Your search keyword '"Genisyuerek S"' showing total 5 results

1. Inositol hexakisphosphate-dependent processing of Clostridium sordellii lethal toxin and Clostridium novyi alpha-toxin.

Author

Guttenberg G, Papatheodorou P, Genisyuerek S, Lü W, Jank T, Einsle O, and Aktories K

Subjects

Bacterial Proteins, Bacterial Toxins chemistry, Clostridium sordellii chemistry, Hydrogen-Ion Concentration, Peptide Fragments pharmacology, Protein Binding, Protein Conformation, Bacterial Toxins metabolism, Clostridium chemistry, Phytic Acid metabolism

Abstract

Clostridium sordellii lethal toxin and Clostridium novyi α-toxin, which are virulence factors involved in the toxic shock and gas gangrene syndromes, are members of the family of clostridial glucosylating toxins. The toxins inactivate Rho/Ras proteins by glucosylation or attachment of GlcNAc (α-toxin). Here, we studied the activation of the autoproteolytic processing of the toxins by inositol hexakisphosphate (InsP(6)) and compared it with the processing of Clostridium difficile toxin B. In the presence of low concentrations of InsP(6) (<1 μM), toxin fragments consisting of the N-terminal glucosyltransferase (or GlcNAc-transferase) domains and the cysteine protease domains (CPDs) of C. sordellii lethal toxin, C. novyi α-toxin, and C. difficile toxin B were autocatalytically processed. The cleavage sites of lethal toxin (Leu-543) and α-toxin (Leu-548) and the catalytic cysteine residues (Cys-698 of lethal toxin and Cys-707 of α-toxin) were identified. Affinity of the CPDs for binding InsP(6) was determined by isothermal titration calorimetry. In contrast to full-length toxin B and α-toxin, autocatalytic cleavage and InsP(6) binding of full-length lethal toxin depended on low pH (pH 5) conditions. The data indicate that C. sordellii lethal toxin and C. novyi α-toxin are InsP(6)-dependently processed. However, full-length lethal toxin, but not its short toxin fragments consisting of the glucosyltransferase domain and the CPD, requires a pH-sensitive conformational change to allow binding of InsP(6) and subsequent processing of the toxin.

Published

2011

2. Structural determinants for membrane insertion, pore formation and translocation of Clostridium difficile toxin B.

Author

Genisyuerek S, Papatheodorou P, Guttenberg G, Schubert R, Benz R, and Aktories K

Subjects

Amino Acid Sequence, Animals, Bacterial Proteins genetics, Bacterial Toxins genetics, Cell Line, Cell Membrane metabolism, Clostridioides difficile chemistry, Clostridioides difficile genetics, Enterocolitis, Pseudomembranous metabolism, Humans, Molecular Sequence Data, Pore Forming Cytotoxic Proteins genetics, Pore Forming Cytotoxic Proteins metabolism, Protein Structure, Tertiary, Protein Transport, Sequence Alignment, Sequence Deletion, Bacterial Proteins chemistry, Bacterial Proteins metabolism, Bacterial Toxins chemistry, Bacterial Toxins metabolism, Cell Membrane microbiology, Clostridioides difficile metabolism, Enterocolitis, Pseudomembranous microbiology, Pore Forming Cytotoxic Proteins chemistry

Abstract

Clostridium difficile toxins A and B bind to eukaryotic target cells, are endocytosed and then deliver their N-terminal glucosyltransferase domain after processing into the cytosol. Whereas glucosyltransferase, autoprocessing and cell-binding domains are well defined, structural features involved in toxin delivery are unknown. Here, we studied structural determinants that define membrane insertion, pore formation and translocation of toxin B. Deletion analyses revealed that a large region, covering amino acids 1501-1753 of toxin B, is dispensable for cytotoxicity in Vero cells. Accordingly, a chimeric toxin, consisting of amino acids 1-1550 and the receptor-binding domain of diphtheria toxin, caused cytotoxic effects. A large N-terminal part of toxin B (amino acids 1-829) was not essential for pore formation (measured by (86) Rb(+) release in mammalian cells). Studies using C-terminal truncation fragments of toxin B showed that amino acid residues 1-990 were still capable of inducing fluorescence dye release from large lipid vesicles and led to increased electrical conductance in black lipid membranes. Thereby, we define the minimal pore-forming region of toxin B within amino acid residues 830 and 990. Moreover, we identify within this region a crucial role of the amino acid pair glutamate-970 and glutamate-976 in pore formation of toxin B., (© 2011 Blackwell Publishing Ltd.)

Published

2011

3. Clostridial glucosylating toxins enter cells via clathrin-mediated endocytosis.

Author

Papatheodorou P, Zamboglou C, Genisyuerek S, Guttenberg G, and Aktories K

Subjects

Bacterial Proteins metabolism, Caveolae drug effects, Caveolae metabolism, Chlorpromazine pharmacology, Coated Pits, Cell-Membrane drug effects, Coated Pits, Cell-Membrane metabolism, Dynamins antagonists & inhibitors, Dynamins metabolism, Genes, Dominant genetics, Glycosylation drug effects, HeLa Cells, Humans, Hydrazones pharmacology, Mutation genetics, RNA Interference drug effects, Sphingomyelin Phosphodiesterase metabolism, Sphingomyelins metabolism, Bacterial Toxins metabolism, Clathrin Heavy Chains metabolism, Endocytosis drug effects

Abstract

Clostridium difficile toxin A (TcdA) and toxin B (TcdB), C. sordellii lethal toxin (TcsL) and C. novyi alpha-toxin (TcnA) are important pathogenicity factors, which represent the family of the clostridial glucosylating toxins (CGTs). Toxin A and B are associated with antibiotic-associated diarrhea and pseudomembraneous colitis. Lethal toxin is involved in toxic shock syndrome after abortion and alpha-toxin in gas gangrene development. CGTs enter cells via receptor-mediated endocytosis and require an acidified endosome for translocation of the catalytic domain into the cytosol. Here we studied the endocytic processes that mediate cell internalization of the CGTs. Intoxication of cells was monitored by analyzing cell morphology, status of Rac glucosylation in cell lysates and transepithelial resistance of cell monolayers. We found that the intoxication of cultured cells by CGTs was strongly delayed when cells were preincubated with dynasore, a cell-permeable inhibitor of dynamin, or chlorpromazine, an inhibitor of the clathrin-dependent endocytic pathway. Additional evidence about the role of clathrin in the uptake of the prototypical CGT family member toxin B was achieved by expression of a dominant-negative inhibitor of the clathrin-mediated endocytosis (Eps15 DN) or by siRNA against the clathrin heavy chain. Accordingly, cells that expressed dominant-negative caveolin-1 were not protected from toxin B-induced cell rounding. In addition, lipid rafts impairment by exogenous depletion of sphingomyelin did not decelerate intoxication of HeLa cells by CGTs. Taken together, our data indicate that the endocytic uptake of the CGTs involves a dynamin-dependent process that is mainly governed by clathrin.

Published

2010

4. Modulation of Ca2+ entry and plasma membrane potential by human TRPM4b.

Author

Fliegert R, Glassmeier G, Schmid F, Cornils K, Genisyuerek S, Harneit A, Schwarz JR, and Guse AH

Subjects

Animals, COS Cells, Calcium Channels genetics, Calcium Channels metabolism, Cell Line, Cell Membrane drug effects, Cell Membrane metabolism, Chlorocebus aethiops, Gene Expression, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Humans, Ionomycin pharmacology, Ionophores pharmacology, Membrane Potentials drug effects, Membrane Potentials genetics, Membrane Potentials physiology, Microscopy, Confocal, Patch-Clamp Techniques, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Recombinant Fusion Proteins physiology, Reverse Transcriptase Polymerase Chain Reaction, TRPM Cation Channels genetics, TRPM Cation Channels metabolism, Calcium metabolism, Calcium Channels physiology, Cell Membrane physiology, TRPM Cation Channels physiology

Abstract

TRPM4b is a Ca(2+)-activated, voltage-dependent monovalent cation channel that has been shown to act as a negative regulator of Ca(2+) entry and to be involved in the generation of oscillations of Ca(2+) influx in Jurkat T-lymphocytes. Transient overexpression of TRPM4b as an enhanced green fluorescence fusion protein in human embryonic kidney (HEK) cells resulted in its localization in the plasma membrane, as demonstrated by confocal fluorescence microscopy. The functionality and plasma membrane localization of overexpressed TRPM4b was confirmed by induction of Ca(2+)-dependent inward and outward currents in whole cell patch clamp recordings. HEK-293 cells stably overexpressing TRPM4b showed higher ionomycin-activated Ca(2+) influx than wild-type cells. In addition, analysis of the membrane potential using the potentiometric dye bis-(1,3-dibutylbarbituric acid)-trimethine oxonol and by current clamp experiments in the perforated patch configuration revealed a faster initial depolarization after activation of Ca(2+) entry with ionomycin. Furthermore, TRPM4b expression facilitated repolarization and thereby enhanced sustained Ca(2+) influx. In conclusion, in cells with a small negative membrane potential, such as HEK-293 cells, TRPM4b acts as a positive regulator of Ca(2+) entry.

Published

2007

5. Accumulation of FlAsH/Lumio Green in active mitochondria can be reversed by beta-mercaptoethanol for specific staining of tetracysteine-tagged proteins.

Author

Langhorst MF, Genisyuerek S, and Stuermer CA

Subjects

Fluoresceins metabolism, Fluorescent Dyes metabolism, HeLa Cells, Humans, Membrane Proteins chemistry, Mercaptoethanol pharmacology, Microscopy, Fluorescence, Mitochondria drug effects, Mitochondria metabolism, Organometallic Compounds metabolism, Repetitive Sequences, Amino Acid, Cysteine analysis, Fluoresceins analysis, Fluorescent Dyes analysis, Mercaptoethanol chemistry, Mitochondria chemistry, Organometallic Compounds analysis, Staining and Labeling methods

Abstract

Recent advances in the field of small molecule labels for live cell imaging promise to overcome some of the limitations set by the size of fluorescent proteins. We tested the tetracysteine-biarsenical labeling system in live cell fluorescence microscopy of reggie-1/flotillin-2 in HeLa and N2a cells. In both cell types, the biarsenical staining reagent FlAsH/Lumio Green accumulated in active mitochondria and led to mitochondrial swelling. This is indicative of toxic side effects caused by arsenic, which should be considered when this labeling system is to be used in live cell imaging. Mitochondrial accumulation of FlAsH/Lumio Green was reversed by addition of low concentrations of thiol-containing reagents during labeling and a subsequent high stringency thiol wash. Both ethanedithiol and beta-mercaptoethanol proved to be effective. We therefore established a staining protocol using beta-mercaptoethanol as thiol binding site competitor resulting in a specific staining of tetracysteine-tagged reggie-1/flotillin-2 of adequate signal to noise ratio, so that the more toxic and inconvenient ethanedithiol could be avoided. Furthermore, we show that staining efficiency was greatly enhanced by introducing a second tetracysteine sequence in tandem.

Published

2006