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将重组前病毒DNA转染到培养细胞中后产生小鼠乳腺肿瘤病毒。

Production of mouse mammary tumor virus upon transfection of a recombinant proviral DNA into cultured cells.

作者信息

Salmons B, Groner B, Calberg-Bacq C M, Ponta H

出版信息

Virology. 1985 Jul 15;144(1):101-14. doi: 10.1016/0042-6822(85)90309-5.

DOI:10.1016/0042-6822(85)90309-5
PMID:2998037
Abstract

We have investigated the intracellular proteins synthesized in rat XC and feline kidney cells transfected with endogenous mouse mammary tumor virus (MMTV) proviral DNA. The endogenous provirus GR40, associated with the Mtv-8 locus, directs the synthesis of gag proteins indistinguishable from those found in MMTV-infected cells. The env precursor Pr73env and the mature gp52 proteins could not be detected in these cells. Instead an env-related protein of 68K is synthesized. In contrast to this endogenous provirus, a cloned exogenous proviral variant directs the synthesis of apparently normal env proteins upon transfection into the same cell lines. These results suggest that the env gene of the endogenous MMTV provirus GR40 is defective. The exogenous proviral variant is not expected to synthesize virus particles since it carries a rearrangement in the gag gene. In order to obtain an MMTV provirus capable of correctly expressing both gag and env functions, we have constructed a hybrid endogenous-exogenous provirus containing the 5' long terminal repeat (LTR)-gag of GR40 and the pol-env-3' LTR of the exogenous provirus. Upon transfection into feline kidney cells, this hybrid provirus directed the synthesis of apparently authentic gag and env proteins. Further, virus particles can be detected in the culture medium of the transfected cells by electron microscopy. Viral proteins obtained from viral particles banded in a sucrose gradient were detected by immunoprecipitation.

摘要

我们研究了用内源性小鼠乳腺肿瘤病毒(MMTV)前病毒DNA转染的大鼠XC细胞和猫肾细胞中合成的细胞内蛋白质。与Mtv-8基因座相关的内源性前病毒GR40指导合成与MMTV感染细胞中发现的gag蛋白无法区分的gag蛋白。在这些细胞中未检测到env前体Pr73env和成熟的gp52蛋白。相反,合成了一种68K的env相关蛋白。与这种内源性前病毒相反,一种克隆的外源性前病毒变体在转染到相同细胞系后指导合成明显正常的env蛋白。这些结果表明内源性MMTV前病毒GR40的env基因有缺陷。由于外源性前病毒变体在gag基因中发生了重排,预计它不会合成病毒颗粒。为了获得一种能够正确表达gag和env功能的MMTV前病毒,我们构建了一种杂交内源性-外源性前病毒,它包含GR40的5'长末端重复序列(LTR)-gag和外源性前病毒的pol-env-3'LTR。将这种杂交前病毒转染到猫肾细胞中后,它指导合成了明显真实的gag和env蛋白。此外,通过电子显微镜可以在转染细胞的培养基中检测到病毒颗粒。通过免疫沉淀检测从蔗糖梯度中条带化的病毒颗粒获得的病毒蛋白。

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