A sequestered fusion peptide in the structure of an HIV-1 transmitted founder envelope trimer

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作者
Neeti Ananthaswamy
Qianglin Fang
Wadad AlSalmi
Swati Jain
Zhenguo Chen
Thomas Klose
Yingyuan Sun
Yue Liu
Marthandan Mahalingam
Subhash Chand
Sodsai Tovanabutra
Merlin L. Robb
Michael G. Rossmann
Venigalla B. Rao
机构
[1] The Catholic University of America,Department of Biology
[2] Purdue University,Department of Biological Sciences
[3] Henry M. Jackson Foundation for the Advancement of Military Medicine,U.S. Military HIV Research Program
[4] Fudan University,The Fifth People’s Hospital of Shanghai & Institutes of Biomedical Sciences
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The envelope protein of human immunodeficiency virus-1 (HIV-1) and its fusion peptide are essential for cell entry and vaccine design. Here, we describe the 3.9-Å resolution structure of an envelope protein trimer from a very early transmitted founder virus (CRF01_AE T/F100) complexed with Fab from the broadly neutralizing antibody (bNAb) 8ANC195. The overall T/F100 trimer structure is similar to other reported “closed” state prefusion trimer structures. In contrast, the fusion peptide, which is exposed to solvent in reported closed structures, is sequestered (buried) in the hydrophobic core of the T/F100 trimer. A buried conformation has previously been observed in “open” state structures formed after CD4 receptor binding. The T/F100 trimer binds poorly to bNAbs including the fusion peptide-specific bNAbs PGT151 and VRC34.01. The T/F100 structure might represent a prefusion state, intermediate between the closed and open states. These observations are relevant to mechanisms of HIV-1 transmission and vaccine design.
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