Membrane Biology Section

Julie G Donaldson, PhD, Principal Investigator

Our group studies the function of the Arf GTP-binding proteins in regulating membrane traffic and structure. A primary focus is on Arf6, which coordinates membrane traffic and the actin cytoskeleton at the plasma membrane (PM). In the active, GTP-bound state, Arf6 activates phosphatidylinositol 4-phosphate 5-kinase, an enzyme that generates phosphatidylinositol 4,5-bisphosphate (PIP2), a major PM phosphoinositide. PIP2 is abundant along the PM where it facilitates actin polymerization and on endosomal membranes associated with Arf6. Stimulated activation of Arf6, by expression of a guanine nucleotide exchange factor (GEF) for Arf6, results in the formation of protrusive ruffling and consequent formation of macropinosomes, which are taken into the cells and the membrane recycled back to the PM. Failure to inactivate Arf6, by GTP hydrolysis, or to turnover the PIP2 leads to a disruption in this membrane flow and a halt in PM ruffling. One area of research in the lab is the identification of additional GEFs that activate Arf6 and studies aimed at identifying factors that regulate GEF activity in cells.

The Arf6-associated endosomal membranes contain PM proteins that enter cells by endocytosis independently of adaptor protein 2 (AP2)/clathrin. We have found that these non-clathrin derived endosomes contain physiologically important PM proteins such as the major histocompatibility complex class I (MHCI) proteins, integrins, "raft" partitioning proteins like GPI-anchored proteins, and other regulators such as Rac1 and src. Upon internalization, these non-clathrin-derived early endosomes fuse with the traditional, Rab5-associated early endosome and from there cargo can proceed to late endosomes and lysosomes where they are degraded or be recycled back to the PM via distinct, tubular, Arf6-associated recycling membranes. This recycling pathway only carries non-clathrin cargo and requires the activities of two Rab GTPases, Rab11 and Rab22. Further studies aimed at elucidating how these endosomal membrane systems interconnect will include identification of other components involved in these pathways (such as Rabs, SNARES, and PIP-kinases) and the development of in vitro endosomal fusion assays that recreate these activities. We also are interested in understanding how clathrin-independent endocytosis is regulated and identifying the molecular machinery that is required for this process.

Arf6 belongs to the Arf Family of GTP binding proteins and is 70% identical to Arf1, the other Arf family member that is well characterized. These two Arfs also exhibit remarkable structural similarity and we have utilized this feature to create chimeras between Arf1 and Arf6 in order to identify sequences critical for localization and function. We have identified residues in Arf6 sequence adjacent to Switch I region that are required for protrusion formation by Arf6. Recently, we have identified a determinant in Arf1 that facilitates Golgi recruitment through binding to the ER-Golgi SNARE protein Membrin. Using yeast 2-hybrid and biochemical affinity approaches, projects have identified candidate, Arf6- and Arf1-specific interacting proteins. Studies of these effector proteins should assist in the discovery of how Arf6 and Arf1 carry out their specific cellular functions.

Selected Publications:

Brown, F.D., Rozelle, A.L., Yin, H.L., Balla, T., and Donaldson, J.G. Phosphatidylinositol-4,5-bisphosphate and Arf6-regulated membrane traffic. J. Cell Biol., 154, 1007-1017, 2001.

Donaldson, J.G. Multiple roles for Arf6: Sorting, structuring, and signaling at the plasma membrane, J. Biol. Chem. 278, 41573-41576, 2003.

Honda, A., Al-Awar, O.S., Hay, J.C., and Donaldson, J.G. Targeting of Arf-1 to the early Golgi by membrin, an ER-Golgi SNARE, J. Cell Biol. 168:1039-1051.

Naslavsky, N., Weigert, R., and Donaldson, J.G. Convergence between non-clathrin and clathrin-derived endosomes involves Arf6 inactivation. Mol. Biol. Cell 14, 417-431, 2003.

Naslavsky, N., Weigert, R. and Donaldson, J.G. Characterization of a non-clathrin endocytic pathway: membrane cargo and lipid requirements, Mol Biol Cell, 15:3542-3552, 2004.

Weigert, R., Yeung, A.C., Li, J. and Donaldson, J.G. Rab22a regulates the recycling of membrane proteins internalized independently of clathrin. Mol Biol Cell, 15:3758-3770, 2004.

Questions, comments and suggestions about this page may be addressed to Julie Donaldson

NHLBI HOME · SEARCH NHLBI · ACCESSIBILITY INFORMATION · NHLBI SITE INDEX · OTHER SITES · PRIVACY STATEMENT · FOIA · CONTACT NHLBI