Cloning, Expression, and Sequence Analysis of Camelysin, a Zinc Metalloprotease from <em>Bacillus anthracis</em> and <em>B. cereus</em>

Myers, Andrew Ross

18 July 2005

Bacillus anthracis and B. cereus are well known etiological agents, which cause disease in healthy and immunocompromised individuals. Considering the abundance and lethality of these organisms it is imperative that research is performed to identify and analyze new factors that may contribute to their pathogenicity. Camelysin is a membrane bound, zinc metalloprotease isolated from B. cereus. Assays performed on purified camelysin demonstrate that the protease exhibits fibrinolytic, collagenolytic, and actin degradation activity, any of which can contribute to the organisms ability to invade host tissues and cause damage. Considering the putative role of camelysin in pathogenicity, it would be beneficial to study the effects of camelysin in tissue cultures or animal models. The goal of this study focused on the cloning and expression of camelysin from B. cereus and its homolog in B. anthracis. Expression of a fusion tagged protein may assist in the purification of camelysin as well as overcoming the native proteins extreme insolubility. Primers were designed to amplify the camelysin gene from B. cereus for cloning into the prokaryotic pBAD TOPO® TA, pET100/D-TOPO®, and the eukaryotic pcDNA3.1/V5-His© TOPO[registered trademark] TA expression vectors. Primers were also designed to amplify the gene from B. anthracis for cloning into the pBAD TOPO® TA vector. The recombinant clones were induced and successful expression of the protein was confirmed by performing SDS-PAGE, Western blotting, and an azocasein protease assay. The recombinant proteins exhibited casein degradation activity which is observed with purified camelysin from B. cereus. This study successfully demonstrated the presence of the camelysin protein in B. anthracis. Furthermore, the recombinant clones obtained will be useful for purification and analysis of camelysin and delineation of its role in the pathogenicity of B. cereus and B. anthracis.

Metalloenzyme

Collagen

Pathogenic factor

Recombinant protein

Nosocomial infections

American Studies

Arts and Humanities

Frequência de Cryptococcus spp. e outras leveduras com potencial patogênico em excretas de aves silvestres em três munícipios do estado de São Paulo / Frequency of Cryptococcus spp. and other yeasts with pathogenic potential in excreta of wild birds in three municipalities of the state of São Paulo

Caldas, Cirlene da Cunha

28 September 2017

Introdução: Nas últimas décadas, as infeções fúngicas invasivas por leveduras tornou-se um importante problema de saúde pública, dado sua incidência crescente relacionada ao aumento da população suscetível. O reconhecimento destes patógenos em aspectos como, distribuicão ambiental e caraterísticas fenotípicas, são pilares essenciais para sua vigilância e controle. Objetivo: Descrever a frequência dos agentes de criptococose e outras leveduras com potencial patogênico e comparar essa frequência em excretas de aves silvestres em três municípios do estado de São Paulo, com vistas a melhor conhecimento da distribuição desses agentes no ambiente, além de determinar o perfil de suscetibilidade in vitro a antifúngicos de uso clínico. Método: No período de 2 anos, aves silvestres foram identificadas em áreas de circulação de 3 municípios de São Paulo (Praia Grande, Santos e Rio Claro) e submetidas à coleta de excretas para isolamento de leveduras com potencial patogênico. Análise microscópica e macroscópica para classificação presuntiva de gênero foram realizados em todas as colônias de leveduras obtidas das amostras de excretas. A suscetibilidade dos isolados de leveduras aos antífúngicos: fluconazol, voriconazol e anfotericina B foi determinada segundo método de referência europeu (AFST-EUCAST). Análise de dados: Foi utilizada a regressão de Poisson com a opção robusta para estimar razões de prevalência e identificar variáveis associadas com os principais isolados identificados, com opção de cluster para agrupar os isolados por excreta. Foi avaliado o nível de concordância entre os dois métodos de identificação (fenotípico e MALDI-TOF), utilizando o coeficiente Kappa. Adicionalmente, foi estimada a correlação entre os MIC´s dos fármacos estudados no total de espécies identificadas, utilizando o coeficiente de correlação de Spearman. Resultados: Das 294 excretas coletadas, 42,2 por cento continham leveduras, incluindo espécies de Candida 62 por cento , seguido por Rhodotorula 16,4 por cento , Cryptococcus 10,4 por cento , Trichosporon 6,6 por cento e Pichia 2,7 por cento . Muitas espécies, verificadas em alta frequência, tem forte potêncial de causar infecção invasiva, como: C. parapsilosis stricto sensu, C. tropicalis, Clavispora lusitaniae, C. krusei, C. orthopsilosis, C. glabrata, C. laurenti, C. albicans, C. metapsilosis, C. nivariensis e Meyerozyma guilliermondii. A resistência ao fluconazol, voriconazol e anfotericina B ocorreu nesses isolados, sendo documentada uma forte correlação entre a susceptibilidade, principalmente entre os azois (fluconazol e voriconazol), no entanto, a correlação mesmo sendo menor também foi significativa entre esses fármacos e a anfotericina. De 13 espécies de aves silvestres dispersoras de leveduras, as de maior frequência foram: Sula leucogaster 26,2 por cento , Turdus leucomelas 17 por cento , Larus dominicanus 15 por cento , Thalasseus maximus 11,2 por cento , Thalasseus acuflavidus 5,4 por cento , Tangara sayaca 4,4 por cento , Turdus amaurochalinus 3,7 por cento , Sterna hirundinacea e Pitangus sulphuratus 2,7 por cento . Os gêneros identificados apresentaram associações entre local, estação do ano e espécies de aves. Conclusões: Dentre as principais espécies de aves estudadas, 3 eram de hábitos migratórios (Thalasseus maximus, Thalasseus acuflavidus e Sterna hirundinacea) o que permite inferir dispersão interamericana de leveduras patogênicas. Diversas espécies resistentes a antifúngicos foram descritas, pela primeira vez, em excretas de aves silvestres conferindo a este estudo o valor de contribuir para o conhecimento da epidemiologia das infecções fúngicas por leveduras. / Background: In recent decades, invasive yeast fungal infections have become an important public health problem, due to their increasing incidence related to the increase in the susceptible population. The recognition of these pathogens in aspects such as environmental distribution and phenotypic characteristics are essential pillars for their surveillance and control. Objective: To describe the frequency of cryptococcosis agents and other yeasts with pathogenic potential and to compare this frequency in excreta of wild birds in three municipalities of the state of São Paulo, with a view to a better knowledge of the distribution of these agents in the environment, in addition to determining the profile of in vitro susceptibility to antifungals for clinical use. Method: During two years, wild birds were identified in circulation areas of three municipalities of São Paulo (Praia Grande, Santos and Rio Claro) and were screened for yeasts with pathogenic potential. Microscopic and macroscopic analysis for presumptive genus classification were performed in all yeast colonies obtained from excreta samples. Susceptibility of yeast isolates to antifungals: fluconazole, amphotericin B and voriconazole was determined according to the European reference method (AFST-EUCAST). Data analysis: Poisson regression was used with the robust option to estimate prevalence ratios and to identify variables associated with the main isolates identified, with option of cluster to group the isolates by excreta. The level of agreement between the two identification methods (phenotype and MALDI-TOF) was evaluated using the Kappa coefficient. Additionally, the correlation was estimated between MICs of the drugs studied in total of species identified, using Spearman\'s correlation coefficients. Results: Of the 294 excreta collected, half contained yeasts, including Candida species (62 per cent ), followed by Rhodotorula (16.4 per cent ), Cryptococcus (10.4 per cent ), Trichosporon (6.3 per cent ) and Pichia (2.7 per cent ). Many species, verified at high frequency, have a strong potential to cause invasive infection, such as: C. parapsilosis stricto sensu, C. tropicalis, Clavispora lusitaniae, C. krusei, C. orthopsilosis, C. glabrata, C. laurentii, C. albicans, C. metapsilosis, C. nivariensis and Meyerozyma guilliermondii. Resistance to fluconazole, voriconazole and amphotericin B occurred in these isolates and a strong correlation was reported between susceptibility, mainly between azole (fluconazole and voriconazole), however, the correlation, even though it was lower, was also significant between these drugs and amphotericin. From 13 species of wild birds dispersing yeasts, the ones with the highest frequency were: Sula leucogaster 26,2 per cent , Turdus leucomelas 17 per cent , Larus dominicanus 15 per cent , Thalasseus maximus 11,2 per cent , Thalasseus acuflavidus 5,4 per cent , Tangara sayaca 4,4 per cent , Turdus amaurochalinus 3,7 per cent , Sterna hirundinacea e Pitangus sulphuratus 2,7 per cent . The identified genera presented associations between site, season of the year and species of birds. Conclusion: Among the main species of birds studied, 3 were of migratory habits (Thalasseus maximus, Thalasseus acuflavidus and Sterna hirundinacea), which allows inferring the inter - American dispersion of pathogenic yeasts. Several species resistant to antifungal were described for the first time in excreta of wild birds, conferring to this study the value of contributing to the knowledge of the epidemiology of fungal infections by yeasts.

Antifungal,Fluconazole

Antifúngicos

Aves

Birds

Criptococose

Cryptococcosis

Eliminação de Excretas

Elimination of Excreta

Fluconazol

Leveduras Patogênicas

Pathogenic Yeasts

Genetic dissection of disease resistance to Phoma medicaginis in Medicago truncatula

lars.kamphuis@csiro.au, Lars Gian Kamphuis

January 2007

Phoma medicaginis is a necrotrophic fungal pathogen, commonly found infecting Medicago truncatula and M. sativa in temperate regions of Australia. To identify, characterize and differentiate eight P. medicaginis isolates from Western Australia, morphological phenotypes and five gene regions (actin, â- tubulin, calmodulin, internal transcribed spacer, translation elongation factor 1-á) were examined. Sequence comparisons showed that specimens isolated from M. truncatula in Western Australia formed a group that was consistently different from, but closely allied to, a P. medicaginis var. medicaginis type specimen. Characterization of three P. medicaginis genotypes showed that all exhibited a narrow host range, causing disease only in M. sativa and M. truncatula among eight commonly cultivated legume species sampled. Infection of 85 M. truncatula accessions showed a continuous distribution in disease phenotypes, with the majority of accessions susceptible. Differences in disease phenotypes suggest that M. truncatula harbours specific and diverse sources of resistance to individual P. medicaginis genotypes. To characterize the genetic basis of resistance to P. medicaginis two F2 populations derived from crosses between the resistant accession SA27063 and the susceptible accessions SA3054 and A17 were phenotyped for disease symptoms. Highly significant recessive QTLs for resistance to P. medicaginis OMT5 were identified in each mapping population. In SA27063 x A17 a QTL named resistance to the necrotroph Phoma medicaginis one (rnpm1) was identified on the short arm of LG4. In SA27063 x SA3054 a QTL (rnpm2) was identified on the long arm of LG8. Further fine mapping of the areas surrounding the QTLs is underway to identify the genes underlying rnpm1 and rnpm2. Examination of the recombination frequencies between genetic markers on the long arms of chromosomes 4 and 8 in the SA27063 x A17 cross revealed an apparent genetic linkage between these chromosomes. Subsequent analysis of other crosses showed this unexpected linkage relationship is characteristic for genetic maps derived from A17. Furthermore F1 individuals derived from crosses involving A17 showed 50% pollen viability or less. This semisterility and the unexpected linkage relationships provide good evidence for a reciprocal translocation in A17 between chromosomes four and eight. The implications of the distinctive chromosomal rearrangement in A17 on genetic mapping, genome sequencing and comparative mapping are discussed. The Mt16kOLI1plus microarray was used to identify transcriptional changes in M. truncatula expressed in defence against P. medicaginis. Three-hundred-and-thirty-four differentially expressed transcripts showed a change of two-fold or more in either the resistant or susceptible interaction, and most of the Phoma-regulated genes could be assigned to functional categories which have been reported to be involved in plant defence responses. RT-qPCR and HPLCUV confirmed involvement of the octadecanoid and phenylpropanoid pathways in response to P. medicaginis infection. Faster induction of lipoxygenase genes and constitutively higher levels of certain phenolic metabolites were observed in resistant plants.

Medicago

Disease and pest resistance

Genetic aspects

Phoma

Pathogenic fungi

Western Australia

Identification and characterisation of in vivo expressed genes of Pasteurella multocida

Boucher, David

January 2004

Abstract not available

Pasteurella multocida

Gene expression

Mutagenesis

Pathogenic bacteria

Studies on the agrocin 84 plasmid of `Agrobacterium radiobacter`

Shim, Je-Seop.

January 1987

Includes two journal articles with contributions by the author Bibliography: leaves 145-154

Pathogenic bacteria

Crown-gall disease

Plasmids

Insertion elements, DNA

Rhizobiaceae Biological control

Deterministic model of microbial sources, fate and transport: a quantitative tool for pathogen catchment budgeting

Ferguson, Christobel Margaret, Biotechnology & Biomolecular Science, UNSW

January 2005

The most important priority for the management of Australian drinking water catchments is the control of pathogen loads delivered to raw water reservoirs and treatment plant intakes. A process-based mathematical model was developed to estimate pathogen catchment budgets (PCB) for Cryptosporidium, Giardia and E. coli loads generated within and exported from catchments. The model quantified key processes affecting the generation and transport of microorganisms from humans and animal excreta using land use and hydrologic data, and catchment specific information including point sources such as sewage treatment plants and on-site systems. The PCB model was applied in the Wingecarribee catchment, Sydney and used to predict and rank pathogen and indicator loads in dry weather, intermediate (<30 mm in 24 h) and large wet weather events (100mm in 24 h). Sensitivity analysis identified that pathogen excretion rates from animals and humans, and manure mobilisation rates were the most significant factors determining the output of the model. Comparison with water quality data indicated that predicted dry weather loads were generally within 1-2 log10 of the measured loads for Cryptosporidium and E. coli and within 1 log10 for Giardia. The model was subsequently used to predict and rank pathogen and indicator loads for the entire (16 000 km2) Sydney drinking water catchment.

pathogen

model

Cryptosporidium

catchment

watershed

pathogenic microorganisms

water

microbiology

drinking water

contamination

The Effects of Phytophthora Cinnamomi on heathland flora and fauna of the Eastern Otway Ranges.

Laidlaw, William Scott, mikewood@deakin.edu.au

January 1997

The plant pathogen, Phytophthora dnnamomi, is a cause of dieback disease observed in sclerophyll vegetation in Australia, The effects of P. dnnamomi on flora and fauna were studied at two locations in heathland vegetation near the coastal town of Anglesea, Victoria. The pathogen was isolated from soils beneath diseased heathland plants. The extent of diseased vegetation was assessed by the presence and absence of highly sensitive indicator species, Xanthorrhoea australis and hopogon ceratophyllus. The characteristics of heathland vegetation exhibiting dieback disease associated with the presence of P. dnnamomi were investigated. Plant species richness was similar between diseased and non-diseased areas however diseased areas were characterised by significant declines in the cover and frequency of susceptible species, increases in resistant species and increases in percent cover of open ground. Compared to non-diseased areas, diseased areas exhibited fewer shrub species and decreased shrub cover. The percentage cover and number of species of sedges, lilies and grasses were higher in diseased areas. Structural differences were significant between 0-0.6 m with decreased cover of vegetation in diseased areas. Differences in structure between diseased and non-diseased areas were not as great as expected due to increases in the cover of resistant species. A number of regenerating X australis were observed in post-disease areas. Cluster analysis of floristic data could clearly separate diseased and non-diseased trap stations. The population dynamics and habitat use of eight small mammal species present were compared in diseased and non-diseased areas using trapping and radio-tracking techniques. The number of small mammal species captured in post-disease areas was significantly lower than non-diseased areas. Mean captures of Antechinus stuartii and Rattus fiisdpes were significantly lower in diseased areas on Grid B. Mean captures of Rattus lutreolus were significantly lower in diseased areas on both study grids. Significant differences were not observed in every season over the two year study period. Radio tracking revealed more observations of Sminthopsis leucopus in non-diseased vegetation than in diseased. Cercartetus nanus was frequently observed to utilise the disease susceptible X. australis for nesting. At one location, the recovery of vegetation and small mammal communities in non-diseased and diseased vegetation after fuel reduction burning was monitored for three years post-fire. Return of plant species after fire in both disease classes were similar, reaching 75% of pre-fire richness after three years. Vegetation cover was slower to return after fire in diseased areas. Of the seven small mammal species captured pre-fire, five were regularly captured in the three years after fire. General linear model analysis revealed a significant influence of disease on capture rates for total small mammals before fire and a significant influence of fire on capture rates for total small mammals after fire. After three years, the influence of fire on capture rates was reduced no significant difference was detected between disease classes. Measurements of microclimate indicate that diseased, burnt heathland was likely to experience greater extremes of temperature and wind speed. Seeding of diseased heathland with X. australis resulted in the establishment of seedlings of this sensitive species. The reported distributions of the mamma] species in Victoria were analysed to determine which species were associated with the reported distribution of dieback disease. Twenty-two species have more than 20% of their known distribution in diseased areas. Five of these species, Pseudomys novaehollandiae, Pseudomys fumeust Pseudomys shortridgei, Potorous longipes and Petrogale pencillata are rare or endangered in Victoria. Four of the twenty-two species, Sminthopsis leucopus, Isoodon obesulus, Cercartetus nanus and Rottus lutreolus am observed in Victorian heathlands. Phytophthora cinnamomi changes both the structure and floristics of heathland vegetation in the eastern Qtway Ranges. Small mammals respond to these changes through decreased utilisation of diseased heathland. The pathogen threatens the diversity of species present and future research efforts should be directed towards limiting its spread and rehabilitating diseased areas.

Phytophtora cinnamomi

Anglesea

otway ranges

heathlands

pathogenic microorganisms

dieback

antechinus

mammals

moor ecology

Survival of Spore forming bacteria during pasteurisation and anaerobic digestion in biogas plants.

Danielsson, Mari

January 2006

<p>ABSTRACT</p><p>Anaerobic digestion is one way of handling biowaste and generating energy in the form of methane, biogas.</p><p>This study shows that spore forming bacterias survive the process of pasteurisation and anaerobic digestion in biogas plants. It has also been established that both the nonpasteurised-and digestion- waste contains pathogen spore forming bacterias. Two Swedish full-scale</p><p>commercial biogas plants were sampled before pasteurisation, after pasteurisation and after digestion on 10 occasions with one week intervals. The samples were analysed quantitatively</p><p>and qualitatively, with biochemical methods, for Clostridium spp and Bacillus spp.</p><p>Polymerase Chain Reaction, a biomolecular method, was used for</p><p>C. chauvei analysis, with C. chauvei specific primers. For this analyse the biogas plants were sampled at 11 occasions.</p><p>Survival of pathogenic spore forming bacteria in digestion residue may be a health risk for both humans and animals. The digested residue may be used as fertiliser on arable land and the risk of contamination by pathogenic Clostridium spp and Bacillus spp is hard to assess, but can not be neglected.</p>

Pathogenic bacteria

Biowaste

Digestion residue

Bacillus spp

Clostridium spp

Microbiology

Mikrobiologi

<i>Campylobacter</i> Pathogenesis and Subunit Vaccine Development

Zeng, Ximin

01 August 2010

Campylobacter jejuni is the leading bacterial cause of human gastroenteritis in the United States. Increasing resistance of Campylobacter to clinical antibiotics raises an urgent need for novel strategies to prevent and control infections in humans and animal reservoirs, which necessitates a better understanding of Campylobacter pathogenesis. We hypothesize that multidrug efflux pump CmeABC and ferric enterobactin (FeEnt) iron acquisition systems, which play a critical role in Campylobacter pathogenesis, are novel targets for developing effective measures against Campylobacter. To test this, the molecular, antigenic, functional, and protective characteristics of two outer membrane proteins, CmeC (an essential component of CmeABC drug efflux pump) and CfrA (a FeEnt receptor), were examined. Both CmeC and CfrA are highly conserved and widely produced in C. jejuni strains. Anti-CmeC and Anti-CfrA antibodies inhibited the function of CmeABC efflux pump and CfrA, resulting enhanced susceptibility to bile salts and reduced utilization of FeEnt of C. jejuni, respectively. Immunoblotting analysis also indicated that CfrA is expressed and immunogenic in vivo. Amino acid substitution mutagenesis demonstrated that a highly conserved basic amino acid R327 in CfrA plays a critical role in FeEnt acquisition. The purified recombinant CmeC and a Salmonella live vaccine expressing the protective epitope of CfrA were evaluated as subunit vaccines against Campylobacter infection in the chicken model. CmeC vaccination elicited immune response but failed to reduce C. jejuni colonization in the intestine. However, Salmonella-vectored vaccine conferred significant protection against C. jejuni challenge. To further elucidate the role of iron acquisition in the pathogenesis of Campylobacter, whole genome sequence of a unique C. jejuni strain was determined using a 454 GS FLX sequencer with Titanium series reagents. Comparative genomics analysis led to the identification of a novel Campylobacter Enterobactin Esterase (Cee) that is essential in the CfrB-dependent FeEnt utilization pathway. Extensive genetic manipulation revealed molecular pathways and mechanistic features of the two orchestrated FeEnt acquisition systems in Campylobacter. This project provides critical information about the feasibility of targeting CmeC and CfrA for immune protection against Campylobacter colonization in the intestine, and increases our understanding of the critical role of FeEnt acquisition in the pathophysiology of Campylobacter.

Campylobacter

vaccine

pathogenesis

CmeABC efflux pump

CfrA

CfrB

ferric enterobactin acquisition

Cee

Pathogenic Microbiology

Evaluation of chromosomally-integrated luxCDABE and plasmid-borne GFP markers for the study of localization and shedding of STEC O91:H21 in calves

Hong, Yingying

01 May 2011

Shiga toxin-producing Escherichia coli (STEC) has been recognized as an important foodborne pathogen. Of this group, O91 is one of the common serogroups frequently isolated from patients and food in some countries, with O91:H21 being previously implicated in hemolytic uremic syndrome (HUS). Cattle are principle reservoirs for STEC, and studies examining STEC shedding in cattle often include experimental inoculation of strains of interest using antibiotic resistance markers for identifiable recovery. However, indigenous fecal microbes exhibiting similar resistance patterns can confound such studies. Such was the case in a study by our group when attempting to characterize shedding patterns of O91:H21 in calves, leading us to seek other, more effective, markers. Among our strategies was the development of a chromosomally integrated bioluminescence marker via transposon mutagenesis using a luxCDABE cassette from Photorhabdus luminescens and a plasmid borne GFP marker via transformation of the pGFP vector. The luxCDABE marker was inserted on host chromosome at a site that was 27 nucleotides before the stop codon of gene yihL and confirmed to have little impact on important virulence genes and growth rate with a very high stability. In contrast, plasmid borne GFP marker showed poor stability without the application of appropriate antibiotic selection pressure. For calves receiving luxCDABE-marked O91:H21, the fecal counts of the organismranged from 1.2 x 10 3 to 1.3 x 10 4CFU/g at two days post inoculation and decreased to 5.8 to 8.7 x 10 2 CFU/g or undetectable level after two weeks.Intestinal contents sampled from various positions at day 14 post inoculation indicated that cecum and descending colon may be the primary localization sites of this O91:H21 strain. Compared to antibiotic resistance markers, the use of bioluminescence markers does not require the restricted pre-inoculation screening of animals. The enumeration of luxCDABE-marked O91:H21 from feces and intestinal contents was easily accomplished and confirmed reliable by M-PCR analysis under the presence of indigenous bacteria which cannot be eliminated by antibiotic-supplemented selective plates. Therefore, the chromosomal integrated luxCDABE marker may be a better model for the study of STEC colonization and shedding in cattle.

shedding

luxCDABE

GFP

marker

O91:H21

Pathogenic Microbiology