Maguire Michael F, Guinea Rosario, Griffin Philip, Macmanus Sarah, Elston Robert C, Wolfram Josie, Richards Naomi, Hanlon Mary H, Porter David J T, Wrin Terri, Parkin Neil, Tisdale Margaret, Furfine Eric, Petropoulos Chris, Snowden B Wendy, Kleim Jörg-Peter
Department of Clinical Virology, GlaxoSmithKline Research and Development, Stevenage SG1 2NY, United Kingdom.
J Virol. 2002 Aug;76(15):7398-406. doi: 10.1128/jvi.76.15.7398-7406.2002.
Human immunodeficiency virus type 1 (HIV-1) Gag protease cleavage sites (CS) undergo sequence changes during the development of resistance to several protease inhibitors (PIs). We have analyzed the association of sequence variation at the p7/p1 and p1/p6 CS in conjunction with amprenavir (APV)-specific protease mutations following PI combination therapy with APV. Querying a central resistance data repository resulted in the detection of significant associations (P < 0.001) between the presence of APV protease signature mutations and Gag L449F (p1/p6 LP1'F) and P453L (p1/p6 PP5'L) CS changes. In population-based sequence analyses the I50V mutant was invariably linked to either L449F or P453L. Clonal analysis revealed that both CS mutations were never present in the same genome. Sequential plasma samples from one patient revealed a transition from I50V M46L P453L viruses at early time points to I50V M46I L449F viruses in later samples. Various combinations of the protease and Gag mutations were introduced into the HXB2 laboratory strain of HIV-1. In both single- and multiple-cycle assay systems and in the context of I50V, the L449F and P453L changes consistently increased the 50% inhibitory concentration of APV, while the CS changes alone had no measurable effect on inhibitor sensitivity. The decreased in vitro fitness of the I50V mutant was only partially improved by addition of either CS change (I50V M46I L449F mutant replicative capacity approximately 16% of that of wild-type virus). Western blot analysis of Pr55 Gag precursor cleavage products from infected-cell cultures indicated accumulation of uncleaved Gag p1-p6 in all I50V viruses without coexisting CS changes. Purified I50V protease catalyzed cleavage of decapeptides incorporating the L449F or P453L change 10-fold and 22-fold more efficiently than cleavage of the wild-type substrate, respectively. HIV-1 protease CS changes are selected during PI therapy and can have effects on both viral fitness and phenotypic resistance to PIs.
1型人类免疫缺陷病毒(HIV-1)的Gag蛋白酶切割位点(CS)在对多种蛋白酶抑制剂(PI)产生耐药性的过程中会发生序列变化。我们分析了在与安普那韦(APV)联合进行PI治疗后,p7/p1和p1/p6 CS处的序列变异与APV特异性蛋白酶突变之间的关联。查询一个中心耐药性数据库后,发现APV蛋白酶特征性突变的存在与Gag的L449F(p1/p6 LP1'F)和P453L(p1/p6 PP5'L)CS变化之间存在显著关联(P < 0.001)。在基于群体的序列分析中,I50V突变体总是与L449F或P453L相关联。克隆分析表明,这两种CS突变从未同时出现在同一个基因组中。一名患者的连续血浆样本显示,在早期时间点为I50V M46L P453L病毒,而在后期样本中转变为I50V M46I L449F病毒。将蛋白酶和Gag突变的各种组合引入HIV-1的HXB2实验室菌株中。在单循环和多循环检测系统中,以及在I50V的背景下,L449F和P453L变化始终会增加APV的50%抑制浓度,而单独的CS变化对抑制剂敏感性没有可测量的影响。I50V突变体体外适应性的降低仅通过添加任何一种CS变化得到部分改善(I50V M46I L449F突变体的复制能力约为野生型病毒的16%)。对感染细胞培养物中Pr55 Gag前体切割产物的蛋白质印迹分析表明,在所有不存在共存CS变化的I50V病毒中,未切割的Gag p1-p6会积累。纯化的I50V蛋白酶催化切割包含L449F或P453L变化的十肽,其效率分别比切割野生型底物高10倍和22倍。HIV-1蛋白酶CS变化在PI治疗期间被选择,并且可能对病毒适应性和对PI类药物的表型耐药性都有影响。
