Identification and structural characterization of a histidinol phosphate phosphatase from Mycobacterium tuberculosis

Jha, Bhavya; Kumar, Deepak; Sharma, Arun; Dwivedy, Abhisek; Singh, Ramandeep; Biswal, B.K.

doi:10.1074/jbc.ra118.002299

Cited by 11 publications

(15 citation statements)

References 56 publications

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“…In order to delineate the role of bacterial histidine biosynthesis in Mtb infection, we examined the dynamics of cellular expression of the histidine biosynthesis pathway enzymes as the infection progresses. For this, three key enzymes of the pathway – imidazole glycerol phosphate dehydratase ( hisB , Rv1601) 24 , histidinol dehydrogenase ( hisD , Rv1599) 18 and histidinol phosphate phosphatase ( hisN , Rv3137) 25 , 26 , well known for their essentiality were chosen. These enzymes were overexpressed and purified to homogeneity using appropriate protocols (Supplementary Fig.…”

Section: Resultsmentioning

confidence: 99%

“…Expression clones of hisB 10 and hisN 25 were available, whereas hisD expression plasmid was prepared. Briefly, the corresponding ORF was amplified using gene specific primers and cloned into an expression vector pYUB-1062, overexpressed in a M. smegmatis mc 2 -4517 system and the protein was purified to homogeneity by using Ni 2+ -NTA affinity chromatography, followed by size exclusion chromatography.…”

Section: Methodsmentioning

confidence: 99%

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De novo histidine biosynthesis protects Mycobacterium tuberculosis from host IFN-γ mediated histidine starvation

et al. 2021

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Intracellular pathogens including Mycobacterium tuberculosis (Mtb) have evolved with strategies to uptake amino acids from host cells to fulfil their metabolic requirements. However, Mtb also possesses de novo biosynthesis pathways for all the amino acids. This raises a pertinent question- how does Mtb meet its histidine requirements within an in vivo infection setting? Here, we present a mechanism in which the host, by up-regulating its histidine catabolizing enzymes through interferon gamma (IFN-γ) mediated signalling, exerts an immune response directed at starving the bacillus of intracellular free histidine. However, the wild-type Mtb evades this host immune response by biosynthesizing histidine de novo, whereas a histidine auxotroph fails to multiply. Notably, in an IFN-γ−/− mouse model, the auxotroph exhibits a similar extent of virulence as that of the wild-type. The results augment the current understanding of host-Mtb interactions and highlight the essentiality of Mtb histidine biosynthesis for its pathogenesis.

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Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

De novo histidine biosynthesis protects Mycobacterium tuberculosis from host IFN-γ mediated histidine starvation

et al. 2021

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“…This entire complex with both dehydratase and phosphatase activities is commonly known as HisB. However, in other organisms, such as Mtb , 26,27 fungi 28 and plants, 29,30 these enzymes are not fused. They operate separately and are encoded by two separate ORFs.…”

Section: Introductionmentioning

confidence: 99%

“…Owing to the absence of both structural and functional homologs of IGPD in mammals, this enzyme has been a major anti‐herbs 31‐33 target. IGPD has also been regarded as a promising anti‐bacterial 34,35 and anti‐fungal 36 drug target.Over the past decade, to derive a mechanistic understanding of histidine production by Mtb , which could assist in developing target‐specific anti‐TB small molecules, we have structurally and biochemically characterized IGPD, 26 HisC 37 and HisN 27 of this pathway. IGPD being an important anti‐bacterial drug target, 38 we sought to determine its 3D structure at a higher resolution to obtain a better model comprising more precise structural information for the design of IGPD specific anti‐TB inhibitors through a structure‐guided approach.…”

Section: Introductionmentioning

confidence: 99%

Characterization of a triazole scaffold compound as an inhibitor of Mycobacterium tuberculosis imidazoleglycerol‐phosphate dehydratase

et al. 2021

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Mycobacterium tuberculosis (Mtb), the causative agent of human tuberculosis (TB), employs ten enzymes including imidazoleglycerol‐phosphate dehydratase (IGPD) for de novo biosynthesis of histidine. The absence of histidine‐biosynthesis in humans combined with its essentiality for Mtb makes the enzymes of this pathway major anti‐TB drug targets. We explored the inhibitory potential of a small molecule β‐(1,2,4‐Triazole‐3‐yl)‐DL‐alanine (DLA) against Mtb IGPD. DLA exhibits an in vitro inhibitory efficacy in the lower micromolar range. Higher‐resolution crystal structures of native and substrate‐bound Mtb IGPD provided additional structural features of this important drug target. Crystal structure of IGPD‐DLA complex at a resolution of 1.75 Å, confirmed that DLA locks down the function of the enzyme by binding in the active site pocket of the IGPD mimicking the substrate‐binding mode to a high degree. In our biochemical study, DLA showed an efficient inhibition of Mtb IGPD. Furthermore, DLA also showed bactericidal activity against Mtb and Mycobacterium smegmatis and inhibited their growth in respective culture medium. Importantly, owing to the favorable ADME and physicochemical properties, it serves as an important lead molecule for further derivatizations.

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“…In order to identify the protein, mass-spectrometric analysis was employed. The protein band of the appropriate size was excised from the SDS polyacrylamide gel and processed as described elsewhere (Jha et al, 2018). The extracted protein was subjected to trypsin digestion, following which the peptides were analyzed by MALDI-TOF MS/MS (TOF/TOF 5800 analyzer, SCIEX, Shanghai, People's Republic of China) for peptide mass fingerprinting.…”

Section: Protein Purification and Crystallizationmentioning

confidence: 99%

Serendipitous crystallization and structure determination of bacterioferritin from Achromobacter

et al. 2018

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Bacterioferritins (Bfrs) are ferritin-like molecules with a hollow spherical 24-mer complex design that are unique to bacterial and archaeal species. They play a critical role in storing iron(III) within the complex at concentrations much higher than the feasible solubility limits of iron(III), thus maintaining iron homeostasis within cells. Here, the crystal structure of bacterioferritin from Achromobacter (Ach Bfr) that crystallized serendipitously during a crystallization attempt of an unrelated mycobacterial protein is reported at 1.95 Å resolution. Notably, Fe atoms were bound to the structure along with a porphyrin ring sandwiched between the subunits of a dimer. Furthermore, the dinuclear ferroxidase center of Ach Bfr has only a single iron bound, in contrast to the two Fe atoms in other Bfrs. The structure of Ach Bfr clearly demonstrates the substitution of a glutamate residue, which is involved in the interaction with the second Fe atom, by a threonine and the consequent absence of another Fe atom there. The iron at the dinuclear center has a tetravalent coordination, while a second iron with a hexavalent coordination was found within the porphyrin ring, generating a heme moiety. Achromobacter spp. are known opportunistic pathogens; this structure enhances the current understanding of their iron metabolism and regulation, and importantly will be useful in the design of small-molecule inhibitors against this protein through a structure-guided approach.

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Identification and structural characterization of a histidinol phosphate phosphatase from Mycobacterium tuberculosis

Cited by 11 publications

References 56 publications

De novo histidine biosynthesis protects Mycobacterium tuberculosis from host IFN-γ mediated histidine starvation

De novo histidine biosynthesis protects Mycobacterium tuberculosis from host IFN-γ mediated histidine starvation

Characterization of a triazole scaffold compound as an inhibitor of Mycobacterium tuberculosis imidazoleglycerol‐phosphate dehydratase

Serendipitous crystallization and structure determination of bacterioferritin from Achromobacter

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