Evaluation of PE_PGRS33 as a potential surface target for humoral responses against Mycobacterium tuberculosis

Minerva, Mariachiara; Maio, Flavio De; Camassa, Serena; Battah, Basem; Palucci, Ivana; Manganelli, Riccardo; Sanguinetti, Maurizio; Sali, Michela; Delogu, Giovanni

doi:10.1093/femspd/ftx100

Cited by 12 publications

(24 citation statements)

References 23 publications

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“…Of note, PE_PGRS33 was able to interact with TLR2 to promote cell death and inflammation [ 42 ] and proper localization of PE_PGRS33 on the mycobacterial surface is required to activate the TLR2 pathway [ 55 ]. Moreover, an antiserum directed against the native form of PE_PGRS33 was able to abolish the secretion of TNF-α following infection of macrophages with M. smegmatis expressing PE_PGRS33, further supporting the key role of PE_PGRS33-TLR2 interaction [ 81 ]. In line with these findings, the Mtb Δ pe_pgrs 33 mutant was impaired, compared to the parental strain, in its ability to enter in macrophages, but not epithelial cells, in a process involving activation of the TLR2-CR3 pathway, which activates the inside-out-signaling to promote Mtb entry in macrophages [ 44 ].…”

Section: Experimental Evidences On Pe_pgrssmentioning

confidence: 94%

“…Heterologous expression of PE_PGRS33 in M. smegmatis promoted cell death and increased mycobacterial survival in macrophages and in intraperitoneally infected mice over the parental strain or the M. smegmatis recombinant strain expressing only the PE domain of PE_PGRS33, pointing for the key role of the PGRS domain in this process [ 42 , 78 , 79 ]. PE_PGRS33 triggered TNF-α and IL-12 secretion promoting cell necrosis and inflammation, as highlighted by the enlarged spleens of mice infected with M. smegmatis expressing PE_PGRS33 compared to controls [ 55 , 78 , 80 , 81 ]. However, experiments carried out with the purified recombinant protein or in eukaryotic cells transfected with a plasmid expressing PE_PGRS33, while confirming the ability of PE_PGRS33 to promote cell death implicated a mechanism involving apoptosis rather than necrosis [ 42 , 79 ].…”

Section: Experimental Evidences On Pe_pgrssmentioning

confidence: 99%

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PE_PGRS proteins ofMycobacterium tuberculosis: A specialized molecular task force at the forefront of host–pathogen interaction

et al. 2020

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To the PE_PGRS protein subfamily belongs a group of surface-exposed mycobacterial antigens that in Mycobacterium tuberculosis ( Mtb ) H37Rv accounts to more than 65 genes, 51 of which are thought to express a functional protein. PE_PGRS proteins share a conserved structural architecture with three main domains: the N-terminal PE domain; the PGRS domain, that can vary in sequence and size and is characterized by the presence of multiple GGA-GGX amino acid repeats; the highly conserved sequence containing the GRPLI motif that links the PE and PGRS domains; the unique C-terminus end that can vary in size from few to up to ≈ 300 amino acids. pe_pgrs genes emerged in slow-growing mycobacteria and expanded and diversified in MTBC and few other pathogenic mycobacteria. Interestingly, despite sequence homology and apparent redundancy, PE_PGRS proteins seem to have evolved a peculiar function. In this review, we summarize the actual knowledge on this elusive protein family in terms of evolution, structure, and function, focusing on the role of PE_PGRS in TB pathogenesis. We provide an original hypothesis on the role of the PE domain and propose a structural model for the polymorphic PGRS domain that might explain how so similar proteins can have different physiological functions.

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Section: Experimental Evidences On Pe_pgrssmentioning

confidence: 94%

Section: Experimental Evidences On Pe_pgrssmentioning

confidence: 99%

PE_PGRS proteins ofMycobacterium tuberculosis: A specialized molecular task force at the forefront of host–pathogen interaction

et al. 2020

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“…Conversely, Mtb infection was carried out using an MOI of 1 (1 : 1 bacterium to cell ratio) and the initial infection was for 1 hour instead of 4 hours, in line with our previous research. 50,51 In the third experimental setting, macrophages were pre-treated with medium alone and medium containing GO (1000 mg ml À1 , 100 mg ml À1 and 10 mg ml À1 ) or gentamycin (10 mg ml À1 ). Four hours later, the macrophages were infected with Ms GFP (MOI 10) or Mtb GFP (MOI 1) and CFUs were obtained as previously described.…”

Section: Mycobacterial Infectionmentioning

confidence: 99%

Graphene oxide prevents mycobacteria entry into macrophages through extracellular entrapment

et al. 2019

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“…Our present results show that Rv1768 is located in the bacterial CW and only exits in H37Rv and H37Ra, not in M. avium, Ms, M. marinum, M. intracellulare, or BCG. Some other members of the M. tb PE_PGRS family, for example, PE_PGRS33, are surface-exposed proteins that interact with TLR2 on host macrophages to induce inflammatory signals and promote entry into macrophages (Minerva et al, 2017). PE_PGRS3 mediates adhesion and persistence in host cells (De Maio et al, 2018).…”

Section: Discussionmentioning

confidence: 99%

PE_PGRS31-S100A9 Interaction Promotes Mycobacterial Survival in Macrophages Through the Regulation of NF-κB-TNF-α Signaling and Arachidonic Acid Metabolism

et al. 2020

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Mycobacterium tuberculosis (M. tb) evades the surveillance of immune responses for survival in macrophages. However, the precise mechanism and toxins/proteins encoded by M. tb involved in the bacterial escape remain elusive. The function of Rv1768 protein (also referred to as PE_PGRS31, belonging to the PE_PGRS family) encoded by the region of deletion 14 (RD-14) in the virulent M. tb H37Rv strain has not, to the best of our knowledge, been reported previously. Here, we found that Rv1768 remarkably promotes bacterial survival in macrophages. Compared to wild type (WT) H37Rv, the Rv1768 deficient strain (H37Rv 1768) showed significantly decreased colony-forming units in the lungs, spleen, and liver of the murine M. tb infection model. The bacterial burdens of WT H37Rv in WT macrophages and C57BL/6 mice were significantly higher than those in S100A9 deficiency cells and mice, but there were no significant differences for H37Rv Rv1768. Rv1768 binds S100A9 with the proline-glutamic acid domain (PE domain) and blocks the interaction between S100A9 and Toll-like receptor 4 (TLR4), and suppresses TLR4-myeloid differentiation factor 88-nuclear factor-kappa B (NF-κB)-tumor necrosis factor α (TNF-α) signaling in macrophages. Interestingly, Rv1768 binding to S100A9 also disturbs the metabolism of arachidonic acid by activating 5-lipoxygenase, increasing lipotoxin A4, and down-regulating cyclooxygenase-2 and prostaglandin E2 expression, thus, promoting mycobacterial survival. Our results revealed that M. tb Rv1768 promotes mycobacterial survival in macrophages by regulating NF-κB-TNF-α signaling and arachidonic acid metabolism via S100A9. Disturbing the interaction between Rv1768 and S100A9 may be a potential therapeutic target for tuberculosis.

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Evaluation of PE_PGRS33 as a potential surface target for humoral responses against Mycobacterium tuberculosis

Cited by 12 publications

References 23 publications

PE_PGRS proteins ofMycobacterium tuberculosis: A specialized molecular task force at the forefront of host–pathogen interaction

PE_PGRS proteins ofMycobacterium tuberculosis: A specialized molecular task force at the forefront of host–pathogen interaction

Graphene oxide prevents mycobacteria entry into macrophages through extracellular entrapment

PE_PGRS31-S100A9 Interaction Promotes Mycobacterial Survival in Macrophages Through the Regulation of NF-κB-TNF-α Signaling and Arachidonic Acid Metabolism

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