2013
DOI: 10.1002/prot.24329
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NMR investigation of the equilibrium partitioning of a water-soluble bile salt protein carrier to phospholipid vesicles

Abstract: Membrane binding by cytosolic fatty acid binding proteins (FABP) appears to constitute a key step of intracellular lipid trafficking. We applied NMR spectroscopy to study the partitioning of a water-soluble bile acid binding protein (BABP), belonging to the FABP family, between its free and lipid-vesicle-bound states. As the lipid-bound protein was NMR-invisible, the signals of the free biomolecule were analyzed to obtain quantitative information on binding affinity and steady-state kinetics. The data indicate… Show more

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Cited by 32 publications
(34 citation statements)
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“…We employed a recently developed NMR approach [55,56] to monitor protein binding to liposomes. This approach allows measurement of the amount of protein that remains free in solution in the presence of liposomes under equilibrium conditions, and is based on the fact that NMR signals are readily detectable for proteins the size of HIV-1 MA (~15kDa) but generally undetectable (or “dark” [55]) for proteins and protein complexes as large as liposomes (>60MDa).…”
Section: Resultsmentioning
confidence: 99%
See 3 more Smart Citations
“…We employed a recently developed NMR approach [55,56] to monitor protein binding to liposomes. This approach allows measurement of the amount of protein that remains free in solution in the presence of liposomes under equilibrium conditions, and is based on the fact that NMR signals are readily detectable for proteins the size of HIV-1 MA (~15kDa) but generally undetectable (or “dark” [55]) for proteins and protein complexes as large as liposomes (>60MDa).…”
Section: Resultsmentioning
confidence: 99%
“…This approach allows measurement of the amount of protein that remains free in solution in the presence of liposomes under equilibrium conditions, and is based on the fact that NMR signals are readily detectable for proteins the size of HIV-1 MA (~15kDa) but generally undetectable (or “dark” [55]) for proteins and protein complexes as large as liposomes (>60MDa). Provided that on/off membrane exchange is intermediate-to-slow on the NMR chemical shift time scale, binding to liposomes is expected to render all but the highly flexible MA residues NMR-invisible [55,56]. As shown in Fig.…”
Section: Resultsmentioning
confidence: 99%
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“…DLS was performed on Qtracker ® 800 using a Zetasizer Nano ZS instrument (Malvern Instruments Ltd, MA, USA) operating with a 633 nm He-Ne laser light source and a fixed detector angle of 173°, as previously described [27]. Qtracker ® 800, 2-μM stock solution of 2 μM in 50 mM borate buffer, pH 8.3 (Life Technologies) was diluted to the range of 40-80 nM either in Ringer solution or in saline solution (See section Chemicals).…”
Section: Hydrodynamic Size Measurements By Dlsmentioning
confidence: 99%