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Targeted mutagenesis of the P22 portal protein reveals the mechanism of signal transmission during DNA packaging

机译:P22门耳蛋白的靶向诱变揭示了DNA包装期间信号传输的机制

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摘要

The portal vertex in dsDNA bacteriophage serves as the site for genome encapsidation and release. In several of these viruses, efficient termination of DNA packaging has been shown to be dependent on the density of packaged DNA. The portal protein has been implicated as being part of the sensor that regulates packaging termination through DNA-dependent conformational changes during packaging. The mechanism by which DNA induces these conformational changes remains unknown. In this study, we explore how point mutants in the portal core can result in changes in genome packaging density in P22. Mutations in the portal core that subtly alter the structure or dynamics of the protein result in an increase in the amount of DNA packaged. The magnitude of the change is amino acid and location specific. Our findings suggest a mechanism wherein compression of the portal core is an essential aspect of signal transmission during packaging.
机译:DSDNA噬菌体中的门瓣顶点用作基因组封装和释放的部位。 在这些病毒中的几种中,已显示DNA包装的有效终止依赖于包装DNA的密度。 门耳蛋白已涉及作为通过在包装期间通过DNA依赖性构象变化调节包装终止的传感器的一部分。 DNA诱导这些构象变化的机制仍然是未知的。 在这项研究中,我们探讨了门芯中的点突变体如何导致P22中基因组包装密度的变化。 门芯中的突变细微改变蛋白质的结构或动态导致包装的DNA的量增加。 变化的大小是氨基酸和位置特异性。 我们的研究结果表明了一种机构,其中门户核心的压缩是包装期间信号传输的必要方面。

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