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Structural-functional characterization of the MIRO1-TRAK1 complex

Nature Communications. 2025-07; 
Erika E Ravitch, Elana E Baltrusaitis, Tania A Perez, Kyle R Barrie, Adam R Fenton, Erika L F Holzbaur, Roberto Dominguez Department of Physiology, Perelman School of Medicine, University of Pennsylvania, Philadelphia, PA, USA
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Bacterial Expression The DNA for human MIRO1 (Addgene, plasmid #127613), human TRAK1 (GenScript, E. coli codon-optimized), and TRAK1416-446,561-623 (GenScript, E. coli codon-optimized) were used as templates for cloning (primers listed in Source Data file). Get A Quote

Abstract

Mitochondrial Rho GTPase (MIRO) features N- and C-terminal GTPase domains (nGTPase and cGTPase) flanking two pairs of EF-hands, and functions as a master scaffold on the outer mitochondrial membrane. It regulates mitochondrial motility by recruiting trafficking kinesin-binding protein (TRAK), which in turn recruits kinesin-1 and dynein-dynactin. The MIRO-TRAK interaction remains incompletely understood. Here, we describe the cryo-electron microscopy structure of TRAK1569-623 bound to MIRO1. The complex forms a dimer, mediated by interactions through the second EF-hand pair, cGTPase, and TRAK1. TRAK1569-623 binds in a cleft between the nGTPase and first EF-hand pair, inserting side chains into hydrophobic pocket... More

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