Mutations that create new promoters suppress the sigma 54 dependence of glnA transcription in Escherichia coli

Abstract: Escherichia coli rpoN mutants lack or4 and are therefore unable to initiate the transcription of ginA at glnAp2, which is required for the production of a high intracellular concentration of glutamine synthetase. We have found that the dependence on a54 can be overcome by iutations that have apparently created a new r70-dependent promoter. The position -35 RNA polymerase contact site of this new promoter overlaps glnAp2.The initiation of transcription at the new promoter is inhibited by r54-RNA polymerase even… Show more

“…The active fraction was eluted at a KCl concentration of approximately 0.25 M, and concentrated to about 10 ml on a Amicon UM-10 membrane. The concentrated enzyme was dialyzed against buffer C (the buffer B containing 10mM (CH 3 COOhMg), and then applied to a Blue-Cellulofine column (2.5 x 20 cm) equilibrated with buffer C. The.column was washed with 0.1 M KCl in buffer C, and the enzyme was then eluted with a linear gradient from 0.1 MKCl, 10 mM (CH 3 COOhMg to 1.0 M KCl, 0 mM (CH 3 COOhMg in buffer C. The active fraction was concentrated on the Amicon membrane and dialyzed against buffer B. The puriffed enzyme could be stored at -70°C without loss of activity for at least one month.…”

“…A nucleotide sequence derived from pKK223-3 was underlined with a double line. (CH 3 COOhMg, 1mM EDTA, 30mM KCl, and 5mM 2-mercaptoethanol) and re-collected by centrifugation. The cells were then suspended in 50 ml of buffer A and disrupted by sonication at O°C.…”

“…1 ) These enzymes are distributed in prokaryotes as Escherichia coli 2 ) and Klebsiella aerogenes 3 ) and encoded by asnA genes. On the other hand, asparagine synthetases from eukaryotes 4 -7) use glutamine as the preferred amido nitrogen donor, although they can also use ammonia.…”

Overexpression and Purification of Asparagine Synthetase fromEscherichia coli

“…The active fraction was eluted at a KCl concentration of approximately 0.25 M, and concentrated to about 10 ml on a Amicon UM-10 membrane. The concentrated enzyme was dialyzed against buffer C (the buffer B containing 10mM (CH 3 COOhMg), and then applied to a Blue-Cellulofine column (2.5 x 20 cm) equilibrated with buffer C. The.column was washed with 0.1 M KCl in buffer C, and the enzyme was then eluted with a linear gradient from 0.1 MKCl, 10 mM (CH 3 COOhMg to 1.0 M KCl, 0 mM (CH 3 COOhMg in buffer C. The active fraction was concentrated on the Amicon membrane and dialyzed against buffer B. The puriffed enzyme could be stored at -70°C without loss of activity for at least one month.…”

“…A nucleotide sequence derived from pKK223-3 was underlined with a double line. (CH 3 COOhMg, 1mM EDTA, 30mM KCl, and 5mM 2-mercaptoethanol) and re-collected by centrifugation. The cells were then suspended in 50 ml of buffer A and disrupted by sonication at O°C.…”

“…1 ) These enzymes are distributed in prokaryotes as Escherichia coli 2 ) and Klebsiella aerogenes 3 ) and encoded by asnA genes. On the other hand, asparagine synthetases from eukaryotes 4 -7) use glutamine as the preferred amido nitrogen donor, although they can also use ammonia.…”

Overexpression and Purification of Asparagine Synthetase fromEscherichia coli

“…On the other hand, asparagine synthetase using glutamine as amido nitrogen donor [Laspartate: L-glutamine amido-ligase (AMP-forming) E.C. 6.3.5.4] is found not only in prokaryotes (Humbert & Simoni, 1980;Reitzer & Magasanik, 1982) but also in eukaryotes (Andrulis, Chen & Ray, 1987;Gantt & Arfin, 1981;Hongo & Sato, 1981 ;, and encoded by the asnB gene. Studies of steady-state kinetic mechanisms for both enzymes have demonstrated that the mechanism of the ammonia-dependent enzymes is different from that of the glutamine-dependent enzymes (Cedar & Schwartz, 1969b;Hongo & Sato, 1985;Mehlhaff, Luehr & Schuster, 1985).…”

“…6.3.1.1] catalyzes the synthesis of L-asparagine from L-aspartate and ammonia, with hydrolyzing ATP to AMP and PPi (Meister, 1974). This enzyme is distributed in prokaryotes as Escherichia coli (Cedar & Schwartz, 1969a) and Klebsiella aerogenes (Reitzer & Magasanik, 1982), and encoded by the asnA gene. On the other hand, asparagine synthetase using glutamine as amido nitrogen donor [Laspartate: L-glutamine amido-ligase (AMP-forming) E.C.…”

Crystallization and preliminary crystallographic study of asparagine synthetase fromEscherichia coli

Regulation of Escherichia coli Glutamine Synthetase