Your search keyword '"Ulrike MacDonald"' showing total 24 results

1. Antibody Dependent Enhancement ofAcinetobacter baumanniiInfection in a Mouse Pneumonia Model

Author

Ruth Olson, Janet M. Beanan, Shun Xin Wang-Lin, Thomas A. Russo, Joseph P. Balthasar, and Ulrike MacDonald

Subjects

0301 basic medicine, Pharmacology, biology, Virulence, biology.organism_classification, Microbiology, Acinetobacter baumannii, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Immune system, In vivo, Monoclonal, biology.protein, Molecular Medicine, Antibody-dependent enhancement, Antibody, Pathogen, 030217 neurology & neurosurgery

Abstract

Acinetobacter baumannii has become a pathogen of increasing medical importance because of the emergence of multidrug-resistant strains and the high rate of mortality of infected patients. Promising animal study results have been reported recently with active and passive immunization against A. baumannii virulence factors. In the present study, a monoclonal IgG3 antibody, 8E3, was developed with specificity for the K2 capsular polysaccharide of A. baumannii, and its therapeutic potential was assessed. 8E3 enhanced macrophage-mediated bactericidal activity against the A. baumannii clinical strain AB899. However, 8E3 treatment (passive immunization) of AB899-infected mice led to a substantial increase in mortality and to substantial increases in bacterial load in blood, lung, and in splenic samples. In vitro investigations showed a large binding capacity in the supernatant of bacterial cultures, suggesting that shed capsule components act as a binding sink for 8E3. Investigations of 8E3 pharmacokinetics in mice demonstrated that unbound concentrations of the antibody dropped below detection limits within 24 hours after a 200 mg/kg dose. However, total concentrations of antibody declined slowly, with an apparent terminal half-life (t1/2) of 6.7–8.0 days, suggesting that the vast majority of 8E3 in blood is bound (e.g., with soluble capsule components in blood). We hypothesize that high concentrations of 8E3-capsule immune complexes act to inhibit bacterial clearance in vivo. To the best of our knowledge, this is the first demonstration of antibody-dependent enhancement of A. baumannii infection, and these observations highlight the complexity of antibody-based therapy for A. baumannii infections.

Published

2019

2. Anatomy of an Extensively Drug Resistant Klebsiella pneumoniae Outbreak in Tuscany, Italy

Author

Lindsey R. Hall, Patrick McGann, Jason W. Bennett, Melissa J. Martin, Francois Lebreton, Giacinta Tordini, Ulrike MacDonald, Thomas A. Russo, Jean Denis Docquier, Katharina Schaufler, Brendan T. Jones, Rosslyn Maybank, Nils-Olaf Hübner, Jason Stam, Stefania Cresti, Emma G. Mills, Filomena Sannio, Marcello Valassina, Karsten Becker, Brendan W. Corey, Yoon I. Kwak, and Maria Grazia Cusi

Subjects

Plasmid, Klebsiella pneumoniae, Colistin, medicine, Outbreak, Virulence, Tigecycline, Drug resistance, Biology, biology.organism_classification, Hybrid plasmid, medicine.drug, Microbiology

Abstract

A protracted outbreak of New Delhi metallo-beta-lactamase (NDM)-producing carbapenem-resistant Klebsiella pneumoniae, started in Tuscany, Italy, in November 2018 and continued in 2020 and through 2021. To understand the regional emergence and transmission dynamics over time, we collected and sequenced the genomes of 117 extensively drug-resistant, NDM-producing K. pneumoniae isolates cultured over a 20-month period from 76 patients at several health care facilities in South-East Tuscany. All isolates belonged to high-risk clone ST-147 and were typically non-susceptible to all first line antibiotics. Albeit sporadic, resistances to colistin, tigecycline and fosfomycin were also observed as a result of repeated, independent mutations. Genomic analysis revealed that ST-147 isolates circulating in Tuscany were monophyletic, highly genetically related (including a network of 42 patients from the same hospital and sharing nearly identical isolates) and shared a recent ancestor with clinical isolates from the Middle East. While the blaNDM–1 gene was carried by an IncFIB-type plasmid, our investigations revealed that the ST-147 lineage from Italy also acquired a hybrid IncH-type plasmid carrying the 16S methyltransferase armA gene as well as key virulence biomarkers often found in hypervirulent isolates. This plasmid shared extensive homologies with mosaic plasmids circulating globally including from ST-11 and ST-307 convergent lineages. Phenotypically, the carriage of this hybrid plasmid resulted in increased siderophore production but did not confer virulence to the level of an archetypical, hypervirulent K. pneumoniae in a subcutaneous model of infection with immunocompetent CD1 mice. Our findings highlight the importance of performing genomic surveillance to identify emerging threats.Significance StatementCarbapenem-resistant Klebsiella pneumoniae belong to the “critical priority” tier of bacterial pathogens as identified by the World Health Organization. Emerging “high-risk” lineages are responsible for difficult-to-treat, hospital-acquired infections and outbreaks around the globe. By integrating genomic and epidemiological data for isolates collected over 20 months, this study revealed both the high, regional prevalence and the rapid spread, within a single hospital, of K. pneumoniae ST-147 in Italy. Besides resistance to nearly all antibiotics, we showed that this lineage carried a hybrid plasmid harboring a set of biomarker genes previously linked to hypervirulence. Convergence of multidrug resistance and hypervirulence is a major concern and these findings highlight the need for robust, global surveillance to monitor the emergence of high-risk K. pneumoniae.

Published

2021

3. An Assessment of Siderophore Production, Mucoviscosity, and Mouse Infection Models for Defining the Virulence Spectrum of Hypervirulent Klebsiella pneumoniae

Author

Sidra Hassan, Patrick McGann, Ellie Camanzo, Brendan W. Corey, Thomas A. Russo, Ulrike MacDonald, and Francois Lebreton

Subjects

Male, 0301 basic medicine, Siderophore, mice, Virulence Factors, Klebsiella pneumoniae, 030106 microbiology, Virulence, Biology, Microbiology, Cohort Studies, 03 medical and health sciences, Plasmid, Animals, infection model, Molecular Biology, Gene, Mice, Inbred BALB C, siderophores, Strain (biology), biology.organism_classification, Phenotype, QR1-502, hypervirulent, pathogenic potential, Klebsiella Infections, Mice, Inbred C57BL, Disease Models, Animal, 030104 developmental biology, mucoviscosity, Bacteria, Research Article, Plasmids

Abstract

Hypervirulent Klebsiella pneumoniae (hvKp) bacteria are more virulent than classical K. pneumoniae (cKp) with resultant differences in clinical manifestations and management. It is unclear whether all hvKp isolates share a similar pathogenic potential. This report assessed the utility of siderophore production, mucoviscosity, and murine infection for defining the virulence spectrum of hvKp. Three strain cohorts were identified and defined based on the CD1 mouse subcutaneous (SQ) challenge model: (i) fully virulent hvKp strains (fvhvKp), lethal at a challenge inoculum (CI) of ≤103 CFU; (ii) partially virulent hvKp strains (pvhvKp), lethal at a CI of >103 to 107 CFU; (iii) classical K. pneumoniae, not lethal at a CI of 107 CFU. Quantitative siderophore and mucoviscosity assays differentiated fvhvKp and pvhvKp strains from cKp strains but were unable to differentiate between the fvhvKP and pvhvKP strain cohorts. However, SQ challenge of CD1 mice and intraperitoneal (IP) challenge of CD1 and BALB/c mice, but not C57BL/6 mice, were able to discriminate between an fvhvKp and a pvhvKp strain; SQ challenge of CD1 mice may have the greatest sensitivity. cKp was differentiated from hvKp both by SQ challenge of CD1 mice and IP challenge of all three mouse strains. These data identify a means to define the relative virulence of hvKP strains. It remains unclear whether the observed differences of hvKp virulence in mice translates to human infection. However, these data can be used to sort random collections of K. pneumoniae strains into fvhvKp and pvhvKp strain cohorts and assess for differences in clinical manifestations and outcomes. IMPORTANCE The pathogenic potential of hvKp strains is primarily mediated by a large virulence plasmid. The minimal set of genes required for the full expression of the hypervirulent phenotype is undefined. A number of reports describe hvKp strains possessing only a portion of the virulence plasmid; the clinical consequences of this are unclear. Therefore, the goal of this report was to determine whether virulence among hvKp strains varied and, if so, how to best identify the relative virulence of hvKp isolates. Data demonstrate hvKp pathogenic potential varies in CD1 and BALB/c murine infection models. In contrast, measurements of siderophore production and mucoviscosity were unable to discriminate the differences in hvKp isolate virulence observed in mice. This information can be used in future studies to determine the mechanisms responsible for differences between fully virulent hvKp and partially virulent hvKp and whether the differences observed in mice translate to disease in humans.

Published

2021

4. Anatomy of an extensively drug-resistant Klebsiella pneumoniae outbreak in Tuscany, Italy

Author

Patrick McGann, Yoon I. Kwak, Ulrike MacDonald, Maria Grazia Cusi, Melissa J. Martin, Jason Stam, Francois Lebreton, Casey Harless, Giacinta Tordini, Emma G. Mills, Jean Denis Docquier, Stefania Cresti, Lindsey R. Hall, Karsten Becker, Rosslyn Maybank, Brendan W. Corey, Brendan T. Jones, Thomas A. Russo, Filomena Sannio, Jason W. Bennett, Katharina Schaufler, Marcello Valassina, and Nils-Olaf Hübner

Subjects

Klebsiella pneumoniae, Antimicrobial resistance, Bacterial pathogenesis, Genomic epidemiology, Nosocomial outbreak, Animals, Anti-Bacterial Agents, Bacterial Proteins, Biomarkers, Carbapenems, Colistin, Computational Biology, Cross Infection, Drug Resistance, Multiple, Bacterial, Humans, Italy, Kaplan-Meier Estimate, Klebsiella Infections, Likelihood Functions, Mice, Microbial Sensitivity Tests, Pharmaceutical Preparations, Plasmids, Polymorphism, Single Nucleotide, beta-Lactamases, Disease Outbreaks, Drug Resistance, Virulence, Tigecycline, Microbiology, Antibiotic resistance, Plasmid, medicine, Polymorphism, Multidisciplinary, biology, Bacterial, Outbreak, Single Nucleotide, Biological Sciences, biology.organism_classification, Hybrid plasmid, Multiple, medicine.drug

Abstract

Significance Carbapenem-resistant Klebsiella pneumoniae belongs to the “critical-priority” tier of bacterial pathogens as identified by the World Health Organization. Emerging “high-risk” lineages are responsible for difficult-to-treat, hospital-acquired infections and outbreaks around the globe. By integrating genomic and epidemiological data for isolates collected over 20 mo, this study revealed both the high, regional prevalence and the rapid spread, within a single hospital, of K. pneumoniae ST-147 in Italy. Besides resistance to nearly all antibiotics, this lineage carried a hybrid plasmid harboring a set of biomarker genes previously linked to hypervirulence. Convergence of resistance and virulence determinants is a major concern and these findings highlight the need for robust, global surveillance to monitor the emergence of high-risk K. pneumoniae., A protracted outbreak of New Delhi metallo-β-lactamase (NDM)–producing carbapenem-resistant Klebsiella pneumoniae started in Tuscany, Italy, in November 2018 and continued in 2020 and through 2021. To understand the regional emergence and transmission dynamics over time, we collected and sequenced the genomes of 117 extensively drug-resistant, NDM-producing K. pneumoniae isolates cultured over a 20-mo period from 76 patients at several healthcare facilities in southeast Tuscany. All isolates belonged to high-risk clone ST-147 and were typically nonsusceptible to all first-line antibiotics. Albeit sporadic, resistances to colistin, tigecycline, and fosfomycin were also observed as a result of repeated, independent mutations. Genomic analysis revealed that ST-147 isolates circulating in Tuscany were monophyletic and highly genetically related (including a network of 42 patients from the same hospital and sharing nearly identical isolates), and shared a recent ancestor with clinical isolates from the Middle East. While the blaNDM-1 gene was carried by an IncFIB-type plasmid, our investigations revealed that the ST-147 lineage from Italy also acquired a hybrid IncFIB/IncHIB–type plasmid carrying the 16S methyltransferase armA gene as well as key virulence biomarkers often found in hypervirulent isolates. This plasmid shared extensive homologies with mosaic plasmids circulating globally including from ST-11 and ST-307 convergent lineages. Phenotypically, the carriage of this hybrid plasmid resulted in increased siderophore production but did not confer virulence to the level of an archetypical, hypervirulent K. pneumoniae in a subcutaneous model of infection with immunocompetent CD1 mice. Our findings highlight the importance of performing genomic surveillance to identify emerging threats.

Published

2021

5. An Evaluation of BfmR-Regulated Antimicrobial Resistance in the Extensively Drug Resistant (XDR) Acinetobacter baumannii Strain HUMC1

Author

Candace M. Marr, Ulrike MacDonald, Grishma Trivedi, Somnath Chakravorty, and Thomas A. Russo

Subjects

Microbiology (medical), Acinetobacter baumannii, BfmR, medicine.drug_class, Polymyxin, lcsh:QR1-502, Drug resistance, Microbiology, Meropenem, biofilm, lcsh:Microbiology, 03 medical and health sciences, Antibiotic resistance, meropenem, polymyxin E, medicine, Pathogen, 030304 developmental biology, 0303 health sciences, extensively drug resistant, biology, 030306 microbiology, Biofilm, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, Antimicrobial, medicine.drug

Abstract

Acinetobacter baumannii is a problematic pathogen due to its common expression of extensive drug resistance (XDR) and ability to survive in the healthcare environment. These characteristics are mediated, in part, by the signal transduction system BfmR/BfmS. We previously demonstrated, in antimicrobial sensitive clinical isolates, that BfmR conferred increased resistance to meropenem and polymyxin E. In this study, potential mechanisms were informed, in part, by a prior transcriptome analysis of the antimicrobial sensitive isolate AB307-0294, which identified the porins OprB and aquaporin (Omp33-36, MapA) as plausible mediators for resistance to hydrophilic antimicrobials such as meropenem. Studies were then performed in the XDR isolate HUMC1, since delineating resistance mechanisms in this genomic background would be more translationally relevant. In HUMC1 BfmR likewise increased meropenem and polymyxin E resistance and upregulated gene expression of OprB and aquaporin. However, the comparison of HUMC1 with isogenic mutant constructs demonstrated that neither OprB nor aquaporin affected meropenem resistance; polymyxin E susceptibility was also unaffected. Next, we determined whether BfmR-mediated biofilm production affected either meropenem or polymyxin E susceptibilities. Interestingly, biofilm formation increased resistance to polymyxin E, but had little, if any effect on meropenem activity. Additionally, BfmR mediated meropenem resistance, and perhaps polymyxin E resistance, was due to BfmR regulated factors that do not affect biofilm formation. These findings increase our understanding of the mechanisms by which BfmR mediates intrinsic antimicrobial resistance in a clinically relevant XDR isolate and suggest that the efficacy of different classes of antimicrobials may vary under biofilm inducing conditions.

Published

2020

6. The Galleria mellonella Infection Model Does Not Accurately Differentiate between Hypervirulent and Classical Klebsiella pneumoniae

Author

Ulrike MacDonald and Thomas A. Russo

Subjects

0301 basic medicine, classical Klebsiella pneumoniae, Klebsiella pneumoniae, Virulence Factors, 030106 microbiology, lcsh:QR1-502, Virulence, Moths, Microbiology, lcsh:Microbiology, outbred mouse systemic infection model, Host-Microbe Biology, 03 medical and health sciences, Mice, Antibiotic resistance, Plasmid, infection models, Genotype, Animals, Molecular Biology, Genetics, hypervirulent Klebsiella pneumoniae, biology, fungi, biology.organism_classification, Phenotype, QR1-502, 3. Good health, Biomarker (cell), Klebsiella Infections, Galleria mellonella, Disease Models, Animal, 030104 developmental biology, Larva, Galleria mellonella infection model, Research Article

Abstract

Hypervirulent Klebsiella pneumoniae (hvKp) is of increasing concern because it can infect individuals in community and health care settings and because such infections are becoming difficult to treat. Identification of hvKp is important for patient care and to track its global spread. The genetic definition of hvKp, which can be used for its identification and the development of diagnostic tests, has not been optimized. Determination of possession of 4 of 5 genes that are present on the hvKp-specific virulence plasmid is highly accurate for identifying hvKp. However, an ongoing issue is whether strains that possess only some of these markers are still hypervirulent. The Galleria mellonella model and, less commonly, the murine infection model have been used to assess the virulence of these ambiguously identifiable strains. This report demonstrates that the murine model but not the G. mellonella model accurately identifies suspected hvKp strains. This information is critical for the development of diagnostics for patient care and for future research studies., Hypervirulent Klebsiella pneumoniae (hvKp) is an emerging pathogen of increasing concern due to its ability to cause serious organ and life-threatening infections in healthy individuals and its increasing acquisition of antimicrobial resistance determinants. Identification of hvKp is critical for patient care and epidemiologic and research studies. Five genotypic markers on the hvKp-specific virulence plasmid can accurately differentiate hvKp from the less virulent classical K. pneumoniae (cKp) strain, but it is unclear whether the possession of fewer markers accurately predicts the hvKp pathotype. Likewise, the effect, if any, of various antimicrobial resistance factors on the pathogenic potential of hvKp has been incompletely explored. The Galleria mellonella infection model is often used to assess virulence, but this tool has not been validated. Therefore, levels of lethality of defined hvKp and cKp strain cohorts were compared in Galleria and outbred mouse models. The murine model, but not the G. mellonella model, accurately differentiated hvKp from cKp strains. Therefore, isolates in which the pathogenic potential is ambiguous due to an incomplete hvKp biomarker profile, an incomplete pLVPK-like hvKp-specific virulence plasmid, antimicrobial resistance that could decrease biofitness, and/or the lack of a characteristic clinical presentation should be validated in an outbred murine model. These data will assist in determining the minimal genomic content needed for full expression of the hypervirulence phenotype. This information, in turn, is critical for the development of the pragmatic point-of-care testing requisite for patient care and for the performance of epidemiologic and research studies going forward. IMPORTANCE Hypervirulent Klebsiella pneumoniae (hvKp) is of increasing concern because it can infect individuals in community and health care settings and because such infections are becoming difficult to treat. Identification of hvKp is important for patient care and to track its global spread. The genetic definition of hvKp, which can be used for its identification and the development of diagnostic tests, has not been optimized. Determination of possession of 4 of 5 genes that are present on the hvKp-specific virulence plasmid is highly accurate for identifying hvKp. However, an ongoing issue is whether strains that possess only some of these markers are still hypervirulent. The Galleria mellonella model and, less commonly, the murine infection model have been used to assess the virulence of these ambiguously identifiable strains. This report demonstrates that the murine model but not the G. mellonella model accurately identifies suspected hvKp strains. This information is critical for the development of diagnostics for patient care and for future research studies.

Published

2020

7. Identification of biomarkers for differentiation of hypervirulent Klebsiella pneumoniae from classical K. pneumoniae

Author

Thomas A. Russo, Ruth Olson, Chi-Tai Fang, Nicole Stoesser, Mark Miller, Ulrike MacDonald, Alan Hutson, Jason H. Barker, Ricardo M. La Hoz, James R. Johnson, Martin Backer, Rajinder Bajwa, Andrew T. Catanzaro, Derrick Crook, Kleper de Almeda, Joshua Fierer, David E. Greenberg, Michael Klevay, Payal Patel, Adam Ratner, Jin-Town Wang, and Jaroslaw Zola

Subjects

Male, 0301 basic medicine, Microbiology (medical), Canada, medicine.medical_specialty, Virulence Factors, Klebsiella pneumoniae, 030106 microbiology, Siderophores, Diagnostic accuracy, Biology, Sepsis, Mice, 03 medical and health sciences, Epidemiology, medicine, Animals, Humans, Genetics, Molecular Epidemiology, Hazard ratio, K pneumoniae, Bacteriology, biology.organism_classification, medicine.disease, Survival Analysis, United Kingdom, Klebsiella Infections, Disease Models, Animal, Molecular Diagnostic Techniques, Genes, Bacterial, Cohort, Prevalence studies, Biomarkers

Abstract

A hypervirulent Klebsiella pneumoniae (hvKp) pathotype is undergoing global dissemination. In contrast to the usual health care-associated epidemiology of classical K. pneumoniae (cKp) infections, hvKp causes tissue-invasive infections in otherwise healthy individuals from the community, often involving multiple sites. An accurate test to identify hvKp strains is needed for improved patient care and epidemiologic studies. To fill this knowledge gap, clinical criteria or random blood isolates from North American and United Kingdom strain collections were used to assemble hvKp-rich (n = 85) and cKp-rich (n = 90) strain cohorts, respectively. The isolates were then assessed for multiple candidate biomarkers hypothesized to accurately differentiate the two cohorts. The genes peg-344, iroB, iucA, plasmid-borne rmpA gene ((p)rmpA), and (p)rmpA2 all demonstrated >0.95 diagnostic accuracy for identifying strains in the hvKp-rich cohort. Next, to validate this epidemiological analysis, all strains were assessed experimentally in a murine sepsis model. peg-344, iroB, iucA, (p)rmpA, and (p)rmpA2 were all associated with a hazard ratio of >25 for severe illness or death, additionally supporting their utility for identifying hvKp strains. Quantitative siderophore production of ≥30 μg/ml also strongly predicted strains as members of the hvKp-rich cohort (accuracy, 0.96) and exhibited a hazard ratio of 31.7 for severe illness or death. The string test, a widely used marker for hvKp strains, performed less well, achieving an accuracy of only 0.90. Last, using the most accurate biomarkers to define hvKp, prevalence studies were performed on two Western strain collections. These data strongly support the utility of several laboratory markers for identifying hvKp strains with a high degree of accuracy.

Published

2019

8. Aerobactin, but Not Yersiniabactin, Salmochelin, or Enterobactin, Enables the Growth/Survival of Hypervirulent (Hypermucoviscous) Klebsiella pneumoniae Ex Vivo and In Vivo

Author

Thomas A. Russo, Ruth Olson, Janet M. Beanan, Bruce A. Davidson, and Ulrike MacDonald

Subjects

Male, Siderophore, Klebsiella pneumoniae, Immunology, Siderophores, Virulence, Hydroxamic Acids, Microbiology, Yersiniabactin, Virulence factor, Enterobactin, Mice, Young Adult, chemistry.chemical_compound, Glucosides, Phenols, Animals, Humans, Microbial Viability, biology, biology.organism_classification, Molecular Pathogenesis, Klebsiella Infections, Thiazoles, Infectious Diseases, chemistry, bacteria, Aerobactin, Parasitology, Ex vivo

Abstract

The siderophore aerobactin is the dominant siderophore produced by hypervirulent Klebsiella pneumoniae (hvKP) and was previously shown to be a major virulence factor in systemic infection. However, strains of hvKP commonly produce the additional siderophores yersiniabactin, salmochelin, and enterobactin. The roles of these siderophores in hvKP infection have not been optimally defined. To that end, site-specific gene disruptions were created in hvKP1 (wild type), resulting in the generation of hvKP1Δ iucA (aerobactin deficient), hvKP1Δ iroB (salmochelin deficient), hvKP1Δ entB (enterobactin and salmochelin deficient), hvKP1Δ irp2 (yersiniabactin deficient), and hvKP1Δ entB Δ irp2 (enterobactin, salmochelin, and yersiniabactin deficient). The growth/survival of these constructs was compared to that of their wild-type parent hvKP1 ex vivo in human ascites fluid, human serum, and human urine and in vivo in mouse systemic infection and pulmonary challenge models. Interestingly, in contrast to aerobactin, the inability to produce enterobactin, salmochelin, or yersiniabactin individually or in combination did not decrease the ex vivo growth/survival in human ascites or serum or decrease virulence in the in vivo infection models. Surprisingly, none of the siderophores increased growth in human urine. In human ascites fluid supplemented with exogenous siderophores, siderophores increased the growth of hvKP1Δ iucA , with the relative activity being enterobactin > aerobactin > yersiniabactin > salmochelin, suggesting that the contribution of aerobactin to virulence is dependent on both innate biologic activity and quantity produced. Taken together, these data confirm and extend a role for aerobactin as a critical virulence factor for hvKP. Since it appears that aerobactin production is a defining trait of hvKP strains, this factor is a potential antivirulence target.

Published

2015

9. Structure of shikimate kinase, anin vivoessential metabolic enzyme in the nosocomial pathogenAcinetobacter baumannii, in complex with shikimate

Author

Ulrike MacDonald, Thomas A. Russo, L.W. Schultz, Ruth Olson, J. Breen, K.A. Sutton, Janet M. Beanan, and Timothy C. Umland

Subjects

Acinetobacter baumannii, Models, Molecular, Protein Conformation, Shikimic Acid, Crystallography, X-Ray, medicine.disease_cause, Shikimate kinase, Microbiology, chemistry.chemical_compound, Structural Biology, medicine, Animals, Humans, Shikimate pathway, Pathogen, biology, Aroa, Pathogenic bacteria, General Medicine, Shikimic acid, biology.organism_classification, Rats, Phosphotransferases (Alcohol Group Acceptor), chemistry, Essential gene, Acinetobacter Infections, Signal Transduction

Abstract

Acinetobacter baumanniiis an opportunistic Gram-negative pathogen that is an important cause of healthcare-associated infections exhibiting high mortality rates. Clinical isolates of multidrug-resistant (MDR) and extremely drug-resistant (XDR)A. baumanniistrains are increasingly being observed. Compounding this concern is the dearth of new antibacterial agents in late-stage development that are effective against MDR and XDRA. baumannii. As part of an effort to address these concerns, two genes (aroAandaroC) of the shikimate pathway have previously been determined to be essential for the growth and survival ofA. baumanniiduring host infection (i.e.to be essentialin vivo). This study expands upon these results by demonstrating that theA. baumannii aroKgene, encoding shikimate kinase (SK), is also essentialin vivoin a rat soft-tissue infection model. The crystal structure ofA. baumanniiSK in complex with the substrate shikimate and a sulfate ion that mimics the binding interactions expected for the β-phosphate of ATP was then determined to 1.91 Å resolution and the enzyme kinetics were characterized. The flexible shikimate-binding domain and LID region are compared with the analogous regions in other SK crystal structures. The impact of structural differences and sequence divergence between SKs from pathogenic bacteria that may influence antibiotic-development efforts is discussed.

Published

2015

10. Metabolite Transporter PEG344 Is Required for Full Virulence of Hypervirulent Klebsiella pneumoniae Strain hvKP1 after Pulmonary but Not Subcutaneous Challenge

Author

Ulrike MacDonald, Thomas A. Russo, Ruth Olson, Janet M. Beanan, and Jeffrey Bulger

Subjects

0301 basic medicine, Klebsiella pneumoniae, Virulence Factors, In silico, medicine.medical_treatment, Immunology, Virulence, Microbiology, Pathogenesis, 03 medical and health sciences, Mice, Plasmid, Bacterial Proteins, Subcutaneous Absorption, medicine, Animals, Humans, Lung, biology, Growth factor, Ascites, Membrane Transport Proteins, Bacterial Infections, biology.organism_classification, Virology, In vitro, Klebsiella Infections, 030104 developmental biology, Infectious Diseases, Parasitology, Ex vivo

Abstract

Hypervirulent Klebsiella pneumoniae (hvKP) is an emerging pathotype that is capable of causing tissue-invasive and organ- and life-threatening infections in healthy individuals from the community. Knowledge on the virulence factors specific to hvKP is limited. In this report, we describe a new factor (PEG344) that increases the virulence of hvKP strain hvKP1. peg-344 is present on the hvKP1 virulence plasmid, is broadly prevalent among hvKP strains, and has increased RNA abundance when grown in human ascites. An isogenic derivative of hvKP1 (hvKP1Δ peg-344 ) was constructed and compared with its wild-type parent strain in in vitro , ex vivo , and infection model studies. Both survival and competition experiments with outbred CD1 mice demonstrated that PEG344 was required for full virulence after pulmonary challenge but, interestingly, not after subcutaneous challenge. In silico analysis suggested that PEG344 serves as an inner membrane transporter. Compared to hvKP1, a small but significant decrease in the growth/survival of hvKP1Δ peg-344 was observed in human ascites, but resistance to the bactericidal activity of complement was similar. These data suggested that PEG344 may transport an unidentified growth factor present in ascites. The data presented are important since they expand our limited knowledge base on virulence factors unique to hvKP, which is needed to lay the groundwork for translational approaches to prevent or treat these devastating infections.

Published

2017

11. The Capsular Polysaccharide of Acinetobacter baumannii Is an Obstacle for Therapeutic Passive Immunization Strategies

Author

Ruth Olson, Janet M. Beanan, Ulrike MacDonald, Shun Xin Wang-Lin, Joseph P. Balthasar, and Thomas A. Russo

Subjects

0301 basic medicine, Acinetobacter baumannii, Blood Bactericidal Activity, medicine.drug_class, 030106 microbiology, Immunology, Monoclonal antibody, Microbiology, Epitope, 03 medical and health sciences, Mice, Sepsis, medicine, Animals, Humans, Antiserum, biology, Polysaccharides, Bacterial, Immunization, Passive, Antibodies, Monoclonal, Complement System Proteins, Bacterial Infections, biology.organism_classification, bacterial infections and mycoses, Virology, Antibodies, Bacterial, Antibody opsonization, Disease Models, Animal, 030104 developmental biology, Infectious Diseases, Treatment Outcome, biology.protein, Hybridoma technology, bacteria, Parasitology, Antibody, Bacterial outer membrane, Acinetobacter Infections, Bacterial Outer Membrane Proteins, Protein Binding

Abstract

Acinetobacter baumannii has become an important concern for human health due to rapid development and wide spread of antimicrobial-resistant strains and high mortality associated with the infection. Passive immunizations with antisera targeting outer membrane proteins (OMPs) have shown encouraging results in protecting mice from A. baumannii infection, but monoclonal anti-OMP antibodies have not been developed, and their potential therapeutic properties have not been explored. The goal of this report is to evaluate the antibacterial activity of monoclonal antibodies (MAbs) targeting outer membrane protein A (OmpA) of A. baumannii . Five anti-OmpA MAbs were developed using hybridoma technology and showed strong binding to strain ATCC 19606. However, low antibody binding was observed when they were tested against six clinical isolates, which included extensively drug-resistant strains. In contrast, high binding to an isogenic K1 capsule-negative mutant (AB307.30) was shown, suggesting that capsular polysaccharide mediated the inhibition of MAb binding to OmpA. Anti-OmpA MAbs increased the macrophage-mediated bactericidal activity of AB307.30 but failed to increase phagocytic killing of capsule-positive strains. Capsular polysaccharide was also protective against complement-mediated bactericidal activity in human ascites in the presence and absence of opsonization. Lastly, passive immunization with anti-OmpA MAbs did not confer protection against challenge with AB307-0294, the encapsulated parent strain of AB307.30, in a mouse sepsis infection model. These results reveal the important role of capsule polysaccharide in shielding OmpA and thereby inhibiting anti-OmpA MAb binding to clinical isolates. This property of capsule hindered the therapeutic utility of anti-OmpA MAbs, and it may apply to other conserved epitopes in A. baumannii .

Published

2017

12. The Response Regulator BfmR Is a Potential Drug Target for Acinetobacter baumannii

Author

Ruth Olson, Janet M. Beanan, Ulrike MacDonald, Thomas A. Russo, Akshay Manohar, Timothy C. Umland, and Jessica Graham

Subjects

0301 basic medicine, Acinetobacter baumannii, Gram-negative bacilli, medicine.drug_class, 030106 microbiology, Antibiotics, Druggability, lcsh:QR1-502, Biology, Microbiology, lcsh:Microbiology, drug discovery, 03 medical and health sciences, Antibiotic resistance, medicine, essential genes, Molecular Biology, antibiotic target, Drug discovery, multidrug resistant, Therapeutics and Prevention, Antimicrobial, biology.organism_classification, QR1-502, 3. Good health, bacterial drug target, Multiple drug resistance, 030104 developmental biology, Colistin, medicine.drug, Research Article

Abstract

Increasing antibiotic resistance in bacteria, particularly Gram-negative bacilli, has significantly affected the ability of physicians to treat infections, with resultant increased morbidity, mortality, and health care costs. In fact, some strains of bacteria are resistant to all available antibiotics, such as Acinetobacter baumannii, which is the focus of this report. Therefore, the development of new antibiotics active against these resistant strains is urgently needed. In this study, BfmR is further validated as an intriguing target for a novel class of antibiotics. Successful inactivation of BfmR would confer the multiple benefits of a decreased ability of A. baumannii to survive in human body fluids, increased sensitivity to complement-mediated bactericidal activity and, importantly, increased sensitivity to other antibiotics. Structural studies support the potential for this “druggable” target, as they identify the potential for small-molecule binding at functionally relevant sites. Next-phase high-throughput screening studies utilizing BfmR are warranted., Identification and validation is the first phase of target-based antimicrobial development. BfmR (RstA), a response regulator in a two-component signal transduction system (TCS) in Acinetobacter baumannii, is an intriguing potential antimicrobial target. A unique characteristic of BfmR is that its inhibition would have the dual benefit of significantly decreasing in vivo survival and increasing sensitivity to selected antimicrobials. Studies on the clinically relevant strain AB307-0294 have shown BfmR to be essential in vivo. Here, we demonstrate that this phenotype in strains AB307-0294 and AB908 is mediated, in part, by enabling growth in human ascites fluid and serum. Further, BfmR conferred resistance to complement-mediated bactericidal activity that was independent of capsular polysaccharide. Importantly, BfmR also increased resistance to the clinically important antimicrobials meropenem and colistin. BfmR was highly conserved among A. baumannii strains. The crystal structure of the receiver domain of BfmR was determined, lending insight into putative ligand binding sites. This enabled an in silico ligand binding analysis and a blind docking strategy to assess use as a potential druggable target. Predicted binding hot spots exist at the homodimer interface and the phosphorylation site. These data support pursuing the next step in the development process, which includes determining the degree of inhibition needed to impact growth/survival and the development a BfmR activity assay amenable to high-throughput screening for the identification of inhibitors. Such agents would represent a new class of antimicrobials active against A. baumannii which could be active against other Gram-negative bacilli that possess a TCS with shared homology. IMPORTANCE Increasing antibiotic resistance in bacteria, particularly Gram-negative bacilli, has significantly affected the ability of physicians to treat infections, with resultant increased morbidity, mortality, and health care costs. In fact, some strains of bacteria are resistant to all available antibiotics, such as Acinetobacter baumannii, which is the focus of this report. Therefore, the development of new antibiotics active against these resistant strains is urgently needed. In this study, BfmR is further validated as an intriguing target for a novel class of antibiotics. Successful inactivation of BfmR would confer the multiple benefits of a decreased ability of A. baumannii to survive in human body fluids, increased sensitivity to complement-mediated bactericidal activity and, importantly, increased sensitivity to other antibiotics. Structural studies support the potential for this “druggable” target, as they identify the potential for small-molecule binding at functionally relevant sites. Next-phase high-throughput screening studies utilizing BfmR are warranted.

Published

2016

13. Biofilm formed by a hypervirulent (hypermucoviscous) variant of Klebsiella pneumoniae does not enhance serum resistance or survival in an in vivo abscess model

Author

Thomas A. Russo, Qingli Kong, Alexander O. Pomakov, Alyssa S. Shon, Daniel J. Metzger, Ruth Olson, Janet M. Beanan, and Ulrike MacDonald

Subjects

Male, Serum, Microbiology (medical), Transposable element, Blood Bactericidal Activity, Editor's Corner, Virulence Factors, Operon, Klebsiella pneumoniae, Immunology, Mutant, Virulence, Biology, Microbiology, Gene Knockout Techniques, Young Adult, Animals, Humans, Rats, Long-Evans, Subcutaneous abscess, Pathogen, Microbial Viability, Polysaccharides, Bacterial, Biofilm, biology.organism_classification, Abscess, Klebsiella Infections, Rats, Disease Models, Animal, Mutagenesis, Insertional, Infectious Diseases, Biofilms, DNA Transposable Elements, Parasitology, Research Paper

Abstract

A new hypervirulent (hypermucoviscous) clinical variant of Klebsiella pneumoniae (hvKP) has emerged over the last decade. Our goal is to identify new mechanisms, which increase the virulence hvKP. It has been shown that hvKP strains produce more biofilm than “classical” stains of K. pneumoniae, therefore we hypothesized that biofilm formation may contribute to the pathogenesis of systemic infection. To test this hypothesis, transposon mutants of the model pathogen hvKP1 were generated and screened for decreased production of biofilm. Three mutant constructs with disruptions in glnA [putatively encodes glutamine synthetase, hvKP1 glnA:: EZ::TN < KAN-2 > (glnA::Tn)], sucD [putatively encodes succinyl-CoA synthase α subunit, hvKP1 sucD:: EZ::TN < KAN-2 > (sucD::Tn)], and tag [putatively encodes transcriptional antiterminator of glycerol uptake operon, hvKP1 tag:: EZ::TN < KAN-2 > (tag::Tn)] were chosen for further characterization and use in biologic studies. Quantitative assays performed in rich laboratory medium and human ascites confirmed the phenotype and a hypermucoviscosity assay established that capsule production was not affected. However, compared with its wild-type parent, neither planktonic cells nor biofilms of glnA::Tn, sucD::Tn and tag::Tn displayed a change to the bactericidal activity of 90% human serum. Likewise, when assessed in a rat subcutaneous abscess model, the growth and survival of glnA::Tn, sucD::Tn and tag::Tn in abscess fluid was similar to hvKP1. In this report we identify three new genes that contribute to biofilm formation in hvKP1. However, decreased biofilm production due to disruption of these genes does not affect the sensitivity of these mutant constructs to 90% human serum when in planktonic form or within a biofilm. Further, their virulence in an in vivo abscess model was unaffected.

Published

2012

14. Clinical and phenotypic differences between classic and hypervirulent Klebsiella pneumonia: an emerging and under-recognized pathogenic variant

Author

Hsiao Cb, Ulrike MacDonald, Pomakova Dk, Ruth Olson, Yoav Keynan, Janet M. Beanan, and Thomas A. Russo

Subjects

Male, Microbiology (medical), medicine.medical_specialty, Liver Abscess, Virulence, Biology, Communicable Diseases, Emerging, Young Adult, Medical microbiology, medicine, Animals, Humans, Rats, Long-Evans, Subcutaneous abscess, General Medicine, Long evans, medicine.disease, Virology, Phenotype, Klebsiella Infections, Rats, Community-Acquired Infections, Disease Models, Animal, Klebsiella pneumoniae, Infectious Diseases, Klebsiella pneumonia, Pneumonia (non-human), Spleen, Liver abscess

Abstract

The purpose of this study was to increase awareness, gain insight into acquisition, and assess the virulence of the hypervirulent (hypermucoviscous) clinical variant (hvKP) that is entrenched in the Pacific Rim but emerging in Western countries. A case of community-acquired liver abscess with metastatic spread to the spleen is described. Comparative in vitro and in vivo virulence studies on this isolate (hvKP1) and four randomly chosen blood isolates of "classic" K. pneumonia strains (cKP1-4) were performed. Cases of hvKP infection are occurring in Western countries and are under-recognized. A hypermucoviscous phenotype is a surrogate laboratory marker for this variant. The propensity of hvKP strains for metastatic spread in non-compromised hosts is both a defining and unusual trait. The mode of acquisition in the described case was unclear but potential means are discussed. hvKP1 was more resistant to complement and neutrophil-mediated bactericidal activity and was more virulent in a rat subcutaneous abscess model than cKP1-4. Recognition of the hypermucoviscous phenotype, defined by a positive "string-test", will alert the microbiologist or clinician that the infecting strain may be a hvKP, which is hypervirulent compared to cKP. This will improve our understanding of the epidemiology and clinical spectrum of infection, which may be more extensive than appreciated.

Published

2011

15. The K1 Capsular Polysaccharide of Acinetobacter baumannii Strain 307-0294 Is a Major Virulence Factor

Author

Ruth Olson, Janet M. Beanan, L. Wayne Schultz, Nicole R. Luke, Anthony A. Campagnari, Shauna L. Sauberan, Ulrike MacDonald, Thomas A. Russo, and Timothy C. Umland

Subjects

Acinetobacter baumannii, Bacterial capsule, Blood Bactericidal Activity, Virulence Factors, Immunology, Mutant, Virulence, Microbiology, Virulence factor, Animals, Humans, Gene, Pathogen, Bacterial Capsules, Antigens, Bacterial, biology, Polysaccharides, Bacterial, Complement System Proteins, biology.organism_classification, Molecular Pathogenesis, Phenotype, Rats, Infectious Diseases, Parasitology

Abstract

Acinetobacter baumannii is a pathogen of increasing medical importance with a propensity to be multidrug resistant, thereby making treatment challenging. Little is known of virulence traits in A. baumannii . To identify virulence factors and potential drug targets, random transposon (Tn) mutants derived from the A. baumannii strain AB307-0294 were screened to identify genes essential for growth in human ascites fluid in vitro , an inflammatory exudative fluid. These studies led to the identification of two genes that were predicted to be required for capsule polymerization and assembly. The first, ptk , encodes a putative protein tyrosine kinase (PTK), and the second, epsA , encodes a putative polysaccharide export outer membrane protein (EpsA). Monoclonal antibodies used in flow cytometric and Western analyses confirmed that these genes are required for a capsule-positive phenotype. A capsule-positive phenotype significantly optimized growth in human ascites fluid, survival in human serum, and survival in a rat soft tissue infection model. Importantly, the clearance of the capsule-minus mutants AB307.30 ( ptk mutant, capsule minus) and AB307.45 ( epsA mutant, capsule minus) was complete and durable. These data demonstrated that the K1 capsule from AB307-0294 was an important protectin. Further, these data suggested that conserved proteins, which contribute to the capsule-positive phenotype, are potential antivirulence drug targets. Therefore, the results from this study have important biologic and translational implications and, to the best of our knowledge, are the first to address the role of capsule in the pathogenesis of A. baumannii infection.

Published

2010

16. Penicillin‐Binding Protein 7/8 Contributes to the Survival ofAcinetobacter baumanniiIn Vitro and In Vivo

Author

Ulrike MacDonald, Shauna L. Sauberan, Thomas A. Russo, L. Wayne Luke, Ian J. MacDonald, Ruth Olson, Janet M. Beanan, and Timothy C. Umland

Subjects

Acinetobacter baumannii, Blood Bactericidal Activity, Penicillin binding proteins, Molecular Sequence Data, Mutant, Urine, Microbiology, Pathogenesis, chemistry.chemical_compound, Microscopy, Electron, Transmission, In vivo, Pneumonia, Bacterial, Animals, Humans, Penicillin-Binding Proteins, Immunology and Allergy, Computer Simulation, Amino Acid Sequence, Pathogen, biology, Soft Tissue Infections, Complement System Proteins, biology.organism_classification, In vitro, Rats, Disease Models, Animal, Infectious Diseases, chemistry, Data Interpretation, Statistical, Mutation, DNA Transposable Elements, bacteria, Peptidoglycan, Acinetobacter Infections

Abstract

BACKGROUND Acinetobacter baumannii is a bacterial pathogen of increasing medical importance. Little is known about genes important for its survival in vivo. METHODS AND RESULTS Screening of random transposon mutants of the model pathogen AB307-0294 identified the mutant AB307.27. AB307.27 contained its transposon insertion in pbpG, which encodes the putative low-molecular-mass penicillin-binding protein 7/8 (PBP-7/8). AB307.27 was significantly killed in ascites (P

Published

2009

17. Capsular polysaccharide and the O-specific antigen impede antibody binding: A potential obstacle for the successful development of an extraintestinal pathogenic Escherichia coli vaccine

Author

John J. Cope, Ruth Olson, Janet M. Beanan, Ulrike MacDonald, and Thomas A. Russo

Subjects

Male, Immunogen, Heterologous, Biology, Epitope, Microbiology, Mice, Antigen, Sepsis, Animals, Bacterial Capsules, Escherichia coli Infections, Extraintestinal Pathogenic Escherichia coli, Microbial Viability, General Veterinary, General Immunology and Microbiology, Escherichia coli Vaccines, Public Health, Environmental and Occupational Health, O Antigens, Antibodies, Bacterial, Survival Analysis, Virology, Mice, Inbred C57BL, Infectious Diseases, Polyclonal antibodies, biology.protein, Molecular Medicine, Female, Bacterial antigen, Antibody, Protein Binding

Abstract

Extraintestinal pathogenic Escherichia coli (ExPEC) cause a wide variety of infections that are responsible for significant morbidity, mortality and costs to our healthcare system. An efficacious vaccine against ExPEC would be desirable. Previously, we demonstrated that nasal immunization with a genetically engineered strain in which capsule and O-antigen are no longer expressed (CP923) was immunogenic, generated antibodies that bound a subset of heterologous ExPEC strains, and enhanced neutrophil-mediated bactericidal activity against the homologous and a heterologous strain in vitro. In the work reported here we tested the hypothesis that nasal immunization with CP923 conferred protection in a mouse intravenous sepsis model. Nasal immunization with the wild-type strain CP9 conferred protection against challenge with itself and this protection was enhanced when IL-12 was used as an adjuvant. However, when CP923 was used the immunogen, protection was not observed against challenge with CP9. Next, we hypothesized that the observed lack of protection may be due to capsule and the O-antigen moiety of lipopolysaccharide (LPS) impeding antibody binding to non-capsule and O-antigen epitopes. This hypothesis was substantiated by in vitro binding assays, which demonstrated that binding of polyclonal anti-CP923 antisera was decreased when capsule and/or O-antigen were present. Lastly, neutrophil-mediated bactericidal activity against CP923, opsonisized with anti-CP923 antisera, was significantly increased compared to CP9. Taken together, these results demonstrate that the capsule and O-antigen form a biologically significant barrier against antibodies directed against non-capsular and O-antigen epitopes. This defense against the acquired immune response will need to be overcome for the development of a successful vaccine against ExPEC.

Published

2009

18. A killed, genetically engineered derivative of a wild-type extraintestinal pathogenic E. coli strain is a vaccine candidate

Author

Thomas A. Russo, Ruth Olson, Brian D. Johnston, Janet M. Beanan, Stacy A. Genagon, Bruce A. Davidson, James R. Johnson, Ulrike MacDonald, and John J. Cope

Subjects

Male, Bacterial capsule, Immunogen, Escherichia coli Vaccines, Heterologous, Biology, Article, Microbiology, Mice, Immune system, Antigen, Formaldehyde, Escherichia coli, Animals, Humans, Administration, Intranasal, Bacterial Capsules, Escherichia coli Infections, General Veterinary, General Immunology and Microbiology, Escherichia coli Proteins, Public Health, Environmental and Occupational Health, O Antigens, Antibodies, Bacterial, Virology, Blood, Infectious Diseases, Vaccines, Inactivated, Immunization, biology.protein, Molecular Medicine, Female, Rabbits, Antibody, Genetic Engineering

Abstract

Infections due to extraintestinal pathogenic E. coli (ExPEC) result in significant morbidity, mortality and increased healthcare costs. An efficacious vaccine against ExPEC would be desirable. In this report, we explore the use of killed-whole E. coli as a vaccine immunogen. Given the diversity of capsule and O-antigens in ExPEC, we have hypothesized that alternative targets are viable vaccine candidates. We have also hypothesized that immunization with a genetically engineered strain that is deficient in the capsule and O-antigen will generate a greater immune response against antigens other than the capsular and O-antigen epitopes than a wild-type strain. Lastly, we hypothesize that mucosal immunization with killed E. coli has the potential to generate a significant immune response. In this study, we demonstrated that nasal immunization with a formalin-killed ExPEC derivative deficient in capsule and O-antigen results in a significantly greater overall humoral response compared to its wild-type derivative (which demonstrates that capsule and/or the O-antigen impede the development of an optimal humoral immune response) and a significantly greater immune response against non-capsular and O-antigen epitopes. These antibodies also bound to a subset of heterologous ExPEC strains and enhanced neutrophil-mediated bactericidal activity against the homologous and a heterologous strain. Taken together, these studies support the concept that formalin-killed genetically engineered ExPEC derivatives are whole cell vaccine candidates to prevent infections due to ExPEC.

Published

2007

19. E. colivirulence factor hemolysin induces neutrophil apoptosis and necrosis/lysis in vitro and necrosis/lysis and lung injury in a rat pneumonia model

Author

Ruth Olson, Janet M. Beanan, Stacy A. Genagon, Patrick D. Pawlicki, Bruce A. Holm, Ulrike MacDonald, Paul R. Knight, Bruce A. Davidson, Natalie M. Warholic, and Thomas A. Russo

Subjects

Pulmonary and Respiratory Medicine, Necrosis, Lipopolysaccharide, Neutrophils, Physiology, Bacterial Toxins, Virulence, Apoptosis, In Vitro Techniques, Biology, Lung injury, Virulence factor, Microbiology, Hemolysin Proteins, chemistry.chemical_compound, In vivo, Physiology (medical), Pneumonia, Bacterial, medicine, Animals, Rats, Long-Evans, Annexin A5, Lung, Caspase 7, L-Lactate Dehydrogenase, Caspase 3, Escherichia coli Proteins, Hemolysin, Cell Biology, Rats, Disease Models, Animal, chemistry, Caspases, medicine.symptom

Abstract

Enteric gram-negative bacilli, such as Escherichia coli are the most common cause of nosocomial pneumonia. In this study a wild-type extraintestinal pathogenic strain of E. coli (ExPEC)(CP9) and isogenic derivatives deficient in hemolysin (Hly) and cytotoxic necrotizing factor (CNF) were assessed in vitro and in a rat model of gram-negative pneumonia to test the hypothesis that these virulence factors induce neutrophil apoptosis and/or necrosis/lysis. As ascertained by in vitro caspase-3/7 and LDH activities and neutrophil morphology, Hly mediated neutrophil apoptosis at lower E. coli titers (1 × 105–6cfu) and necrosis/lysis at higher titers (≥1 × 107cfu). Data suggest that CNF promotes apoptosis but not necrosis or lysis. We also demonstrate that annexin V/7-amino-actinomycin D staining was an unreliable assessment of apoptosis using live E. coli. The use of caspase-3/7 and LDH activities and neutrophil morphology supported the notion that necrosis, not apoptosis, was the primary mechanism by which neutrophils were affected in our in vivo gram-negative pneumonia model using live E. coli. In addition, in vivo studies demonstrated that Hly mediates lung injury. Neutrophil necrosis was not observed when animals were challenged with purified lipopolysaccharide, demonstrating the importance of using live bacteria. These findings establish that Hly contributes to ExPEC virulence by mediating neutrophil toxicity, with necrosis/lysis being the dominant effect of Hly on neutrophils in vivo and by lung injury. Whether Hly-mediated lung injury is due to neutrophil necrosis, a direct effect of Hly, or both is unclear.

Published

2005

20. Aerobactin Mediates Virulence and Accounts for Increased Siderophore Production under Iron-Limiting Conditions by Hypervirulent (Hypermucoviscous) Klebsiella pneumoniae

Author

Andrew M. Gulick, Ulrike MacDonald, Lauren M. Maltese, Eric J. Drake, Daniel J. Metzger, Ruth Olson, and Thomas A. Russo

Subjects

Siderophore, Klebsiella pneumoniae, Virulence Factors, Iron, Immunology, Gene Dosage, Virulence, Siderophores, Hydroxamic Acids, Microbiology, Gene dosage, Virulence factor, chemistry.chemical_compound, Mice, Animals, Humans, biology, Ascites, Limiting, biology.organism_classification, Virology, Molecular Pathogenesis, Klebsiella Infections, Disease Models, Animal, Infectious Diseases, chemistry, Culture Media, Conditioned, Aerobactin, Parasitology, Ex vivo

Abstract

Hypervirulent (hypermucoviscous) Klebsiella pneumoniae (hvKP) strains are an emerging variant of “classical” K. pneumoniae (cKP) that cause organ and life-threatening infection in healthy individuals. An understanding of hvKP-specific virulence mechanisms that enabled evolution from cKP is limited. Observations by our group and previously published molecular epidemiologic data led us to hypothesize that hvKP strains produced more siderophores than cKP strains and that this trait enhanced hvKP virulence. Quantitative analysis of 12 hvKP strains in iron-poor minimal medium or human ascites fluid showed a significant and distinguishing 6- to 10-fold increase in siderophore production compared to that for 14 cKP strains. Surprisingly, high-pressure liquid chromatography (HPLC)-mass spectrometry and characterization of the hvKP strains hvKP1, A1142, and A1365 and their isogenic aerobactin-deficient (Δ iucA ) derivatives established that aerobactin accounted for the overwhelming majority of increased siderophore production and that this was not due to gene copy number. Further, aerobactin was the primary factor in conditioned medium that enhanced the growth/survival of hvKP1 in human ascites fluid. Importantly the ex vivo growth/survival of hvKP1 Δ iucA was significantly less than that of hvKP1 in human ascites fluid, and the survival of outbred CD1 mice challenged subcutaneously or intraperitoneally with hvKP1 was significantly less than that of mice challenged with hvKP1 Δ iucA . The lowest subcutaneous and intraperitoneal challenge inocula of 3 × 10 2 and 3.2 × 10 1 CFU, respectively, resulted in 100% mortality, demonstrating the virulence of hvKP1 and its ability to cause infection at a low dose. These data strongly support that aerobactin accounts for increased siderophore production in hvKP compared to cKP (a potential defining trait) and is an important virulence factor.

Published

2014

21. The K1 capsular polysaccharide from Acinetobacter baumannii Is a potential therapeutic target via passive immunization

Author

Frank St. Michael, Ulrike MacDonald, Evgeny Vinogradov, Andrew D. Cox, Anthony A. Campagnari, Nicole R. Luke-Marshall, Thomas A. Russo, Brad Spellberg, Ruth Olson, and Janet M. Beanan

Subjects

Serotype, Bacterial capsule, Acinetobacter baumannii, Male, opsonization, Magnetic Resonance Spectroscopy, bacterial growth, immunogenicity, Mass Spectrometry, Epitopes, Mice, rat, molecular mimicry, serotype, epitope, biology, seroprevalence, soft tissue infection, Polysaccharides, Bacterial, neutrophil, Antibodies, Monoclonal, Flow Cytometry, unclassified drug, Bacterial vaccine, Antibody opsonization, Infectious Diseases, Microbial Immunity and Vaccines, bacterial survival, Bacterial Vaccines, Antibody, Acinetobacter Infections, K1 capsular polysaccharide, Immunology, animal experiment, bactericidal activity, Microbiology, bacterial capsule, bacterial clearance, Antibiotic resistance, Animals, carbohydrate analysis, Rats, Long-Evans, mouse, Bacterial Capsules, Antigens, Bacterial, animal model, Immunization, Passive, Gene Expression Regulation, Bacterial, biology.organism_classification, bacterial strain, Virology, Rats, nuclear magnetic resonance, Immunization, monoclonal antibody, polysaccharide, biology.protein, Parasitology, passive immunization

Abstract

The emergence of extremely resistant and panresistant Gram-negative bacilli, such as Acinetobacter baumannii , requires consideration of nonantimicrobial therapeutic approaches. The goal of this report was to evaluate the K1 capsular polysaccharide from A. baumannii as a passive immunization target. Its structure was determined by a combination of mass spectrometric and nuclear magnetic resonance (NMR) techniques. Molecular mimics that might raise the concern for autoimmune disease were not identified. Immunization of CD1 mice demonstrated that the K1 capsule is immunogenic. The monoclonal antibody (MAb) 13D6, which is directed against the K1 capsule from A. baumannii , was used to determine the seroprevalence of the K1 capsule in a collection of 100 A. baumannii strains. Thirteen percent of the A. baumannii isolates from this collection were seroreactive to MAb 13D6. Opsonization of K1-positive strains, but not K1-negative strains, with MAb 13D6 significantly increased neutrophil-mediated bactericidal activity in vitro ( P < 0.05). Lastly, treatment with MAb 13D6 3 and 24 h after bacterial challenge in a rat soft tissue infection model resulted in a significant decrease in the growth/survival of a K1-positive strain compared to that of a K1-negative strain or to treatment with a vehicle control ( P < 0.0001). These data support the proof of principle that the K1 capsule is a potential therapeutic target via passive immunization. Other serotypes require assessment, and pragmatic challenges exist, such as the need to serotype infecting strains and utilize serotype-specific therapy. Nonetheless, this approach may become an important therapeutic option with increasing antimicrobial resistance and a diminishing number of active antimicrobials.

Published

2013

22. In Vivo-Validated Essential Genes Identified in Acinetobacter baumannii by Using Human Ascites Overlap Poorly with Essential Genes Detected on Laboratory Media

Author

Ulrike MacDonald, Ruth Olson, Janet M. Beanan, L. Wayne Schultz, Thomas A. Russo, and Timothy C. Umland

Subjects

Acinetobacter baumannii, Mutagenesis (molecular biology technique), Human pathogen, Biology, Microbiology, Skin Diseases, In vivo, Virology, Putative gene, Animals, Humans, Gene, Genes, Essential, Ascites, Enterobacter, Antimicrobial, biology.organism_classification, QR1-502, Abscess, Culture Media, Rats, Disease Models, Animal, Mutagenesis, Insertional, Genes, Bacterial, Gene Deletion, Research Article

Abstract

A critical feature of a potential antimicrobial target is the characteristic of being essential for growth and survival during host infection. For bacteria, genome-wide essentiality screens are usually performed on rich laboratory media. This study addressed whether genes detected in that manner were optimal for the identification of antimicrobial targets since the in vivo milieu is fundamentally different. Mutant derivatives of a clinical isolate of Acinetobacter baumannii were screened for growth on human ascites, an ex vivo medium that reflects the infection environment. A subset of 34 mutants with unique gene disruptions that demonstrated little to no growth on ascites underwent evaluation in a rat subcutaneous abscess model, establishing 18 (53%) of these genes as in vivo essential. The putative gene products all had annotated biological functions, represented unrecognized or underexploited antimicrobial targets, and could be grouped into five functional categories: metabolic, two-component signaling systems, DNA/RNA synthesis and regulation, protein transport, and structural. These A. baumannii in vivo essential genes overlapped poorly with the sets of essential genes from other Gram-negative bacteria catalogued in the Database of Essential Genes (DEG), including those of Acinetobacter baylyi, a closely related species. However, this finding was not due to the absence of orthologs. None of the 18 in vivo essential genes identified in this study, or their putative gene products, were targets of FDA-approved drugs or drugs in the developmental pipeline, indicating that a significant portion of the available target space within pathogenic Gram-negative bacteria is currently neglected., IMPORTANCE The human pathogen Acinetobacter baumannii is of increasing clinical importance, and a growing proportion of isolates are multiantimicrobial-resistant, pan-antimicrobial-resistant, or extremely resistant strains. This scenario is reflective of the general problem of a critical lack of antimicrobials effective against antimicrobial-resistant Gram-negative bacteria, such as Pseudomonas aeruginosa, Klebsiella pneumoniae, Enterobacter sp., and Escherichia coli. This study identified a set of A. baumannii genes that are essential for growth and survival during infection and demonstrated the importance of using clinically relevant media and in vivo validation while screening for essential genes for the purpose of developing new antimicrobials. Furthermore, it established that if a gene is absent from the Database of Essential Genes, it should not be excluded as a potential antimicrobial target. Lastly, a new set of high-value potential antimicrobial targets for pathogenic Gram-negative bacteria has been identified.

Published

2012

23. Rat Pneumonia and Soft-Tissue Infection Models for the Study of Acinetobacter baumannii Biology▿

Author

Nicole R. Luke, Steven R. Gill, Anthony A. Campagnari, Thomas A. Russo, Ruth Olson, Janet M. Beanan, and Ulrike MacDonald

Subjects

Acinetobacter baumannii, Blood Bactericidal Activity, Neutrophils, Virulence Factors, Immunology, Colony Count, Microbial, Virulence, Biology, Lung injury, Microbiology, In vivo, medicine, Animals, Pathogen, Lung, Host factor, Skin, Extraintestinal Pathogenic Escherichia coli, Soft Tissue Infections, Proteins, Bacterial Infections, Pneumonia, medicine.disease, biology.organism_classification, Survival Analysis, Rats, Disease Models, Animal, Mutagenesis, Insertional, Infectious Diseases, Cytokines, Parasitology, Pneumonia (non-human), Bronchoalveolar Lavage Fluid, Acinetobacter Infections

Abstract

Acinetobacter baumannii is a bacterial pathogen of increasing medical importance. Little is known about its mechanisms of pathogenesis, and safe reliable agents with predictable activity against A. baumannii are presently nonexistent. The availability of relevant animal infection models will facilitate the study of Acinetobacter biology. In this report we tested the hypothesis that the rat pneumonia and soft-tissue infection models that our laboratory had previously used for studies of extraintestinal pathogenic Escherichia coli were clinically relevant for A. baumannii . Advantages of these models over previously described models were that the animals were not rendered neutropenic and they did not receive porcine mucin with bacterial challenge. Using the A. baumannii model pathogen 307-0294 as the challenge pathogen, the pneumonia model demonstrated all of the features of infection that are critical for a clinically relevant model: namely, bacterial growth/clearance, an ensuing host inflammatory response, acute lung injury, and, following progressive bacterial proliferation, death due to respiratory failure. We were also able to demonstrate growth of 307-0294 in the soft-tissue infection model. Next we tested the hypothesis that the soft-tissue infection model could be used to discriminate between the inherent differences in virulence of various A. baumannii clinical isolates. The ability of A. baumannii to grow and/or be cleared in this model was dependent on the challenge strain. We also hypothesized that complement is an important host factor in protecting against A. baumannii infection in vivo. In support of this hypothesis was the observation that the serum sensitivity of various A. baumannii clinical isolates in vitro roughly paralleled their growth/clearance in the soft-tissue infection model in vivo. Lastly we hypothesized that the soft-tissue infection model would serve as an efficient screening mechanism for identifying gene essentiality for drug discovery. Random mutants of 307-0294 were initially screened for lack of growth in human ascites in vitro. Selected mutants were subsequently used for challenge in the soft-tissue infection model to determine if the disrupted gene was essential for growth in vivo. Using this approach, we have been able to successfully identify a number of genes essential for the growth of 307-0294 in vivo. In summary, these models are clinically relevant and can be used to study the innate virulence of various Acinetobacter clinical isolates and to assess potential virulence factors, vaccine candidates, and drug targets in vivo and can be used for pharmacokinetic and chemotherapeutic investigations.

Published

2008

24. Hypervirulent K. Pneumoniae Secretes More and More Active Iron-Acquisition Molecules than 'Classical' K. Pneumoniae Thereby Enhancing its Virulence

Author

Ulrike MacDonald, Mark P. Visitacion, Ruth Olson, Alyssa S. Shon, Janet M. Beanan, Thomas A. Russo, and Alexander O. Pomakov

Subjects

Bacterial Diseases, Siderophore, Klebsiella pneumoniae, Iron, Mutant, lcsh:Medicine, Virulence, Pathogenesis, Gastroenterology and Hepatology, Microbiology, Mice, 03 medical and health sciences, Model Organisms, In vivo, Animals, Secretion, lcsh:Science, Biology, Microbial Pathogens, 030304 developmental biology, 0303 health sciences, Multidisciplinary, biology, Strain (chemistry), 030306 microbiology, lcsh:R, Quorum Sensing, Klebsiella Pneumonia, biology.organism_classification, Bacterial Pathogens, Klebsiella Infections, 3. Good health, Host-Pathogen Interaction, Infectious Diseases, Culture Media, Conditioned, Models, Animal, Medicine, Clinical Immunology, lcsh:Q, Ex vivo, Research Article

Abstract

Background A new hypervirulent (hypermucoviscous) clinical variant of Klebsiella pneumoniae (hvKP) has emerged over the last decade. Our goal is to identify new mechanisms, which increase the virulence hvKP compared to “classic” K. pneumoniae (cKP). Methodology/Principal Findings Various growth assays were performed in human ascites, human serum, and laboratory medium with the hvKP strain hvKP1 (wt), randomly chosen blood isolates of cKP strains (cKP1-4), and mutant constructs deficient in the secretion of selected compounds. An in vivo mouse model that mimics infection due to hvKP and a quantitative siderophore assay were also used. It was established that a molecule(s)/factor(s) was secreted by hvKP1 significantly enhanced its growth and/or survival in human ascites. This molecule(s)/factor(s) also increased the growth and/or survival of hvKP1 in serum ex vivo and in an in vivo mouse model that measures metastatic spread after subcutaneous challenge, thereby further establishing biologic significance. Although features such as a size of

Published

2011