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Flow Cytometry of the Side Population: Tips & Tricks

Background: The Side Population (SP) has become an important hallmark for the definition of the stem cell compartment, especially in the detection of these cells and in their physical isolation by fluorescence-activated cell sorting (FACS). SP cells are CD34(neg) and were discovered using ultraviole...

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Autores principales: Sales-Pardo, Irene, Avendaño, Ariadna, Martinez-Muñoz, Vanessa, García-Escarp, Marta, Celis, Raquel, Whittle, Phil, Barquinero, Jordi, Domingo, Joan Carles, Marin, Pedro, Petriz, Jordi
Formato: Online Artículo Texto
Lenguaje:English
Publicado: IOS Press 2006
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4617814/
https://www.ncbi.nlm.nih.gov/pubmed/16675880
http://dx.doi.org/10.1155/2006/536519
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author Sales-Pardo, Irene
Avendaño, Ariadna
Martinez-Muñoz, Vanessa
García-Escarp, Marta
Celis, Raquel
Whittle, Phil
Barquinero, Jordi
Domingo, Joan Carles
Marin, Pedro
Petriz, Jordi
author_facet Sales-Pardo, Irene
Avendaño, Ariadna
Martinez-Muñoz, Vanessa
García-Escarp, Marta
Celis, Raquel
Whittle, Phil
Barquinero, Jordi
Domingo, Joan Carles
Marin, Pedro
Petriz, Jordi
author_sort Sales-Pardo, Irene
collection PubMed
description Background: The Side Population (SP) has become an important hallmark for the definition of the stem cell compartment, especially in the detection of these cells and in their physical isolation by fluorescence-activated cell sorting (FACS). SP cells are CD34(neg) and were discovered using ultraviolet excitation based on the efflux of Hoechst 33342 (Ho342). Although the method works as originally described, we believe that this method is difficult for most investigators. First, because the ability to discriminate SP cells is based on the differential retention of Ho342 during a functional assay; second, because of the difficulties in setting the right experimental and acquisition conditions; and third, because the analysis of the acquired data requires an extensive expertise on flow cytometry to accurately detect the SP events. Methods: First of all and mainly for the SP application, the laser beam paths were exhaustively checked to ensure the lowest coefficients of variation. Blood suspensions were prepared by erythrocyte lysis with ammonium chloride and hematopoietic cells were labeled with Ho342. Results: The Ho342 concentration and the staining procedure are critical for the optimal resolution of the SP cells. Although UV laser alignment is very important to resolve the dim tail that outlines the SP, the problem with Ho342 excitation is not the Hoechst Blue emission, but rather the Hoechst Red's (because of the weak emission). Conclusions: Each laboratory must establish its own expected ranges based on its instrument and results may vary slightly due to instrument differences such as the narrowness of the band pass filters, laser power, laser emission wavelength, nozzle type, differential of pressure, light collection system (cuvette versus jet-in-air) and beam shaping optics.
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spelling pubmed-46178142016-01-12 Flow Cytometry of the Side Population: Tips & Tricks Sales-Pardo, Irene Avendaño, Ariadna Martinez-Muñoz, Vanessa García-Escarp, Marta Celis, Raquel Whittle, Phil Barquinero, Jordi Domingo, Joan Carles Marin, Pedro Petriz, Jordi Cell Oncol Other Background: The Side Population (SP) has become an important hallmark for the definition of the stem cell compartment, especially in the detection of these cells and in their physical isolation by fluorescence-activated cell sorting (FACS). SP cells are CD34(neg) and were discovered using ultraviolet excitation based on the efflux of Hoechst 33342 (Ho342). Although the method works as originally described, we believe that this method is difficult for most investigators. First, because the ability to discriminate SP cells is based on the differential retention of Ho342 during a functional assay; second, because of the difficulties in setting the right experimental and acquisition conditions; and third, because the analysis of the acquired data requires an extensive expertise on flow cytometry to accurately detect the SP events. Methods: First of all and mainly for the SP application, the laser beam paths were exhaustively checked to ensure the lowest coefficients of variation. Blood suspensions were prepared by erythrocyte lysis with ammonium chloride and hematopoietic cells were labeled with Ho342. Results: The Ho342 concentration and the staining procedure are critical for the optimal resolution of the SP cells. Although UV laser alignment is very important to resolve the dim tail that outlines the SP, the problem with Ho342 excitation is not the Hoechst Blue emission, but rather the Hoechst Red's (because of the weak emission). Conclusions: Each laboratory must establish its own expected ranges based on its instrument and results may vary slightly due to instrument differences such as the narrowness of the band pass filters, laser power, laser emission wavelength, nozzle type, differential of pressure, light collection system (cuvette versus jet-in-air) and beam shaping optics. IOS Press 2006 2006-04-28 /pmc/articles/PMC4617814/ /pubmed/16675880 http://dx.doi.org/10.1155/2006/536519 Text en Copyright © 2006 Hindawi Publishing Corporation and the authors.
spellingShingle Other
Sales-Pardo, Irene
Avendaño, Ariadna
Martinez-Muñoz, Vanessa
García-Escarp, Marta
Celis, Raquel
Whittle, Phil
Barquinero, Jordi
Domingo, Joan Carles
Marin, Pedro
Petriz, Jordi
Flow Cytometry of the Side Population: Tips & Tricks
title Flow Cytometry of the Side Population: Tips & Tricks
title_full Flow Cytometry of the Side Population: Tips & Tricks
title_fullStr Flow Cytometry of the Side Population: Tips & Tricks
title_full_unstemmed Flow Cytometry of the Side Population: Tips & Tricks
title_short Flow Cytometry of the Side Population: Tips & Tricks
title_sort flow cytometry of the side population: tips & tricks
topic Other
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4617814/
https://www.ncbi.nlm.nih.gov/pubmed/16675880
http://dx.doi.org/10.1155/2006/536519
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