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5. Ulceroglandular tularemia

Author

Potz-Biedermann, C, Schwendemann, L, Schröppel, K, Sönnichsen, K, Schmidt, D, Schaller, M, University of Zurich, and Schaller, M

Subjects
2708 Dermatology, 10042 Clinic for Diagnostic and Interventional Radiology, 610 Medicine & health
Published
2011

6. High-throughput-screening-based identification and structure-activity relationship characterization defined (S)-2-(1-aminoisobutyl)-1-(3-chlorobenzyl) benzimidazole as a highly antimycotic agent nontoxic to cell lines

Author

Bauer, J., Kinast, S., Burger-Kentischer, A., Finkelmeier, D., Kleymann, G., Rayyan, W.A., Schröppel, K., Singh, A., Jung, G., Wiesmüller, K.-H., Rupp, S., Eickhoff, H., and Publica

Abstract

Novel nontoxic (S)-2-aminoalkylbenzimidazole derivatives were found to be effective against Candida spp. at low micromolar concentrations using high-throughput screening with infected HeLa cells. A collection of analogues defined the chemical groups relevant for activity. The most active compound was characterized by transcriptional analysis of the response of C. albicans Sc5314. (S)-2-(1-Aminoisobutyl)-1-(3-chlorobenzyl)benzimidazole had a strong impact on membrane biosynthesis. Testing different clinically relevant pathogenic fungi showed the selectivity of the antimycotic activity against Candida species.

Published
2011

7. Identification and Characterization of Cor33p, a novel protein implicated in tolerance towards oxidative stress in Candida albicans

Author

Sohn, K., Röhm, M., Urban, C.F., Saunders, N., Rothenstein, D., Lottspeich, F., Schröppel, K., Rupp, S., and Publica

Abstract

We applied two-dimensional gel electrophoresis to identify downstream effectors of CPH1 and EFG1 under hypha-inducing conditions in Candida albicans. Among the proteins that were expressed in wild-type cells but were strongly downregulated in a cph1 Delta/efg1 Delta double mutant in alpha-minimal essential medium at 37 degrees C, we could identify not-yet-characterized proteins, including Cor33-1p and Cor33-2p. The two proteins are almost identical (97% identity) and represent products of allelic isoforms of the same gene. Cor33p is highly similar to Cip1p from Candida sp. but lacks any significant homology to proteins from Saccharomyces cerevisiae. Strikingly, both proteins share homology with phenylcoumaran benzylic ether reductases and isoflavone reductases from plants. For other hypha-inducing media, like yeast-peptone-dextrose (YPD) plus serum at 37 degrees C, we could not detect any transcription for COR33 in wild-type cells, indicating that Cor33p is not hypha specific. In contrast, we found a strong induction for COR33 when cells were treated with 5 mM hydrogen peroxide. However, under oxidative conditions, transcription of COR33 was not dependent on EFG1, indicating that other regulatory factors are involved. In fact, upregulation depends on CAP1 at least, as transcript levels were clearly reduced in a Delta cap1 mutant strain under oxidative conditions. Unlike in wild-type cells, transcription of COR33 in a tsa1 Delta mutant can be induced by treatment with 0.1 mM hydrogen peroxide. This suggests a functional link between COR33 and thiol-specific antioxidant-like proteins that are important in the oxidative-stress response in yeasts. Concordantly, cor33 Delta deletion mutants show retarded growth on YPD plates supplemented with hydrogen peroxide, indicating that COR33 in general is implicated in conferring tolerance toward oxidative stress on Candida albicans.

Published
2005

8. The moonlighting protein Tsa1p is implicated in oxidative stress response and in cell wall biogenesis in Candida albicans

Author

Urban, C.F., Sohn, K., Schröppel, K., Brunner, H., Rupp, S., and Publica

Abstract

Candida albicans is one of the most common fungal pathogens in humans. The cell wall is the first contact site between host and pathogen and thus is critical for colonization and infection of the host. We have identified Tsa1p, a protein that is differentially localized to the cell wall of C. albicans in hyphal cells but remains in the cytosol and nucleus in yeast-form cells. This is different from Saccharomyces cerevisiae, where the homologous protein solely has been found in the cytoplasm. We report here that TSA1 confers resistance towards oxidative stress as well as is involved in the correct composition of hyphal cell walls. However, no significant change of the cell wall composition was observed in a TSA1 deletion strain in yeast-form cells, which is in good agreement with the observation that Tsa1p is absent from the yeast-form cell wall. This indicates that Tsa1p of C. albicans might represent a moonlighting protein with specific functions correlating to its respective localization. Furthermore, the translocation of Tsa1p to the hyphal cell wall of C. albicans depends on Efg1p, suggesting a contribution of the cAMP/PKA pathway to the localization of this protein. In a strain deleted for TUP1 that filaments constitutively Tsa1p can be found in the cell wall under all conditions tested, confirming the result that Tsa1p localization to the cell wall is correlated to the morphology of C. albicans.

Published
2005

10. Identification and characterization of Cor33p, a novel protein implicated in tolerance towards oxidative stress in Candida albicans

Author

Sohn, K, Roehm, M, Urban, Constantin, Saunders, N, Rothenstein, D, Lottspeich, F, Schröppel, K, Brunner, H, Rupp, S, Sohn, K, Roehm, M, Urban, Constantin, Saunders, N, Rothenstein, D, Lottspeich, F, Schröppel, K, Brunner, H, and Rupp, S

Abstract

We applied two-dimensional gel electrophoresis to identify downstream effectors of CPH1 and EFG1 under hypha-inducing conditions in Candida albicans. Among the proteins that were expressed in wild-type cells but were strongly downregulated in a cph1Delta/efg1Delta double mutant in alpha-minimal essential medium at 37 degrees C, we could identify not-yet-characterized proteins, including Cor33-1p and Cor33-2p. The two proteins are almost identical (97% identity) and represent products of allelic isoforms of the same gene. Cor33p is highly similar to Cip1p from Candida sp. but lacks any significant homology to proteins from Saccharomyces cerevisiae. Strikingly, both proteins share homology with phenylcoumaran benzylic ether reductases and isoflavone reductases from plants. For other hypha-inducing media, like yeast-peptone-dextrose (YPD) plus serum at 37 degrees C, we could not detect any transcription for COR33 in wild-type cells, indicating that Cor33p is not hypha specific. In contrast, we found a strong induction for COR33 when cells were treated with 5 mM hydrogen peroxide. However, under oxidative conditions, transcription of COR33 was not dependent on EFG1, indicating that other regulatory factors are involved. In fact, upregulation depends on CAP1 at least, as transcript levels were clearly reduced in a Deltacap1 mutant strain under oxidative conditions. Unlike in wild-type cells, transcription of COR33 in a tsa1Delta mutant can be induced by treatment with 0.1 mM hydrogen peroxide. This suggests a functional link between COR33 and thiol-specific antioxidant-like proteins that are important in the oxidative-stress response in yeasts. Concordantly, cor33Delta deletion mutants show retarded growth on YPD plates supplemented with hydrogen peroxide, indicating that COR33 in general is implicated in conferring tolerance toward oxidative stress on Candida albicans.

Published
2005
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14. Is zoom-endoscopic subaqual mucosa evaluation able to replace biopsy in the diagnostics of acute tissue rejection in patients with small intestine transplantation?

Author

Kratt, T, primary, Stüker, D, additional, Minkley, L, additional, Steurer, W, additional, Ladurner, R, additional, Nadalin, S, additional, Feilitzsch, M von, additional, Küper, M, additional, Thiel, C, additional, Lamprecht, HG, additional, Fend, F, additional, Hann von Weyhern, C, additional, Schröppel, K, additional, and Königsrainer, A, additional

Published
2010
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15. IS ZOOM-ENDOSCOPIC SUBAQUAL MUCOSA EVALUATION ABLE TO REPLACE BIOPSY IN THE DIAGNOSTICS OF ACUTE TISSUE REJECTION IN PATIENTS WITH SMALL INTESTINE TRANSPLANTATION?

Author

Kratt, T., primary, Minkley, L., additional, Stueker, D., additional, Steurer, W., additional, Ladurner, R., additional, Küper, M., additional, Thiel, C., additional, Lamprecht, H. G., additional, Fend, F., additional, von Weyhern, Hann C., additional, Schröppel, K., additional, Königsrainer, A., additional, and Nadalin, S., additional

Published
2010
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25. IL-4 enhances IL-3 and IL-8 gene expression in a human leukemic mast cell line.

Author

Gessner, A., Will, A., Vieth, M., Schröppel, K., and Röllinghoff, M.

Subjects
INTERLEUKIN-4, INTERLEUKIN-3, INTERLEUKIN-8, LYMPHOCYTES, MAST cells, CYTOKINES
Abstract

We examined the capacity of interleukin (IL)-4 to induce or enhance the expression of certain cytokines in resting and activated cells of the HMC-1 human leukemic mast cell line. The HMC-1 mast cells were cultured with or without recombinant human IL-4 and then activated with the calcium ionophore ionomycin. Stimulation of non-IL-4-treated cells with ionomycin (10 µM) for periods of 30 min to 8 hr induced expression of mRNA encoding IL-3, IL-4 and IL-8 but was without effect on levels of mRNA for tumour necrosis factor (TNF)-α or Β-actin. Culture of the cells with IL-4 (100 ng/ml) for 24 hr led to a small increase in resting levels of m RNA for IL-3 and IL-8 but not for IL-4, TNF-α or Β-actin. More notably, the IL-4 treatment produced a pronounced elevation of mRNA for IL-3 and IL-8 when the cells were subsequently activated with ionomycin. The IL-4 treatment produced a negligible effect on IL-4 mRNA, and no effect on TNF-α or Β-actin mRNA levels in ionomycin-activated cells. Quantitation of cDNA by competitive polymerase chain reaction (PCR) revealed that the IL-4 treatment produced a sixfold increase in ionomycin-induced levels of cellular IL-3 mRNA, a fourfold increase in induced IL-8 mRNA and less than a twofold increase in induced IL-4 mRNA. The IL-4 treatment led to a 15- to 20-fold increase in ionomycin-induced secretion of IL-3 product and a doubling of induced IL-8 product. These effects of IL-4 were not associated with increased mast cell numbers. We conclude that IL-4 alone is a weak activator of IL-3 and IL-8 gene expression in mast cells, but is able to enhance activation signals in stimulated mast cells leading to transcription and secretion of these two cytokines. [ABSTRACT FROM AUTHOR]

Published
1995

26. Interleukin-10 Inhibits Antimicrobial Activity Against Leishmania major in Murine Macrophages.

Author

Vieth, M., Will, A., Schröppel, K., Röllinghoff, M., and Gessner, A.

Subjects
INTERLEUKIN-10, MICROORGANISMS, LEISHMANIA, BONE marrow, MACROPHAGES
Abstract

The stimulation of macrophages is of importance to the defense against intracellularly replicating microorganisms such as Leishmania. In this study the direct effect of recombinant interleukin-10 (IL-10) on the leishmanicidal effector functions of murine peritoneal or bone marrow derived macrophages was investigated. IL-10 almost completely inhibited the killing of intracellular leishmania at concentrations above 10ng/ml. This inhibitory effect was independent of the stimulus used as the activation of macrophages by IFN-γ and IL-7, recently shown to possess macrophage activating properties, were suppressed by IL-10. Kinetic experiments revealed that IL-10 must be present during the process of macrophage activation and that the leishmanicidal effector function of fully activated macrophages was not influenced. Furthermore, in the absence of exogenously added IL-10, the addition of neutralizing antibodies against IL-10 or IL-10-specific antisense phosphorothioate DNA-oligonucleotide led to an enhanced killing of parasites after stimulation with either IFN-γ or IL-7. In accordance with this, IL-10 mRNA was readily detectable in murine macrophages by PCR with reverse transcribed mRNA. These results indicate that IL-10, which is endogenously produced by macrophages, acts as an autocrine deactivating factor supporting the survival of the parasite. [ABSTRACT FROM AUTHOR]

Published
1994
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27. Roles of the Candida albicans mitogen-activated protein kinase homolog, Cek1p, in hyphal development and systemic candidiasis.

Author

Csank, C, Schröppel, K, Leberer, E, Harcus, D, Mohamed, O, Meloche, S, Thomas, D Y, and Whiteway, M

Abstract

Extracellular signal-regulated protein kinase (ERK, or mitogen-activated protein kinase [MAPK]) regulatory cascades in fungi turn on transcription factors that control developmental processes, stress responses, and cell wall integrity. CEK1 encodes a Candida albicans MAPK homolog (Cek1p), isolated by its ability to interfere with the Saccharomyces cerevisiae MAPK mating pathway. C. albicans cells with a deletion of the CEK1 gene are defective in shifting from a unicellular budding colonial growth mode to an agar-invasive hyphal growth mode when nutrients become limiting on solid medium with mannitol as a carbon source or on glucose when nitrogen is severely limited. The same phenotype is seen in C. albicans mutants in which the homologs (CST20, HST7, and CPH1) of the S. cerevisiae STE20, STE7, and STE12 genes are disrupted. In S. cerevisiae, the products of these genes function as part of a MAPK cascade required for mating and invasiveness of haploid cells and for pseudohyphal development of diploid cells. Epistasis studies revealed that the C. albicans CST20, HST7, CEK1, and CPH1 gene products lie in an equivalent, canonical, MAPK cascade. While Cek1p acts as part of the MAPK cascade involved in starvation-specific hyphal development, it may also play independent roles in C. albicans. In contrast to disruptions of the HST7 and CPH1 genes, disruption of the CEK1 gene adversely affects the growth of serum-induced mycelial colonies and attenuates virulence in a mouse model for systemic candidiasis.

Published
1998

28. Repression of hyphal proteinase expression by the mitogen-activated protein (MAP) kinase phosphatase Cpp1p of Candida albicans is independent of the MAP kinase Cek1p.

Author

Schröppel, K, Sprösser, K, Whiteway, M, Thomas, D Y, Röllinghoff, M, and Csank, C

Abstract

Cpp1p is a putative mitogen-activated protein (MAP) kinase phosphatase that suppresses Candida albicans hyphal formation at 25 degrees C through its probable substrate, the Cek1p filamentation MAP kinase. Here we report that expression of the serum-induced genes SAP4-6 and HYR1 increased several fold in hyphal forms of a cpp1/cpp1 null mutant, while the rate and extent of hyphal development up to 5 h were normal. Therefore, we provide evidence that Cpp1p represses hyphal gene expression by acting through a Cek1p-independent mechanism. SAP4-6 and HYR1 transcripts were undetectable in a null mutant of another key regulator of filamentation, Efg1p; thus, Efg1p and Cpp1p oppose each other during the expression of these genes in hyphal forms.

Published
2000

30. Analysis of a long-term outbreak of XDR Pseudomonas aeruginosa: a molecular epidemiological study.

Author

Willmann M, Bezdan D, Zapata L, Susak H, Vogel W, Schröppel K, Liese J, Weidenmaier C, Autenrieth IB, Ossowski S, and Peter S

Subjects
Disease Transmission, Infectious, Environmental Microbiology, Epidemiologic Studies, Genome, Bacterial, Germany epidemiology, Hospitals, University, Humans, Molecular Epidemiology, Molecular Typing, Pseudomonas Infections transmission, Pseudomonas aeruginosa genetics, Pseudomonas aeruginosa isolation & purification, Sequence Analysis, DNA, Spatio-Temporal Analysis, Disease Outbreaks, Drug Resistance, Multiple, Bacterial, Pseudomonas Infections epidemiology, Pseudomonas Infections microbiology, Pseudomonas aeruginosa classification, Pseudomonas aeruginosa drug effects
Abstract

Objectives: Here we report on a long-term outbreak from 2009 to 2012 with an XDR Pseudomonas aeruginosa on two wards at a university hospital in southern Germany., Methods: Whole-genome sequencing was performed on the outbreak isolates and a core genome was constructed for molecular epidemiological analysis. We applied a time-place-sequence algorithm to improve estimation of transmission probabilities., Results: By using conventional infection control methods we identified 49 P. aeruginosa strains, including eight environmental isolates that belonged to ST308 (by MLST) and carried the metallo-β-lactamase IMP-8. Phylogenetic analysis on the basis of a non-recombinant core genome that contained 22 outbreak-specific SNPs revealed a pattern of four dominant clades with a strong phylogeographic structure and allowed us to determine the potential temporal origin of the outbreak to July 2008, 1 year before the index case was diagnosed. Superspreaders at the root of clades exhibited a high number of probable and predicted transmissions, indicating their exceptional position in the outbreak., Conclusions: Our results suggest that the initial expansion of dominant sublineages was driven by a few superspreaders, while environmental contamination seemed to sustain the outbreak for a long period despite regular environmental control measures., (© The Author 2015. Published by Oxford University Press on behalf of the British Society for Antimicrobial Chemotherapy. All rights reserved. For Permissions, please e-mail: journals.permissions@oup.com.)

Published
2015
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31. Time to positivity as prognostic tool in patients with Pseudomonas aeruginosa bloodstream infection.

Author

Willmann M, Kuebart I, Vogel W, Flesch I, Markert U, Marschal M, Schröppel K, Autenrieth IB, Hölzl F, and Peter S

Subjects
Adolescent, Adult, Aged, Aged, 80 and over, Analysis of Variance, Area Under Curve, Bacteremia diagnosis, Female, Humans, Male, Middle Aged, Prognosis, Pseudomonas Infections diagnosis, Retrospective Studies, Bacteremia microbiology, Pseudomonas Infections microbiology, Pseudomonas aeruginosa isolation & purification
Abstract

Objectives: The time to positivity (TTP), measured as the time span between the start of incubation and the alert signal from the blood culture device, has been described as useful tool of prognosis in patients suffering from blood stream infection with Staphylococcus aureus, Escherichia coli and Klebsiella pneumonia. The present study investigates the relationship between TTP and in-hospital mortality in patients with monomicrobial Pseudomonas aeruginosa blood stream infection (PA-BSI)., Methods: From 2006 until 2012 a retrospective cohort study was undertaken in 3 hospitals in the region surrounding Tübingen, Germany. Seventy-four patients with monomicrobial PA-BSI were studied. TTP and clinical parameters were determined and analyzed by receiver operating characteristic (ROC) analysis and Cox regression., Results: The in-hospital mortality of our clinical cohort was 33.78%. In multivariate Cox regression, a TTP ≤ 18 h proved to be independently associated with mortality (HR 3.83, P = 0.012) along with SAPS II score (HR 1.04, P = 0.006), cardiac disease (HR 0.33, P = 0.008) and appropriate definitive antimicrobial treatment (HR 0.21, P = 0.013)., Conclusions: TTP is an easy-to-measure laboratory tool for prognosis in patients with monomicrobial PA-BSI, providing useful information in addition to clinical parameters., (Copyright © 2013 The British Infection Association. Published by Elsevier Ltd. All rights reserved.)

Published
2013
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32. Effect of metallo-β-lactamase production and multidrug resistance on clinical outcomes in patients with Pseudomonas aeruginosa bloodstream infection: a retrospective cohort study.

Author

Willmann M, Kuebart I, Marschal M, Schröppel K, Vogel W, Flesch I, Markert U, Autenrieth IB, Hölzl F, and Peter S

Subjects
Aged, Anti-Bacterial Agents pharmacology, Bacteremia diagnosis, Bacteremia epidemiology, Bacteremia mortality, Cohort Studies, Cross Infection epidemiology, Cross Infection microbiology, Drug Resistance, Multiple, Bacterial, Female, Germany epidemiology, Hospital Mortality, Hospitals, Humans, Male, Middle Aged, Prognosis, Pseudomonas Infections diagnosis, Pseudomonas Infections epidemiology, Pseudomonas Infections mortality, Pseudomonas aeruginosa genetics, Retrospective Studies, Treatment Outcome, beta-Lactamases genetics, beta-Lactamases metabolism, Bacteremia microbiology, Pseudomonas Infections microbiology, Pseudomonas aeruginosa drug effects, Pseudomonas aeruginosa enzymology, beta-Lactamases biosynthesis
Abstract

Background: Blood stream infections (BSI) with Pseudomonas aeruginosa lead to poor clinical outcomes. The worldwide emergence and spread of metallo-β-lactamase (MBL) producing, often multidrug-resistant organisms may further aggravate this problem. Our study aimed to investigate the effect of MBL-producing P. aeruginosa (MBL-PA) and various other resistance phenotypes on clinical outcomes., Methods: A retrospective cohort study was conducted in three German hospitals. Medical files from 2006 until 2012 were studied, and a number of 113 patients with P. aeruginosa BSI were included. The presence of VIM, IMP and NDM genes was detected using molecular techniques. Genetic relatedness was assessed through multilocus sequence typing (MLST). The effect of resistance patterns or MBL production on clinical outcomes was investigated by using multivariate Cox regression models., Results: In-hospital mortality was significantly higher in patients with MBL-PA and multidrug-resistant P. aeruginosa. However, neither BSI with MBL-PA nor BSI with various resistance phenotypes of P. aeruginosa were independently associated with mortality or length of hospital stay. In multivariate models, the SAPS II score (HR 1.046), appropriate definitive treatment (HR range 0.25-0.26), and cardiovascular disease (HR range 0.44-0.46) were independent predictors of mortality. Concomitant infections were associated with an excess length of stay (HR < 1)., Conclusions: Medication with appropriate antimicrobial agents at any time during the course of infection remains the key for improving clinical outcomes in patients with P. aeruginosa BSI and should be combined with a strict implementation of routine infection control measures.

Published
2013
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33. Time series analysis as a tool to predict the impact of antimicrobial restriction in antibiotic stewardship programs using the example of multidrug-resistant Pseudomonas aeruginosa.

Author

Willmann M, Marschal M, Hölzl F, Schröppel K, Autenrieth IB, and Peter S

Subjects
Drug Resistance, Multiple, Bacterial, Microbial Sensitivity Tests, Anti-Bacterial Agents pharmacology, Pseudomonas aeruginosa drug effects
Abstract

The association between antimicrobial consumption and resistance in nonfermentative Gram-negative bacteria is well-known. Antimicrobial restriction, implemented in clinical routines by antibiotic stewardship programs (ASPs), is considered a means to reduce resistance rates. Whether and how antimicrobial restriction can accomplish this goal is still unknown though. This leads to an element of uncertainty when designing strategies for ASPs. From January 2002 until December 2011, an observational study was performed at the University Hospital Tübingen, Tübingen, Germany, to investigate the association between antimicrobial use and resistance rates in Pseudomonas aeruginosa. Transfer function models were used to determine such associations and to simulate antimicrobial restriction strategies. Various positive associations between antimicrobial consumption and resistance were observed in our setting. Surprisingly, impact estimations of different antimicrobial restriction strategies revealed relatively low intervention expenses to effectively attenuate the observed increase in resistance. For example, a simulated intervention of an annual 4% reduction in the use of meropenem over 3 years from 2009 until 2011 yielded a 62.5% attenuation (95% confidence interval, 15% to 110%) in the rising trend of multidrug-resistant Pseudomonas aeruginosa (three- and four-class-resistant P. aeruginosa [34MRGN-PA]). Time series analysis models derived from past data may be a tool to predict the outcome of antimicrobial restriction strategies, and could be used to design ASPs.

Published
2013
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34. High-throughput-screening-based identification and structure-activity relationship characterization defined (S)-2-(1-aminoisobutyl)-1-(3-chlorobenzyl)benzimidazole as a highly antimycotic agent nontoxic to cell lines.

Author

Bauer J, Kinast S, Burger-Kentischer A, Finkelmeier D, Kleymann G, Rayyan WA, Schröppel K, Singh A, Jung G, Wiesmüller KH, Rupp S, and Eickhoff H

Subjects
Antifungal Agents chemical synthesis, Antifungal Agents pharmacology, Antifungal Agents toxicity, Antimitotic Agents pharmacology, Antimitotic Agents toxicity, Benzimidazoles pharmacology, Benzimidazoles toxicity, Candida drug effects, Candida genetics, Cell Line, Tumor, Drug Screening Assays, Antitumor, High-Throughput Screening Assays, Humans, Imidazoles chemical synthesis, Imidazoles pharmacology, Imidazoles toxicity, Microbial Sensitivity Tests, Mycology methods, Stereoisomerism, Structure-Activity Relationship, Transcription, Genetic drug effects, Antimitotic Agents chemical synthesis, Benzimidazoles chemical synthesis
Abstract

Novel nontoxic (S)-2-aminoalkylbenzimidazole derivatives were found to be effective against Candida spp. at low micromolar concentrations using high-throughput screening with infected HeLa cells. A collection of analogues defined the chemical groups relevant for activity. The most active compound was characterized by transcriptional analysis of the response of C. albicans Sc5314. (S)-2-(1-Aminoisobutyl)-1-(3-chlorobenzyl)benzimidazole had a strong impact on membrane biosynthesis. Testing different clinically relevant pathogenic fungi showed the selectivity of the antimycotic activity against Candida species.

Published
2011
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35. A screening assay based on host-pathogen interaction models identifies a set of novel antifungal benzimidazole derivatives.

Author

Burger-Kentischer A, Finkelmeier D, Keller P, Bauer J, Eickhoff H, Kleymann G, Abu Rayyan W, Singh A, Schröppel K, Lemuth K, Wiesmüller KH, and Rupp S

Subjects
Animals, Antifungal Agents chemistry, Antifungal Agents toxicity, Benzimidazoles chemistry, Benzimidazoles pharmacology, Benzimidazoles toxicity, CHO Cells, Candida genetics, Candida isolation & purification, Candidiasis drug therapy, Candidiasis microbiology, Cell Line, Cricetinae, Drug Resistance, Fungal, Ergosterol antagonists & inhibitors, Genome, Fungal, HeLa Cells, High-Throughput Screening Assays, Humans, Microbial Sensitivity Tests, Oligonucleotide Array Sequence Analysis, Structure-Activity Relationship, Transcription, Genetic, Antifungal Agents pharmacology, Candida drug effects, Host-Pathogen Interactions drug effects
Abstract

Fungal infections are a serious health problem in clinics, especially in the immune-compromised patient. Disease ranges from widespread superficial infections like vulvovaginal infections to life-threatening systemic candidiasis. Especially for systemic mycoses, only a limited arsenal of antifungals is available. The most commonly used classes of antifungal compounds used include azoles, polyenes, and echinocandins. Due to emerging resistance to standard therapy, significant side effects, and high costs for several antifungals, there is a medical need for new antifungals in the clinic and general practice. In order to expand the arsenal of compounds with antifungal activities, we screened a compound library including more than 35,000 individual compounds derived from organic synthesis as well as combinatorial compound collections representing mixtures of compounds for antimycotic activity. In total, more than 100,000 compounds were screened using a new type of activity-selectivity assay, analyzing both the antifungal activity and the compatibility with human cells at the same time. One promising hit, an (S)-2-aminoalkyl benzimidazole derivative, was developed among a series of lead compounds showing potent antifungal activity. (S)-2-(1-Aminoisobutyl)-1-(3-chlorobenzyl) benzimidazole showed the highest antifungal activity and the best compatibility with human cells in several cell culture models and against a number of clinical isolates of several species of pathogenic Candida yeasts. Transcriptional profiling indicates that the newly discovered compound is a potential inhibitor of the ergosterol pathway, in contrast to other benzimidazole derivatives, which target microtubules.

Published
2011
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36. Ulceroglandular tularemia.

Author

Potz-Biedermann C, Schwendemann L, Schröppel K, Sönnichsen K, Schmidt D, and Schaller M

Subjects
Abscess drug therapy, Administration, Oral, Aged, Animals, Anti-Bacterial Agents therapeutic use, Bites and Stings complications, Disease Vectors, Doxycycline therapeutic use, Humans, Injections, Intramuscular, Leg Ulcer drug therapy, Lymphadenitis drug therapy, Male, Streptomycin therapeutic use, Ticks, Tularemia drug therapy, Tularemia transmission, Abscess diagnosis, Leg Ulcer diagnosis, Lymphadenitis diagnosis, Tularemia diagnosis, Zoonoses
Abstract

An increasing number of patients with the zoonosis tularemia have been reported in the last few years in Europe. Tularemia can be divided into different forms depending on its appearance. Tularemia must be considered in the differential diagnosis of diseases that present with an ulcer and regional lymphadenopathy. The diagnosis can be confirmed by culturing Francisella tularensis. With effective antibiotic intervention, the prognosis is favorable. Typically tularemia develops after outdoor activities; it is generally transferred by blood-sucking arthropods from infected wild animals to humans., (© The Authors • Journal compilation © Blackwell Verlag GmbH, Berlin.)

Published
2011
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37. Integrated detection of extended-spectrum-beta-lactam resistance by DNA microarray-based genotyping of TEM, SHV, and CTX-M genes.

Author

Leinberger DM, Grimm V, Rubtsova M, Weile J, Schröppel K, Wichelhaus TA, Knabbe C, Schmid RD, and Bachmann TT

Subjects
Bacteria genetics, DNA, Bacterial chemistry, DNA, Bacterial genetics, Humans, Molecular Sequence Data, Oligonucleotide Array Sequence Analysis, Sensitivity and Specificity, Sequence Analysis, DNA, Bacteria drug effects, Bacteria enzymology, Genes, Bacterial genetics, Microarray Analysis methods, Microbial Sensitivity Tests methods, beta-Lactam Resistance, beta-Lactamases genetics
Abstract

Extended-spectrum beta-lactamases (ESBL) of the TEM, SHV, or CTX-M type confer resistance to beta-lactam antibiotics in gram-negative bacteria. The activity of these enzymes against beta-lactam antibiotics and their resistance against inhibitors can be influenced by genetic variation at the single-nucleotide level. Here, we describe the development and validation of an oligonucleotide microarray for the rapid identification of ESBLs in gram-negative bacteria by simultaneously genotyping bla(TEM), bla(SHV), and bla(CTX-M). The array consists of 618 probes that cover mutations responsible for 156 amino acid substitutions. As this comprises unprecedented genotyping coverage, the ESBL array has a high potential for epidemiological studies and infection control. With an assay time of 5 h, the ESBL microarray also could be an attractive option for the development of rapid antimicrobial resistance tests in the future. The validity of the DNA microarray was demonstrated with 60 blinded clinical isolates, which were collected during clinical routines. Fifty-eight of them were characterized phenotypically as ESBL producers. The chip was characterized with regard to its resolution, phenotype-genotype correlation, and ability to resolve mixed genotypes. ESBL phenotypes could be correctly ascribed to ESBL variants of bla(CTX-M) (76%), bla(SHV) (22%), or both (2%), whereas no ESBL variant of bla(TEM) was found. The most prevalent ESBLs identified were CTX-M-15 (57%) and SHV-12 (18%).

Published
2010
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38. [Methicillin-resistant Staphylococcus aureus (MRSA) infections. Epidemiology, diagnostics, therapy, and prevention].

Author

Heeg P and Schröppel K

Subjects
Animals, Bacterial Proteins genetics, Bacteriological Techniques, Carrier State, Community-Acquired Infections diagnosis, Community-Acquired Infections drug therapy, Community-Acquired Infections prevention & control, Cross Infection diagnosis, Cross Infection drug therapy, Cross Infection prevention & control, Cross-Sectional Studies, Germany, Humans, Incidence, Penicillin-Binding Proteins, Risk Factors, Staphylococcal Infections diagnosis, Staphylococcal Infections drug therapy, Staphylococcal Infections prevention & control, Universal Precautions, Community-Acquired Infections epidemiology, Cross Infection epidemiology, Methicillin-Resistant Staphylococcus aureus genetics, Staphylococcal Infections epidemiology
Abstract

The increasing number of complicated soft-tissue or invasive infections caused by methicillin-resistant Staphylococcus aureus (MRSA) is a frequent reason for elaborate treatment regimens. Unidentified MRSA carriers may be the origin of endemic spread to other patients and medical staff. Recently, community-associated cMRSA with particular virulence factors were isolated from persons without the typical history of hospital contacts. Molecular tools for the timely detection of the mecA resistance gene for the identification of MRSA in medical test specimens have become a standard approach in MRSA-related diagnostic procedures. The actual therapy of MRSA infections requires consideration of both the appropriate spectrum of activity and the adequate pharmacological properties of a chosen antimicrobial. Preventive strategies rely on the consistent application of standard hygiene precautions, which have to be supplemented with increased barriers for the isolation of identified MRSA patients.

Published
2009
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39. Experimental infection of rodent mammals for fungal virulence testing.

Author

Schweizer A and Schröppel K

Subjects
Animals, Candida albicans genetics, Candidiasis etiology, Female, Fungemia etiology, Humans, Mice, Mice, Inbred BALB C, Mutation, Virulence genetics, Candida albicans pathogenicity, Mycology methods
Abstract

Invasive fungal infections comprise a group of serious and life-threatening diseases affecting immunocompromised patients. Molecular analysis of fungal virulence involves the deletion of genes that are suspected for contributing to fungal pathogenesis. Phenotypic analysis of the generated mutants includes in vivo infection experiments in order to assign a function during fungal disease to a gene of interest.

Published
2009
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40. Ureaplasma urealyticum meningitis in an adult patient.

Author

Geissdörfer W, Sandner G, John S, Gessner A, Schoerner C, and Schröppel K

Subjects
Adult, Anti-Bacterial Agents pharmacology, Anti-Bacterial Agents therapeutic use, Cerebrospinal Fluid microbiology, Chloramphenicol therapeutic use, DNA Gyrase genetics, DNA Topoisomerase IV genetics, Doxycycline therapeutic use, Drug Resistance, Bacterial genetics, Humans, Male, Meningitis, Bacterial drug therapy, Molecular Sequence Data, Quinolones pharmacology, Sequence Analysis, DNA, Treatment Outcome, Ureaplasma Infections drug therapy, Ureaplasma urealyticum classification, Ureaplasma urealyticum drug effects, Ureaplasma urealyticum genetics, Kidney Transplantation adverse effects, Meningitis, Bacterial microbiology, Ureaplasma Infections microbiology, Ureaplasma urealyticum isolation & purification
Abstract

A 38-year-old patient developed meningitis after a complicated kidney transplantation and organ rejection. Ureaplasma urealyticum was identified as the etiological agent by molecular and microbiological analyses of the cerebrospinal fluid. The patient was successfully treated with doxycycline and chloramphenicol. This is the first report of Ureaplasma urealyticum meningitis in an adult.

Published
2008
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41. Analysis of the Candida albicans - specific T-cell response and oropharyngeal Candida colonization in a cohort of HIV-1-infected patients.

Author

Bäuerle M, Schröppel K, Taylor B, Bergmann S, Schmitt-Haendle M, and Harrer T

Subjects
AIDS-Related Opportunistic Infections immunology, CD4 Lymphocyte Count, Candidiasis, Oral immunology, Case-Control Studies, Cohort Studies, Enzyme-Linked Immunosorbent Assay, Female, Humans, Immunity, Mucosal, Interferon-gamma metabolism, Male, Viral Load, AIDS-Related Opportunistic Infections microbiology, CD4-Positive T-Lymphocytes immunology, Candida albicans physiology, Candidiasis, Oral microbiology, Oropharynx microbiology
Abstract

To investigate Candida epidemiology and immunologic correlates of protection in HIV-1 infected patients, we analyzed oral Candida colonization in correlation to the Candida-specific T-cell response measured by g-IFN ELISPOT using different Candida (C.) albicans strains. In 16/46 patients (13 asymptomatic, 3 with oral thrush), but in 0/28 controls, Candida (13 C. albicans, 1 C. lusitaniae, 1 C. krusei, 1 C. parapsilosis) was isolated. Candida specific T-cells were detected more frequently in controls (20/28) than in HIV-1+ subjects (16/46, p= 0.03). We observed a significant association of higher CD4 cell numbers with both detection of Candida specific T-cells and lack of oral Candida colonization, but there was no significant correlation of oral Candida colonization to the detection of Candida specific T-cells, viral load or antiretroviral therapy. Thus, local mucosal immunity seems to be more important in the pathogenesis of Candida colonization than circulating Candida specific T-cells. The pathogenic C. albicans strain K24122 was less frequently recognized by patients (6/46) than the laboratory adapted strain SC5314 (14/46, p= 0.03), whereas a similar recognition of both strains was observed in healthy controls. This indicates an impaired Candida-specific T-cell repertoire in HIV+ patients that could increase the risk of immune evasion by C. albicans.

Published
2006

42. Role of calcineurin in stress resistance, morphogenesis, and virulence of a Candida albicans wild-type strain.

Author

Bader T, Schröppel K, Bentink S, Agabian N, Köhler G, and Morschhäuser J

Subjects
Animals, Calcineurin genetics, Candida albicans genetics, Candida albicans physiology, Candidiasis immunology, Candidiasis microbiology, Disease Models, Animal, Female, Gene Silencing, Immunity, Innate genetics, Mice, Oxidative Stress genetics, Virulence genetics, Calcineurin physiology, Candida albicans growth & development, Candida albicans pathogenicity, Oxidative Stress physiology
Abstract

By generating a calcineurin mutant of the Candida albicans wild-type strain SC5314 with the help of a new recyclable dominant selection marker, we confirmed that calcineurin mediates tolerance to a variety of stress conditions but is not required for the ability of C. albicans to switch to filamentous growth in response to hypha-inducing environmental signals. While calcineurin was essential for virulence of C. albicans in a mouse model of disseminated candidiasis, deletion of CMP1 did not significantly affect virulence during vaginal or pulmonary infection, demonstrating that the requirement for calcineurin for a successful infection depends on the host niche.

Published
2006
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43. Fungal adenylyl cyclase integrates CO2 sensing with cAMP signaling and virulence.

Author

Klengel T, Liang WJ, Chaloupka J, Ruoff C, Schröppel K, Naglik JR, Eckert SE, Mogensen EG, Haynes K, Tuite MF, Levin LR, Buck J, and Mühlschlegel FA

Subjects
Animals, Bicarbonates metabolism, Candida albicans genetics, Candida albicans growth & development, Candidiasis mortality, Carbonic Anhydrases metabolism, Cryptococcus neoformans metabolism, Enzyme Induction physiology, Female, Genetic Complementation Test, Mice, Mice, Inbred BALB C, Survival Analysis, Virulence, Adenylyl Cyclases metabolism, Candida albicans enzymology, Candida albicans pathogenicity, Carbon Dioxide metabolism, Cryptococcus neoformans enzymology, Cyclic AMP metabolism, Signal Transduction physiology
Abstract

The ascomycete Candida albicans is the most common fungal pathogen in immunocompromised patients . Its ability to change morphology, from yeast to filamentous forms, in response to host environmental cues is important for virulence . Filamentation is mediated by second messengers such as cyclic adenosine 3',5'-monophosphate (cAMP) synthesized by adenylyl cyclase . The distantly related basidiomycete Cryptococcus neoformans is an encapsulated yeast that predominantly infects the central nervous system in immunocompromised patients . Similar to the morphological change in C. albicans, capsule biosynthesis in C. neoformans, a major virulence attribute, is also dependent upon adenylyl cyclase activity . Here we demonstrate that physiological concentrations of CO2/HCO3- induce filamentation in C. albicans by direct stimulation of cyclase activity. Furthermore, we show that CO2/HCO3- equilibration by carbonic anhydrase is essential for pathogenesis of C. albicans in niches where the available CO2 is limited. We also demonstrate that adenylyl cyclase from C. neoformans is sensitive to physiological concentrations of CO2/HCO3-. These data demonstrate that the link between cAMP signaling and CO2/HCO3- sensing is conserved in fungi and reveal CO2 sensing to be an important mediator of fungal pathogenesis. Novel therapeutic agents could target this pathway at several levels to control fungal infections.

Published
2005
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44. Induction of SAP7 correlates with virulence in an intravenous infection model of candidiasis but not in a vaginal infection model in mice.

Author

Taylor BN, Hannemann H, Sehnal M, Biesemeier A, Schweizer A, Röllinghoff M, and Schröppel K

Subjects
Animals, Aspartic Acid Endopeptidases genetics, Candida genetics, Disease Models, Animal, Female, Fungal Proteins genetics, Gene Deletion, Mice, Mutation, Vagina microbiology, Virulence, Aspartic Acid Endopeptidases metabolism, Candida enzymology, Candida pathogenicity, Candidiasis microbiology, Fungal Proteins metabolism, Vaginal Diseases microbiology
Abstract

SAP7 of Candida albicans is induced after vaginal infection of mice. Conversely, virulence during vaginal infection was not affected in a Deltasap7/Deltasap7 mutant strain. Only a partial virulence phenotype was detectable after intravenous injection. In conclusion, SAP7 expression does not correlate with C. albicans virulence in mice.

Published
2005
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45. The moonlighting protein Tsa1p is implicated in oxidative stress response and in cell wall biogenesis in Candida albicans.

Author

Urban C, Xiong X, Sohn K, Schröppel K, Brunner H, and Rupp S

Subjects
Candida albicans pathogenicity, Candida albicans ultrastructure, Cell Nucleus chemistry, Cell Wall chemistry, Cell Wall genetics, Cell Wall metabolism, Cytoplasm chemistry, DNA-Binding Proteins genetics, Fungal Proteins genetics, Gene Deletion, Gene Expression Regulation, Fungal, Hyphae growth & development, Hyphae metabolism, Nuclear Proteins metabolism, Peroxidases analysis, Peroxidases genetics, Peroxiredoxins, Protein Transport, Repressor Proteins genetics, Repressor Proteins metabolism, Thioredoxin-Disulfide Reductase genetics, Transcription Factors genetics, Transcription, Genetic, Virulence, Vitamin K 3 pharmacology, Water pharmacology, Candida albicans metabolism, Fungal Proteins physiology, Oxidative Stress genetics, Peroxidases physiology
Abstract

Candida albicans is one of the most common fungal pathogens in humans. The cell wall is the first contact site between host and pathogen and thus is critical for colonization and infection of the host. We have identified Tsa1p, a protein that is differentially localized to the cell wall of C. albicans in hyphal cells but remains in the cytosol and nucleus in yeast-form cells. This is different from Saccharomyces cerevisiae, where the homologous protein solely has been found in the cytoplasm. We report here that TSA1 confers resistance towards oxidative stress as well as is involved in the correct composition of hyphal cell walls. However, no significant change of the cell wall composition was observed in a TSA1 deletion strain in yeast-form cells, which is in good agreement with the observation that Tsa1p is absent from the yeast-form cell wall. This indicates that Tsa1p of C. albicans might represent a moonlighting protein with specific functions correlating to its respective localization. Furthermore, the translocation of Tsa1p to the hyphal cell wall of C. albicans depends on Efg1p, suggesting a contribution of the cAMP/PKA pathway to the localization of this protein. In a strain deleted for TUP1 that filaments constitutively Tsa1p can be found in the cell wall under all conditions tested, confirming the result that Tsa1p localization to the cell wall is correlated to the morphology of C. albicans.

Published
2005
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46. Profile of Candida albicans-secreted aspartic proteinase elicited during vaginal infection.

Author

Taylor BN, Staib P, Binder A, Biesemeier A, Sehnal M, Röllinghoff M, Morschhäuser J, and Schröppel K

Subjects
Animals, Aspartic Acid Endopeptidases genetics, Candida albicans enzymology, Candida albicans growth & development, Candidiasis, Vulvovaginal microbiology, Female, Fungal Proteins genetics, Gene Expression Profiling, Gene Expression Regulation, Enzymologic, Humans, Hyphae enzymology, Hyphae growth & development, Mice, Mice, Inbred BALB C, Aspartic Acid Endopeptidases metabolism, Candida albicans pathogenicity, Candidiasis, Vulvovaginal physiopathology, Fungal Proteins metabolism, Gene Expression Regulation, Fungal
Abstract

Vaginal infections caused by the opportunistic yeast Candida albicans are a significant problem in women of child-bearing age. Several factors are recognized as playing a crucial role in the pathogenesis of superficial candidiasis; these factors include hyphal formation, phenotypic switching, and the expression of virulence factors, including a 10-member family of secreted aspartic proteinases. In the present investigation, we analyzed the secreted aspartic proteinase gene (SAP) expression profile of C. albicans that is elicited in the course of vaginal infection in mice and how this in vivo expression profile is associated with hyphal formation. We utilized two different genetic reporter systems that allowed us to observe SAP expression on a single-cell basis, a recombination-based in vivo expression technology and green fluorescent protein-expressing Candida reporter strains. Of the six SAP genes that were analyzed (SAP1 to SAP6), only SAP4 and SAP5 were detectably induced during infection in this model. Expression of both of these genes was associated with hyphal growth, although not all hyphal cells detectably expressed SAP4 and SAP5. SAP5 expression was induced soon after infection, whereas SAP4 was expressed at later times and in fewer cells compared with SAP5. These findings point to a link between morphogenetic development and expression of virulence genes during Candida vaginitis in mice, where host signals induce both hyphal formation and expression of SAP4 and SAP5, but temporal gene expression patterns are ultimately controlled by other factors.

Published
2005
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47. PMT family of Candida albicans: five protein mannosyltransferase isoforms affect growth, morphogenesis and antifungal resistance.

Author

Prill SK, Klinkert B, Timpel C, Gale CA, Schröppel K, and Ernst JF

Subjects
Animals, Candida albicans drug effects, Candida albicans enzymology, Candidiasis microbiology, Candidiasis physiopathology, Female, Humans, Isoenzymes, Mannosyltransferases genetics, Mice, Mice, Inbred BALB C, Microbial Sensitivity Tests, Morphogenesis, Mutation, Virulence, Antifungal Agents pharmacology, Candida albicans growth & development, Candida albicans pathogenicity, Gene Expression Regulation, Fungal, Mannosyltransferases metabolism, Multigene Family
Abstract

Protein O-mannosyltransferases (Pmt proteins) initiate O-mannosylation of secretory proteins. The PMT gene family of the human fungal pathogen Candida albicans consists of PMT1 and PMT6, as well as three additional PMT genes encoding Pmt2, Pmt4 and Pmt5 isoforms described here. Both PMT2 alleles could not be deleted and growth of conditional strains, containing PMT2 controlled by the MET3- or tetOScHOP1-promoters, was blocked in non-permissive conditions, indicating that PMT2 is essential for growth. A homozygous pmt4 mutant was viable, but synthetic lethality of pmt4 was observed in combination with pmt1 mutations. Hyphal morphogenesis of a pmt4 mutant was defective under aerobic induction conditions, yet increased in embedded or hypoxic conditions, suggesting a role of Pmt4p-mediated O-glycosylation for environment-specific morphogenetic signalling. Although a PMT5 transcript was detected, a homozygous pmt5 mutant was phenotypically silent. All other pmt mutants showed variable degrees of supersensitivity to antifungals and to cell wall-destabilizing agents. Cell wall composition was markedly affected in pmt1 and pmt4 mutants, showing a significant decrease in wall mannoproteins. In a mouse model of haematogenously disseminated infection, PMT4 was required for full virulence of C. albicans. Functional analysis of the first complete PMT gene family in a fungal pathogen indicates that Pmt isoforms have variable and specific roles for in vitro and in vivo growth, morphogenesis and antifungal resistance.

Published
2005
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48. Tec1p-independent activation of a hypha-associated Candida albicans virulence gene during infection.

Author

Staib P, Binder A, Kretschmar M, Nichterlein T, Schröppel K, and Morschhäuser J

Subjects
Animals, Aspartic Acid Endopeptidases genetics, Candida albicans genetics, Candida albicans growth & development, Candidiasis microbiology, Candidiasis physiopathology, DNA-Binding Proteins genetics, Disease Models, Animal, Gene Deletion, Humans, Mice, Peritonitis microbiology, Promoter Regions, Genetic, Transcription Factors genetics, Virulence, Aspartic Acid Endopeptidases metabolism, Candida albicans pathogenicity, DNA-Binding Proteins metabolism, Fungal Proteins, Gene Expression Regulation, Fungal, Hyphae growth & development, Peritonitis physiopathology, Transcription Factors metabolism
Abstract

The Tec1p transcription factor is involved in the expression of hypha-specific genes in Candida albicans. Although the induction of the hypha-associated SAP5 gene by serum in vitro depends on Tec1p, deletion of all Tec1p binding site consensus sequences from the SAP5 promoter did not affect its activation. In two different animal models of candidiasis, the SAP5 promoter was induced even in a Deltatec1 deletion mutant, demonstrating that the requirement for Tec1p in gene expression in C. albicans depends on the environmental conditions within the host.

Published
2004
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49. High diversity of ankA sequences of Anaplasma phagocytophilum among Ixodes ricinus ticks in Germany.

Author

von Loewenich FD, Baumgarten BU, Schröppel K, Geissdörfer W, Röllinghoff M, and Bogdan C

Subjects
Anaplasma phagocytophilum classification, Anaplasma phagocytophilum isolation & purification, Animals, Base Sequence, DNA Primers, Germany, Phylogeny, Polymerase Chain Reaction, Anaplasma phagocytophilum genetics, Bacterial Proteins genetics, Genetic Variation genetics, Ixodes microbiology
Abstract

In Germany humans with acute granulocytic ehrlichiosis have not yet been described. Here, we characterized three different genes of Anaplasma phagocytophilum strains infecting German Ixodes ricinus ticks in order to test whether they differ from strains in other European countries and the United States. A total of 1,022 I. ricinus ticks were investigated for infection with A. phagocytophilum by nested PCR and sequence analysis. Forty-two (4.1%) ticks were infected. For all positive ticks, parts of the 16S rRNA and groESL genes were sequenced. The complete coding sequence of the ankA gene could be determined in 24 samples. The 16S rRNA and groESL gene sequences were as much as 100% identical to known sequences. Fifteen ankA sequences were >/=99.37% identical to sequences derived from humans with granulocytic ehrlichiosis in Europe and from a horse with granulocytic ehrlichiosis in Germany. Thus, German I. ricinus ticks most likely harbor A. phagocytophilum strains that can cause disease in humans. Nine additional sequences were clearly different from known ankA sequences. Because these newly described sequences have never been obtained from diseased humans or animals, their biological significance is currently unknown. Based on this unexpected sequence heterogeneity, we propose to use the ankA gene for further phylogenetic analyses of A. phagocytophilum and to investigate the biology and pathogenicity of strains that differ in the ankA gene.

Published
2003
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50. Calcineurin is essential for virulence in Candida albicans.

Author

Bader T, Bodendorfer B, Schröppel K, and Morschhäuser J

Subjects
Amino Acid Sequence, Animals, Base Sequence, Calcineurin chemistry, Calcineurin genetics, Candida albicans genetics, Candida albicans growth & development, Candida albicans physiology, Candidiasis etiology, DNA, Fungal genetics, Female, Gene Deletion, Genes, Fungal, Humans, Hydrogen-Ion Concentration, Mice, Mice, Inbred BALB C, Molecular Sequence Data, Protein Subunits, Sequence Homology, Amino Acid, Virulence genetics, Calcineurin physiology, Candida albicans pathogenicity
Abstract

Calcineurin is a conserved Ca(2+)-calmodulin-activated, serine/threonine-specific protein phosphatase that regulates a variety of physiological processes, e.g., cell cycle progression, polarized growth, and adaptation to salt and alkaline pH stresses. In the pathogenic yeast Cryptococcus neoformans, calcineurin is also essential for growth at 37 degrees C and virulence. To investigate whether calcineurin plays a role in the virulence of Candida albicans, the major fungal pathogen of humans, we constructed C. albicans mutants in which both alleles of the CMP1 gene, encoding the calcineurin catalytic subunit, were deleted. The C. albicans Delta cmp1 mutants displayed hypersensitivity to elevated Na(+), Li(+), and Mn(2+) concentrations and to alkaline pH, phenotypes that have been described after calcineurin inactivation in the related yeast Saccharomyces cerevisiae. Unlike S. cerevisiae calcineurin mutants, which exhibit reduced susceptibility to high Ca(2+) concentrations, growth of C. albicans was inhibited in the presence of 300 mM CaCl(2) after the deletion of CMP1, demonstrating that there are also differences in calcineurin-mediated cellular responses between these two yeast species. In contrast to C. neoformans, inactivation of calcineurin did not cause temperature sensitivity in C. albicans. In addition, hyphal growth, an important virulence attribute of C. albicans, was not impaired in the Delta cmp1 mutants under a variety of inducing conditions. Nevertheless, the virulence of the mutants was strongly attenuated in a mouse model of systemic candidiasis, demonstrating that calcineurin signaling is essential for virulence in C. albicans.

Published
2003
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