Live cell imaging of LC3 dynamics

Giulia Cerrato; Allan Sauvat; Oliver Kepp; Guido Kroemer

doi:10.1016/bs.mcb.2020.10.003

Live cell imaging of LC3 dynamics

Giulia Cerrato, Allan Sauvat, Oliver Kepp, Guido Kroemer

Résultats de recherche: Le chapitre dans un livre, un rapport, une anthologie ou une collection › !!Chapter › Revue par des pairs

1 Citation (Scopus)

Résumé

Macroautophagy (hereafter referred to as autophagy) serves the liberation of energy resources through the degradation of cellular components and is characterized by the formation of double-membraned vesicles, commonly referred to as autophagosomes. Microtubule-associated proteins 1A/1B light chain 3B (hereafter referred to as LC3) plays a crucial role during autophagosome formation, as cleavage of its immature form and subsequent conjugation to phosphatidylethanolamine facilitates autophagosomal membrane biogenesis. Indeed, the redistribution of green fluorescent protein (GFP)-conjugated LC3 from a diffuse cytosolic pattern into forming autophagosomes constitutes a morphological phenotype (commonly referred to as LC3 puncta) applicable to phenotypic analysis. The quantification of LC3 puncta in end-point assays has extensively been used in the past, allowing for the identification of autophagy modulators. Here, we describe a robust method employing automated confocal live cell imaging for the study of time-resolved LC3 dynamics. Furthermore, this method can be used to differentiate between phenotypes such as the homogeneous distribution of LC3 puncta in the cytoplasm, and the aggregation of LC3 clusters juxtaposed to the nucleus thus allowing for functional predictions.

langue originale	Anglais
titre	Monitoring vesicular trafficking in cellular responses to stress - Part A
rédacteurs en chef	Oliver Kepp, Lorenzo Galluzzi
Editeur	Academic Press Inc.
Pages	27-38
Nombre de pages	12
ISBN (imprimé)	9780128235447
Les DOIs	https://doi.org/10.1016/bs.mcb.2020.10.003
état	Publié - 1 janv. 2021

Série de publications

Nom	Methods in Cell Biology
Volume	164
ISSN (imprimé)	0091-679X

Accès au document

10.1016/bs.mcb.2020.10.003

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abstract = "Macroautophagy (hereafter referred to as autophagy) serves the liberation of energy resources through the degradation of cellular components and is characterized by the formation of double-membraned vesicles, commonly referred to as autophagosomes. Microtubule-associated proteins 1A/1B light chain 3B (hereafter referred to as LC3) plays a crucial role during autophagosome formation, as cleavage of its immature form and subsequent conjugation to phosphatidylethanolamine facilitates autophagosomal membrane biogenesis. Indeed, the redistribution of green fluorescent protein (GFP)-conjugated LC3 from a diffuse cytosolic pattern into forming autophagosomes constitutes a morphological phenotype (commonly referred to as LC3 puncta) applicable to phenotypic analysis. The quantification of LC3 puncta in end-point assays has extensively been used in the past, allowing for the identification of autophagy modulators. Here, we describe a robust method employing automated confocal live cell imaging for the study of time-resolved LC3 dynamics. Furthermore, this method can be used to differentiate between phenotypes such as the homogeneous distribution of LC3 puncta in the cytoplasm, and the aggregation of LC3 clusters juxtaposed to the nucleus thus allowing for functional predictions.",

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Live cell imaging of LC3 dynamics. / Cerrato, Giulia; Sauvat, Allan; Kepp, Oliver et al.
Monitoring vesicular trafficking in cellular responses to stress - Part A. Ed. / Oliver Kepp; Lorenzo Galluzzi. Academic Press Inc., 2021. p. 27-38 (Methods in Cell Biology; Vol 164).

Résultats de recherche: Le chapitre dans un livre, un rapport, une anthologie ou une collection › !!Chapter › Revue par des pairs

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