首页> 美国卫生研究院文献>The Journal of Clinical Investigation >Liposome-mediated transfection of intact viral particles reveals that plasma membrane penetration determines permissivity of tissue culture cells to rotavirus.
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Liposome-mediated transfection of intact viral particles reveals that plasma membrane penetration determines permissivity of tissue culture cells to rotavirus.

机译:脂质体介导的完整病毒颗粒的转染表明质膜渗透决定了组织培养细胞对轮状病毒的介导性。

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摘要

Rotaviruses are an important cause of gastroenteritis in human infants. In vivo, rotavirus displays striking cell tropism with viral replication generally restricted to the villus tip enterocytes of the small intestine. We studied a panel of cell lines that vary significantly in their permissivity to rotavirus infection. L cells and HEp2 cells were relatively resistant to rotavirus infection compared with permissive Ma104 cells and HT29 cells. RNA transcription among the cell lines was proportional to antigen synthesis making a translational or posttranslational block an unlikely source of observed differences in susceptibility. All of the cell lines bound and internalized radiolabeled virus equally well, as measured by escape from surface protease treatment. Analysis of the escape of cell bound virus from neutralizing monoclonal antibody revealed that rotavirus did not immediately enter an eclipse phase in nonpermissive cells, but was internalized in an infectious form for several hours, possibly sequestered within endocytic vacuoles. L cells and HEp2 cells were as permissive as Ma104 and HT29 cells when rotavirus infection was mediated by transfection of single- or double-shelled rotavirus particles with cationic liposomes (Lipofectin). Rotavirus cell tropism in tissue culture cells is determined by the ability of infecting virions to traverse the plasma membrane of the cells into the cytoplasmic compartment.
机译:轮状病毒是人类婴儿胃肠炎的重要原因。在体内,轮状病毒表现出惊人的细胞嗜性,其病毒复制通常局限于小肠的绒毛尖端肠上皮细胞。我们研究了一组细胞系,它们对轮状病毒感染的允许率差异很大。与允许的Ma104细胞和HT29细胞相比,L细胞和HEp2细胞对轮状病毒感染具有相对抗性。细胞系之间的RNA转录与抗原合成成正比,使得翻译或翻译后阻滞不可能是观察到的敏感性差异的来源。如通过从表面蛋白酶处理中逃逸所测量的,所有细胞系均同样良好地结合并内化了放射性标记的病毒。分析细胞结合病毒从中和性单克隆抗体中逃逸的过程表明,轮状病毒不会立即在非许可细胞中进入蚀相阶段,而是会以感染性形式内化几个小时,可能被隔离在胞吞液泡中。当用阳离子脂质体(Lipofectin)转染单或双壳轮状病毒颗粒介导轮状病毒感染时,L细胞和HEp2细胞与Ma104和HT29细胞一样宽松。组织培养细胞中轮状病毒细胞的嗜性是由感染病毒粒子穿过细胞质膜进入细胞质区室的能力决定的。

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