Analysis of synaptic vesicle endocytosis in synaptosomes by high-content screening

被引：39

作者：

Daniel, James A. ^{[1
]}

Malladi, Chandra S. ^{[2
]}

Kettle, Emma ^{[1
]}

McCluskey, Adam ^{[3
]}

Robinson, Phillip J. ^{[1
]}

机构：

[1] Univ Sydney, Childrens Med Res Inst, Cell Signalling Unit, Westmead, NSW 2145, Australia

[2] Univ Western Sydney, Sch Med, Dept Mol Physiol, Mol Med Res Grp, Penrith, NSW 1797, Australia

[3] Univ Newcastle, Dept Chem, Sch Environm & Life Sci, Callaghan, NSW 2308, Australia

来源：

NATURE PROTOCOLS | 2012年 / 7卷 / 08期

基金：

英国医学研究理事会;

关键词：

FROG NEUROMUSCULAR-JUNCTION; PERCOLL GRADIENT PROCEDURE; CLATHRIN-MEDIATED ENDOCYTOSIS; PIG BRAIN SYNAPTOSOMES; MOTOR-NERVE TERMINALS; WIDOW SPIDER VENOM; TRANSMITTER RELEASE; DYNAMIN-I; PLASMA-MEMBRANE; SUBCELLULAR-FRACTIONS;

D O I：

10.1038/nprot.2012.070

中图分类号：

Q5 [生物化学];

学科分类号：

070307 [化学生物学];

摘要：

Small molecules modulating synaptic vesicle endocytosis (SVE) may ultimately be useful for diseases where pathological neurotransmission is implicated. Only a small number of specific SVE modulators have been identified to date. Slow progress is due to the laborious nature of traditional approaches to study SVE, in which nerve terminals are identified and studied in cultured neurons, typically yielding data from 10-20 synapses per experiment. We provide a protocol for a quantitative, high-throughput method for studying SVE in thousands of nerve terminals. Rat forebrain synaptosomes are attached to 96-well microplates and depolarized; SVE is then quantified by uptake of the dye FM4-64, which is imaged by high-content screening. Synaptosomes that have been frozen and stored can be used in place of fresh synaptosomes, reducing the experimental time and animal numbers required. With a supply of frozen synaptosomes, the assay can be performed within a day, including data analysis.

引用

页码：1439 / 1455

页数：17

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