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The Q motif of a viral packaging motor governs its force generation and communicates ATP recognition to DNA interaction

机译:病毒包装马达的Q主题控制着力量的产生并将ATP识别传达给DNA相互作用

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摘要

A key step in the assembly of many viruses is the packaging of DNA into preformed procapsids by an ATP-powered molecular motor. To shed light on the motor mechanism we used single-molecule optical tweezers measurements to study the effect of mutations in the large terminase subunit in bacteriophage λ on packaging motor dynamics. A mutation, K84A, in the putative ATPase domain driving DNA translocation was found to decrease motor velocity by ≈40% but did not change the force dependence or decrease processivity substantially. These findings support the hypothesis that a deviant “Walker A-like” phosphate-binding motif lies adjacent to residue 84. Another mutation, Y46F, was also found to decrease motor velocity by ≈40% but also increase slipping during DNA translocation by >10-fold. These findings support the hypothesis that viral DNA packaging motors contain an adenine-binding motif that regulates ATP hydrolysis and substrate affinity analogous to the “Q motif” recently identified in DEAD-box RNA helicases. We also find impaired force generation for the Y46F mutant, which shows that the Q motif plays an important role in determining the power and efficiency of the packaging motor.
机译:组装许多病毒的关键步骤是通过ATP驱动的分子马达将DNA包装成预先形成的衣壳。为了阐明运动机制,我们使用了单分子光学镊子测量来研究噬菌体λ中大末端酶亚基的突变对包装运动动力学的影响。发现推定的ATPase域驱动DNA易位的突变K84A使运动速度降低了约40%,但并未显着改变力的依赖性或降低了生产力。这些发现支持了这样一个假说,即残基84附近存在一个异常的“ Walker A样”磷酸结合基序。另一个突变Y46F也被发现可将运动速度降低≈40%,但在DNA转运过程中也可增加滑动率> 10。 -折。这些发现支持以下假设:病毒DNA包装马达包含一个腺嘌呤结合基序,该基序与最近在DEAD-box RNA解旋酶中鉴定的“ Q基序”相似,可调节ATP水解和底物亲和力。我们还发现Y46F突变体的力产生受损,这表明Q基序在确定包装电机的功率和效率中起着重要作用。

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