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Literature DB >> 27768059

Determination of the Relative Cell Surface and Total Expression of Recombinant Ion Channels Using Flow Cytometry.

Benoîte Bourdin¹, Emilie Segura¹, Marie-Philippe Tétreault¹, Sylvie Lesage², Lucie Parent³.

Abstract

Inherited or de novo mutations in cation-selective channels may lead to sudden cardiac death. Alteration in the plasma membrane trafficking of these multi-spanning transmembrane proteins, with or without change in channel gating, is often postulated to contribute significantly in this process. It has thus become critical to develop a method to quantify the change of the relative cell surface expression of cardiac ion channels on a large scale. Herein, a detailed protocol is provided to determine the relative total and cell surface expression of cardiac L-type calcium channels CaV1.2 and membrane-associated subunits in tsA-201 cells using two-color fluorescent cytometry assays. Compared with other microscopy-based or immunoblotting-based qualitative methods, flow cytometry experiments are fast, reproducible, and large-volume assays that deliver quantifiable end-points on large samples of live cells (ranging from 104 to 106 cells) with similar cellular characteristics in a single flow. Constructs were designed to constitutively express mCherry at the intracellular C-terminus (thus allowing a rapid assessment of the total protein expression) and express an extracellular-facing hemagglutinin (HA) epitope to estimate the cell surface expression of membrane proteins using an anti-HA fluorescence conjugated antibody. To avoid false negative, experiments were also conducted in permeabilized cells to confirm the accessibility and proper expression of the HA epitope. The detailed procedure provides: (1) design of tagged DNA (deoxyribonucleic acid) constructs, (2) lipid-mediated transfection of constructs in tsA-201 cells, (3) culture, harvest, and staining of non-permeabilized and permeabilized cells, and (4) acquisition and analysis of fluorescent signals. Additionally, the basic principles of flow cytometry are explained and the experimental design, including the choice of fluorophores, titration of the HA antibody and control experiments, is thoroughly discussed. This specific approach offers objective relative quantification of the total and cell surface expression of ion channels that can be extended to study ion pumps and plasma membrane transporters.

Entities: Chemical Disease Gene

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Year: 2016 PMID： 27768059 PMCID： PMC5092078 DOI： 10.3791/54732

Source DB: PubMed Journal: J Vis Exp ISSN： 1940-087X Impact factor: 1.355

39 in total

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Journal: Circ Cardiovasc Genet Date: 2016-01-22

10. A CACNA1C variant associated with reduced voltage-dependent inactivation, increased CaV1.2 channel window current, and arrhythmogenesis.

Authors: Jessica A Hennessey; Nicole J Boczek; Yong-Hui Jiang; Joelle D Miller; William Patrick; Ryan Pfeiffer; Brittan S Sutphin; David J Tester; Hector Barajas-Martinez; Michael J Ackerman; Charles Antzelevitch; Ronald Kanter; Geoffrey S Pitt
Journal: PLoS One Date: 2014-09-03 Impact factor: 3.240

5 in total

1. A three-way inter-molecular network accounts for the Ca_Vα2δ1-induced functional modulation of the pore-forming Ca_V1.2 subunit.

Authors: Julie Briot; Olivier Mailhot; Benoîte Bourdin; Marie-Philippe Tétreault; Rafael Najmanovich; Lucie Parent
Journal: J Biol Chem Date: 2018-03-27 Impact factor: 5.157

2. Proteolytic cleavage of the hydrophobic domain in the Ca_Vα2δ1 subunit improves assembly and activity of cardiac Ca_V1.2 channels.

Authors: Emilie Segura; Benoîte Bourdin; Marie-Philippe Tétreault; Julie Briot; Bruce G Allen; Gaétan Mayer; Lucie Parent
Journal: J Biol Chem Date: 2017-05-11 Impact factor: 5.157

3. Calcium-regulatory proteins as modulators of chemotherapy in human neuroblastoma.

Authors: Ana-Maria Florea; Elizabeth Varghese; Jennifer E McCallum; Safa Mahgoub; Irfan Helmy; Sharon Varghese; Neha Gopinath; Steffen Sass; Fabian J Theis; Guido Reifenberger; Dietrich Büsselberg
Journal: Oncotarget Date: 2017-04-04

4. Tracking the motion of the K_V 1.2 voltage sensor reveals the molecular perturbations caused by a de novo mutation in a case of epilepsy.

Authors: Antonios Pantazis; Maki Kaneko; Marina Angelini; Federica Steccanella; Annie M Westerlund; Sarah H Lindström; Michelle Nilsson; Lucie Delemotte; Sulagna C Saitta; Riccardo Olcese
Journal: J Physiol Date: 2020-09-21 Impact factor: 5.182

5. Negatively charged residues in the first extracellular loop of the L-type Ca_V1.2 channel anchor the interaction with the Ca_Vα2δ1 auxiliary subunit.

Authors: Benoîte Bourdin; Julie Briot; Marie-Philippe Tétreault; Rémy Sauvé; Lucie Parent
Journal: J Biol Chem Date: 2017-09-01 Impact factor: 5.157

5 in total