Journal article
Roles of PucR, G1nR, and TnrA in regulating expression of the Bacillus subtilis ure p3 promoter
Expression of the P3 promoter of the Bacillus subtilis ureABC operon is activated during nitrogen-limited growth by PucR, the transcriptional regulator of the purine-degradative genes. Addition of allantoic acid, a purine-degradative intermediate, to nitrogen-limited cells stimulated transcription of ure P3 twofold.
Since urea is produced during purine degradation in B. subtilis, regulation of ureABC expression by PucR allows purines to be completely degraded to ammonia. The nitrogen transcription factor TnrA was found to indirectly regulate ure P3 expression by activating pucR expression. The two consensus GlnR/TnrA binding sites located in the ure P3 promoter region were shown to be required for negative regulation by GlnR.
Mutational analysis indicates that a cooperative interaction occurs between GlnR dimers bound at these two sites. B. subtilis is the first example where urease expression is both nitrogen regulated and coordinately regulated with the enzymes involved in purine transport and degradation.
| Language: | English |
|---|---|
| Publisher: | American Society for Microbiology |
| Year: | 2002 |
| Pages: | 6060-6064 |
| ISSN: | 10985530 , 00219193 and 10678832 |
| Types: | Journal article |
| DOI: | 10.1128/JB.184.21.6060-6064.2002 |
| ORCIDs: | Jarmer, Hanne Østergaard |
Bacillus subtilis Bacterial Proteins Base Sequence Culture Media DNA-Binding Proteins Gene Expression Regulation, Bacterial Genes, Bacterial GlnR protein, Streptomyces coelicolor Molecular Sequence Data Nitrogen Promoter Regions, Genetic Repressor Proteins ScgR protein, Bacillus subtilis Trans-Activators Transcription Factors
