Banapour B, Marthas M L, Ramos R A, Lohman B L, Unger R E, Gardner M B, Pedersen N C, Luciw P A
Department of Medical Pathology, California Regional Primate Research Center, Davis.
J Virol. 1991 Nov;65(11):5798-805. doi: 10.1128/JVI.65.11.5798-5805.1991.
Simian immunodeficiency virus (SIV), a lymphocytopathic lentivirus, induces an AIDS-like disease in rhesus macaques (Macaca mulatta). A pathogenic molecular clone of rhesus macaque SIV (SIVmac), SIVmac-239, replicates and induces cytopathology in T lymphocytes but is restricted for replication in macrophages. In contrast, a nonpathogenic molecular clone of SIVmac, SIVmac-1A11, replicates and induces syncytia (multinucleated giant cells) in cultures of both T lymphocytes and macrophages. SIVmac-1A11 does not cause disease in macaques. To map the viral determinants of macrophage tropism, reciprocal recombinant genomes were constructed between molecular clones of SIVmac-239 and SIVmac-1A11. Infectious recombinant viruses were rescued by transfection of cloned viral genomes into permissive lymphoid cells. Analysis of one pair of reciprocal recombinants revealed that an internal 6.2-kb DNA fragment of SIVmac-1A11 was necessary and sufficient for both syncytium formation and efficient replication in macrophages. This region includes the coding sequences for a portion of the gag gene, all of the pol, vif, vpr, and vpx genes, the first coding exons of tat and rev, and the external env glycoprotein gp130. Thus, the transmembrane glycoprotein of env, the nef gene, the second coding exons of tat and rev, and the long terminal repeats are not essential for in vitro macrophage tropism. Analysis of additional recombinants revealed that syncytium formation, but not virus production, was controlled by a 1.4-kb viral DNA fragment in SIVmac-1A11 encoding only the external env glycoprotein gp130. Thus, gp130 env of SIVmac-1A11 is necessary for entry of virus into macrophages but is not sufficient for a complete viral replication cycle in this cell type. We therefore conclude that gp130 env and one or more genetic elements (exclusive of the long terminal repeats, transmembrane glycoprotein of env, and second coding exons of tat and rev, and nef) are essential for a complete replication cycle of SIVmac in rhesus macaque macrophages.
猴免疫缺陷病毒(SIV)是一种致淋巴细胞病变的慢病毒,可在恒河猴(猕猴)中引发类似艾滋病的疾病。恒河猴SIV(SIVmac)的致病分子克隆SIVmac - 239可在T淋巴细胞中复制并诱导细胞病变,但在巨噬细胞中的复制受到限制。相比之下,SIVmac的非致病分子克隆SIVmac - 1A11在T淋巴细胞和巨噬细胞培养物中均可复制并诱导形成多核巨细胞(合胞体)。SIVmac - 1A11不会在猕猴中引发疾病。为了确定病毒巨噬细胞嗜性的决定因素,在SIVmac - 239和SIVmac - 1A11的分子克隆之间构建了相互重组基因组。通过将克隆的病毒基因组转染到允许的淋巴细胞中拯救出有感染性的重组病毒。对一对相互重组体的分析表明,SIVmac - 1A11的一个6.2 kb内部DNA片段对于合胞体形成和在巨噬细胞中的有效复制是必需且充分的。该区域包括gag基因一部分的编码序列、所有的pol、vif、vpr和vpx基因、tat和rev的第一个编码外显子以及外膜糖蛋白gp130。因此,env的跨膜糖蛋白、nef基因、tat和rev的第二个编码外显子以及长末端重复序列对于体外巨噬细胞嗜性并非必需。对其他重组体的分析表明,合胞体形成而非病毒产生受SIVmac - 1A11中仅编码外膜糖蛋白gp130的一个1.4 kb病毒DNA片段控制。因此,SIVmac - 1A11的gp130 env对于病毒进入巨噬细胞是必需的,但对于该细胞类型中的完整病毒复制周期并不充分。我们因此得出结论,gp130 env和一个或多个遗传元件(不包括长末端重复序列、env的跨膜糖蛋白、tat和rev的第二个编码外显子以及nef)对于SIVmac在恒河猴巨噬细胞中的完整复制周期至关重要。
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