Protocol to measure centrosome cohesion deficits mediated by pathogenic LRRK2 in cultured cells using confocal microscopy

Elena Fdez; Rachel Fasiczka; Antonio Jesús Lara Ordóñez; Belén Fernández; Yahaira Naaldijk; Sabine Hilfiker

doi:10.1016/j.xpro.2022.102024

Protocol to measure centrosome cohesion deficits mediated by pathogenic LRRK2 in cultured cells using confocal microscopy

Elena Fdez, Rachel Fasiczka, Antonio Jesús Lara Ordóñez, Belén Fernández, Yahaira Naaldijk, Sabine Hilfiker

New Jersey Medical School (NJMS), Anesthesiology

Research output: Contribution to journal › Article › peer-review

3 Scopus citations

Abstract

The present protocol allows for quantification of inter-centrosome distances in G2 phase cells by confocal fluorescence microscopy to determine centrosome cohesion deficits. We describe transfection and immunofluorescence approaches followed by image acquisition and analysis of inter-centrosome distances. This protocol is for adherent A549 cells transiently overexpressing pathogenic LRRK2 and for immortalized murine embryonic fibroblasts endogenously expressing LRRK2 but is amenable to any other cultured cell type as well. For complete details on the use and execution of this protocol, please refer to Fdez et al.¹ and Lara Ordóñez et al.²

Original language	English (US)
Article number	102024
Journal	STAR Protocols
Volume	4
Issue number	1
DOIs	https://doi.org/10.1016/j.xpro.2022.102024
State	Published - Mar 17 2023

All Science Journal Classification (ASJC) codes

General Neuroscience
General Biochemistry, Genetics and Molecular Biology
General Immunology and Microbiology

Keywords

Cell Biology
Cell Culture
Cell-based Assays
Microscopy

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10.1016/j.xpro.2022.102024

Cite this

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abstract = "The present protocol allows for quantification of inter-centrosome distances in G2 phase cells by confocal fluorescence microscopy to determine centrosome cohesion deficits. We describe transfection and immunofluorescence approaches followed by image acquisition and analysis of inter-centrosome distances. This protocol is for adherent A549 cells transiently overexpressing pathogenic LRRK2 and for immortalized murine embryonic fibroblasts endogenously expressing LRRK2 but is amenable to any other cultured cell type as well. For complete details on the use and execution of this protocol, please refer to Fdez et al.1 and Lara Ord{\'o}{\~n}ez et al.2",

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T1 - Protocol to measure centrosome cohesion deficits mediated by pathogenic LRRK2 in cultured cells using confocal microscopy

AU - Fdez, Elena

AU - Fasiczka, Rachel

AU - Lara Ordóñez, Antonio Jesús

AU - Fernández, Belén

AU - Naaldijk, Yahaira

AU - Hilfiker, Sabine

PY - 2023/3/17

Y1 - 2023/3/17

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AB - The present protocol allows for quantification of inter-centrosome distances in G2 phase cells by confocal fluorescence microscopy to determine centrosome cohesion deficits. We describe transfection and immunofluorescence approaches followed by image acquisition and analysis of inter-centrosome distances. This protocol is for adherent A549 cells transiently overexpressing pathogenic LRRK2 and for immortalized murine embryonic fibroblasts endogenously expressing LRRK2 but is amenable to any other cultured cell type as well. For complete details on the use and execution of this protocol, please refer to Fdez et al.1 and Lara Ordóñez et al.2

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KW - Cell Culture

KW - Cell-based Assays

KW - Microscopy

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Protocol to measure centrosome cohesion deficits mediated by pathogenic LRRK2 in cultured cells using confocal microscopy

Abstract

All Science Journal Classification (ASJC) codes

Keywords

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