A High Precision Survey of the Molecular Dynamics of Mammalian Clathrin-Mediated Endocytosis

被引:592
作者
Taylor, Marcus J. [1 ]
Perrais, David [2 ,3 ]
Merrifield, Christien J. [1 ]
机构
[1] MRC, Mol Biol Lab, Cambridge CB2 2QH, England
[2] Univ Bordeaux, Interdisciplinary Inst Neurosci, UMR 5297, Bordeaux, France
[3] CNRS, Interdisciplinary Inst Neurosci, UMR 5297, Bordeaux, France
基金
英国医学研究理事会;
关键词
ACTIN-BINDING PROTEIN; COATED PITS; DIFFERENTIAL REQUIREMENTS; MEMBRANE INVAGINATION; VESICLE FORMATION; MONOMERIC RED; BAR DOMAINS; RECRUITMENT; CYTOSKELETON; COFILIN;
D O I
10.1371/journal.pbio.1000604
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
070307 [化学生物学]; 071010 [生物化学与分子生物学];
摘要
Dual colour total internal reflection fluorescence microscopy is a powerful tool for decoding the molecular dynamics of clathrin-mediated endocytosis (CME). Typically, the recruitment of a fluorescent protein-tagged endocytic protein was referenced to the disappearance of spot-like clathrin-coated structure (CCS), but the precision of spot-like CCS disappearance as a marker for canonical CME remained unknown. Here we have used an imaging assay based on total internal reflection fluorescence microscopy to detect scission events with a resolutionof similar to 2 s. We found that scission events engulfed comparable amounts of transferrin receptor cargo at CCSs of different sizes and CCS did not always disappear following scission. We measured the recruitment dynamics of 34 types of endocytic protein to scission events: Abp1, ACK1, amphiphysin1, APPL1, Arp3, BIN1, CALM, CIP4, clathrin light chain (Clc), cofilin, coronin1B, cortactin, dynamin1/2, endophilin2, Eps15, Eps8, epsin2, FBP17, FCHo1/2, GAK, Hip1R, lifeAct, mu2 subunit of the AP2 complex, myosin1E, myosin6, NECAP, N-WASP, OCRL1, Rab5, SNX9, synaptojanin2 beta 1, and syndapin2. For each protein we aligned similar to 1,000 recruitment profiles to their respective scission events and constructed characteristic "recruitment signatures" that were grouped, as for yeast, to reveal the modular organization of mammalian CME. A detailed analysis revealed the unanticipated recruitment dynamics of SNX9, FBP17, and CIP4 and showed that the same set of proteins was recruited, in the same order, to scission events at CCSs of different sizes and lifetimes. Collectively these data reveal the fine-grained temporal structure of CME and suggest a simplified canonical model of mammalian CME in which the same core mechanism of CME, involving actin, operates at CCSs of diverse sizes and lifetimes.
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页数:23
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