A synthetic method to assay polycystin channel biophysics

Author:

Larmore Megan1,Palomero Orhi Esarte1,Kamat Neha P23,DeCaen Paul G134ORCID

Affiliation:

1. Department of Pharmacology, Feinberg School of Medicine, Northwestern University

2. Department of Biomedical Engineering, McCormick School of Engineering and Applied Science, Northwestern University

3. Center for Synthetic Biology, Northwestern University

4. Chemistry of Life Processes Institute, Northwestern University

Abstract

Ion channels are biological transistors that control ionic flux across cell membranes to regulate electrical transmission and signal transduction. They are found in all biological membranes and their conductive states are frequently disrupted in human diseases. Organelle ion channels are among the most resistant to functional and pharmacological interrogation. Traditional channel protein reconstitution methods rely upon exogenous expression and/or purification from endogenous cellular sources which are frequently contaminated by resident ionophores. Here we describe a fully synthetic method to assay the functional properties of the polycystin subfamily of transient receptor potential (TRP) channels that natively traffic to primary cilia and endoplasmic reticulum organelles. Using this method, we characterize their membrane integration, orientation and conductance while comparing these results to their endogenous channel properties. Outcomes define a novel synthetic approach that can be applied broadly to investigate other channels resistant to biophysical analysis and pharmacological characterization.

Publisher

eLife Sciences Publications, Ltd

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