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小鼠MusD逆转座子:一种“细胞内化”逆转录病毒的结构与分子进化

Murine MusD retrotransposon: structure and molecular evolution of an "intracellularized" retrovirus.

作者信息

Ribet David, Harper Francis, Dewannieux Marie, Pierron Gérard, Heidmann Thierry

机构信息

Unité des Rétrovirus Endogènes et Eléments Rétroïdes des Eucaryotes Supérieurs, UMR 8122 CNRS, Institut Gustave Roussy, 39 Rue Camille Desmoulins, 94805 Villejuif Cedex, France.

出版信息

J Virol. 2007 Feb;81(4):1888-98. doi: 10.1128/JVI.02051-06. Epub 2006 Dec 6.

Abstract

We had previously identified active autonomous copies of the MusD long terminal repeat-retrotransposon family, which have retained transpositional activity. These elements are closely related to betaretroviruses but lack an envelope (env) gene. Here we show that these elements encode strictly intracellular virus-like particles that can unambiguously be identified by electron microscopy. We demonstrate intracellular maturation of the particles, with a significant proportion of densely packed cores for wild-type MusD but not for a protease mutant. We show that the molecular origin of this unexpected intracellular localization is solely dependent on the N-terminal part of the Gag protein, which lacks a functional sequence for myristoylation and plasma membrane targeting: replacement of the N-terminal domain of the MusD matrix protein by that of its closest relative-the Mason-Pfizer monkey virus-led to targeting of the MusD Gag to the plasma membrane, with viral particles budding and being released into the cell supernatant. These particles can further be pseudotyped with a heterologous envelope protein and become infectious, thus "reconstituting" a functional retrovirus prone to proviral insertions. Consistent with its retroviral origin, a sequence with a constitutive transport element-like activity can further be identified at the MusD 3' untranslated region. A molecular scenario is proposed that accounts for the transition, during evolution, from an ancestral infectious betaretrovirus to the strictly intracellular MusD retrotransposon, involving not only the loss of the env gene but also an inability to escape the cell--via altered targeting of the Gag protein--resulting de facto in the generation of a very successful "intracellularized" insertional mutagen.

摘要

我们之前鉴定出了MusD长末端重复逆转录转座子家族的活性自主拷贝,这些拷贝保留了转座活性。这些元件与β逆转录病毒密切相关,但缺少包膜(env)基因。在这里,我们表明这些元件编码严格的细胞内病毒样颗粒,通过电子显微镜可以明确识别。我们证明了颗粒在细胞内的成熟过程,野生型MusD有很大比例的致密堆积核心,而蛋白酶突变体则没有。我们表明,这种意外的细胞内定位的分子起源仅取决于Gag蛋白的N端部分,该部分缺乏肉豆蔻酰化和质膜靶向的功能序列:用其最密切相关的梅森- Pfizer猴病毒的N端结构域取代MusD基质蛋白的N端结构域,导致MusD Gag靶向质膜,病毒颗粒出芽并释放到细胞上清液中。这些颗粒可以进一步用异源包膜蛋白进行假型化并具有感染性,从而“重建”一种易于前病毒插入的功能性逆转录病毒。与其逆转录病毒起源一致,在MusD 3'非翻译区可以进一步鉴定出具有组成型转运元件样活性的序列。我们提出了一种分子假说,解释了在进化过程中从祖先感染性β逆转录病毒到严格细胞内的MusD逆转录转座子的转变,这不仅涉及env基因的丢失,还涉及无法通过改变Gag蛋白的靶向作用逃离细胞,事实上导致了一种非常成功的“细胞内化”插入诱变剂的产生。

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