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A new mode of SAM domain mediated oligomerization observed in the CASKIN2 neuronal scaffolding protein
Authors:Ekaterina?Smirnova  Jamie?J?Kwan  Ryan?Siu  Xin?Gao  Georg?Zoidl  Borries?Demeler  Vivian?Saridakis  Email author" target="_blank">Logan?W?DonaldsonEmail author
Institution:1.Department of Biology,York University,Toronto,Canada;2.Division of Computer, Computational Bioscience Research Center, Electrical and Mathematical Science and Engineering,King Abdullah University of Science and Technology,Thuwal,Kingdom of Saudi Arabia;3.Department of Psychology,York University,Toronto,Canada;4.Department of Biochemistry,University of Texas Health Science Center at San Antonio,San Antonio,USA
Abstract:

Background

CASKIN2 is a homolog of CASKIN1, a scaffolding protein that participates in a signaling network with CASK (calcium/calmodulin-dependent serine kinase). Despite a high level of homology between CASKIN2 and CASKIN1, CASKIN2 cannot bind CASK due to the absence of a CASK Interaction Domain and consequently, may have evolved undiscovered structural and functional distinctions.

Results

We demonstrate that the crystal structure of the Sterile Alpha Motif (SAM) domain tandem (SAM1-SAM2) oligomer from CASKIN2 is different than CASKIN1, with the minimal repeating unit being a dimer, rather than a monomer. Analytical ultracentrifugation sedimentation velocity methods revealed differences in monomer/dimer equilibria across a range of concentrations and ionic strengths for the wild type CASKIN2 SAM tandem and a structure-directed double mutant that could not oligomerize. Further distinguishing CASKIN2 from CASKIN1, EGFP-tagged SAM tandem proteins expressed in Neuro2a cells produced punctae that were distinct both in shape and size.

Conclusions

This study illustrates a new way in which neuronal SAM domains can assemble into large macromolecular assemblies that might concentrate and amplify synaptic responses.
Keywords:
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