Dwyer John J, Wilson Karen L, Martin Kimberly, Seedorff Jennifer E, Hasan Aisha, Medinas Robyn J, Davison Donna K, Feese Michael D, Richter Hans-Thomas, Kim Hidong, Matthews Thomas J, Delmedico Mary K
Trimeris, Inc., Protein Engineering Group, Morrisville, North Carolina 27560, USA.
Protein Sci. 2008 Apr;17(4):633-43. doi: 10.1110/ps.073307608.
HIV fusion is mediated by a conformational transition in which the C-terminal region (HR2) of gp41 interacts with the N-terminal region (HR1) to form a six-helix bundle. Peptides derived from the HR1 form a well-characterized, trimeric coiled-coil bundle in the presence of HR2 peptides, but there is little structural information on the isolated HR1 trimer. Using protein design, we have designed synthetic HR1 peptides that form soluble, thermostable HR1 trimers. In vitro binding of HR2 peptides to the engineered trimer suggests that the design strategy has not significantly impacted the ability to form the six-helix bundle. The peptides have enhanced antiviral activity compared to wild type, with up to 30-fold greater potency against certain viral isolates. In vitro passaging was used to generate HR1-resistant virus and the observed resistance mutations map to the HR2 region of gp41, demonstrating that the peptides block the fusion process by binding to the viral HR2 domain. Interestingly, the activity of the HR2 fusion inhibitor, enfuvirtide (ENF), against these resistant viruses is maintained or improved up to fivefold. The 1.5 A crystal structure of one of these designs has been determined, and we show that the isolated HR1 is very similar to the conformation of the HR1 in the six-helix bundle. These results provide an initial model of the pre-fusogenic state, are attractive starting points for identifying novel fusion inhibitors, and offer new opportunities for developing HIV therapeutics based on HR1 peptides.
HIV融合由一种构象转变介导,其中gp41的C末端区域(HR2)与N末端区域(HR1)相互作用形成六螺旋束。在存在HR2肽的情况下,源自HR1的肽形成了一种特征明确的三聚体卷曲螺旋束,但关于分离的HR1三聚体的结构信息很少。通过蛋白质设计,我们设计了能够形成可溶性、热稳定的HR1三聚体的合成HR1肽。HR2肽与工程化三聚体的体外结合表明,该设计策略并未显著影响形成六螺旋束的能力。与野生型相比,这些肽具有增强的抗病毒活性,对某些病毒分离株的效力提高了30倍。体外传代用于产生对HR1耐药的病毒,观察到的耐药突变定位在gp41的HR2区域,这表明这些肽通过与病毒HR2结构域结合来阻断融合过程。有趣的是,HR2融合抑制剂恩夫韦肽(ENF)对这些耐药病毒的活性保持不变或提高了五倍。已确定其中一种设计的1.5埃晶体结构,我们表明分离的HR1与六螺旋束中HR1的构象非常相似。这些结果提供了融合前状态的初始模型,是识别新型融合抑制剂的有吸引力的起点,并为基于HR1肽开发HIV治疗药物提供了新机会。