Análise da ação do meropenem e Polimixina E com a IgG humana frente isolados de Pseudomonas aeruginosa provenientes de infecções relacionadas à Assistência à Saúde

LIMA, Fernanda Cristina Gomes de

23 February 2015

Submitted by Fabio Sobreira Campos da Costa (fabio.sobreira@ufpe.br) on 2015-05-26T17:40:43Z No. of bitstreams: 2 license_rdf: 1232 bytes, checksum: 66e71c371cc565284e70f40736c94386 (MD5) Dissertação_de_mestrado FERNANDA correção após apresentação FINALIZADA DIGITAL.pdf: 1967282 bytes, checksum: 8e1bd13e2a7cb2f2b493bb443c3db0f9 (MD5) / Made available in DSpace on 2015-05-26T17:40:43Z (GMT). No. of bitstreams: 2 license_rdf: 1232 bytes, checksum: 66e71c371cc565284e70f40736c94386 (MD5) Dissertação_de_mestrado FERNANDA correção após apresentação FINALIZADA DIGITAL.pdf: 1967282 bytes, checksum: 8e1bd13e2a7cb2f2b493bb443c3db0f9 (MD5) Previous issue date: 2015-02-23 / Pseudomonas aeruginosa é uma importante causa de infecções apresentando, no Brasil, altas taxas de morbidade e mortalidade. Os principais mecanismos de resistência utilizados por P. aeruginosa são a produção de β-lactamases e a expressão de bombas de efluxo. O uso de IgG e antibióticos para tratamento destas infecções tem apresentado resultados bem sucedidos, o que motiva a realização de estudos quanto a atividade in vitro da IgG humana com antibióticos frente a isolados de P. aeruginosa. O objetivo deste estudo foi detectar a presença dos genes de resistência, a relação clonal, o tempo de morte em isolados de P. aeruginosa provenientes de Infecções relacionadas à saúde (IrAS) de hospitais públicos do Recife-PE, em 2014, e verificar in vitro a taxa de fagocitose e a produção de oxido nítrico (NO) por monócitos humanos quando infectados por P. aeruginosa tratada com IgG humana em associação a Meropenem e Polimixina E. Foram avaliados 32 isolados para a detecção de genes de resistência por PCR, e para a avaliação de similaridade genética por ERIC-PCR. Destes, foram selecionados os 5 isolados apresentando maior número de genes de resistência e menor similaridade genética. Esses cinco isolados foram submetidos às associações dos sub-CIMs destes antibióticos com a IgG humana, para a determinação do tempo de morte, da taxa de fagocitose de células bacterianas e para a dosagem de NO por monócitos humanos. Foi detectado a presença do gene blaKPC em dois isolados de P. aeruginosa. Todos os isolados possuem os genes mexR, mexB, mexE e rpsL, apenas um isolado foi negativo para os genes mexA e mexF. Foram detectados 30 perfis genéticos distintos entre os isolados bacterianos. O tempo de morte dos isolados revelou que os tratamentos combinados com antibióticos, principalmente Polimixina E, são mais letais para as células bacterianas. A taxa de fagocitose por monócitos humanos revelou que quando infectados com bactéria tratada com IgG mais antibiótico, os monócitos ficam mais ativos à fagocitose e reduz drasticamente a quantidade de células bacterianas. Houve diferença significativa na produção de NO naqueles tratados com Meropenem e IgG. Com o presente estudo concluiu-se que a combinação de IgG mais antibiótico pode ser uma alternativa para o tratamento dessas infecções, pois a bactéria estará em número reduzido facilitando a fagocitose.

Pseudomonas aeruginosa

IgG

Antibióticos

Infecções

Interaction of macrophage cationic proteins with the outer membrane of Pseudomonas Aeruginosa

Sawyer, Janet Gail

January 1987

Purified macrophage cationic proteins were used in functional assays to determine their interactions with the outer membrane and lipopolysaccharide of Pseudomonas aeruginosa. A fluorescent derivative of polymyxin B (dansyl-polymyxin) was found to bind to saturation to purified lipopolysaocharide, with similar affinity for the aminoglycoside supersensitive strain H215 and wild type strain H103 lipopolysaocharide. MCP-1 could displace more dansyl-polymyxin bound to the lipopolysaocharide of both strains, and bound with greater affinity than MCP-2. When whole cells were used, MCPs also displaced bound dansyl-polymyxin. Effects on the outer membrane of whole cells were examined by determining the initial rate of uptake of the hydrophobic fluorescent probe 1-N-phenylnaphthylamine. Uptake was enhanced in the presence of MCPs, indicating permeabilization of the outer membrane. MCP-1 caused maximal uptake of the probe at 40 µg/ml, MCP-2 at 70 µg/ml, and crude extract at only 20 µg/ml. Uptake of the probe was found to be enhanced at add pH, with maximal uptake occurring with only 7.5 µg/ml MCP-1 at pH 6.5. The data suggested that MCPs act to permeabilize the outer membranes of P. aeruginosa in a manner analagous to that defined for other polycationic agents. / Science, Faculty of / Microbiology and Immunology, Department of / Graduate

Pseudomonas aeruginosa

Macrophages

Proteins -- Analysis

Characterization of genetic elements up-regulated in Pseudomonas aeruginosa PAO biofilms and transcriptional activity of the flagellar hook protein gene, flgE, during biofilm development

Meiring, Maria Susanna

27 June 2008

Please read the abstract (Summary) in the section, 00front, of this document / Dissertation (MSc (Microbiology))--University of Pretoria, 2008. / Microbiology and Plant Pathology / unrestricted

Biofilms development

Pseudomonas aeruginosa

UCTD

Regulation of rhamnolipid biosynthesis in the Pseudomonas aeruginosa PAOI biofilm population

Du Plessis, David Johannes Francois

18 August 2008

Pseudomonas aeruginosa, a ubiquitous environmental bacterium and an opportunistic human pathogen, forms biofilms through a series of interactions between the cells and adherence to surfaces. Not only does rhamnolipid contribute to the pathogenic potential of P. aeruginosa, but it has also been reported that the bacterium utilises rhamnolipid to actively maintain the void spaces surrounding microcolonies, thus contributing to the architecture of P. aeruginosa biofilms. The P. aeruginosa rhlAB operon encodes the enzyme rhamnosyltransferase I, which produces mono-rhamnolipid, and the induction of rhlAB is dependent on the quorum sensing transcription activator RhIR complexed with the auto inducer N-butyryl-homoserine lactone. In this study, several aspects related to rhamnolipid biosynthesis and regulation in P. aeruginosa PAO1 were investigated. As a first step, a biochemical assay was developed and optimised whereby the concentration of rhamnolipid could be accurately quantified following its extraction from small sample volumes. Although the optimised rhamnolipid assay is not able to distinguish between different rhamnolipids or between different homologs of a specific rhamnolipid, it is, however, simple to perform, cost¬effective and does not rely on the use of specialised equipment. Subsequently an rhlAB-deficient mutant strain of P. aeruginosa PAOI strain was generated. For this purpose, three allelic exchange strategies, i.e. plasmid incompatibility, the use of a SacB counter-selectable marker and a combination of these approaches, were investigated by making use of newly constructed allelic exchange vector systems. The results that were obtained indicated that, of the three approaches, the latter was most efficient in generating the desired P. aeruginosa mutant strain, and 90% of the derived strains were found to be double reciprocal mutants. Reporter gene technology, using the genes encoding for stable and unstable variants of the green fluorescent protein (GFP), was finally used to investigate the transcriptional activity of the rhlA promoter in P. aeruginosa biofilms under conditions of continuous flow using glass as substratum. For this purpose, mini-CTX-GFP reporter vectors, containing stable and unstable variants of the gfp reporter gene, were constructed that allow for integration of a single copy of the transcriptional fusion in a defined, non-essential region onto the P. aeruginosa genome. Several global regulators have been reported to playa role in regulating quorum sensing and/or rhamnolipid biosynthesis in P. aeruginosa, amongst other, the sigma factors RpoS and RpoN. Therefore, rhlA promoter activity was also investigated in biofilms of P. aeruginosa strains lacking either RpoN or RpoS. Although structural differences between the biofilms formed by the P. aeruginosa wild-type PAD 1 and respective mutant strains were noted, transcription of rhlA appeared to be constitutive from 24 h onwards and did not appear to be localised to specific areas within the microcolonies or biofilms. These results, combined with those obtained by batch analysis, indicated that RpoS positively regulates rhlA transcription, whilst RpoN did not appear to influence rhlA promoter activity under the conditions used in this study. / Dissertation (MSc)--University of Pretoria, 2009. / Microbiology and Plant Pathology / unrestricted

Rhamnolipid biosynthesis

Pseudomonas aeruginosa

UCTD

A study of RNA bacteriophage 7s infection of Pseudomonas aeruginosa

Benson, Deanne

23 August 1974

A study was conducted to find the effect of magnesium, calcium, manganese and zinc ions on the infection of Psudomonas aeruginosa strain 1C by RNA bacteriophage 7s. When an 18 hour progeny experiment was performed, it was found that magnesium, calcium and manganese had different effects on bacteriophage production and was dependent on the bacterial growth conditions. RNA bacteriophage 7s progeny production was significantly enhanced by the addition of magnesium to cultures of Psudomonas aeruginosa 1C grown in a magnesium deficient medium. Under these environmental conditions there was a slight increase in progeny in the presence of calcium. When Psudomonas aeruginosa 1c was grown in a complete medium, the infection of cells by bacteriophage 7s was enhanced by magnesium and calcium but not manganese or zinc, as demonstrated by the One Step Growth Curve.

Bacteriophages

Pseudomonas aeruginosa

Biochemistry

Biology

Critical factors controlling regrowth of opportunistic pathogens in premise plumbing

Wang, Hong

28 March 2013

Opportunistic pathogens (e.g., Legionella pneumophila, Mycobacterium avium complex, Acanthamoeba polyphaga, Pseudomonas aeruginosa) residing in human-made water systems, particularly premise plumbing, are now the primary source of water-borne disease in developed countries. The prevention and control of opportunistic pathogens is a new challenge in premise plumbing due to the limited knowledge concerning the factors driving their occurrence and regrowth mechanisms, and also the complexity of premise plumbing conditions. The goal of this study is to identify key factors governing occurrence of opportunistic pathogens in drinking water distribution systems, particularly premise plumbing, via field investigations and lab-scale experiments. A molecular survey of three opportunistic pathogens (L. pneumophila, M. avium, P. aeruginosa), related groups (Legionella and mycobacteria) and two amoeba hosts (Acanthamoeba spp. and Hartmanella vermiformis) was performed in two real-word chloraminated drinking water distribution systems using quantitative polymerase chain reaction (q-PCR). A high occurrence of Legionella (" 69.0%) and mycobacteria (100%), lower occurrence of L. pneumophila (" 20%) and M. avium (" 33.3%), and rare detection of Pseudomonas aeruginosa (" 13.3%) was observed in both systems. Hartmanella vermiformis was more prevalent than Acanthamoeba. Three-minute flushing resulted in reduced gene copies of Legionella, mycobacteria, H. vermiformis and 16S rRNA genes (P<0.05) and distinct microbial community structure in postflushing water, implying strong regrowth potential of opportunistic pathogens in premise pluming. In order to examine the influence of pipe material, disinfectant type, and water age on occurrence and persistence of the target microorganisms, triplicate simulated distribution systems (SDSs) comparing iron, cement and PVC pipe materials were fed either chlorinated or chloraminated tap water, and were sampled at water ages ranging from 1d to 5.7d. q-PCR quantification of target microorganisms in both biofilm and bulk water revealed that Legionella, mycobacteria, P. aeruginosa and both amoebas naturally colonized the six SDSs, but L. pneumophila and M. avium were not detected. Disinfectant type and dose have the strongest influence on the microbiota. Disinfectant decay was noted with water age, particularly in chloraminated SDSs (due to nitrification), generally resulting in increased microbial detection frequencies and densities with water age. Influence of pipe material became apparent at water ages corresponding to low disinfectant residual. Natural colonization of Legionella spp., Mycobacterium spp., Acanthamoeba spp., H. vermiformis and M. avium was also observed in biofilms from five annular reactors, which were used to investigate effects of prior granular activated carbon (GAC) biofiltration and disinfectant type (chlorine, chloramine) on opportunistic pathogens under premise plumbing conditions. GAC pre-treatment effectively reduced total organic carbon (TOC). In most cases, total bacteria and opportunistic pathogens were higher in undisinfected annular reactors, but the levels were not proportional to the level of GAC pre-treatment/TOC. Chlorine was more effective for controlling mycobacteria and Acanthamoeba, whereas chloramine was more effective for controlling Legionella. Both chlorine and chloramine effectively reduced M. avium and H. vermiformis numbers. Pyrosequencing of 16S rRNA genes in biofilms revealed a significant effect of GAC pre-treatment and disinfectant type on the microbial community structure. Overall, the study provides insights to critical factors triggering proliferation of opportunistic pathogens in drinking water systems. Knowledge gained from this study can assist in formulating practical guidance for drinking water utilities and water consumers in terms of opportunistic pathogen prevention and control. / Ph. D.

Legionella

mycobacteria

Pseudomonas aeruginosa

amoeba

Characterization of the Response of Pseudomonas Aeruginosa to the Novel Bactericidal Agent AB569 and its use as a Model Organism in Microbial Fuel Cells

McDaniel, Cameron T.

29 October 2018

No description available.

Microbiology

EDTA

Nitrite

Pseudomonas aeruginosa

The Regulation and Dynamics of Type IV Pili / THE REGULATION AND DYNAMICS OF TYPE IV PILI IN PSEUDOMONAS AERUGINOSA

Graham, Katherine

January 2021

Type IV pili (T4P) are hair-like adhesins involved in many processes, including surface attachment, twitching, DNA uptake, electron transfer, and pathogenesis. These flexible filaments are expressed in various pathogens, including the opportunistic pathogen Pseudomonas aeruginosa. The pilus fibre is primarily composed of the major pilin structural subunit, PilA, which is rapidly polymerized or depolymerized during pilus extension or retraction, respectively. The transcription of pilA is tightly controlled by the PilS-PilR two-component system, which responds to fluctuating levels of PilA in the inner membrane. In addition to pilA, the response regulator, PilR, also regulates a subset of other non-T4P related genes. Here, we used hyperactivating point mutants in the PilS-PilR two-component system, which induce hyperpiliation without loss of pilus function, to assess the effects of increased surface pili expression on virulence against Caenorhabditis elegans, and to identify additional non-T4P genes regulated by the PilS-PilR two-component system. We hypothesized that dysregulation of the PilS-PilR two-component system impacts the expression of pilA and other genes, which impacts both surface piliation and T4P dynamics, resulting in altered P. aeruginosa virulence. C. elegans slow killing assays revealed that hyperpiliation, independently of T4P function, reduces virulence of model P. aeruginosa strains PAK and PA14. We propose a model whereby a surfeit of pili reduces virulence, potentially through impeding effective engagement of contact-dependent antagonism systems, such as the type III secretion system. Transcriptomic analysis of the hyperactive PilR point mutant also identified a subset of 26 genes, including those related to phenazine biosynthesis, quorum sensing, and ethanol oxidation, regulated by the PilS-PilR two-component system. Last, a T4P cysteine-labelling system was implemented for P. aeruginosa, allowing for the visualization of real-time pilus dynamics. Together, this work provides new insights into the consequences of hyperpiliation and the scope of the PilS-PilR signalling network, as well as novel tools for investigating P. aeruginosa T4P dynamics in vivo. / Thesis / Master of Science (MSc) / Pseudomonas aeruginosa is a major contributor to hospital-acquired infections and is of particular concern due to its intrinsic resistance to many frontline antibiotics. To aid in infection, Pseudomonas encodes an arsenal of virulence factors, including type IV pili (T4P), hair-like adhesins involved in many processes, such as twitching motility and surface attachment. T4P are primarily composed of the major pilin, PilA, whose expression is tightly regulated by the PilS-PilR two-component system. The sensor kinase, PilS, monitors the inner membrane PilA inventory and modifies activity of the response regulator, PilR, to regulate pilA transcription. Here, we demonstrate that P. aeruginosa virulence in a roundworm infection model is reduced when the amount of T4P expressed at the cell surface increases, regardless of the ability of the bacteria to twitch. We propose that inappropriate increases in surface T4P expression may impair pathogenicity-associated systems which require intimate host-cell contact. New genes in the regulon of the PilS-PilR two-component system were also identified. A tool to fluorescently label and image T4P in real-time using microscopy was established in the lab. This work highlights the consequences of increased surface T4P expression, providing potential new targets for antipseudomonal therapeutics which act on components involved in T4P expression and function.

type IV pili

Pseudomonas aeruginosa

Enhancement of the humoral immune response to Pseudomonas aeruginosa

Douthett, Rebecca L.

07 October 2005

No description available.

flagella

PSEUDOMONAS AERUGINOSA

fliC

vaccine

The effect of subinhibitory concentrations of antibiotics on Pseudomonas aeruginosa infection /

Geers, Teresa Anne

January 1986

No description available.

Biology

Pseudomonas aeruginosa

Antibiotics

Trachea