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Merck

Imaging autophagy.

Current protocols in cytometry (2014-07-06)
Eleftherios Karanasios, Eloise Stapleton, Maria Manifava, Nicholas T Ktistakis
ABSTRACT

Autophagy is a membrane-trafficking pathway activated to deliver cytosolic material for degradation to lysosomes through a novel membrane compartment, the autophagosome. Fluorescence microscopy is the most common method used to visualize proteins inside cells, and it is widely used in the autophagy field. To distinguish it from the cellular background, the protein of interest (POI) is either fused with a genetically encoded fluorescent protein or stained with an antibody that is conjugated to an inorganic fluorescent compound. Genetic tagging of the POI allows its visualization in live cells, while immunostaining of the POI requires the fixation of cells and the permeabilization of cell membranes. Here we describe detailed protocols on how to visualize autophagy dynamics using fluorescence microscopy in live and fixed cells. We discuss the critical parameters of each technique, their advantages, and why the robustness is increased when they are used in tandem.

MATERIALS
Product Number
Brand
Product Description

Sigma-Aldrich
Anti-Atg13 Antibody, clone 2H4.2, clone 2H4.2, from mouse
Sigma-Aldrich
Anti-Atg101 antibody produced in rabbit, ~1.0 mg/mL, affinity isolated antibody
Sigma-Aldrich
Anti-ATG13 antibody produced in rabbit, ~1.0 mg/mL, affinity isolated antibody
Sigma-Aldrich
Anti-LC3B antibody produced in rabbit, ~1 mg/mL, affinity isolated antibody, buffered aqueous solution
Sigma-Aldrich
PP242 hydrate, ≥98% (HPLC), powder