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Novel tsg101 binding partners regulate viral l domain trafficking

  • Madeleine Strickland
  • , David Nyenhuis
  • , Susan M. Watanabe
  • , Nico Tjandra
  • , Carol A. Carter
  • National Institutes of Health
  • Stony Brook University

Research output: Contribution to journalReview articlepeer-review

11 Scopus citations

Abstract

Two decades ago, Tsg101, a component of the Endosomal Sorting Complexes Required for Transport (ESCRT) complex 1, was identified as a cellular factor recruited by the human immunodefi-ciency virus type 1 (HIV-1) to facilitate budding of viral particles assembled at the cell periphery. A highly conserved Pro-(Thr/Ser)-Ala-Pro [P(T/S)AP] motif in the HIV-1 structural polyprotein, Gag, engages a P(T/S)AP-binding pocket in the Tsg101 N-terminal domain. Since the same domain in Tsg101 that houses the pocket was found to bind mono-ubiquitin (Ub) non-covalently, Ub binding was speculated to enhance P(T/S)AP interaction. Within the past five years, we found that the Ub-binding site also accommodates di-Ub, with Lys63-linked di-Ub exhibiting the highest affinity. We also identified small molecules capable of disrupting Ub binding and inhibiting budding. The structural similarity of these molecules, prazoles, to nucleosides prompted testing for nucleic acid binding and led to identification of tRNA as a Tsg101 binding partner. Here, we discuss these recently identified interactions and their contribution to the viral assembly process. These new partners may provide additional insight into the control and function of Tsg101 as well as identify opportunities for anti-viral drug design.

Original languageEnglish
Article number1147
JournalViruses
Volume13
Issue number6
DOIs
StatePublished - Jun 2021

Keywords

  • Anti-viral
  • E2 enzyme
  • ESCRT
  • HIV-1
  • Herpesvirus
  • L do-main
  • Prazoles
  • RNA
  • Tsg101
  • UEV
  • Ubiquitin

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