Communications Biology (Dec 2024)

Quantitative single-molecule analysis of assembly and Ca2+-dependent disassembly of synaptotagmin oligomers on lipid bilayers

  • Feng Li,
  • Jeff Coleman,
  • Lorena Redondo-Morata,
  • R. Venkat Kalyana Sundaram,
  • Ekaterina Stroeva,
  • James E. Rothman,
  • Frédéric Pincet

DOI
https://doi.org/10.1038/s42003-024-07317-9
Journal volume & issue
Vol. 7, no. 1
pp. 1 – 14

Abstract

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Abstract Synaptotagmin-1 (Syt-1) self-assembles into ring-like oligomers, and genetic and biochemical evidence suggest that oligomerization is needed to clamp synaptic vesicles and stabilize them for Ca2+-evoked release. However, oligomerization has not yet been demonstrated on lipid bilayers or studied in quantitative biophysical terms. Here we utilize single-molecule imaging methods to monitor the assembly and disassembly of oligomeric clusters of Syt-1 on lipid bilayers in real-time. Syt-1 assembled into two distinct classes of oligomers, small (5 ± 2 subunits) and large (15 ± 2 subunits). Each class assembled at a constant k on that was always proportional to its ultimate size, but both classes disassembled at the same unit rate (k off ) independent of its size. Both large and small oligomers explosively disassembled when Ca2+ was added. The F349A mutation in the Syt-1 nearly eliminates the large class of oligomers but does not reduce the small class. Altogether, the physical-chemical properties of Syt-1 oligomers meet or exceed the physiologic requirements to function as such a clamp.