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包含鼠白血病病毒基质的嵌合型1型人类免疫缺陷病毒在鼠细胞中组装。

Chimeric human immunodeficiency virus type 1 containing murine leukemia virus matrix assembles in murine cells.

作者信息

Reed Margaret, Mariani Roberto, Sheppard Liana, Pekrun Katja, Landau Nathaniel R, Soong Nay-Wei

机构信息

Maxygen, Inc, Redwood City, California 94063, USA.

出版信息

J Virol. 2002 Jan;76(1):436-43. doi: 10.1128/jvi.76.1.436-443.2002.

Abstract

Murine cells do not support efficient assembly and release of human immunodeficiency virus type 1 (HIV-1) virions. HIV-1-infected mouse cells that express transfected human cyclin T1 synthesize abundant Gag precursor polyprotein, but inefficiently assemble and release virions. This assembly defect may result from a failure of the Gag polyprotein precursor to target to the cell membrane. Plasma membrane targeting of the precursor is mediated by the amino-terminal region of polyprotein. To compensate for the assembly block, we substituted the murine leukemia virus matrix coding sequences into an infectious HIV-1 clone. Transfection of murine fibroblasts expressing cyclin T1 with the chimeric proviruses resulted in viruses that were efficiently assembled and released. Chimeric viruses, in which the cytoplasmic tail of the transmembrane subunit, gp41, was truncated to prevent potential interference between the envelope glycoprotein and the heterologous matrix, could infect human and murine cells. They failed to further replicate in the murine cells, but replicated with delayed kinetics in human MT-4 cells. These findings may be useful for establishing a murine model for HIV-1 replication.

摘要

鼠细胞不支持1型人类免疫缺陷病毒(HIV-1)病毒粒子的高效组装和释放。表达转染人细胞周期蛋白T1的HIV-1感染的小鼠细胞能合成大量的Gag前体多聚蛋白,但病毒粒子的组装和释放效率低下。这种组装缺陷可能是由于Gag多聚蛋白前体未能靶向细胞膜所致。前体的细胞膜靶向由多聚蛋白的氨基末端区域介导。为了弥补组装障碍,我们将鼠白血病病毒基质编码序列替换到一个感染性HIV-1克隆中。用嵌合前病毒转染表达细胞周期蛋白T1的鼠成纤维细胞,产生了能高效组装和释放的病毒。在嵌合病毒中,跨膜亚基gp41的胞质尾巴被截断,以防止包膜糖蛋白与异源基质之间的潜在干扰,这种嵌合病毒能感染人和鼠细胞。它们在鼠细胞中无法进一步复制,但在人MT-4细胞中复制动力学延迟。这些发现可能有助于建立HIV-1复制的鼠模型。

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