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宿主细胞能量代谢对噬菌体PRD1 DNA进入的响应变化。

Changes in host cell energetics in response to bacteriophage PRD1 DNA entry.

作者信息

Daugelavicius R, Bamford J K, Bamford D H

机构信息

Department of Biosciences, Biocenter, University of Helsinki, Finland.

出版信息

J Bacteriol. 1997 Aug;179(16):5203-10. doi: 10.1128/jb.179.16.5203-5210.1997.

Abstract

Double-stranded DNA bacteriophage PRD1 infects a variety of gram-negative bacteria harboring an IncP-type conjugative plasmid. The plasmid codes for the DNA transfer phage receptor complex in the cell envelope. Our goal was, by using a collection of mutant phage particles for which the variables are the DNA content and/or the presence of the receptor-binding protein, to obtain information on the energy requirements for DNA entry as well as on alterations in the cellular energetics taking place during the first stages of infection. We studied the fluxes of tetraphenylphosphonium (TPP+), phenyldicarbaundecaborane (PCB-), and K+ ions as well as ATP through the envelope of Salmonella typhimurium cells. The final level of the membrane voltage (delta psi) indicator TPP+ accumulated by the infected cells exceeds the initial level before the infection. Besides the effects on TPP+ accumulation, PRD1 induces the leakage of ATP and K+ from the cytosol. All these events were induced only by DNA-containing infectious particles and were cellular ATP and delta psi dependent. PRD1-caused changes in delta psi and in PCB- binding differ considerably from those observed in other bacteriophage infections studied. These results are in accordance with the presence of a specific channel engaged in phage PRD1 DNA transport.

摘要

双链DNA噬菌体PRD1可感染多种携带IncP型接合质粒的革兰氏阴性菌。该质粒编码位于细胞包膜中的DNA转移噬菌体受体复合物。我们的目标是,通过使用一系列突变噬菌体颗粒(其变量为DNA含量和/或受体结合蛋白的存在情况),获取有关DNA进入的能量需求以及感染初期细胞能量学变化的信息。我们研究了四苯基鏻离子(TPP+)、苯基二碳硼烷(PCB-)和钾离子以及ATP通过鼠伤寒沙门氏菌细胞膜的通量。被感染细胞积累的膜电压(δψ)指示剂TPP+的最终水平超过感染前的初始水平。除了对TPP+积累的影响外,PRD1还会诱导ATP和钾离子从细胞质中泄漏。所有这些事件仅由含DNA的感染性颗粒诱导,并且依赖于细胞内的ATP和δψ。PRD1引起的δψ和PCB-结合变化与在其他研究的噬菌体感染中观察到的变化有很大不同。这些结果与存在参与噬菌体PRD1 DNA转运的特定通道一致。

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