Abstract

We are studying the mechanisms of protein translocation into, and across, biological membranes. The process is basic to subcellular compartmentation and is a vital aspect of processes from hormone secretion to bacterial pathogenesis. We have purified and reconstituted E. coli preprotein translocase, the complex protein which transports preproteins across the plasma membrane. We have identified its major subunits and established the fundamentals of its catalytic cycle. Preprotein translocase has a SecA peripheral membrane domain, which is bound to both acidic lipids and to a membrane-embedded, heterohexameric integral membrane domain of SecYEGDFyajC. The SecA subunit carries successive loops of preprotein across the membrane, driven in its insertion and de-insertion cycle by the energy of ATP binding and hydrolysis. We now propose to purify the overproduced, epitope-tagged translocase, collaboratively determine its structure, and explore the environment of the transiting chain, the leader (signal) peptide, and the SecA subunit as it inserts across the membrane with the preprotein. Dynamic questions of translocase function will include the topology of subunits, their exchange among holoenzyme complexes during the catalytic cycle, and the roles of lipid and proton-flux in translocation. Finally, we will study the assembly of integral membrane proteins, whether through this translocase or via spontaneous insertion. This phase of the work can now actually address the fundamental mechanistic questions of secretion and membrane assembly.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM023377-24
Application #
6018472
Study Section
Microbial Physiology and Genetics Subcommittee 2 (MBC)
Project Start
1976-05-01
Project End
2001-06-30
Budget Start
1999-07-01
Budget End
2000-06-30
Support Year
24
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
Dartmouth College
Department
Biochemistry
Type
Schools of Medicine
DUNS #
041027822
City
Hanover
State
NH
Country
United States
Zip Code
03755

  Publications

Orr, Amy; Song, Hongki; Rusin, Scott F et al. (2017) HOPS catalyzes the interdependent assembly of each vacuolar SNARE into a SNARE complex. Mol Biol Cell 28:975-983
Song, Hongki; Wickner, William (2017) A short region upstream of the yeast vacuolar Qa-SNARE heptad-repeats promotes membrane fusion through enhanced SNARE complex assembly. Mol Biol Cell 28:2282-2289
Song, Hongki; Orr, Amy; Duan, Mengtong et al. (2017) Sec17/Sec18 act twice, enhancing membrane fusion and then disassembling cis-SNARE complexes. Elife 6:
Schwartz, Matthew L; Nickerson, Daniel P; Lobingier, Braden T et al. (2017) Sec17 (?-SNAP) and an SM-tethering complex regulate the outcome of SNARE zippering in vitro and in vivo. Elife 6:
Zick, Michael; Wickner, William (2016) Improved reconstitution of yeast vacuole fusion with physiological SNARE concentrations reveals an asymmetric Rab(GTP) requirement. Mol Biol Cell 27:2590-7
Zick, Michael; Orr, Amy; Schwartz, Matthew L et al. (2015) Sec17 can trigger fusion of trans-SNARE paired membranes without Sec18. Proc Natl Acad Sci U S A 112:E2290-7
Orr, Amy; Wickner, William; Rusin, Scott F et al. (2015) Yeast vacuolar HOPS, regulated by its kinase, exploits affinities for acidic lipids and Rab:GTP for membrane binding and to catalyze tethering and fusion. Mol Biol Cell 26:305-15
Baker, Richard W; Jeffrey, Philip D; Zick, Michael et al. (2015) A direct role for the Sec1/Munc18-family protein Vps33 as a template for SNARE assembly. Science 349:1111-4
Zick, Michael; Wickner, William T (2014) A distinct tethering step is vital for vacuole membrane fusion. Elife 3:e03251
Zick, Michael; Stroupe, Christopher; Orr, Amy et al. (2014) Membranes linked by trans-SNARE complexes require lipids prone to non-bilayer structure for progression to fusion. Elife 3:e01879

Showing the most recent 10 out of 39 publications