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真核细胞对人乳头瘤病毒33型病毒样颗粒的结合与内化作用。

Binding and internalization of human papillomavirus type 33 virus-like particles by eukaryotic cells.

作者信息

Volpers C, Unckell F, Schirmacher P, Streeck R E, Sapp M

机构信息

Institut für Medizinische Mikrobiologie und Hygiene, Universität Mainz, Germany.

出版信息

J Virol. 1995 Jun;69(6):3258-64. doi: 10.1128/JVI.69.6.3258-3264.1995.

Abstract

Infection of cells by human papillomaviruses (HPVs) associated with malignant genital lesions has not been studied because of the lack of an in vitro system and the unavailability of virions. We have now used virus-like particles (VLPs) of HPV type 33 to analyze the initial events in the interaction of the HPV capsid with cell lines. Binding of VLPs to HeLa cells was observed in biochemical assays and by immunofluorescence. VLP binding was inhibited by antisera raised against VLPs but not by monoclonal antibodies recognizing either L1 or L2 epitopes accessible on VLPs. Under saturating conditions, approximately 2 x 10(4) VLPs were bound per cell, with a dissociation constant of about 100 pM. VLPs composed of L1 alone bound as well as VLPs composed of both capsid proteins, indicating that L2 is not required for initial binding. VLPs dissociated into capsomers did not bind, demonstrating that intercapsomer contacts are required. Neither capsomers nor simian virus 40 virions competed with VLP binding. Uptake of VLPs by small and smooth endocytic vesicles was demonstrated by immunoelectron microscopy. Cellular binding of VLPs was sensitive to trypsin but not to sialidase, N-glycosidase, or octyl-beta-D-glycopyranoside treatment, suggesting that a cell surface protein is involved in the VLP binding. Cell lines originating from a variety of tissues and organisms as distantly related as insects and humans bound VLPs with similar efficiency and specificity. Therefore, the putative receptor mediating VLP attachment should be highly conserved and cannot be responsible for the species and tissue specificity of HPVs.

摘要

由于缺乏体外系统且无法获得病毒粒子,与恶性生殖器病变相关的人乳头瘤病毒(HPV)对细胞的感染尚未得到研究。我们现在已使用33型HPV的病毒样颗粒(VLP)来分析HPV衣壳与细胞系相互作用的初始事件。在生化分析和免疫荧光实验中均观察到VLP与HeLa细胞的结合。抗VLP血清可抑制VLP结合,但识别VLP上可及的L1或L2表位的单克隆抗体则无此作用。在饱和条件下,每个细胞约结合2×10⁴个VLP,解离常数约为100 pM。仅由L1组成的VLP与由两种衣壳蛋白组成的VLP结合情况相同,这表明初始结合不需要L2。解离成衣壳粒的VLP不发生结合,这表明衣壳粒间的接触是必需的。衣壳粒和猴病毒40病毒粒子均不与VLP结合竞争。免疫电子显微镜显示VLP被小而光滑的内吞囊泡摄取。VLP的细胞结合对胰蛋白酶敏感,但对唾液酸酶、N-糖苷酶或辛基-β-D-吡喃葡萄糖苷处理不敏感,这表明细胞表面蛋白参与了VLP结合。源自各种组织和生物(如昆虫和人类等亲缘关系甚远的生物)的细胞系以相似的效率和特异性结合VLP。因此,介导VLP附着的假定受体应高度保守,且不能解释HPV的物种和组织特异性。

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