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Unbiased Identification of the Liposome Protein Corona using Photoaffinity-based Chemoproteomics
Author(s) -
Roy Pattipeiluhu,
Stefan Crielaard,
Iris Klein-Schiphorst,
Bogdan I. Florea,
Alexander Kros,
Frederick Campbell
Publication year - 2020
Publication title -
acs central science
Language(s) - English
Resource type - Journals
eISSN - 2374-7951
pISSN - 2374-7943
DOI - 10.1021/acscentsci.9b01222
Subject(s) - liposome , photoaffinity labeling , biophysics , chemistry , nanoparticle , plasma protein binding , in vivo , computational biology , biochemistry , nanotechnology , binding site , biology , materials science , microbiology and biotechnology
Protein adsorption to the surface of a nanoparticle can fundamentally alter the character, behavior, and fate of a nanoparticle in vivo. Current methods to capture the protein corona rely on physical separation techniques and are unable to resolve key, individual protein-nanoparticle interactions. As a result, the precise link between the "synthetic" and the "biological" identity of a nanoparticle remains unclear. Herein, we report an unbiased photoaffinity-based approach to capture, characterize, and quantify the protein corona of liposomes in their native state. Compared to conventional methods, our photoaffinity approach reveals markedly different interacting proteins as well as reduced total protein binding to liposome surfaces. Identified proteins do not follow protein abundancy patterns of human serum, as has been generally reported, but are instead dominated by soluble apolipoproteins-endogenous serum proteins that have evolved to recognize the lipidic surface of circulating lipoproteins. We believe our findings are the most accurate characterization of a liposome's biological identity but, more fundamentally, reveal liposome-protein binding is, in many cases, significantly less complex than previously thought.

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