TY - THES A1 - Gonzalez-Leal, Iris Janet T1 - Roles of cathepsins B and L in the Th1/Th2 polarization by dendritic cells T1 - Die Rolle von Kathepsinen B und L während der Th1/Th2 Polarisierung durch Dendritische Zellen N2 - Leishmaniasis is a neglected tropical disease that can be manifested through different clinical forms, ranging from cutaneous to visceral. The host response against Leishmania spp. is greatly dependent on T cell-mediated immunity, in which T helper 1 responses are associated with macrophage activation and elimination of the parasite, while regulatory T cells and T helper 2 responses are correlated with parasite survival and persistence of infection. Leishmania uses different virulence factors as strategies for evading the immune response of the host. One of them are cathepsin-like cysteine proteases, which are currently under extensive investigation as targets for drug development. Previous studies with inhibitors of cathepsins B and L in vivo revealed an outstanding modulation of the host T helper cell response. However, the mechanisms behind these observations were not further investigated. Given the urgent need for better treatments against leishmaniasis, the aim of this study was to investigate the effects that the lack of cathepsin B and L activity have on the signals that dendritic cells use to instruct T helper cell polarization in response to infection with Leishmania major. The cathepsin inhibitors tested showed low or no cytotoxicity in bone marrow-derived dendritic cells, and dendritic cells and macrophages could be generated from cathepsin B and cathepsin L-deficient mice without apparent alterations in their phenotype in comparison to wild-type controls. Furthermore, lack of cathepsin B and L activity showed no impact in the rate of promastigote processing by dendritic cells. Cathepsin B and cathepsin L-deficient macrophages showed no differences in parasite proliferation and capacity to produce nitric oxide in comparison to wild-type macrophages. In response to the parasite, dendritic cells treated with a cathepsin B inhibitor and dendritic cells from cathepsin B-deficient mice showed higher levels of expression of major histocompatibility complex (MHC) class II molecules than dimethyl sulfoxide (DMSO) or wild-type controls, but it was not accompanied by changes in the expression of costimulatory molecules. Wild-type dendritic cells and macrophages are not able to express the pro-inflammatory cytokine interleukin (IL)-12 in response to promastigotes. However, cells treated with a cathepsin B inhibitor or cells deficient for cathepsin B were able to express IL-12, whilethe expression of other cytokines -including IL-6 and tumor necrosis factor (TNF)-alpha-remained unchanged. These characteristics point towards a more “pro-Th1” profile of dendritic cells in the absence of cathepsin B. This data is the first report on IL-12 regulation depending on cathepsin B. The IL-12 up-regulation observed was already present at the transcriptional level. Furthermore, it was also present in macrophages and dendritic cells in response to LPS, and the latter had a higher capacity to induce T cell helper 1 polarization in vitro than wild-type dendritic cells. The activation of different signaling pathways was analyzed, but the up-regulation of IL-12 could not be attributed to modulation of nuclear factor-kappaB (NFkappaB), p38 mitogen activated protein kinase (MAPK) and extra-cellular signal-regulated kinase (ERK)1/2 pathways. Thus, the mechanism behind IL-12 regulation by cathepsin B remains to be elucidated, and the impact of these effects is yet to be confirmed in vivo. Altogether it is tempting to speculate that cathepsin B, in addition to its role in processing endocytosed material, is involved in the modulation of the pro-inflammatory cytokine IL-12. N2 - Leishmaniose ist eine hauptsächlich in den Tropen vorkommende Infektionskrankheit, die sich in verschiedenen klinischen Formen, von kutan bis viszeral, manifestieren kann. Die Reaktion des Wirtes gegen Leishmania spp. hängt stark von der T-Zell-vermittelten Immunantwort ab, wobei die Antwort der T1-Helferzellen assoziiert ist mit der Aktivierung von Makrophagen und der Beseitigung des Parasiten, während die regulatorischen T-Zellen und T2-Helferzellen mit dem Überleben der Parasiten und der Fortdauer der Infektion in Verbindung stehen. Leishmania verwendet verschiedene Virulenzfaktoren als Strategie zur Umgehung der Immunantwort des Wirtes. Darunter zählen Cathepsin-ähnliche Cysteinproteasen, die derzeit Gegenstand umfangreicher Untersuchungen sind mit dem Ziel, für die Arzneimittelentwicklung eingesetzt werden zu können. Frühere Studien mit Inhibitoren von Cathepsin B und L in vivo zeigten eine hervorragende Modulation der Wirt-T-Helferzellantwort. Jedoch wurden die Mechanismen, die diesen Beobachtungen zu Grunde liegen, nicht weiter untersucht. Angesichts der dringenden Notwendigkeit einer besseren Behandlung gegen Leishmaniose war das Ziel dieser Studie die Auswirkungen zu untersuchen, die das Fehlen von Cathepsin B und L-Aktivität auf die Signale hat, welche die dendritischen Zellen verwenden, um die Reaktion der T-Helferzellen auf eine Infektion mit Leishmania major zu beeinflussen. Die getesteten Cathepsin-Inhibitoren zeigten geringe oder keine Cytotoxizität in den aus dem Knochenmark präparierten dendritischen Zellen. Dendritische Zellen und Makrophagen von Cathepsin B- und Cathepsin L-defizienten Mäusen zeigten keine offensichtlichen Veränderungen ihres Phänotyps im Vergleich zu Wildtypkontrollen. Weiterhin zeigte das Fehlen von Cathepsin B- und L-Aktivität keine Auswirkung auf die Prozessierung der Promastigoten durch dendritische Zellen. Auch zeigten Cathepsin Bund Cathepsin L-defiziente Makrophagen keine Unterschiede in der Parasitenproliferation und der Fähigkeit Stickoxid zu produzieren im Vergleich zu Wildtyp-Makrophagen. In Reaktion auf den Parasiten war bei mit einem Cathepsin-B-Inhibitor behandelten dendritischen Zellen und dendritischen Zellen von Cathepsin-B-defizienten Mäusen eine höhere Expression von MHC-Klasse-II-Molekülen ersichtlich im Vergleich zu DMSO oder Wildtyp-Kontrollen, aber es wurden keine Veränderungen in der Expression von costimulatorischen Molekülen festgestellt. Dendritische Zellen und Makrophagen von Wildtyp-Mäusen sind nicht in der Lage das pro-inflammatorische Zytokin IL-12 als Reaktion auf die Promastigoten zu exprimieren. Jedoch konnten dendritische Zellen, die mit einem Cathepsin-B-Inhibitor behandelt waren oder Cathepsin-B-defiziente Zellen, IL-12 exprimieren, während die Expression von anderen Zytokinen - einschließlich IL-6 und TNF-alpha- unverändert blieb. Diese Eigenschaften weisen in die Richtung einer "pro-Th1"-Antwort der dendritischen Zellen in Abwesenheit von Cathepsin B. Diese Daten sind der erste Bericht über die IL-12-Regulierung in Abhängigkeit von Cathepsin B. Die Hochregulation von IL-12 war bereits auf der Transkriptionsebene zu beobachten. Weiterhin war sie in Makrophagen und dendritischen Zellen auch als Reaktion auf LPS vorhanden. Dendritische Zellen von Cathepsin B-defizienten Mäusen hatten eine höhere Kapazität zur Induktion einer eine T1-Helferzell-Polarisierung in vitro als dendritische Zellen von Wildtyp-Mäusen. Die Aktivierung von verschiedenen Signalwegen wurde untersucht, jedoch konnte die Hochregulierung von IL-12 nicht auf die Modulation von NF_B, p38 MAPK und ERK1/2-Signalwege zurückgeführt werden. Damit ist der für die IL-12-Regulierung durch Cathepsin B verantwortliche Mechanismus noch nicht geklärt; auch die Auswirkungen dieser Effekte in vivo müssen noch bestätigt werden. Insgesamt lässt die vorliegende Studie vermuten, dass Cathepsin B nicht nur an der Prozessierung von endozytiertem Material sondern auch an der Regulierung des pro-inflammatorischen Zytokins IL-12 beteiligt ist. KW - Leishmaniose KW - Dendritische Zelle KW - leishmaniasis KW - dendritic cells KW - th1/th2 polarization KW - T-Lymphozyt KW - Helferzelle KW - Immunologie KW - Infektionsbiologie Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-114397 ER - TY - JOUR A1 - Hacker, Jörg A1 - Kestler, H. A1 - Hoschützky, H. A1 - Jann, K. A1 - Lottspeich, F. A1 - Korhonen, T. K. T1 - Cloning and characterization of the S fimbrial adhesin (SfaII) complex of an Escherichia coli O18:K1 meningitis isolate N2 - S fimbrial adbesins (Sfa), which are able to recognize sialic acid-containing receptors on eukaryotic cells, are produced by Escherichia coli strains causing urinary tract infections or newbom meningitis. We recently described tbe cloning and molecular cbaracterization of a determinant, termed sftJI, from the chromosome of an E. coli urinary tract infection strain. Herewe present data conceming a S fimbria-specific gene duster, designated sfall, of an E. coli newbom meningitis strain. Like tbe Sfal complex, Sfall consists of tbe major subunit protein SfaA (16 kDa) and the minor subunit proteins SfaG (17 kDa), SfaS (15 kDa), and SfaH (29 kDa). The genes encoding tbe subunit proteins of Sfall were identified and sequenced. Their protein sequences were calculated from the DNA sequences and compared with tbose of the Sfal complex subunits. Altbough the sequences ofthe two major SfaA subunits ditf'ered markedly, tbe sequences ofthe minor subunits sbowed only a few amino acid exchanges (SfaG, SfaH) or were completely identical (SfaS). The introduction of a site-specific mutation into the gene sfaSII and subsequent analysis of an SfaS-negative clone indicated that sfaSII codes for the sialic acid-specific adhesin of tbe meninigitis isolate. These data were confirmed by tbe isolation and characterization of tbe SfaSII protein and the determination of its N-terminal amino acid sequence. The identity between the sialic acid-specific adhesins of Sfal and Sfall revealed that difl'erences between the two Sfa complexes with respect to tbeir capacities to agglutinate erythrocytes must result from sequence alterations of subunit proteins other tban SfaS. KW - Infektionsbiologie Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59853 ER - TY - JOUR A1 - Zingler, G. A1 - Blum, G. A1 - Falkenhagen, U. A1 - Orskov, I. A1 - Orskov, F. A1 - Hacker, Jörg A1 - Ott, M T1 - Clonal differentiation of uropathogenic E. coli isolates of serotype O6:K5 by fimbrial antigen typing and DNA long-range mapping techniques N2 - Escherichia coli isolates of serotype 06: K5 are the most common causative agents of cystitis and pyelonephritis in adults. To answer the question, as to whether strains of this particular serotype represent one special clonal group, out of a collection of 34 serotype 06: K5 isolates [Zingler et al. ( 1990) Zentralbl. Bakteriol Mikrobiol Hyg [A] 274:372-381] 15 strains were selected andanalyzed in detail. The flagellar (H) antigen and the outer membrane protein (OMP) pattern were determined. Furtherserum resistance properties and the genetic presence and expression of other virulence factors, including hemolysin, aerobactin, P fimbriae, S/F1C fimbriae and type 1 fimbriae was evaluated. In~laddition the Xbalmacrorestriction pattern of ten representative isolates was elaborated and the fimbrial (F) antigentype ofthe P fimbriae was determined, to obtain the complete 0: K: H: F pattern. These analyses could clearly show that the 06: K5 isolates do not represent one clonal group. The Xbal-macrorestriction profiles were heterogeneaus and marked differences in the hybridization patterns, using virulenceassociated gene probes in Southern hybridization of long-range-separated genomic DNA, were observed among the strains. However, some of strains showed similarities in the genomic profiles, arguing for clonal groupings among the 06: K5 isolates. lnterstingly the strains grouped tagether exhibited the same fimbrial F typethat many indicate a coincidence of this phenotypic trait with clonality. KW - Infektionsbiologie Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59865 ER - TY - JOUR A1 - Hacker, Jörg A1 - Ott, M. A1 - Hof, H. T1 - Effects of low, subinhibitory concentrations of antibiotics on expression of a virulence gene cluster of pathogenic E. coli by using a wild-type gene fusion N2 - No abstract available KW - Infektionsbiologie Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59874 ER - TY - JOUR A1 - Morschhäuser, J. A1 - Uhlin, B. E. A1 - Hacker, Jörg T1 - Transcriptional analysis and regulation of the sfa determinant coding for S fimbria of pathogenic E. coli strains N2 - The sfa determinant codes for S fimbrial adhesins which constitute adherence factors of pathogenic Escherichia coli strains. Wehave recently shown that the sfa determinant is transcribed from three prömoters, pA, pB, and pC. In comparison with the promoters pB and pC, promoter pA, which is located in front of the structural gene sfaA, showed very weak activity. Herewe have determined the exact positions ofthe mRNA start points by primer extension studies. We have also shown that mRNAs of 500, 700 and 1400 bases can be detected using oligonucleotide probes specific for the genes sfaB, sfaC and sfaA. SfaB and SfaC arepositive regulators infiuencing fimbriation and the production of the S-specific adhesin which is encoded by the gene sfaS Iocated in the distal half of the determinant. In addition, it is demonstrated that SfaB and SfaC interfere with the regulatory effect of the histone-like protein H-NS, encoded by a locus termed drdX or osmZ. In a drdx+ strain the regulators are necessary for transcription of the sfa determinant. In contrast, sfa expression is activator-independent in a drdx- strain. In this latter genetic background, a substantial fraction of the sfa transcripts is initiated from promoter pA. On the basis of these data we discuss a model for the regulation of this adhesin-specific determinant. KW - Infektionsbiologie KW - Gene regulation KW - Fimbriae KW - Adhesion KW - Transcription KW - trans-activation Y1 - 1993 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59844 ER - TY - JOUR A1 - Linhardt, F. A1 - Ziebuhr, W. A1 - Meyer, P. A1 - Witte, W. A1 - Hacker, Jörg T1 - Pulsed-field gel electrophoresis of genomic restriction fragments as a tool for the epidemiological analysis of Staphylococcus aureus and coagulase-negative Staphylococci N2 - Thirtccn StttJ1hylococcus dw·eus and s: <'pid<'l'· midis strains ohtaincd from nnsc and hand nf twn cmployccs and onc paticnt uf a mcdical ward as weil as two S. hemol.\"licus strains wcrc analyscd according to thcir rcstrktion fmgmcnt lcngth pattcrns ( RFLP) hy pulscd-ficld gcl clcctrophorcsis (PFGE) using thc rcslriction cnzymcs SmaJ and s.. .· tll. Spccics idcntification nf thc isolatcs was pcrformcd hy a systcm which includcs :!O hiochcmical rc"ctions. Furthcrmorc. thc antillintic resistancc pattcrns of thc stmins wcrc dctcrmincd. Whilc scvcral isolatcs cxhihitcd idcnticaf antihiotic susccptihilitics and hiochcmical prnfilcs. diffcrences in thc RFLP wcrc ohtaincd. ln thrcc cascs, S. epidermülis strains colonizing thc skin showcd an idcntical rcstriction profilc as isollltcs from thc mucous mcmhrancs of thc samc pcrson. Wc C(mcludcd that thc analysis of staphylococcal strains hy PFGE is an important cpidcmiolngical tnnl with high discrimination power. KW - Infektionsbiologie Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59811 ER - TY - JOUR A1 - Ott, M. A1 - Bender, L. A1 - Lück, P. C. A1 - Meyer, P. A1 - Hacker, Jörg T1 - Distribution of Legionellae in a hospital water system: prevalence of immunologically and genetically related Legionella pneumophila serogroup 6 isolates N2 - A hospital warm water system was monitored for the prcsence and distribution of lcgionellac. Subtyping of ten scletled Legionella pneumophiltl isolates. originating from four different sites in the system by using serogroup spccific antisera in an indircct immunofluorcscence tcst, rcvcalcd that nine of the tcn isolatcs belonged to scrogroup 6, while the remaining one was serogroup I 0. Two monoclonal antibodics (mAbs) spccific for a subgroup of serogroup 6 strains were further used for characterization. None of the strains reactcd with these mAbs. Genome analysis by elaborating Not I profiles using the pulscd field gel electrophoresis (PFGE) technique revealed that nearly all serogroup 6 isolates dcrived from different sites, including a new building connected hy a ring pipe. wcrc identical according to restriction fragment pattems. The patterns were distinguishable from those of the two L. pnewnophi/a serogroup 6 rcfcrencc strains, and ftom that of thc L. pneumophila scrogroup 10 isolate. These data arguc for a relatively homogeneaus L. pneunwpltila serogroup 6 population in the entire watcr system. KW - Infektionsbiologie KW - Legionella pneumophila KW - Hospital water system KW - Environmental isolate KW - Serogroup KW - Genomic profile Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59827 ER - TY - JOUR A1 - Schroten, H. A1 - Steinig, M. A1 - Plogmann, R. A1 - Hanisch, F. G. A1 - Hacker, Jörg A1 - Herzig, P. A1 - Wahn, V T1 - S-fimbriae mediated adhesin of Escherichia coli to human buccal epithelial cells is age independent N2 - S-fimbriated Escherichia coli, which cause sepsis and meningitis in the newbom, bind to sialic acid-containing glycoprotein structures on the surface of human buccal epithelial cells. The dependence of · this binding on host age was examined. S-fimbriated · E. coli adhered in comparable numbers to cells in newborns, infants, children and adults (23.0 ± 8.6; 23.1 ± 11.5; 24.7 ± 7.9; 28.9 ± 8.8). Thus, the increased susceptibility of neonates to infections caused by S-fimbriated E. coli cannot be explained by enhanced · adhesion to epithelial cells N2 - Die S-Fimbrien vermittelte Adhiision von Escherichia coli an menschliche Mundschleimhautzellen ist altersunabhängig. S-Fimbrien tragende Escherichia coli, die Sepsis und Meningitis . im Neugeborenenalter verursachen, binden an sialinsäurehaltige Glycoproteine atif der Oberfläche menschlicher Mundschleimhautzellen. Wir untersuchten die Abhängigkeit · der Bindung vom Alter des Schleimhautzellenspenders. S-Fimbrien tragende. E. coli banden in vergleichbarer Zahl an Zellen von Neugeborenen, Säuglingen, älteren · Kindern und Erwachsenen (23,0 ± 8,6; 23,1 ± 11,5; 24,7 ± 7,9; 28,9 ± 8,8). Die vermehrte Empfänglichkeit von Neugeborenen für Infektionen, die durch S- Fimbrien tragende E. coli verursacht werden, kann nicht mit einer verstärkten Adhäsion an Mundschleimhautzellen erklärt wer.den. KW - Infektionsbiologie Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59830 ER - TY - JOUR A1 - Fischer, G. A1 - Bang, H. A1 - Ludwig, B. A1 - Mann, K. H. A1 - Hacker, Jörg T1 - Mip protein of Legionella pneumophila exhibits peptidyl-prolyl cis-trans-isomerase (PPIase) activity N2 - Legfonells pneumoph/la is an intracellular paraslte which ts able to survtve and multipJy in human monocytes and alveolar macrophages. The Mtp (macrophage lnfectiv1ty potentlator) protein has been shown to be an essential virulente factor. A search of translated nuclelt .acld data ba.ses has shown that the Mip proteJn from strain Wadsworth possesses reglons homologaus to those found in the FK.506-bindfng proteins (FKBPs) of several different eukaryotlc organisms. FKBPs are abte to bind to the fmmunosuppressant macrollde FK506 and possess peptidyf .. prolyl cisltrans Isomerase (PPiase) activlty. The gene coding for the Mlp proteln was cloned from the ehromo. some of L. pneumophila straln Philadelph·a I and sequenced. II was synthesl%ed in Escherichla coll ·K- 12 and alter purlfication it exhibited PPiase activity catalyslng the slow clsltrans lsomerization of prolyl peptlde bonds. ln ollgopeptides. Mip ls inhibi~ted by FK506 and fully reslstant to cyclosporln A, as was also found for the recently characterlzed FKBP-type PPiases of eukaryotes. However, the N-terminal extenslon of Mip and/or the substltutrons of the vari· ab1e amlno acrds ln the C-termlnal FKBP core Iead to variatlons,. when compared with eukaryotlc FKBPs, Jn substrate specfflclty wlth the Oligopeptide substrates of' type Suc-Aia-Xaa-Pro-Phe·4·nitroanUide. Never· theless, the Legionella Mip factor represents a bacte· rial gene product whtch shares some characteristics normally found in eukaryotic proteins. ln view of the activity of PPiases in protein-folding reactlonsf such prokaryotic FKBP analogues may represent a new class of bacterial. pathogenicity factors. KW - Infektionsbiologie Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59778 ER - TY - JOUR A1 - Schroten, H. A1 - Hanisch, F. G. A1 - Plogmann, R. A1 - Hacker, Jörg A1 - Uhlenbruck, G. A1 - Wahn, V. T1 - Inhibition of Adhesion of S-fimbriated Escherichia coli to buccal epithelial cells by human milk fat globule membrane components: a novel aspect of protective function of mucins in the non-immunoglobulin fraction N2 - We investigated the presence of factors in human milkthat inhibit Invasion of pathogenic bacteria. The efl'ect of human milk fat globule membrane (HMFGM) components on adhesion of cloned S-fimbriated Escherichia coli to human buccal epithelial cells was analyzed. S fimbriae are a common feature of E. coli strains causing sepsis and meningitis in newborns and are bound to epithelia via sialyl-(a-2-3)galactoside structures. Human milk fat globules (HMFG) could be agglutinated by the above-mentioned bacteria. Agglutination could be inhibited by fetuin, human glycophorin, and a 1-acid glycoprotein. In addition, pretreatment of HMFG with Jlibrio cholerae neuraminidase markedly reduced bacterium-induced agglutinations, indicating the involvement of neuraminic acid-containing glycoproteins. In contrast, Iipid droplets of infant formula or artificiallipid emulsions (Intralipid) could not be agglutinated. HMFG were present in stools of breast-fed neonates as shown by indirect immunofluorescence staining with a monoclonal antibody directed against carbohydrate residues present on HMFGM. These HMFG could be agglutinated by bacteria. HMFG inhibited E. coli adhesion to buccal epithelial cells. To further characterize relevant E. coli binding structures, HMFGM components w~re separated by gel chromatography. The mucin fraction showed the most pronounced inhibitory efrect on adhesion of S-fimbriated E. coli to human buccal epithelial cells. Our data soggest that HMFG inhibit bacterial adhesion in the entire intestine and thereby may provide protection against bacterial infection. KW - Infektionsbiologie Y1 - 1992 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-59793 ER -