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小鼠乳腺肿瘤细胞对小鼠乳腺肿瘤病毒(MuMTV)包膜基因产物的表达与分布

Expression and disposition of the murine mammary tumor virus (MuMTV) envelope gene products by murine mammary tumor cells.

作者信息

Sarkar N H, Racevskis J

出版信息

Virology. 1983 Apr 15;126(1):279-300. doi: 10.1016/0042-6822(83)90479-8.

DOI:10.1016/0042-6822(83)90479-8
PMID:6302986
Abstract

Three murine mammary tumor virus (MuMTV)-producing epithelial cell lines derived from murine mammary tumors were examined in order to identify the MuMTV-specific cell surface antigens and their distribution on the cell surface, to study the kinetics of the MuMTV envelope precursor processing, virus assembly, and release, and to characterize the soluble MuMTV antigens that are shed into culture medium. Cell surface labeling experiments showed that only the mature MuMTV envelope glycoproteins gp52 and gp36 were exposed on the cell surface, and that gp52 was more abundant than gp36. In cells producing large quantities of MuMTV, expression of gp52 on the cell surface was shown by immunoelectron microscopy to be localized predominantly on the surface of budding virions and not on smooth areas of the cell surface where virus was not budding. The cell surface associated gp36 was found not to be incorporated into budding virions. A few cells in all three cell lines were found to produce only a few or no MuMTV particles and in these cells, unlike in the high virus-producing cells, considerable quantities of gp52 were expressed on the surface membrane. All three cell lines were found to shed large amounts of the MuMTV env precursor polyprotein as well as the mature non-virion-associated glycoprotein, gp52, into the culture medium. The envelope precursor protein (P75env) that was shed into the culture medium was found to differ from the predominant form of the cellular env precursor (Pr70env) in that (1) P75env migrated with an apparent higher molecular weight than Pr70env in SDS gels; (2) Pr70env contained only the core oligosaccharide, whereas P75env contained fucose in addition to the core sugars; (3) two-dimensional gel electrophoretic analysis showed that Pr70env could be resolved into three to four components migrating in the basic region of the isoelectric focussing gel (pH 7-8), whereas P75env was resolved into 9-13 components migrating in a more acidic region of the gel (pH 5-7). The molecular structure of the exfoliated gp52 was found to be similar to that of the gp52 that was incorporated into the virions although the virion-associated gp52 was not the source of the gp52 in the medium. Our quantitative pulse-chase studies suggest that of the two populations of MuMTV env precursors that are present in MuMTV-producing cells, only Pr70env is processed intracellularly to give rise to the mature MuMTV envelope proteins gp52 and gp36.

摘要

为了鉴定小鼠乳腺肿瘤病毒(MuMTV)特异性细胞表面抗原及其在细胞表面的分布,研究MuMTV包膜前体加工、病毒组装和释放的动力学,并表征分泌到培养基中的可溶性MuMTV抗原,对三种源自小鼠乳腺肿瘤的产生MuMTV的上皮细胞系进行了检测。细胞表面标记实验表明,只有成熟的MuMTV包膜糖蛋白gp52和gp36暴露在细胞表面,且gp52比gp36更丰富。在大量产生MuMTV的细胞中,免疫电子显微镜显示细胞表面gp52的表达主要定位于出芽病毒粒子的表面,而非病毒未出芽的细胞表面光滑区域。发现细胞表面相关的gp36未被整合到出芽病毒粒子中。在所有三种细胞系中,发现少数细胞仅产生少量或不产生MuMTV颗粒,与高病毒产生细胞不同,在这些细胞的表面膜上表达了相当数量的gp52。发现所有三种细胞系都将大量的MuMTV env前体多蛋白以及成熟的非病毒相关糖蛋白gp52分泌到培养基中。分泌到培养基中的包膜前体蛋白(P75env)与细胞env前体(Pr70env)的主要形式不同,在于:(1)在SDS凝胶中,P75env迁移时的表观分子量高于Pr70env;(2)Pr70env仅含有核心寡糖,而P75env除核心糖外还含有岩藻糖;(3)二维凝胶电泳分析表明,Pr70env可解析为在等电聚焦凝胶碱性区域(pH 7 - 8)迁移的三到四个组分,而P75env可解析为在凝胶酸性更强区域(pH 5 - 7)迁移的9 - 13个组分。发现脱落的gp52的分子结构与整合到病毒粒子中的gp52相似,尽管病毒粒子相关的gp52不是培养基中gp52的来源。我们的定量脉冲追踪研究表明,在产生MuMTV的细胞中存在的两种MuMTV env前体群体中,只有Pr70env在细胞内被加工产生成熟的MuMTV包膜蛋白gp52和gp36。

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引用本文的文献

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