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Structural Basis for the Inhibition of Voltage-gated Sodium Channels by Conotoxin μO§-GVIIJ

Journal of Biological Chemistry(2016)

Cited 5|Views30
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Abstract
Cone snail toxins are well known blockers of voltage-gated sodium channels, a property that is of broad interest in biology and therapeutically in treating neuropathic pain and neurological disorders. Although most conotoxin channel blockers function by direct binding to a channel and disrupting its normal ion movement, conotoxin O -GVIIJ channel blocking is unique, using both favorable binding interactions with the channel and a direct tether via an intermolecular disulfide bond. Disulfide exchange is possible because conotoxin O -GVIIJ contains an S-cysteinylated Cys-24 residue that is capable of exchanging with a free cysteine thiol on the channel surface. Here, we present the solution structure of an analog of O -GVIIJ (GVIIJ[C24S]) and the results of structure-activity studies with synthetic O -GVIIJ variants. GVIIJ[C24S] adopts an inhibitor cystine knot structure, with two antiparallel -strands stabilized by three disulfide bridges. The loop region linking the -strands (loop 4) presents residue 24 in a configuration where it could bind to the proposed free cysteine of the channel (Cys-910, rat Na(V)1.2 numbering; at site 8). The structure-activity study shows that three residues (Lys-12, Arg-14, and Tyr-16) located in loop 2 and spatially close to residue 24 were also important for functional activity. We propose that the interaction of O -GVIIJ with the channel depends on not only disulfide tethering via Cys-24 to a free cysteine at site 8 on the channel but also the participation of key residues of O -GVIIJ on a distinct surface of the peptide.
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Key words
disulfide,high performance liquid chromatography (HPLC),nuclear magnetic resonance (NMR),peptide chemical synthesis,sodium channel,conotoxin,cysteine,structure-activity relationship studies,two-electrode voltage clamp electrophysiology
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