Published: Vol 8, Iss 23, Dec 5, 2018 DOI: 10.21769/BioProtoc.3104 Views: 4311
Reviewed by: Ralph Thomas BoettcherPiyali SahaRAMESH KUDIRA
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Abstract
To enable cells to move forward, cell surface integrins are internalized into an endosomal compartment and subsequently intracellularly transported to be re-exposed at a new site on the cell membrane. Leukocytes are the fastest migrating cell type in the human body, which express the leukocyte-specific integrin LFA-1. Here, we describe a flow cytometry-based assay that allows the quantification of LFA-1 internalization and its re-expression on the cell surface in T lymphocytes. An advantage of using flow cytometry-based assay over biochemical methods is the low number of needed cells. This protocol can be also used to measure recycling of other receptors.
Keywords: Flow cytometryBackground
Leukocytes need to be quick to extravasate from the vascular in order to defeat invading pathogens. To become effector cells, T lymphocytes need to migrate in the lymph nodes where they can encounter their specific antigen (Ley et al., 2007). LFA-1, which is the major integrin used by T lymphocytes to adhere and migrate, binds to its ligand intercellular adhesion molecule-1 (ICAM-1) on the endothelial or the antigen presenting cell (Evans et al., 2009). The reuse of LFA-1 is a dynamic process as it is internalized and intracellularly transported to be re-exposed to a new sight on the cell membrane for the cell to move forward (Svensson et al., 2012). The lysosomotropic amine Primaquine can be used to block intracellular transport and when used in T cells LFA-1 dependent migration is impaired (Stanley et al., 2012). The exact mechanism how LFA-1 is internalized and recycled isn’t fully understood. One method to investigate the internalization and re-exposure of LFA-1 in low number of cells is to label cells with the non-blocking antibody for LFA-1 (TS-2) and analyze the internalization and re-exposure of LFA-1 at different time points by flow cytometry (Samuelsson et al., 2017).
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Acknowledgments
The protocol was adapted from Samuelsson et al. (2017). This work was supported by Swedish Research Council awards K2010-80P-21592-01-4 and K2010-80X-215917-01-4, Foundation Olle Engquist Byggmästare, I&A Lundberg Research Foundation, Royal Swedish Academy of science, Royal Physiographic Society of Lund, Åke Wiberg, Jeanssons Foundation, Kocks Foundation, P&U Schybergs Foundation, Gyllenstiernska Krapperup Foundation, Gustav V 80 Jubilee Fund, Österlund Foundation, Nanna Svartz and Crafoord awards (to LS). Anna-Greta Crafoord postdoctoral fellowship and Royal Physiographic Society of Lund (KP) and Royal Physiographic Society of Lund (MS).
Competing interests
The authors declare no competing interest.
References
Article Information
Publication history
Accepted: Oct 31, 2018
Published: Dec 5, 2018
Copyright
© 2018 The Authors; exclusive licensee Bio-protocol LLC.
How to cite
Potrzebowska, K., Lehtonen, J., Samuelsson, M. and Svensson, L. (2018). Flow Cytometry Assay for Recycling of LFA-1 in T-lymphocytes. Bio-protocol 8(23): e3104. DOI: 10.21769/BioProtoc.3104.
Category
Immunology > Immune cell staining > Flow cytometry
Cell Biology > Cell staining > Protein
Biochemistry > Protein > Immunodetection
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