11.2-kbp linear duplex DNAs at a rate of ∼250 bp s(-1), while hydrolyzing ∼5 ATPs per bp unwound. Crippling the AdnA phosphohydrolase active site did not affect the rate of unwinding but lowered energy consumption slightly, to ∼4.2 ATPs bp(-1). Mutation of the AdnB phosphohydrolase abolished duplex unwinding, consistent with a model in which the "leading" AdnB motor propagates a Y-fork by translocation along the 3' DNA strand, ahead of the "lagging" AdnA motor domain. By tracking the resection of the 5' and 3' strands at the DSB ends, we illuminated a division of labor among the AdnA and AdnB nuclease modules during dsDNA unwinding, whereby the AdnA nuclease processes the unwound 5' strand to liberate a short oligonucleotide product, and the AdnB nuclease incises the 3' strand on which the motor translocates. These results extend our understanding of presynaptic DSB processing by AdnAB and engender instructive comparisons with the RecBCD and AddAB clades of bacterial helicase-nuclease machines.

摘要

分枝杆菌 AdnAB 是一种异源二聚体 DNA 解旋酶-核酸酶和 3' 到 5' DNA 转位酶,与双链断裂 (DSB) 的修复有关。AdnA 和 AdnB 亚基均由 N 端的马达结构域和 C 端的核酸酶结构域组成。在包含线性质粒 dsDNA 的反应中加入分枝杆菌单链 DNA 结合蛋白 (SSB),使我们能够在解开的单链被 SSB 覆盖的条件下研究 AdnAB 解旋酶,从而防止其重新退火或促进持续的 ATP 水解。我们发现,AdnAB 马达以 ∼250 bp s(-1) 的速度催化 2.7-11.2-kbp 线性双链 DNA 的连续解旋,同时水解每个解开的碱基对约 5 个 ATP。破坏 AdnA 磷酸水解酶活性位点不会影响解旋速度,但略微降低能量消耗,至 ∼4.2 ATPs bp(-1)。突变 AdnB 磷酸水解酶会使双链解旋失活,这与“领头”AdnB 马达通过沿 3' DNA 链向前移动来推进 Y 型分叉的模型一致,而“滞后”的 AdnA 马达结构域则在后面。通过跟踪 DSB 末端 5' 和 3' 链的切除,我们阐明了 AdnA 和 AdnB 核酸酶模块在 dsDNA 解旋过程中的分工,其中 AdnA 核酸酶处理解开的 5' 链以释放短寡核苷酸产物,而 AdnB 核酸酶在马达转位的 3' 链上切割。这些结果扩展了我们对 AdnAB 进行前突触 DSB 处理的理解,并与细菌解旋酶-核酸酶机器的 RecBCD 和 AddAB 分支进行了有益的比较。

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