Microbiology & Immunology - Research Publications

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Author: Pidot, Sacha × End date: 2019 × Start date: 2010 × Type: Journal Article ×

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    Struktur und Biosynthese der Isatropolone, bioaktiver und Amin‐reaktiver fluoreszierender Naturstoffe aus Streptomyces Gö66
    Cai, X ; Shi, Y ; Pöhlmann, N ; Revermann, O ; Bahner, I ; Pidot, SJ ; Wesche, F ; Lackner, H ; Büchel, C ; Kaiser, M ; Richter, C ; Schwalbe, H ; Stinear, TP ; Zeeck, A ; Bode, HB (Wiley, 2017-04-24)
    Abstract Die Naturstoffe Isatropolon A–C (1–3) wurden aus Streptomyces Gö66 reisoliert, und insbesondere 1 und 3 zeigen sehr gute Aktivität gegen Leishmania donovani. Sie tragen einen ungewöhnlichen Tropolonring, der über einen Typ‐II‐Polyketid‐Biosyntheseweg aufgebaut wird. Ihre Biosynthese wurde mithilfe von Markierungsexperimenten, einer Analyse des Biosynthese‐Genclusters, heterologer Expression des Hauptteils des Genclusters und strukturelle Charakterisierung verschiedener Intermediate aufgeklärt. Aufgrund eines 1,5‐Diketon‐Strukturelementes können die Isatropolone mit Ammoniak und Aminen und insbesondere Lysin sowie Lysin‐tragenden Peptiden und Proteinen reagieren und einen Pyridinring bilden. Dabei ändern sich die Fluoreszenz‐Eigenschaften so deutlich, dass die so markierten Peptide und Proteine sehr einfach sichtbar gemacht werden können.
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    Biosynthesis and Ether-Bridge Formation in Nargenicin Macrolides
    Pidot, SJ ; Herisse, M ; Sharkey, L ; Atkin, L ; Porter, JL ; Seemann, T ; Howden, BP ; Rizzacasa, MA ; Stinear, TP (WILEY-V C H VERLAG GMBH, 2019-03-18)
    The nargenicin family of antibiotics are macrolides containing a rare ether-bridged cis-decalin motif. Several of these compounds are highly active against multi-drug resistant organisms. Despite the identification of the first members of this family almost 40 years ago, the genetic basis for the production of these molecules and the enzyme responsible for formation of the oxa bridge, remain unknown. Here, the 85 kb nargenicin biosynthetic gene cluster was identified from a human pathogenic Nocardia arthritidis isolate and this locus is solely responsible for nargenicin production. Further investigation of this locus revealed a putative iron-α-ketoglutarate-dependent dioxygenase, which was found to be responsible for the formation of the ether bridge from the newly identified deoxygenated precursor, 8,13-deoxynargenicin. Uncovering the nargenicin biosynthetic locus provides a molecular basis for the rational bioengineering of these interesting antibiotic macrolides.
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    Mining the Methylome Reveals Extensive Diversity in Staphylococcus epidermidis Restriction Modification
    Lee, JYH ; Carter, GP ; Pidot, SJ ; Guerillot, R ; Seemann, T ; da Silva, AG ; Foster, TJ ; Howden, BP ; Stinear, TP ; Monk, IR ; Torres, VJ (AMER SOC MICROBIOLOGY, 2019-12-17)
    Staphylococcus epidermidis is a significant opportunistic pathogen of humans. Molecular studies in this species have been hampered by the presence of restriction-modification (RM) systems that limit introduction of foreign DNA. Here, we establish the complete genomes and methylomes for seven clinically significant, genetically diverse S. epidermidis isolates and perform the first systematic genomic analyses of the type I RM systems within both S. epidermidis and Staphylococcus aureus Our analyses revealed marked differences in the gene arrangement, chromosomal location, and movement of type I RM systems between the two species. Unlike S. aureus, S. epidermidis type I RM systems demonstrate extensive diversity even within a single genetic lineage. This is contrary to current assumptions and has important implications for approaching the genetic manipulation of S. epidermidis Using Escherichia coli plasmid artificial modification (PAM) to express S. epidermidishsdMS, we readily overcame restriction barriers in S. epidermidis and achieved electroporation efficiencies equivalent to those of modification-deficient mutants. With these functional experiments, we demonstrated how genomic data can be used to predict both the functionality of type I RM systems and the potential for a strain to be electroporation proficient. We outline an efficient approach for the genetic manipulation of S. epidermidis strains from diverse genetic backgrounds, including those that have hitherto been intractable. Additionally, we identified S. epidermidis BPH0736, a naturally restriction-defective, clinically significant, multidrug-resistant ST2 isolate, as an ideal candidate for molecular studies.IMPORTANCEStaphylococcus epidermidis is a major cause of hospital-acquired infections, especially those related to implanted medical devices. Understanding how S. epidermidis causes disease and devising ways to combat these infections have been hindered by an inability to genetically manipulate clinically significant hospital-adapted strains. Here, we provide the first comprehensive analyses of the barriers to the uptake of foreign DNA in S. epidermidis and demonstrate that these are distinct from those described for S. aureus Using these insights, we demonstrate an efficient approach for the genetic manipulation of S. epidermidis to enable the study of clinical isolates for the first time.
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    Biosynthesis and Ether‐Bridge Formation in Nargenicin Macrolides
    Pidot, SJ ; Herisse, M ; Sharkey, L ; Atkin, L ; Porter, JL ; Seemann, T ; Howden, BP ; Rizzacasa, MA ; Stinear, TP (Wiley, 2019)
    Abstract: The nargenicin family of antibiotics are macrolides containing a rare ether‐bridged cis‐decalin motif. Several of these compounds are highly active against multi‐drug resistant organisms. Despite the identification of the first members of this family almost 40 years ago, the genetic basis for the production of these molecules and the enzyme responsible for formation of the oxa bridge, remain unknown. Here, the 85 kb nargenicin biosynthetic gene cluster was identified from a human pathogenic Nocardia arthritidis isolate and this locus is solely responsible for nargenicin production. Further investigation of this locus revealed a putative iron‐α‐ketoglutarate‐dependent dioxygenase, which was found to be responsible for the formation of the ether bridge from the newly identified deoxygenated precursor, 8,13‐deoxynargenicin. Uncovering the nargenicin biosynthetic locus provides a molecular basis for the rational bioengineering of these interesting antibiotic macrolides.
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    Zinc-binding to the cytoplasmic PAS domain regulates the essential WalK histidine kinase of Staphylococcus aureus
    Monk, IR ; Shaikh, N ; Begg, SL ; Gajdiss, M ; Sharkey, LKR ; Lee, JYH ; Pidot, SJ ; Seemann, T ; Kuiper, M ; Winnen, B ; Hvorup, R ; Collins, BM ; Bierbaum, G ; Udagedara, SR ; Morey, JR ; Pulyani, N ; Howden, BP ; Maher, MJ ; McDevitt, CA ; King, GF ; Stinear, TP (NATURE PUBLISHING GROUP, 2019-07-11)
    WalKR (YycFG) is the only essential two-component regulator in the human pathogen Staphylococcus aureus. WalKR regulates peptidoglycan synthesis, but this function alone does not explain its essentiality. Here, to further understand WalKR function, we investigate a suppressor mutant that arose when WalKR activity was impaired; a histidine to tyrosine substitution (H271Y) in the cytoplasmic Per-Arnt-Sim (PASCYT) domain of the histidine kinase WalK. Introducing the WalKH271Y mutation into wild-type S. aureus activates the WalKR regulon. Structural analyses of the WalK PASCYT domain reveal a metal-binding site, in which a zinc ion (Zn2+) is tetrahedrally-coordinated by four amino acids including H271. The WalKH271Y mutation abrogates metal binding, increasing WalK kinase activity and WalR phosphorylation. Thus, Zn2+-binding negatively regulates WalKR. Promoter-reporter experiments using S. aureus confirm Zn2+ sensing by this system. Identification of a metal ligand recognized by the WalKR system broadens our understanding of this critical S. aureus regulon.
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    Genomics-Driven Discovery of NO-Donating Diazeniumdiolate Siderophores in Diverse Plant-Associated Bacteria
    Hermenau, R ; Mehl, JL ; Ishida, K ; Dose, B ; Pidot, S ; Stinear, TP ; Hertweck, C (WILEY-V C H VERLAG GMBH, 2019-09-09)
    Siderophores are key players in bacteria-host interactions, with the main function to provide soluble iron for their producers. Gramibactin from rhizosphere bacteria expands siderophore function and diversity as it delivers iron to the host plant and features an unusual diazeniumdiolate moiety for iron chelation. By mutational analysis of the grb gene cluster, we identified genes (grbD and grbE) necessary for diazeniumdiolate formation. Genome mining using a GrbD-based network revealed a broad range of orthologous gene clusters in mainly plant-associated Burkholderia/Paraburkholderia species. Two new types of diazeniumdiolate siderophores, megapolibactins and plantaribactin were fully characterized. In vitro assays and in vivo monitoring experiments revealed that the iron chelators also liberate nitric oxide (NO) in plant roots. This finding is important since NO donors are considered as biofertilizers that maintain iron homeostasis and increase overall plant fitness.
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    A Major Role for Mammals in the Ecology of Mycobacterium ulcerans
    Fyfe, JAM ; Lavender, CJ ; Handasyde, KA ; Legione, AR ; O'Brien, CR ; Stinear, TP ; Pidot, SJ ; Seemann, T ; Benbow, ME ; Wallace, JR ; McCowan, C ; Johnson, PDR ; Zinsstag, J (PUBLIC LIBRARY SCIENCE, 2010-08)
    BACKGROUND: Mycobacterium ulcerans is the causative agent of Buruli ulcer (BU), a destructive skin disease found predominantly in sub-Saharan Africa and south-eastern Australia. The precise mode(s) of transmission and environmental reservoir(s) remain unknown, but several studies have explored the role of aquatic invertebrate species. The purpose of this study was to investigate the environmental distribution of M. ulcerans in south-eastern Australia. METHODOLOGY/PRINCIPAL FINDINGS: A range of environmental samples was collected from Point Lonsdale (a small coastal town southwest of Melbourne, Australia, endemic for BU) and from areas with fewer or no reported incident cases of BU. Mycobacterium ulcerans DNA was detected at low levels by real-time PCR in soil, sediment, water residue, aquatic plant biofilm and terrestrial vegetation collected in Point Lonsdale. Higher levels of M. ulcerans DNA were detected in the faeces of common ringtail (Pseudocheirus peregrinus) and common brushtail (Trichosurus vulpecula) possums. Systematic testing of possum faeces revealed that M. ulcerans DNA could be detected in 41% of faecal samples collected in Point Lonsdale compared with less than 1% of faecal samples collected from non-endemic areas (p<0.0001). Capture and clinical examination of live possums in Point Lonsdale validated the accuracy of the predictive value of the faecal surveys by revealing that 38% of ringtail possums and 24% of brushtail possums had laboratory-confirmed M. ulcerans skin lesions and/or M. ulcerans PCR positive faeces. Whole genome sequencing revealed an extremely close genetic relationship between human and possum M. ulcerans isolates. CONCLUSIONS/SIGNIFICANCE: The prevailing wisdom is that M. ulcerans is an aquatic pathogen and that BU is acquired by contact with certain aquatic environments (swamps, slow-flowing water). Now, after 70 years of research, we propose a transmission model for BU in which terrestrial mammals are implicated as reservoirs for M. ulcerans.
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    Mycobacterium ulcerans and Other Mycolactone-Producing Mycobacteria Should Be Considered a Single Species
    Pidot, SJ ; Asiedu, K ; Kaeser, M ; Fyfe, JAM ; Stinear, TP ; Phillips, RO (PUBLIC LIBRARY SCIENCE, 2010-07)
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    Single Nucleotide Polymorphism Typing of Mycobacterium ulcerans Reveals Focal Transmission of Buruli Ulcer in a Highly Endemic Region of Ghana
    Roeltgen, K ; Qi, W ; Ruf, M-T ; Mensah-Quainoo, E ; Pidot, SJ ; Seemann, T ; Stinear, TP ; Kaeser, M ; Yeboah-Manu, D ; Pluschke, G ; Picardeau, M (PUBLIC LIBRARY SCIENCE, 2010-07)
    Buruli ulcer (BU) is an emerging necrotizing disease of the skin and subcutaneous tissue caused by Mycobacterium ulcerans. While proximity to stagnant or slow flowing water bodies is a risk factor for acquiring BU, the epidemiology and mode of M. ulcerans transmission is poorly understood. Here we have used high-throughput DNA sequencing and comparisons of the genomes of seven M. ulcerans isolates that appeared monomorphic by existing typing methods. We identified a limited number of single nucleotide polymorphisms (SNPs) and developed a real-time PCR SNP typing method based on these differences. We then investigated clinical isolates of M. ulcerans on which we had detailed information concerning patient location and time of diagnosis. Within the Densu river basin of Ghana we observed dominance of one clonal complex and local clustering of some of the variants belonging to this complex. These results reveal focal transmission and demonstrate, that micro-epidemiological analyses by SNP typing has great potential to help us understand how M. ulcerans is transmitted.
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    Serological Evaluation of Mycobacterium ulcerans Antigens Identified by Comparative Genomics
    Pidot, SJ ; Porter, JL ; Marsollier, L ; Chauty, A ; Migot-Nabias, F ; Badaut, C ; Benard, A ; Ruf, M-T ; Seemann, T ; Johnson, PDR ; Davies, JK ; Jenkin, GA ; Pluschke, G ; Stinear, TP ; Phillips, RO (PUBLIC LIBRARY SCIENCE, 2010-11)
    A specific and sensitive serodiagnostic test for Mycobacterium ulcerans infection would greatly assist the diagnosis of Buruli ulcer and would also facilitate seroepidemiological surveys. By comparative genomics, we identified 45 potential M. ulcerans specific proteins, of which we were able to express and purify 33 in E. coli. Sera from 30 confirmed Buruli ulcer patients, 24 healthy controls from the same endemic region and 30 healthy controls from a non-endemic region in Benin were screened for antibody responses to these specific proteins by ELISA. Serum IgG responses of Buruli ulcer patients were highly variable, however, seven proteins (MUP045, MUP057, MUL_0513, Hsp65, and the polyketide synthase domains ER, AT propionate, and KR A) showed a significant difference between patient and non-endemic control antibody responses. However, when sera from the healthy control subjects living in the same Buruli ulcer endemic area as the patients were examined, none of the proteins were able to discriminate between these two groups. Nevertheless, six of the seven proteins showed an ability to distinguish people living in an endemic area from those in a non-endemic area with an average sensitivity of 69% and specificity of 88%, suggesting exposure to M. ulcerans. Further validation of these six proteins is now underway to assess their suitability for use in Buruli ulcer seroepidemiological studies. Such studies are urgently needed to assist efforts to uncover environmental reservoirs and understand transmission pathways of the M. ulcerans.