Novel Structure, Properties and Inactivation of Glutamine Synthetase Cloned from Bacteroides fragilis

1 State Vaccine Institute, Alexandra Road, Pinelands 7405, South Africa 2 Department of Microbiology, University of Cape Town, Rondebosch 7700, South Africa ABSTRACT SUMMARY: The cloned Bacteroides fragilis glutamine synthetase (GS) subunit produced in Escherichia coli had the same apparent M r of a...

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Published inJournal of general microbiology Vol. 133; no. 9; pp. 2437 - 2446
Main Authors SOUTHERN, JAMES A, PARKER, JOAN R, WOODS, DAVID R
Format Journal Article
LanguageEnglish
Published London Soc General Microbiol 01.09.1987
New York, NY Cambridge University Press
Subjects
Bacteriology
Bacteroides fragilis
Biological and medical sciences
Fundamental and applied biological sciences. Psychology
glutamate-ammonia ligase
Metabolism. Enzymes
Microbiology
Regulation(control)
Gene
Molecular structure
Bacteroides fragilis
Enzyme
Escherichia coli
Bacteria
Glutamine synthetase
Molecular cloning
Escherichieae
Bacteroidaceae
Enterobacteriaceae
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ISSN0022-1287
1350-0872
1465-2080
DOI10.1099/00221287-133-9-2437

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Summary:1 State Vaccine Institute, Alexandra Road, Pinelands 7405, South Africa 2 Department of Microbiology, University of Cape Town, Rondebosch 7700, South Africa ABSTRACT SUMMARY: The cloned Bacteroides fragilis glutamine synthetase (GS) subunit produced in Escherichia coli had the same apparent M r of approximately 75000 as the GS subunit from B. fragilis cells. The B. fragilis GS enzyme had an apparent M r of approximately 490000 and it is concluded that the GS is a hexamer. The cloned GS did not appear to be regulated by adenylylation and deadenylylation and the cloned enzyme was inactivated by snake venom phosphodiesterase. The pH profiles of the cloned GS, assayed by the -glutamyl transferase (GGT) assay were similar for NH 4 + -shocked and unshocked cell extracts and an isoactivity point was not obtained from these curves. The cloned GS was subject to feedback inhibition by amino acids but not by AMP. The GGT activity of the cloned GS in NH 4 + -shocked and unshocked cell-free extracts was inhibited by Mg 2+ . Mn 2+ stimulated the cloned GS GGT activity of NH 4 + -shocked cell-free extracts. Western blotting indicated that GS production was regulated by nitrogen in B. fragilis cells but cell extracts showed no GGT activity. Cloned B. fragilis GS produced in E. coli was specifically and irreversibly inactivated by B. fragilis cell extracts.
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ISSN:0022-1287
1350-0872
1465-2080
DOI:10.1099/00221287-133-9-2437