Issue 8, 2017
From the journal:

Chemical Science

A flow cytometry assay to quantify intercellular exchange of membrane components

Dimitrios Poulcharidis, ORCID logo ab   Kimberley Belfor,a   Alexander Kros ORCID logo *b  and  Sander I. van Kasteren ORCID logo *a  

* Corresponding authors

a Division of Bio-organic Synthesis, Leiden Institute of Chemistry, Gorlaeus Laboratories, Leiden University, Leiden, The Netherlands
E-mail: s.i.van.kasteren@chem.leidenuniv.nl

b Division of Supramolecular and Biomaterials Chemistry, Leiden Institute of Chemistry, Leiden University, Einsteinweg 55, 2333 CC Leiden, The Netherlands
E-mail: a.kros@chem.leidenuniv.nl

Abstract

Membrane-compound exchange is vital for cell-to-cell communication, yet quantification of this process is difficult. Here we present a method using flow cytometry in combination with bioorthogonal and fluorescent labelling techniques to quantify the amount of exchange of cholesterol and sialylated compounds between cells. We demonstrate that direct cell–cell contact is the likely mechanism of sterol-exchange and show that by manipulating the contact time between cells using complementary coiled-coil peptides results in an enhanced exchange rate of membrane components between cells.

Graphical abstract: A flow cytometry assay to quantify intercellular exchange of membrane components

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Article information

DOI
https://doi.org/10.1039/C7SC00260B
Article type
Edge Article
Submitted
18 Jan 2017
Accepted
20 May 2017
First published
24 May 2017
This article is Open Access

All publication charges for this article have been paid for by the Royal Society of Chemistry
Creative Commons BY-NC license

Chem. Sci., 2017,8, 5585-5590

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A flow cytometry assay to quantify intercellular exchange of membrane components

D. Poulcharidis, K. Belfor, A. Kros and S. I. van Kasteren, Chem. Sci., 2017, 8, 5585 DOI: 10.1039/C7SC00260B

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