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Image-based Quantification of Macropinocytosis Using Dextran Uptake into Cultured Cells

Anh Le, Laura Machesky

2022BIO-PROTOCOL12 citationsDOIOpen Access PDF

Abstract

Macropinocytosis is an evolutionarily conserved process, which is characterized by the formation of membrane ruffles and the uptake of extracellular fluid. We recently demonstrated a role for CYFIP-related Rac1 Interactor (CYRI) proteins in macropinocytosis. High-molecular weight dextran (70kDa or higher) has generally been used as a marker for macropinocytosis because it is too large to fit in smaller endocytic vesicles, such as those of clathrin or caveolin-mediated endocytosis. Through the use of an image-based dextran uptake assay, we showed that cells lacking CYRI proteins internalise less dextran compared to their wild-type counterparts. Here, we will describe a step-by-step experimentation procedure to detect internalised dextran in cultured cells, and an image pipeline to analyse the acquired images, using the open-access software ImageJ/Fiji. This protocol is detailed yet simple and easily adaptable to different treatment conditions, and the analysis can also be automated for improved processing speed.

Topics & Concepts

PinocytosisDextranEndocytosisEndocytic cycleCell biologyChemistryBiochemistryCell cultureExtracellularBiologyIntracellularMembrane proteinMolecular biologyRAC1PhagocytosisClathrinYeastCentrifugationCellEndosomeCellular transport and secretionCaveolin-1 and cellular processesLipid Membrane Structure and Behavior
Image-based Quantification of Macropinocytosis Using Dextran Uptake into Cultured Cells | Litcius