Abstract

Visinin-like protein 1 (VILIP-1) belongs to the neuronal calcium sensor family of Ca(2+)-myristoyl switch proteins that regulate signal transduction in the brain and retina. Here we analyze Ca(2+) and Mg(2+) binding, characterize metal-induced conformational changes, and determine structural effects of myristoylation and dimerization. Mg(2+) binds functionally to VILIP-1 at EF3 (ΔH = +1.8 kcal/mol and K(D) = 20 μM). Unmyristoylated VILIP-1 binds two Ca(2+) sequentially at EF2 and EF3 (K(EF3) = 0.1 μM and K(EF2) = 1-4 μM), whereas myristoylated VILIP-1 binds two Ca(2+) with lower affinity (K(D) = 1.2 μM) and positive cooperativity (Hill slope = 1.5). NMR assignments and structural analysis indicate that Ca(2+)-free VILIP-1 contains a sequestered myristoyl group like that of recoverin. NMR resonances of the attached myristate exhibit Ca(2+)-dependent chemical shifts and NOE patterns consistent with Ca(2+)-induced extrusion of the myristate. VILIP-1 forms a dimer in solution independent of Ca(2+) and myristoylation. The dimerization site is composed of residues in EF4 and the loop region between EF3 and EF4, confirmed by mutagenesis. We present the structure of the VILIP-1 dimer and a Ca(2+)-myristoyl switch to provide structural insights into Ca(2+)-induced trafficking of nicotinic acetylcholine receptors.

Highlights

  • Visinin-like protein 1 (VILIP-1)2 is a neuronal Ca2ϩ sensor (NCS) protein belonging to the calmodulin superfamily of calcium sensor proteins [1,2,3,4]

  • We report on the structural analysis of Ca2ϩ and Mg2ϩ binding to VILIP-1 to characterize the structural mechanism of the Ca2ϩ-myristoyl switch and determine its dimeric structure

  • The Ca2ϩ binding data for VILIP-1 indicate that N-terminal myristoylation both lowers the apparent affinity (KD ϭ 1.2 ␮M) and induces positive cooperativity (␣ ϭ 1.5) like that observed for recoverin [28] and neurocalcin [29], which is an important hallmark of a Ca2ϩ-myristoyl switch

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Summary

EXPERIMENTAL PROCEDURES

Preparation and Purification of Recombinant VILIPs—Human VILIP-1 and VILIP-3 genes were subcloned in pET3d(ϩ) plasmids. All triple-resonance experiments were performed and analyzed as described [37] on a sample of Mg2ϩ-bound 13C/15N-labeled myristoylated VILIP-1 (in 95% H2O, 5% 2H2O) with the following number of complex points and acquisition times: HNCO (15N (F1) 32, 23.7 ms; 13CO (F2) 64, 42.7 ms; 1H (F3) 512, 64 ms); HNCACB (15N (F1) 32, 23.7 ms; 13C (F2) 48, 6.3 ms; 1H (F3) 512, 64 ms); CBCACONNH (15N (F1) 32, 23.7 ms; 13C (F2) 48, 6.3 ms; 1H (F3) 512, 64 ms); CBCACOCAHA (13C (F1) 52, 6.8 ms, 13CO (F2) 64, 42 ms, 1H (F3) 384, 64 ms); and HBHACONNH (15N (F1) 32, 23.7 ms, 1Hab (F2) 64 21 ms, 1H (F3) 512, 64 ms). The docking calculation of the VILIP-1 dimer appears to be well determined by the experimental restraints

RESULTS
C3 C4–C11 C12 C13 C14
DISCUSSION

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