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-Structure paper
| タイトル | Simulation-driven design of stabilized SARS-CoV-2 spike S2 immunogens. |
|---|---|
| ジャーナル・号・ページ | Nat Commun, Vol. 15, Issue 1, Page 7370, Year 2024 |
| 掲載日 | 2024年8月27日 |
著者 | Xandra Nuqui / Lorenzo Casalino / Ling Zhou / Mohamed Shehata / Albert Wang / Alexandra L Tse / Anupam A Ojha / Fiona L Kearns / Mia A Rosenfeld / Emily Happy Miller / Cory M Acreman / Surl-Hee Ahn / Kartik Chandran / Jason S McLellan / Rommie E Amaro / ![]() |
| PubMed 要旨 | The full-length prefusion-stabilized SARS-CoV-2 spike (S) is the principal antigen of COVID-19 vaccines. Vaccine efficacy has been impacted by emerging variants of concern that accumulate most of the ...The full-length prefusion-stabilized SARS-CoV-2 spike (S) is the principal antigen of COVID-19 vaccines. Vaccine efficacy has been impacted by emerging variants of concern that accumulate most of the sequence modifications in the immunodominant S1 subunit. S2, in contrast, is the most evolutionarily conserved region of the spike and can elicit broadly neutralizing and protective antibodies. Yet, S2's usage as an alternative vaccine strategy is hampered by its general instability. Here, we use a simulation-driven approach to design S2-only immunogens stabilized in a closed prefusion conformation. Molecular simulations provide a mechanistic characterization of the S2 trimer's opening, informing the design of tryptophan substitutions that impart kinetic and thermodynamic stabilization. Structural characterization via cryo-EM shows the molecular basis of S2 stabilization in the closed prefusion conformation. Informed by molecular simulations and corroborated by experiments, we report an engineered S2 immunogen that exhibits increased protein expression, superior thermostability, and preserved immunogenicity against sarbecoviruses. |
リンク | Nat Commun / PubMed:39191724 / PubMed Central |
| 手法 | EM (単粒子) |
| 解像度 | 2.8 Å |
| 構造データ | EMDB-43097, PDB-8vao: |
| 化合物 | ![]() ChemComp-NAG: |
| 由来 |
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キーワード | VIRAL PROTEIN / SARS-CoV-2 / spike protein / viral fusion / viral glycoprotein |
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