The thrH Gene Product of Pseudomonas aeruginosa Is a Dual Activity Enzyme with a Novel Phosphoserine:Homoserine Phosphotransferase Activity

Singh, Shivendra Kumar; Yang, Kun; Karthikeyan, Subramanian; Huynh, Tan‐Phat; Zhang, Xuejun; Phillips, Margaret A.; Zhang, Hong

doi:10.1074/jbc.m311393200

Cited by 20 publications

(23 citation statements)

References 33 publications

(31 reference statements)

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“…These kinetic constants were observed to be lower in comparison with those obtained for PSP enzymes characterized from either Hydrogenobacter thermophiles (K m of 1.6 mM), P. gingivalis (K m of 2.0 mM and 2.6 mM for phosphoserine peptides), or Pseudomonas aeruginosa (K m of 207 M) (26,36,37). We also observed that maximal SerB2 activity was observed in the initial 5 min and that inclusion of 0.01% Triton X-100 enhanced SerB2 activity by 15-20% (Fig.…”

mentioning

confidence: 80%

High Throughput Screen Identifies Small Molecule Inhibitors Specific for Mycobacterium tuberculosis Phosphoserine Phosphatase

Arora

Tiwari

Mandal

et al. 2014

Journal of Biological Chemistry

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Background: Phosphoserine phosphatase (PSP) is an essential enzyme involved in L-serine biosynthesis. Results: High throughput screen was performed to identify specific PSP inhibitors with activity against intracellular bacteria. Conclusion: Validation of PSP as a drug target would lead to identification of scaffolds with a novel mechanism. Significance: This is the first report demonstrating selective inhibition of M. tuberculosis PSP enzyme.

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confidence: 80%

High Throughput Screen Identifies Small Molecule Inhibitors Specific for Mycobacterium tuberculosis Phosphoserine Phosphatase

Arora

Tiwari

Mandal

et al. 2014

Journal of Biological Chemistry

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“…Specific roles in amino acid metabolism continued to be acquired in specific lineages of the bacterial tree; for example, the enolase phosphatase and the phosphoserine:homoserine phosphotransferase respectively in methionine and threonine metabolism. 139,140,150 The other major bacterial innovations were related to sugar metabolism and appear to have occurred somewhat later in bacterial evolution. These sugar metabolism enzymes arose throughout the HAD superfamily, though the cof assemblage appears to be the most dominant amongst them.…”

Section: Post-luca Evolution Of Had Superfamilymentioning

confidence: 99%

“…The related ThrH subfamily, which is restricted to the proteobacteria, participates in the threonine biosynthesis pathway by catalyzing a phosphoserine-homoserine phosphotransfer reaction, similar to the phosphate exchange reaction of SerB. 149,150 The PHOSPHO1 subfamily contains a peculiar C2 cap, which has three conserved cysteine residues, suggesting that it is stabilized by metal chelation. The vertebrate versions of this subfamily are believed to mobilize inorganic phosphate for skeletal matrix mineralization mineralization through their action on phosphocholine and phosphoethanolamine.…”

Section: Tetra-helical Caps: Psp-p5n-1 Assemblagementioning

confidence: 99%

Evolutionary Genomics of the HAD Superfamily: Understanding the Structural Adaptations and Catalytic Diversity in a Superfamily of Phosphoesterases and Allied Enzymes

Burroughs¹,

Allen²,

Dunaway‐Mariano³

et al. 2006

Journal of Molecular Biology

386

520

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The HAD (haloacid dehalogenase) superfamily includes phosphoesterases, ATPases, phosphonatases, dehalogenases, and sugar phosphomutases acting on a remarkably diverse set of substrates. The availability of numerous crystal structures of representatives belonging to diverse branches of the HAD superfamily provides us with a unique opportunity to reconstruct their evolutionary history and uncover the principal determinants that led to their diversification of structure and function. To this end we present a comprehensive analysis of the HAD superfamily that identifies their unique structural features and provides a detailed classification of the entire superfamily. We show that at the highest level the HAD superfamily is unified with several other superfamilies, namely the DHH, receiver (CheY-like), von Willebrand A, TOPRIM, classical histone deacetylases and PIN/FLAP nuclease domains, all of which contain a specific form of the Rossmannoid fold. These Rossmannoid folds are distinguished from others by the presence of equivalently placed acidic catalytic residues, including one at the end of the first core β-strand of the central sheet. The HAD domain is distinguished from these related Rossmannoid folds by two key structural signatures, a "squiggle" (a single helical turn) and a "flap" (a beta hairpin motif) located immediately downstream of the first β-strand of their core Rossmanoid fold. The squiggle and the flap motifs are predicted to provide the necessary mobility to these enzymes for them to alternate between the "open" and "closed" conformations. In addition, most members of the HAD superfamily contains inserts, termed caps, occurring at either of two positions in the core Rossmannoid fold. We show that the cap modules have been independently inserted into these two stereotypic positions on multiple occasions in evolution and display extensive evolutionary diversification independent of the core catalytic domain. The first group of caps, the C1 caps, is directly inserted into the flap motif and regulates access of reactants to the active site. The second group, the C2 caps, forms a roof over the active site, and access to their internal cavities might be in part regulated by the movement of the flap. The diversification of the cap module was a major factor in the exploration of a vast substrate space in the course of the evolution of this superfamily. We show that the HAD superfamily contains 33 major families distributed across the three superkingdoms of life. Analysis of the phyletic patterns suggests that at least five distinct HAD proteins are traceable to the last universal common ancestor (LUCA) of all extant organisms. While these prototypes diverged prior to the emergence Abbreviations used: HAD, haloacid dehalogenase; PNKP, polynucleotide kinase phosphatase; KDO 8-P, deoxy-Dmannose-octulosonate 8-phosphate; CTD, carboxyl-terminal domain; PNKP, polynucleotide kinase phosphatase; LUCA, last universal common ancestor.E-mail address of the corresponding author: aravind@ncbi.nlm.nih.gov of the LUCA, t...

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“…These included GTP, CTP, UTP, PEP, and acetyl-and carbamoylphosphate. Phosphoserine and phosphothreonine were also tested, since they are known substrates of some phosphotransferase enzymes (21,22). The reaction mixture with PEP was subsequently analyzed by the two enzymecoupled assay, while the rest of the reaction mixtures were analyzed by ESI-MS for the presence of 4Ј-phosphopantothenate.…”

Section: Characterization Of a Third Isoform Of Pantothenate Kinase 2mentioning

confidence: 99%

Characterization of a New Pantothenate Kinase Isoform from Helicobacter pylori

Brand

Strauss

2005

Journal of Biological Chemistry

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Pantothenate kinase (PanK) catalyzes the first step in the biosynthesis of the essential and ubiquitous cofactor coenzyme A (CoA) in all organisms. Two well characterized isoforms of the enzyme are known: a prokaryotic PanK that predominates in eubacteria and a eukaryotic isoform that has primarily been characterized from mammalian and plant sources. Curiously, the genomes of certain pathogenic bacteria, including Helicobacter pylori and Pseudomonas aeruginosa, do not contain a PanK similar to either isoform, although these organisms possess all the other biosynthetic machinery required for CoA production. In this study we cloned, overexpressed and characterized an enzyme from Bacillus subtilis and its homologue from H. pylori and show that they catalyze the ATP-dependent phosphorylation of pantothenate. These enzymes do not share sequence homology with any known PanK, and unlike the bacterial and eukaryotic PanK isoforms their activity is not regulated by either CoA or acetyl-CoA. They also do not accept the pantothenic acid antimetabolite N-pentylpantothenamide as a substrate or are inhibited by it. Taken together, these results point to the identification of a third distinct isoform of PanK that accounts for the only known activity of the enzyme in pathogens such as H. pylori and P. aeruginosa.

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The thrH Gene Product of Pseudomonas aeruginosa Is a Dual Activity Enzyme with a Novel Phosphoserine:Homoserine Phosphotransferase Activity

Cited by 20 publications

References 33 publications

High Throughput Screen Identifies Small Molecule Inhibitors Specific for Mycobacterium tuberculosis Phosphoserine Phosphatase

High Throughput Screen Identifies Small Molecule Inhibitors Specific for Mycobacterium tuberculosis Phosphoserine Phosphatase

Evolutionary Genomics of the HAD Superfamily: Understanding the Structural Adaptations and Catalytic Diversity in a Superfamily of Phosphoesterases and Allied Enzymes

Characterization of a New Pantothenate Kinase Isoform from Helicobacter pylori

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