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Specificity of Plasma Membrane Targeting by the Rous Sarcoma Virus Gag Protein

机译:劳斯肉瘤病毒gag蛋白靶向血浆膜的特异性

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摘要

Budding of C-type retroviruses begins when the viral Gag polyprotein is directed to the plasma membrane by an N-terminal membrane-binding (M) domain. While dispersed basic amino acids within the M domain are critical for stable membrane association and consequent particle assembly, additional residues or motifs may be required for specific plasma membrane targeting and binding. We have identified an assembly-defective Rous sarcoma virus (RSV) Gag mutant that retains significant membrane affinity despite having a deletion of the fourth alpha-helix of the M domain. Examination of the mutant protein's subcellular distribution revealed that it was not localized to the plasma membrane but instead was mistargeted to intracytoplasmic membranes. Specific plasma membrane targeting was restored by the addition of myristate plus a single basic residue, by multiple basic residues, or by the heterologous hydrophobic membrane-binding domain from the cellular Fyn protein. These results suggest that the fourth alpha-helix of the RSV M domain promotes specific targeting of Gag to the plasma membrane, either through a direct interaction with plasma membrane phospholipids or a membrane-associated cellular factor or by maintaining the conformation of Gag to expose specific plasma membrane targeting sequences.
机译:当病毒Gag多蛋白通过N端膜结合(M)域导向质膜时,C型逆转录病毒开始萌芽。尽管在M结构域内分散的碱性氨基酸对于稳定的膜缔合和随后的颗粒组装至关重要,但特定质膜的靶向和结合可能还需要其他残基或基序。我们已经确定了一个装配缺陷的劳斯肉瘤病毒(RSV)Gag突变体,尽管该突变体保留了M结构域的第四个α-螺旋,但仍保留了明显的膜亲和力。检查突变蛋白的亚细胞分布表明,它不局限于质膜,而是被错误地靶向了细胞质膜。通过添加肉豆蔻酸酯加上单个碱性残基,多个碱性残基或细胞Fyn蛋白的异源疏水膜结合结构域,可以恢复特定的质膜靶向。这些结果表明,RSV M结构域的第四个α螺旋通过与质膜磷脂或与膜相关的细胞因子直接相互作用或通过维持Gag构象以暴露特异性,从而促进Gag对质膜的特异性靶向。质膜靶向序列。

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