The degradation of <scp>l</scp>-histidine, imidazolyl-<scp>l</scp>-lactate and imidazolylpropionate by <i>Pseudomonas testosteroni</i>

Coote, J. G.; Hassall, H.

doi:10.1042/bj1320409

Cited by 22 publications

(26 citation statements)

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“…Very recently, the complete genome sequence of C. resistens DSM 45100 has been determined to delineate the putative lifestyle of this opportunistic pathogen on the human body (Schröder et al, 2012). The protein products of orthologous genes catalyze the four-step conversion of L-histidine to L-glutamate (Coote & Hassall, 1973). 1).…”

Section: Introductionmentioning

confidence: 99%

“…1). The protein products of orthologous genes catalyze the four-step conversion of L-histidine to L-glutamate (Coote & Hassall, 1973). The presence of this pathway in C. resistens is remarkable, as this species probably colonizes the fatty and histidine-rich inguinal and perineal regions of the human body and thus lives in close proximity to the female genital tract (Schröder et al, 2012).…”

Section: Introductionmentioning

confidence: 99%

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Binding of the IclR-type regulator HutR in the histidine utilization (hut) gene cluster of the human pathogen Corynebacterium resistens DSM 45100

Schröder

Maus

Ostermann

et al. 2012

FEMS Microbiol Lett

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The genome of the human pathogen Corynebacterium resistens DSM 45100 is equipped with a histidine utilization (hut) gene cluster encoding a four‐step pathway for the catabolism of l‐histidine and a transcriptional regulator of the IclR superfamily, now named HutR. The utilization of l‐histidine might be relevant for the growth of C. resistens in its natural habitat, probably the histidine‐rich inguinal and perineal areas of the human body. The ability of C. resistens to utilize l‐histidine as a sole source of nitrogen was demonstrated by growth assays in synthetic minimal media. Reverse transcriptase PCRs revealed enhanced transcript levels of the hut genes in C. resistens cells grown in the presence of l‐histidine. Promoter‐probe assays showed that the hut genes are organized in three transcription units: hutHUI, hutR, and hutG. The respective transcriptional start sites were mapped by 5′ RACE‐PCR to detected putative promoter regions. DNA band shift assays with purified HutR protein identified the 14‐bp DNA sequence TCTGwwATwCCAGA located upstream of the mapped promoters. This DNA motif includes a 4‐bp terminal palindrome, which turned out to be essential for HutR binding in vitro. These data add a new physiological function to the large IclR family of transcriptional regulators.

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Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Binding of the IclR-type regulator HutR in the histidine utilization (hut) gene cluster of the human pathogen Corynebacterium resistens DSM 45100

Schröder

Maus

Ostermann

et al. 2012

FEMS Microbiol Lett

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“…In bacteria, catabolism of histidine occurs via either a four or a five-step enzymatic pathway (Coote and Hassall 1973a;Magasanik 1978). The first three steps, from histidine to urocanate, to imidazolone propionate (IPA), to formiminoglutamate (FIGLU), are catalyzed by the gene products of hutH, hutU, and hutI, respectively, and are common to both the four-step and the five-step pathways (outlined in Figure 1A).…”

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Genetic Analysis of the Histidine Utilization (hut) Genes in Pseudomonas fluorescens SBW25

2007

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The histidine utilization (hut) locus of Pseudomonas fluorescens SBW25 confers the ability to utilize histidine as a sole carbon and nitrogen source. Genetic analysis using a combination of site-directed mutagenesis and chromosomally integrated lacZ fusions showed the hut locus to be composed of 13 genes organized in 3 transcriptional units: hutF, hutCD, and 10 genes from hutU to hutG (which includes 2 copies of hutH, 1 of which is nonfunctional). Inactivation of hutF eliminated the ability to grow on histidine, indicating that SBW25 degrades histidine by the five-step enzymatic pathway. The 3 hut operons are negatively regulated by the HutC repressor with urocanate (the first intermediate of the histidine degradation pathway) as the physiological inducer. 59-RACE analysis of transcriptional start sites revealed involvement of both s 54 (for the hutU-G operon) and s 70 (for hutF ); the involvement of s 54 was experimentally demonstrated. CbrB (an enhancer binding protein for s 54 recruitment) was required for bacterial growth on histidine, indicating positive control of hut gene expression by CbrB. Recognition that a gene (named hutD) encoding a widely distributed conserved hypothetical protein is transcribed along with hutC led to analysis of its role. Mutational and gene fusion studies showed that HutD functions independently of HutC. Growth and fitness assays in laboratory media and on sugar beet seedlings suggest that HutD acts as a governor that sets an upper bound to the level of hut activity.

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“…The histidine degradation pathway in Pseudomonas species consists of five reactions (8,16), while four steps are required in most other organisms which have been studied, e.g., Salmonella typhimurium (18), Klebsiella aerogenes (17), Bacillus subtilis (6), and mammalian species (26). The enzymes and their genes required by Pseudomonas putida for the conversion of histidine to glutamate plus formate and ammonia are: histidase (hutH), urocanase (hutU), imidazolone propionate hydrolase (IPAase) (hutl), formiminoglutamate iminohydrolase (FIGLUase) (hutF), and formylglutamate amidohydrolase (FGase) (hutG).…”

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Organization and multiple regulation of histidine utilization genes in Pseudomonas putida

Phillips

1988

J Bacteriol

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The arrangement of the histidine utilization (hut) genes in Pseudomonas putida was established by examining the structure of a DNA segment that had been cloned into Eschericaha coli via a cosmid vector. Southern blot analysis revealed that the restriction patterns of the hut genes cloned into E. coli and present in the P. putida genome were identical, indicating that no detectable DNA rearrangement took place during the cloning. Expression of the hut genes from a series of overlapping clones indicated the gene order to be hutG-hutl-hutHhutU-hutC-hutF. The transcription directions of the different hut genes were determined by cloning the genes under control of the lambda PL promoter. This showed that hutF, encoding formiminoglutamate hydrolase, was transcribed in a direction opposite to that of the other genes. Inactivation of the cloned hut genes by Tn)000 insertion revealed that the hut genes were divided into three major transcriptional units (hutF, huiC [the repressor gene], and hutUHIG), but huiG may also be independently transcribed. When cloned individually with hutC on the same vector, hutF and hutU (which encodes urocanase) expression was induced by urocanate, indicating that these two genes each possess an operator-promoter element. TnlOOO insertions (in the cloned genes) or Tn5 insertions (in the P. putida genome) affecting the hutI or hutH gene only partially eliminated huiG expression. Furthermore, hutG, which specifies N-formylglutamate amidohydrolase, was regulated by the huic product when the two genes were cloned on the same vector and expressed in E. coli. Therefore, hutG can be expressed independently from its own promoter, in keeping with earlier observations that N-formylglutamate amidohydrolase synthesis is not coordinated with that of urocanase and histidase and can be induced by N-formylglutamiate or urocanate.

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The degradation of l-histidine, imidazolyl-l-lactate and imidazolylpropionate by Pseudomonas testosteroni

Cited by 22 publications

References 26 publications

Binding of the IclR-type regulator HutR in the histidine utilization (hut) gene cluster of the human pathogen Corynebacterium resistens DSM 45100

Binding of the IclR-type regulator HutR in the histidine utilization (hut) gene cluster of the human pathogen Corynebacterium resistens DSM 45100

Genetic Analysis of the Histidine Utilization (hut) Genes in Pseudomonas fluorescens SBW25

Organization and multiple regulation of histidine utilization genes in Pseudomonas putida

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