Literature DB >> 20847230

A charged prominence in the linker domain of the cysteine-string protein Cspα mediates its regulated interaction with the calcium sensor synaptotagmin 9 during exocytosis.

Frédéric Boal1, Michel Laguerre, Alexandra Milochau, Jochen Lang, Pier A Scotti.   

Abstract

The cochaperone cysteine-string protein (Csp) is located on vesicles and participates in the control of neurotransmission and hormone exocytosis. Csp contains several domains, and our previous work demonstrated the requirement of the Csp linker domain in regulated exocytosis of insulin in rodent pancreatic β cells. We now address the molecular details to gain insight into the sequence of events during exocytosis. According to pulldown experiments and in vitro binding assays, Cspα interacts indirectly with SNAP-25 and directly with the calcium sensor synaptotagmin 9 (Syt9), which could be an intermediate between the chaperone and the t-SNARE. The C(2)A calcium binding domain of Syt9 and the linker domain of Cspα constituted the minimal interacting module. FRET-FLIM experiments confirmed the interaction between Syt9 and Cspα. Moreover, the point mutation E93V in the linker domain of Cspα significantly reduced the interaction between the two proteins. Molecular modeling revealed that this point mutation abolished a charged prominence on the surface of Cspα required for interaction. Strikingly, free calcium in the physiological low micromolar range enhanced the interaction between Syt9 and the linker domain of Cspα in vitro. These data indicate that Cspα interacts with Syt9, and such a complex may be relevant in the calcium-mediated control of a late stage of exocytosis by triggering the specific recruitment of a folding catalyst at the fusion point.

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Year:  2010        PMID: 20847230     DOI: 10.1096/fj.09-152033

Source DB:  PubMed          Journal:  FASEB J        ISSN: 0892-6638            Impact factor:   5.191


  12 in total

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8.  Phosphomimetic mutation of cysteine string protein-α increases the rate of regulated exocytosis by modulating fusion pore dynamics in PC12 cells.

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9.  Cysteine string protein limits expression of the large conductance, calcium-activated K⁺ (BK) channel.

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10.  Phosphorylation of Cysteine String Protein Triggers a Major Conformational Switch.

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Journal:  Structure       Date:  2016-07-21       Impact factor: 5.006

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