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Controlling bacteriophage phi29 DNA-packaging motor by addition or discharge of a peptide at N-terminus of connector protein that interacts with pRNA

机译:通过在与pRNA相互作用的连接蛋白N端添加或释放肽来控制噬菌体phi29 DNA包装电机

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摘要

Bacteriophage phi29 utilizes a motor to translocate genomic DNA into a preformed procapsid. The motor contains six pRNAs, an enzyme and one 12-subunit connector with a central channel for DNA transportation. A 20-residue peptide containing a His-tag was fused to the N-terminus of the connector protein gp10. This fusion neither interfered with procapsid assembly nor affected the morphology of the prolate-shaped procapsid. However, the pRNA binding and virion assembly activity were greatly reduced. Such decreased functions can be switched back on by the removal of the tag via protease cleavage, supporting the previous finding that the N-terminus of gp10 is essential for the pRNA binding. The DNA-packaging efficiency with dimeric pRNA was more seriously affected by the extension than with monomeric pRNA. It is speculated that the fusion of the tag generated physical hindrance to pRNA binding, with greater influence for the dimers than the monomers due to their size. These results reveal a potential to turn off and turn on the motor by attaching or removing, respectively, a component to outer part of the motor, and offers an approach for the inhibition of viral replication by using a drug or a small peptide targeted to motor components.
机译:噬菌体phi29利用马达将基因组DNA转移到预先形成的前壳体中。该马达包含6个pRNA,一种酶和一个12个亚基连接器,带有一个用于DNA转运的中央通道。将含有His标签的20个残基的肽融合到连接蛋白gp10的N端。这种融合既不会干扰衣壳的装配,也不会影响扁长形衣壳的形态。但是,pRNA结合和病毒体组装活性大大降低。可以通过通过蛋白酶切割去除标签来重新启动这种降低的功能,从而支持先前的发现,即gp10的N端对于pRNA结合至关重要。与单体pRNA相比,二聚体pRNA的DNA包装效率受到扩展的影响更大。据推测,标签的融合产生了对pRNA结合的物理障碍,由于其大小,对二聚体的影响比对单体的影响大。这些结果揭示了通过分别在电动机的外部连接或移除部件来关闭和打开电动机的潜力,并提供了一种通过使用针对电动机的药物或小肽来抑制病毒复制的方法组件。

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