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Direct Visualization of Actin Filaments and Actin-Binding Proteins in Neuronal Cells

Authors
Jung, MinkyoKim, DooryMun, Ji Young
Issue Date
Nov-2020
Publisher
FRONTIERS MEDIA SA
Keywords
electron microscopy; super-resolution microscopy; correlative light and electron microscopy; actin binding protein; actin; neuronal cell
Citation
FRONTIERS IN CELL AND DEVELOPMENTAL BIOLOGY, v.8
Journal Title
FRONTIERS IN CELL AND DEVELOPMENTAL BIOLOGY
Volume
8
URI
http://scholarworks.bwise.kr/kbri/handle/2023.sw.kbri/567
DOI
10.3389/fcell.2020.588556
ISSN
2296-634X
Abstract
Actin networks and actin-binding proteins (ABPs) are most abundant in the cytoskeleton of neurons. The function of ABPs in neurons is nucleation of actin polymerization, polymerization or depolymerization regulation, bundling of actin through crosslinking or stabilization, cargo movement along actin filaments, and anchoring of actin to other cellular components. In axons, ABP-actin interaction forms a dynamic, deep actin network, which regulates axon extension, guidance, axon branches, and synaptic structures. In dendrites, actin and ABPs are related to filopodia attenuation, spine formation, and synapse plasticity. ABP phosphorylation or mutation changes ABP-actin binding, which regulates axon or dendritic plasticity. In addition, hyperactive ABPs might also be expressed as aggregates of abnormal proteins in neurodegeneration. Those changes cause many neurological disorders. Here, we will review direct visualization of ABP and actin using various electron microscopy (EM) techniques, super resolution microscopy (SRM), and correlative light and electron microscopy (CLEM) with discussion of important ABPs in neuron.
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연구본부 (신경회로 연구그룹)
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