Abstract
AbstractReconstitution of membrane proteins into model membranes is an essential approach for their functional analysis under chemically defined conditions. Established model-membrane systems used in ensemble average measurements are limited by sample heterogeneity and insufficient knowledge of lipid and protein content at the single vesicle level, which limits quantitative analysis of vesicle properties and prevents their correlation with protein activity. Here, we describe a versatile total internal reflection fluorescence microscopy-based bleaching protocol that permits parallel analyses of multiple parameters (physical size, tightness, unilamellarity, membrane protein content and orientation) of individual proteoliposomes prepared with fluorescently tagged membrane proteins and lipid markers. The approach makes use of commercially available fluorophores including the commonly used nitrobenzoxadiazole (NBD) dye and may be applied to deduce functional molecular characteristics of many types of reconstituted fluorescently tagged membrane proteins.
Publisher
Cold Spring Harbor Laboratory
Reference43 articles.
1. Allan, D.B. , Caswell, T. , Keim, N.C. , van der Wel, C.M. , Verweij, R.W. , 2021. soft-matter/trackpy: Trackpy v0.5.0. Zenodo. https://doi.org/10.5281/zenodo.4682814
2. Current problems and future avenues in proteoliposome research;Biochem. Soc. Trans,2020
3. The Astropy Project: Building an Open-science Project and Status of the v2.0 Core;Astropy Collaboration;Package. Astron. J,2018
4. Astropy: A community Python package for astronomy
5. Quantification of nano-scale intermembrane contact areas by using fluorescence resonance energy transfer