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Lipid- and protein-directed photosensitizer proximity labeling captures the cholesterol interactome
by
Julio, Ashley R
, Tontonoz, Peter
, Nagari, Rohith T
, Mack, Julia J
, Biletch, Elijah
, Kennelly, John Paul
, Burton, Nikolas R
, Becker, Andrew P
, Villaneuva, Miranda
, Fukuta, Tomoyuki
, Backus, Keriann M
, Cui, Liujuan
, Hong, Soon-Gook
, Turner, Daniel W
, Xiao, Xu
in
Biochemistry
2024
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Lipid- and protein-directed photosensitizer proximity labeling captures the cholesterol interactome
by
Julio, Ashley R
, Tontonoz, Peter
, Nagari, Rohith T
, Mack, Julia J
, Biletch, Elijah
, Kennelly, John Paul
, Burton, Nikolas R
, Becker, Andrew P
, Villaneuva, Miranda
, Fukuta, Tomoyuki
, Backus, Keriann M
, Cui, Liujuan
, Hong, Soon-Gook
, Turner, Daniel W
, Xiao, Xu
in
Biochemistry
2024
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Do you wish to request the book?
Lipid- and protein-directed photosensitizer proximity labeling captures the cholesterol interactome
by
Julio, Ashley R
, Tontonoz, Peter
, Nagari, Rohith T
, Mack, Julia J
, Biletch, Elijah
, Kennelly, John Paul
, Burton, Nikolas R
, Becker, Andrew P
, Villaneuva, Miranda
, Fukuta, Tomoyuki
, Backus, Keriann M
, Cui, Liujuan
, Hong, Soon-Gook
, Turner, Daniel W
, Xiao, Xu
in
Biochemistry
2024
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Lipid- and protein-directed photosensitizer proximity labeling captures the cholesterol interactome
Journal Article
Lipid- and protein-directed photosensitizer proximity labeling captures the cholesterol interactome
2024
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Overview
The physical properties of cellular membranes, including fluidity and function, are influenced by protein and lipid interactions. In situ labeling chemistries, most notably proximity-labeling interactomics are well suited to characterize these dynamic and often fleeting interactions. Established methods require distinct chemistries for proteins and lipids, which limits the scope of such studies. Here we establish a singlet-oxygen-based photocatalytic proximity labeling platform (POCA) that reports intracellular interactomes for both proteins and lipids with tight spatiotemporal resolution using cell-penetrant photosensitizer reagents. Using both physiologically relevant lipoprotein-complexed probe delivery and genetic manipulation of cellular cholesterol handling machinery, cholesterol-directed POCA captured established and unprecedented cholesterol binding proteins, including protein complexes sensitive to intracellular cholesterol levels and proteins uniquely captured by lipoprotein uptake. Protein-directed POCA accurately mapped known intracellular membrane complexes, defined sterol-dependent changes to the non-vesicular cholesterol transport protein interactome, and captured state-dependent changes in the interactome of the cholesterol transport protein Aster-B. More broadly, we find that POCA is a versatile interactomics platform that is straightforward to implement, using the readily available HaloTag system, and fulfills unmet needs in intracellular singlet oxygen-based proximity labeling proteomics. Thus, we expect widespread utility for POCA across a range of interactome applications, spanning imaging to proteomics.
Publisher
Cold Spring Harbor Laboratory
Subject
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