Abstract

Protein secretion is one of the most important and complex physiological processes in growing cells. The main aim of this proposal is to analyze the molecular details of this process in vitro, i.e. protein translocation into bacterial membrane vesicles. In addition, we will examine further how proteins are excreted past a double membrane in certain Gram-negative bacteria. The elucidation of the mechanism of protein translocation is greatly facilitated by our newly developed, efficient system utilizing extracts, mRNA for alkaline phosphatase and OmpA protein, and inner membrane vesicles, all from E. coli. This system can separate the stage of translocation from that of translation, which makes the biochemical analysis of protein translocation much simpler. With this system we will pursue indications that protein translocation requires ATP as well as protonmotive force, and whether a complex of proteins that may be the bacterial equivalent of the eukaryotic signal recognition particle, and other cytoplasmic proteins, are involved. To identify membrane proteins involved in translocation we will use partial reconstitution, protease inactivation, cross-linking of precursors of secreted proteins to membrane proteins, specific antibodies to block function, and mutants defective in secretion. To study protein excretion past a double membrane in Gram-negative bacteria, we will examine the biosynthesis and excretion pathway of Pseudomonas aeruginosa hemolysin and Vibrio cholera toxin. Building on evidence that excretion of toxin to the exterior requires genes not present in E. coli cells, we will introduce additional genes from Pseudomonas into E. coli and will seek transformants that excrete toxin to the exterior instead of secreting it into the periplasm. If the results are positive, the required gene(s) and protein(s) will be identified. An understanding of mechanisms discovered in bacteria is likely to have implications for secretion of proteins by human cells, and should have important practical implications for the medical-industrial use of recombinant DNA in bacteria. Furthermore, the studies of microbial toxins are directly relevant to medical bacteriology.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
1R01GM034766-01
Application #
3286294
Study Section
Microbial Physiology and Genetics Subcommittee 2 (MBC)
Project Start
1985-07-01
Project End
1990-06-30
Budget Start
1985-07-01
Budget End
1986-06-30
Support Year
1
Fiscal Year
1985
Total Cost
Indirect Cost

  Institution

Name
Boston Biomedical Research Institute
Department
Type
DUNS #
058893371
City
Watertown
State
MA
Country
United States
Zip Code

  Publications

Hsieh, Ying-Hsin; Huang, Ying-Ju; Zhang, Hao et al. (2017) Dissecting structures and functions of SecA-only protein-conducting channels: ATPase, pore structure, ion channel activity, protein translocation, and interaction with SecYEG/SecDF•YajC. PLoS One 12:e0178307
Na, Bing; You, Zhipeng; Yang, Hsiuchin et al. (2015) Characterization of the minimal length of functional SecA in Escherichia coli. Biochem Biophys Res Commun 456:213-8
Hsieh, Ying-Hsin; Zou, Juan; Jin, Jin-Shan et al. (2015) Monitoring channel activities of proteoliposomes with SecA and Cx26 gap junction in single oocytes. Anal Biochem 480:58-66
Yang, Chun-Kai; Tai, Phang C; Lu, Chung-Dar (2014) Time-related transcriptome analysis of B. subtilis 168 during growth with glucose. Curr Microbiol 68:12-20
Hsieh, Ying-Hsin; Huang, Ying-Ju; Jin, Jin-Shan et al. (2014) Mechanisms of Rose Bengal inhibition on SecA ATPase and ion channel activities. Biochem Biophys Res Commun 454:308-12
Floyd, Jeanetta Holley; You, Zhipeng; Hsieh, Ying-Hsin et al. (2014) The dispensability and requirement of SecA N-terminal aminoacyl residues for complementation, membrane binding, lipid-specific domains and channel activities. Biochem Biophys Res Commun 453:138-42
Wang, Hongyun; Ma, Yamin; Hsieh, Ying-Hsin et al. (2014) SecAAA trimer is fully functional as SecAA dimer in the membrane: existence of higher oligomers? Biochem Biophys Res Commun 447:250-4
Yang, Chun-Kai; Zhang, Xiao-Zhou; Lu, Chung-Dar et al. (2014) An internal hydrophobic helical domain of Bacillus subtilis enolase is essential but not sufficient as a non-cleavable signal for its secretion. Biochem Biophys Res Commun 446:901-5
Zhang, Hao; Hsieh, Ying-Hsin; Lin, Bor-Ruei et al. (2013) Specificity of SecYEG for PhoA precursors and SecA homologs on SecA protein-conducting channels. Biochem Biophys Res Commun 437:212-216
Yang, Chun-Kai; Lu, Chung-Dar; Tai, Phang C (2013) Differential expression of secretion machinery during bacterial growth: SecY and SecF decrease while SecA increases during transition from exponential phase to stationary phase. Curr Microbiol 67:682-7

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