Membrane interaction and mechanism of LC3 lipidation machinery in autophagy – Raw GUV data

By Lisa Strong, BSc, Shanlin Rao, PhD and James Hurley
View Published Dataset

Output Details

Description
Raw GUV data of fluorescent protein imaged on a Nikon A1 confocal microscope with a 63 × Plan Apochromat 1.4 NA objective. Three biological replicates were performed for each experimental condition. Identical laser power and gain settings were used during the course of all conditions.
Identifier (DOI)
10.5281/zenodo.7988132
Tags
  • GUVs (Giant unilamellar vesicles)
  • Human
  • In Vitro
  • LC3 lipidation
  • Microscopy - optical
Team
Team Hurley
Program
Collaborative Research Network
Theme
PD Functional Genomics

Meet the Authors

  • Lisa Strong, BSc

    Key Personnel: Team Hurley

    University of California, Berkeley

  • User avatar fallback logo

    Shanlin Rao, PhD

    Key Personnel: Team Hurley

    Max Planck Institute of Biophysics

  • James Hurley

    Lead PI (Core Leadership): Team Hurley

    University of California, Berkeley

Related Research

Three-step docking by WIPI2, ATG16L1 and ATG3 delivers LC3 to the phagophore

In this manuscript, in a near-complete pathway from initial membrane recruitment to LC3 lipidation reaction, we show how a three-step targeting mechanism of the ATG12-ATG5-ATG16L1 machinery ensures a high level of regulatory control on autophagy.

View Article

GUV preparation

Protocol for GUV preparation for membrane tube assay application.

View Protocol

Surface Density Calculation

This protocol details Surface Density Calculation.

View Protocol
View More Outputs