A Chemical Controller of SNARE-Driven Membrane Fusion That Primes Vesicles for Ca(2+)-Triggered Millisecond Exocytosis.

J Am Chem Soc

Department of Genetic Engineering, College of Biotechnology and Bioengineering, and Center for Human Interface Nano Technology, Sungkyunkwan University, Suwon, Gyeonggi-do 440-746, South Korea.

Published: April 2016

AI Article Synopsis

  • Membrane fusion involves the SNARE complex, which acts like a zipper to bring membranes together, and researchers developed a chemical controller using myricetin to pause this process.
  • Enzyme laccase can remove myricetin from the SNARE complex, allowing a hemifusion state to resume, which lasts about 39 minutes.
  • The study showed that with the right priming using myricetin and calcium, vesicles can fuse rapidly in milliseconds, indicating the potential of this approach to explore how different proteins influence membrane fusion.

Article Abstract

Membrane fusion is mediated by the SNARE complex which is formed through a zippering process. Here, we developed a chemical controller for the progress of membrane fusion. A hemifusion state was arrested by a polyphenol myricetin which binds to the SNARE complex. The arrest of membrane fusion was rescued by an enzyme laccase that removes myricetin from the SNARE complex. The rescued hemifusion state was metastable and long-lived with a decay constant of 39 min. This membrane fusion controller was applied to delineate how Ca(2+) stimulates fusion-pore formation in a millisecond time scale. We found, using a single-vesicle fusion assay, that such myricetin-primed vesicles with synaptotagmin 1 respond synchronously to physiological concentrations of Ca(2+). When 10 μM Ca(2+) was added to the hemifused vesicles, the majority of vesicles rapidly advanced to fusion pores with a time constant of 16.2 ms. Thus, the results demonstrate that a minimal exocytotic membrane fusion machinery composed of SNAREs and synaptotagmin 1 is capable of driving membrane fusion in a millisecond time scale when a proper vesicle priming is established. The chemical controller of SNARE-driven membrane fusion should serve as a versatile tool for investigating the differential roles of various synaptic proteins in discrete fusion steps.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4852477PMC
http://dx.doi.org/10.1021/jacs.5b13449DOI Listing

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