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Myristoylation Restricts Orientation of the GRASP Domain on Membranes and Promotes Membrane Tethering
Authors:Frank Heinrich  Hirsh Nanda  Haw Zan Goh  Collin Bachert  Mathias L?sche  Adam D Linstedt
Institution:From the Departments of Physics.;Biological Sciences, and ;Biomedical Engineering, Carnegie Mellon University, Pittsburgh, Pennsylvania 15213 and ;the §National Institute of Standards and Technology (NIST) Center for Neutron Research, Gaithersburg, Maryland 20899
Abstract:The mammalian Golgi reassembly stacking protein (GRASP) proteins are Golgi-localized homotypic membrane tethers that organize Golgi stacks into a long, contiguous ribbon-like structure. It is unknown how GRASPs undergo trans pairing given that cis interactions between the proteins in the plane of the membrane are intrinsically favored. To test the hypothesis that myristoylation of the self-interacting GRASP domain restricts its orientation on the membrane to favor trans pairing, we established an in vitro assay that recapitulates GRASP-dependent membrane tethering and used neutron reflection under similar conditions to determine the orientation of the GRASP domain. In vivo, the membrane association of GRASP proteins is conferred by the simultaneous insertion of an N-terminal myristic acid and binding to a Golgi-associated binding partner. In our assay, the latter contact was replaced using a C-terminal hexa-His moiety, which bound to Ni2+-conjugated lipids incorporated into a substrate-supported bilayer lipid membrane. Nonmyristoylated protein lacked a fixed orientation on the membrane and inefficiently tethered liposomes. In contrast, myristoylated GRASP promoted tethering and exhibited a unique membrane complex. Thus, myristoylation restricts the membrane orientation of the GRASP domain favoring interactions in trans for membrane tethering.
Keywords:Fluorescence  Golgi  Membrane Bilayer  Membrane Fusion  Membrane Trafficking  Neutron Scattering
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