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HtrA proteases and chaperones exhibit important roles in periplasmic protein quality control and stress responses. The genetic inactivation of htrA has been described for many bacterial pathogens. However, in some cases such as the gastric pathogen Helicobacter pylori, HtrA is secreted where it cleaves the tumour-suppressor E-cadherin interfering with gastric disease development, but the generation of htrA mutants is still lacking. Here, we show that the htrA gene locus is highly conserved in worldwide strains. HtrA presence was confirmed in 992 H.pylori isolates in gastric biopsy material from infected patients. Differential RNA-sequencing (dRNA-seq) indicated that htrA is encoded in an operon with two subsequent genes, HP1020 and HP1021. Genetic mutagenesis and complementation studies revealed that HP1020 and HP1021, but not htrA, can be mutated. In addition, we demonstrate that suppression of HtrA proteolytic activity with a newly developed inhibitor is sufficient to effectively kill H.pylori, but not other bacteria. We show that Helicobacter htrA is an essential bifunctional gene with crucial intracellular and extracellular functions. Thus, we describe here the first microbe in which htrA is an indispensable gene, a situation unique in the bacterial kingdom. HtrA can therefore be considered a promising new target for anti-bacterial therapy.
Flagellar motility and chemotaxis are essential virulence traits required for the ability of Helicobacter pylori to colonize the gastric mucosa. The flagellar regulatory network and the complex chemotaxis system of H. pylori are fundamentally different from other bacteria, despite many similarities. In H. pylori expression of the flagella is controlled by a complex regulatory cascade involving the two-component system FlgR-HP244, the sigma factors 54 and 28 and the anti-sigma 28 factor FlgM. Thus far, the input signal for histidine kinase HP244, which activates the transcriptional regulator FlgR, which triggers sigma factor 54-dependent transcription of the flagellar class 2 genes, is not known. Based on a yeast two-hybrid screen a highly significant protein-protein interaction between the H. pylori protein HP137 and both the histidine kinase HP244 and the flagellar hook protein HP908 (FlgE´) has been reported recently (Rain et al., 2001). So far, no function could be assigned to HP137. Interestingly, the interaction between HP137 and histidine kinase HP244 was observed in the characteristic block N sequence motif of the C-terminal ATP-binding kinase domain. In this work a potential role of HP137 in a feedback regulatory mechanism controlling the activity of histidine kinase HP244 in the flagellar regulation of H. pylori was investigated. Although the substitution of the gene encoding HP137 by a kanamycin cassette resulted in non-motile bacteria, the failure to restore motility by the reintroduction of hp137 in cis into the mutant strain, and the observation that HP137 has no significant effect on the activity of histidine kinase HP244 in vitro indicated that HP137 is not directly involved in flagellar regulation. Therefore, it was demonstrated that HP137 does not participate in the regulation of flagellar gene expression, neither in H. pylori nor in the closely related bacterium C. jejuni. Chemotactic signal transduction in H. pylori differs from the enterobacterial paradigm in several respects. In addition to a CheY response regulator protein (CheY1) H. pylori contains a CheY-like receiver domain (CheY2) which is C-terminally fused to the histidine kinase CheA. Furthermore, the genome of H. pylori encodes three CheV proteins consisting of an N-terminal CheW-like domain and a C-terminal receiver domain, while there are no orthologues of the chemotaxis genes cheB, cheR, and cheZ. To obtain insight into the mechanism controlling the chemotactic response of H. pylori the phosphotransfer reactions between the purified two-component signalling modules were investigated in vitro. Using in vitro phosphorylation assays it was shown that both H. pylori histidine kinases CheAY2 and CheA´ lacking the CheY-like domain (CheY2) act as ATP-dependent autokinases. Similar to other CheA proteins CheA´ shows a kinetic of phosphorylation represented by an exponential time course, while the kinetics of phosphorylation of CheAY2 is characterized by a short exponential time course followed by the hydrolysis of CheAY2~P. Therefore, it was demonstrated that the presence of the CheY2-like receiver domain influences the stability of the phosphorylated P1 domain of the CheA part of the bifunctional protein. Furthermore, it was proven that both CheY1 and CheY2 are phosphorylated by CheAY2 and CheA´~P and that the three CheV proteins mediate the dephosphorylation of CheA´~P, although with a clearly reduced efficiency as compared to CheY1 and CheY2. Moreover, CheA´ is capable of donating its phospho group to the CheY1 protein from C. jejuni and to CheY protein from E. coli. Retrophosphorylation experiments indicated that CheY1~P is able to transfer the phosphate group back to the HK CheAY2 and the receiver domain present in the bifunctional CheAY2 protein acts as a phosphate sink fine tuning the activity of the freely diffusible CheY1 protein, which is thought to interact with the flagellar motor. Hence, in this work evidence of a complex phosphorelay in the chemotaxis system was obtained which has similarities to other systems with multiple CheY proteins. The role of the CheV proteins remain unclear at the moment, but they might be engaged in a further fine regulation of the phosphate flow in this complex chemotaxis system and the independent function of the two domains CheA´ and CheY2 is not sufficient for normal chemotactic signalling in vivo.
Helicobacter pylori ist ein pathogenes Bakterium, das verantwortlich gemacht wird für verschiedene Erkrankungen des Magens und Duodenums, wie beispielsweise chronische Gastritis, peptische Ulzera und maligne Lymphome. Das Bakterium zeichnet sich durch eine hohe Rekombinationsrate aus und besitzt ein hohes Maß an genetischer Allelvielfalt. Im ersten Teil dieser Arbeit wurde die Rekombinationsrate und die Länge der rekombinerten DNA-Importe anhand von sequentiellen Isolaten, die zu definierten Zeitpunkten aus dem selben Patienten isoliert wurden, untersucht. Es wurden zehn Gene, darunter sieben 'housekeeping' Gene und drei virulenzassoziierte Gene, amplifiziert und sequenziert. Die Ergebnisse zeigten eine bis dahin noch nicht für Bakterien beschriebene Fragmentlänge der DNA-Importe von durchschnittlich lediglich 417 Basenpaaren. Die Rekombinationsrate war außergewöhnlich hoch. DNA-Microarray-Analysen konnten zeigen, dass es trotz dieser hohen Rekombinationsrate nur wenige Veränderungen in der genomischen Genausstattung gab. Jedoch hing das Auftreten von Rekombinationsereignissen direkt mit Veränderungen der Genausstattung zusammen. Im zweiten Teil der Arbeit wurde ein neues in vitro-Transformationsmodell entwickelt, das die in vivo ermittelten Resultate nachvollziehen sollte. Das Modell konnte sowohl die in vivo gefundene Rekombinationsrate als auch den Import von kurzen DNA-Fragmenten bestätigen, die zu einem Allelmosaik zwischen DNA-Rezipient und Donor führten. Auffällig war eine stark verminderte Transformierbarkeit mit Donor-DNA aus asiatischen H. pylori-Stämmen. Um eine mögliche Beteiligung des Nukleotid-Excisions-Reparatur (NER) Mechanismus an der Rekombination zu ermitteln, wurden zwei Gene des Mechanismus ausgeschaltet. Die Ergebnisse der NER--Mutanten (uvrA-, uvrD-) zeigten eine starke Verminderung der Transformierbarkeit. Diese Verminderung hatte jedoch keinen Einfluss auf die Länge der rekombinierten DNA-Importe. Das Ausschalten des uvrA-Gens führte zudem zu einer erhöhten Sensibilität gegenüber UV-Licht. Der NER-Mechanismus ist bei H. pylori in einer noch nicht aufgeklärten Weise an der Rekombination beteiligt. In einem Rhesusaffen-Tiermodell wurde die initiale Besiedlung mit H. pylori untersucht. Die Tiere stellen einen natürlichen Wirt dar und zeigen ähnliche Krankheitssymptome wie menschliche Patienten. Die Rhesusaffen wurden experimentell mit zwei klinischen H. pylori-Isolaten infiziert. Die Reisolation zu bestimmten Zeitpunkten zeigte, dass sich nur einer der beiden Stämme im Affenmagen etablieren konnte und der zweite Stamm verdrängt worden war. In einem zweiten Versuchsansatz wurden die persistent infizierten Affen mit vier weiteren H. pylori-Stämmen infiziert, um eine transiente Koinfektion zu simulieren. Diese Stämme verdrängten jedoch den bereits etablierten Stamm, und es konnte keine in vivo-Rekombination festgestellt werden. Dennoch ist dieses Modell das Erste, in dem eine persistierende experimentelle H. pylori-Infektion in Rhesusaffen über einen Zeitraum von mehr als vier Jahren nachgewiesen werden konnte. Die Ergebnisse liefern wichtige Hinweise auf den beim Menschen meist unentdeckten Anfang der H. pylori-Infektion. Die Untersuchungen an weiteren Spezies des Genus Helicobacter zeigten, dass die beschriebene Spezies Heelicobacter nemestrinae keine eigene Spezies darstellt, sondern der Spezies H. pylori zugeordnet werden konnte. Den damit nächsten 'Verwandten' stellt die Spezies H. acinonychis dar, deren Stämme sich untereinander wesentlich weniger stark unterscheiden als H. pylori-Stämme. Die Ergebnisse dieser Arbeit liefern wichtige Daten zum Verständnis der Evolution und Mikroevolution innerhalb eines Wirtes von H. pylori, die zu besseren Strategien in der Bekämpfung dieses pathogenen Bakteriums führen können.
Bekanntermaßen führt die H.pylori Infektion des Magens über eine komplexe Modulation des Chemokinsystems zur Ausbildung der H.pylori Gastritis. Die Chemokinrezeptorexpression in der H.pylori Gastritis ist jedoch bisher noch fast nicht untersucht. Das Ziel der Arbeit war die Charakterisierung der Chemokinrezeptorexpression im Magen und die Testung eines Einfluss von H.pylori auf die Expression von Chemokinrezeptoren. In vitro führt die Inkubation von neutrophilen Granulozyten mit H. pylori zu einer schnellen Herunterregulation von CXCR1 und CXCR2 auf Proteinebene durch Rezeptorinternalisation und intrazellulären Abbau. Der Effekt ist unabhängig vom cag Status von H. pylori, sowie von TNF-α- oder IL-8. Als möglicher Signaltransduktionsmechanismus für diesen Effekt wäre die direkte Interaktion von H. pylori mit „toll-like receptors“ (TLRs) denkbar. Auf mRNA Ebene kommt es in vitro bei der Inkubation von neutrophilen Granulozyten mit H. pylori zu einer Herunterregulation von CXCR1 und CXCR2 mRNA nach 3 Stunden. Dieser Effekt tritt bei Inkubation mit einem cag positiven H. pylori Stamm verstärkt auf und könnte bedingt sein durch autokrine Herunterregulation der Expression von CXCR1 und CXCR2 durch IL-8. In vivo exprimieren neutrophile Granulozyten in der H. pylori Gastritis in den Krypten ebenfalls vermindert CXCR1 und CXCR2. Sowohl die Expression der Chemokine als auch der korrespondierenden Chemokinrezeptoren wird somit durch H.pylori beeinflusst. Es lässt sich somit der folgende Pathomechanismus postulieren: Nach dem Eintritt der neutrophilen Granulozyten in die Schleimhaut, kommt es über den direkten Kontakt mit H.pylori zum Verlust der Chemokinrezeptoren. Die neutrophilen Granulozyten können somit nicht mehr auf Chemokinsignale reagieren und werden in der Magenschleimhaut immobilisiert. Dort setzen sie reaktive Sauerstoffradikale, proinflammatorische Zytokine und Chemokine frei, die zur Schleimhautschädigung führen. Magenkarzinome exprimieren die Chemokinrezeptoren CXCR4 und CCR7. Die Expression wird mit der Neigung zur Metastasierung und einer schlechten klinischen Prognose assoziiert. In unseren Untersuchungen wird CXCR4 in vivo während des Prozess der Karzinogenese im Magen ab dem Stadium der intestinalen Metaplasie exprimiert. Bei Inkubation der Zelllinien mit cagA positiven und cagA negativen H. pylori – Stämmen, kommt es zu keiner Änderung der Expression von CXCR4. Die Infektion mit H. pylori ist zwar die Voraussetzung für die Genese der intestinalen Metaplasie, scheint jedoch nicht ursächlich an der Expression von CXCR4 beteiligt zu sein. CCR7 tritt in vivo auf den Magenepithelien der H. pylori Gastritis, der intestinalen Metaplasie, Dysplasie und Magenkarzinomen auf. In vitro führt die Koinkubation von CCR7 tragenden Magenzelllinien mit H. pylori zur Hochregulation von CCR7 kommt. Die Expression von CCR7 auf Karzinomzellen wird ebenfalls möglicherweise durch eine begleitende Infektion mit H. pylori begünstigt. Der Effekt der CCR7 Induktion durch H. pylori in vitro ist unabhängig vom cag Status des für die Infektion verwendeten H. pylori Stammes. Die Hochregulation von CCR7 ist möglicherweise bedingt durch die intrazelluläre Aktivierung von NFκB infolge der H. pylori Infektion. Denkbar wäre auch eine Induktion der Expression von CCR7 in den Magenepithelzellen in TLR abhängiger Weise, äquivalent zu Mechanismen, die in dendritischen Zellen beschrieben wurden. Es lässt sich abschließend feststellen, dass die H.pylori Infektion nicht nur die Freisetzung von Chemokinen, sondern auch die Expression von Chemokinrezeptoren wesentlich beeinflusst. Neutrophile Granulozyten verlieren in direktem Kontakt zu H.pylori die Chemokinrezeptoren CXCR1 und CXCR2. Auf Epithelzellen führt der direkte Kontakt zu H.pylori zur vermehrten Expression von CCR7. Die direkte Regulation von Chemokinrezeptoren durch H.pylori scheint also sowohl bei der H.pylori Gastritis, als auch bei der Entstehung und Progression von Magenkarzinomen eine Rolle zu spielen.
Low pH is the main environmental stress encountered by Helicobacter pylori in the human stomach. To ensure its survival under acidic conditions, this bacterium utilizes urease (encoded by the ureAB operon), a nickel-activated metalloenzyme, which cleaves urea into ammonia to buffer the periplasmic space. Expression of the ureAB operon is tightly regulated at the transcriptional level. Moreover, the urease activity is modulated post translationally via the activity of nickel-binding proteins such as HP1432 that act as nickel sponges to either sequester or release nickel depending on the pH. However, little is known how the levels of these nickel-binding proteins are regulated at the post-transcriptional level. Interestingly, more than 60 candidate small regulatory RNAs (sRNAs) have been identified in a differential RNA-seq approach in H. pylori strain 26695, suggesting an uncharacterized layer of post-transcriptional riboregulation in this pathogen. sRNAs control their trans- or cis- encoded targets by direct binding. Many of the characterized sRNAs are expressed in response to specific environmental cues and are ideal candidates to confer post-transcriptional regulation under different growth conditions.
This study demonstrates that a small RNA termed ArsZ (Acid Responsive sRNA Z) and its target HP1432 constitute yet another level of urease regulation. In-vitro and in-vivo experiments show that ArsZ interacts with the ribosome binding site (RBS) of HP1432 mRNA, effectively repressing translation of HP1432. During acid adaptation, the acid-responsive ArsRS two-component system represses expression of ArsZ. ArsRS and ArsZ work in tandem to regulate expression of HP1432 via a coherent feedforward loop (FFL). ArsZ acts as a delay mechanism in this feedforward loop to ensure that HP1432 protein levels do not abruptly change upon transient pH drops encountered by the bacteria. ArsZ “fine-tunes” the dynamics of urease activity after pH shift presumably by altering nickel availability through post transcriptional control of HP1432 expression. Interestingly, after adaptation to acid stress, ArsZ indirectly activates the transcription of HP1432 and forms an incoherent FFL with ArsRS to regulate HP1432. This study identified a non-standard FFL in which ArsZ can participate directly or indirectly in two different network configurations depending on the state of acid stress adaptation. The importance of ArsZ in the acid response of H. pylori is further supported by bioinformatics analysis showing that the evolution of ArsZ is closely related to the emergence of modern H. pylori strains that globally infect humans. No homologs of arsZ were found in the non-pylori species of Helicobacter. Moreover, this study also demonstrates that the physiological role of a sRNA can be elucidated without the artificial overexpression of the respective sRNA, a method commonly used to characterize sRNAs. Coupled with time-course experiments, this approach allows the kinetics of ArsZ regulation to be studied under more native conditions. ArsZ is the first example of a trans-acting sRNA that regulates a nickel storage protein to modulate apo-urease maturation. These findings may have important implications in understanding the details of urease activation and hence the colonization capability of H. pylori, the only bacterial class I carcinogen to date (WHO, 1994).
Bacterial small non-coding RNAs (sRNAs) play fundamental roles in controlling and finetuning gene expression in a wide variety of cellular processes, including stress responses, environmental signaling and virulence in pathogens. Despite the identification of hundreds of sRNA candidates in diverse bacteria by genomics approaches, the mechanisms and regulatory capabilities of these posttranscriptional regulators have most intensively been studied in Gram-negative Gammaproteobacteria such as Escherichia coli and Salmonella. So far, almost nothing is known about sRNA-mediated regulation (riboregulation) in Epsilonproteobacteria, including the major human pathogen Helicobacter pylori. H. pylori was even thought to be deficient for riboregulation as none of the sRNAs known from enterobacteria are conserved in Helicobacter and since it lacks the major RNA chaperone Hfq, which is crucial for sRNA function as well as stability in many bacteria. Nonetheless, more than 60 cis- and trans-acting sRNA candidates were recently identified in H. pylori by a global RNA sequencing approach, indicating that this pathogen, in principle, has the capability to use riboregulation for its gene expression control. However, the functions and underlying mechanisms of H. pylori sRNAs remained unclear.
This thesis focused on the first functional characterization and target gene identification of a trans-acting sRNA, RepG (Regulator of polymeric G-repeats), in H. pylori. Using in-vitro and in-vivo approaches, RepG was shown to directly base-pair with its C/Urich terminator loop to a variable homopolymeric G-repeat in the 5’ untranslated region (UTR) of the tlpB mRNA, thereby regulating expression of the chemotaxis receptor TlpB. While the RepG sRNA is highly conserved, the length of the G-repeat in the tlpB mRNA leader varies among different H. pylori isolates, resulting in a strain-specific tlpB regulation. The modification of the number of guanines within the G-stretch in H. pylori strain 26695 demonstrated that the length of the homopolymeric G-repeat determines the outcome of posttranscriptional control (repression or activation) of tlpB by RepG. This lengthdependent targeting of a simple sequence repeat by a trans-acting sRNA represents a new twist in sRNA-mediated regulation and a novel mechanism of gene expression control, since it uniquely links phase variation by simple sequence repeats to posttranscriptional regulation.
In almost all sequenced H. pylori strains, tlpB is encoded in a two gene operon upstream of HP0102, a gene of previously unknown function. This study provided evidence that HP0102 encodes a glycosyltransferase involved in LPS O-chain and Lewis x antigen production. Accordingly, this glycosyltransferase was shown to be essential for mice colonization by H. pylori. The coordinated posttranscriptional regulation of the tlpB-HP0102 operon by antisense base-pairing of RepG to the phase-variable G-repeat in the 5’ UTR of the tlpB mRNA allows for a gradual, rather than ON/OFF, control of HP0102 expression, thereby affecting LPS biosynthesis in H. pylori. This fine-tuning of O-chain and Lewis x antigen expression modulates H. pylori antibiotics sensitivity and thus, might be advantageous for Helicobacter colonization and persistence.
Whole transcriptome analysis based on microarray and RNA sequencing was used to identify additional RepG target mRNAs and uncover the physiological role of this riboregulator in H. pylori. Altogether, repG deletion affected expression of more than 40 target gene candidates involved various cellular processes, including membrane transport and adhesion, LPS modification, amino acid metabolism, oxidative and nitrosative stress, and nucleic acid modification. The presence of homopolymeric G-repeats/G-rich sequences in almost all target mRNA candidates indicated that RepG hijacks a conserved motif to
recognize and regulate multiple target mRNAs in H. pylori.
Overall, this study demonstrates that H. pylori employs riboregulation in stress response and virulence control. In addition, this thesis has successfully established Helicobacter as a new model organism for investigating general concepts of gene expression control by Hfq-independent sRNAs and sRNAs in bacterial pathogens.
Bakterien sind in der Lage, sich schnell an wechselnde Umweltbedingungen anzupassen. Eine wichtige Rolle bei der Wahrnehmung von verschiedensten Umweltreizen und der zellulären Antwort spielt die Genregulation durch Zweikomponenten-Systeme. Gut charakterisiert ist das ArsRS Zweikomomponenten-System in H. pylori, welches an der Ausbildung der Säureresistenz beteiligt ist und dem Bakterium so die Kolonisierung der Magenschleimhaut ermöglicht. Die Histidin-Kinase ArsS wird in Gegenwart von Säure aktiviert und phosphoryliert den Response-Regulator ArsR, der die Transkription von Target-Genen reguliert. In der periplasmatischen Sensordomäne der Histidin-Kinase ArsS sind sieben Histidinreste vorhanden, die aufgrund ihres pKa-Wertes von 6,0 bei Absenken des pH Wertes von pH 7 auf pH 5, was eine Aktivierung der Histidin-Kinase zur Folge hat, protoniert werden könnten. Es konnte gezeigt werden, dass der Histidinrest H94 der periplasmatischen Sensordomäne einen wesentliche Rolle bei der Säurewahrnehmung durch die Histidin-Kinase ArsS spielt. Die Einführung einer positiv geladenen AS an dieser Position allein reicht jedoch nicht aus, um die Kinase zu aktivieren, weshalb unklar bleibt, ob eine Protonierung des Histidinrestes H94 in vivo die Säurewahrnehmung vermittelt. Weiterhin konnten Indizien darauf erhalten werden, dass neben dem Histidinrest H94 noch weitere Aminosäuren an der Säurewahrnehmung durch die Histidin-Kinase beteiligt sind. Der Aspartatrest D124 leistet unter den negativ geladenen AS vermutlich den größten Beitrag zur Säurewahrnehmung. In den mit H. pylori nahe verwandten Arten Helicobacter hepaticus, Wolinella succinogenes und Campylobacter jejuni sind Orthologe zu dem ArsRS Zweikomponenten-System vorhanden. Um zu untersuchen, ob es sich bei der Säurewahrnehmung durch die Histidin-Kinase ArsS um eine spezifische Anpassung von H. pylori an sein Habitat handelt oder ob Säure einen allgemeinen Stimulus der ArsS-orthologen Kinasen darstellt, wurden Mutanten im genetischen Hintergrund von H. pylori G27 konstruiert, in welchen die Histidin-Kinase ArsS durch die orthologen Kinasen HH1608, CJ1262 und WS1818 substituiert wurde. Durch Transkriptionsstudien konnte gezeigt werden, dass die Kinase WS1818 eine gesteigerte Aktivität bei saurem pH-Wert aufweist. Auch die Kinase HH1607 kann Säure als einen Umweltreiz wahrnehmen, jedoch deutlich weniger effektiv als die Kinasen ArsS und WS1818. Ob die Zweikomponenten-Systeme HH1608/HH1607 und WS1817/WS1818 in vivo in H. hepaticus und W. succinogenes an der Wahrnehmung von Säure und evtl. an der Ausbildung einer Säureresistenz beteiligt sind, ist unklar, da über die Funktion dieser Zweikomponenten-Systeme bisher nichts bekannt ist. Die Kinase CJ1262 ist nicht in der Lage, Säure als einen Umweltreiz wahrzunehmen. Die beiden Response-Regulatoren HP1043 und HP1021 spielen vermutlich eine Rolle bei der Regulation von Genen, deren Produkte eine wichtige Funktion für das vegetative Zellwachstum haben. Die Aktivität der beiden RR wird entgegen dem gängigen Zweikomponenten-System-Paradigma nicht über eine Phosphorylierung moduliert. In der vorliegenden Arbeit wurde analysiert, ob eine strikte Expressionskontrolle für die wachstumsassoziierten Funktion dieser Response-Regulatoren von Bedeutung ist. Zu diesem Zweck wurden verschieden Mutanten konstruiert, in welchen die Transkription der Gene hp1021 und hp1043 unter der Kontrolle von unterschiedlich regulierten Promotoren stattfindet. Es konnte gezeigt werden, dass die Expression des Gens hp1043 sowohl transkriptionell als auch posttranskriptionell und/oder posttranslational strikt reguliert wird. Es kann deshalb postuliert werden, dass die Aktivität des RR HP1043 über die vorhandene Konzentration an Regulator in der Bakterienzelle beeinflusst wird. Die Expression des Gens hp1021 wird nicht strikt reguliert. Auf welche Weise die Aktivität des RR HP1021 moduliert wird, bleibt unklar.
More than 150 different RNA modifications have been detected in all kingdoms of life and 60 are known to decorate bacterial RNA. Among them, pseudouridine is universally conserved and one of the most abundant modifications present in bacterial stable RNAs such as tRNAs and rRNAs. In bacteria, the nucleotide is posttranscriptionally generated by dedicated enzymes called pseudouridine synthases (PUSs). With the advent of sophisticated deep-sequencing technologies, this modification has been identified in different types of RNA classes (tRNAs, rRNAs, mRNAs, snRNAs, and lncRNAs) in diverse eukaryotic organisms. However, these techniques have never been applied to bacteria, generating a knowledge gap about the location of the modified nucleotide in prokaryotic RNAs. Mutations or deletions of specific eukaryotic PUS enzymes are linked to human diseases and therefore their absence is deleterious for the correct function of the cell. However, deletion of tRNA or rRNA PUS enzymes in the bacterial model organism E. coli have not revealed any such drastic phenotypes, suggesting a different role and function of the modification itself and of the enzymes in different kingdoms of life.
Since the roles of tRNA PUS enzymes in bacteria is still poorly understood, a functional characterization of these proteins is pursued in the Epsilonproteobacteria Campylobacter jejuni and Helicobacter pylori. While C. jejuni is the leading cause of bacterial foodborne gastroenteritis in humans, infection with H. pylori is associated with the development of gastric cancer. In particular, phenotypes were explored for the tRNA PUS enzymes TruA, TruB, and TruD in C. jejuni as well as TruA and TruD in H. pylori. Upon deletion of truD, a severe growth defect is observed for C. jejuni but not for H. pylori, highlighting a potential difference in function of the enzyme in the two related bacterial pathogens.
Moreover, a genome-wide approach called Pseudo-seq is established and applied for RNA of these two pathogens, which allows, for the first time, the global identification of pseudouridine modifications at single-nucleotide resolution in the bacterial transcriptome. Applying Pseudo-seq in RNAs of wildtype and diverse PUS enzyme deletion mutants enabled the identification of the distinct RNA substrates of tRNA PUS enyzmes in C. jejuni and H. pylori. Hereby, the tRNA-Glu was determined to be the major tRNA substrate of TruD in C. jejuni. Interestingly, the tRNA-Glu is expressed as a single copy in the C. jejuni genome. To link the growth defect observed for a C. jejuni ∆truD mutant strain to the pseudouridine modification of the tRNA-Glu, a catalytically inactive TruD complementation was generated. This strain is unable to restore the tRNA-Glu modification but surprisingly, was able to complement the growth defect. The same observation was made for a cross-complementation with a copy of H. pylori TruD. This indicates that there is a potential additional function of the TruD PUS enzyme in C. jejuni that is independent of the pseudouridine modification. Using a combination of deep-sequencing technologies (RIP-seq, RNA-seq, Ribo-seq, and CLIP-seq), the dual function of TruD is investigated.
Overall, this study provides the first in-depth investigation into pseudouridylation of bacteria in general and the bacterial pathogens C. jejuni and H. pylori in particular. The work presented in this thesis reveals not only a global map of pseudouridine in tRNAs and rRNAs of the two bacteria but it also explores the function of the responsible tRNA PUS enzymes. In addition, this study provides evidence for a dual function of the C. jejuni PUS enzyme TruD that goes beyond its RNA modifying function. Future research could focus on unravelling the function of TruD and its potential interaction partners and thus reveal new mechanisms of regulation of a protein previously only described as an RNA modification enzyme.
Background
MicroRNAs, post-transcriptional regulators of eukaryotic gene expression, are implicated in host defense against pathogens. Viruses and bacteria have evolved strategies that suppress microRNA functions, resulting in a sustainable infection. In this work we report that Helicobacter pylori, a human stomach-colonizing bacterium responsible for severe gastric inflammatory diseases and gastric cancers, downregulates an embryonic stem cell microRNA cluster in proliferating gastric epithelial cells to achieve cell cycle arrest.
Results
Using a deep sequencing approach in the AGS cell line, a widely used cell culture model to recapitulate early events of H. pylori infection of gastric mucosa, we reveal that hsa-miR-372 is the most abundant microRNA expressed in this cell line, where, together with hsa-miR-373, it promotes cell proliferation by silencing large tumor suppressor homolog 2 (LATS2) gene expression. Shortly after H. pylori infection, miR-372 and miR-373 synthesis is highly inhibited, leading to the post-transcriptional release of LATS2 expression and thus, to a cell cycle arrest at the G1/S transition. This downregulation of a specific cell-cycle-regulating microRNA is dependent on the translocation of the bacterial effector CagA into the host cells, a mechanism highly associated with the development of severe atrophic gastritis and intestinal-type gastric carcinoma.
Conclusions
These data constitute a novel example of host-pathogen interplay involving microRNAs, and unveil the couple LATS2/miR-372 and miR-373 as an unexpected mechanism in infection-induced cell cycle arrest in proliferating gastric cells, which may be relevant in inhibition of gastric epithelium renewal, a major host defense mechanism against bacterial infections.
Helicobacter pylori (H. pylori) is a gram-negative, microaerophilic, spiral-shaped bacterium. It resides in the gastric mucous layer and epithelial lining of the stomach, often clustering at the junction of epithelial cells. H. pylori colonization usually occurs during childhood, and, when left untreated, generally persists for the host’s lifetime. Persistent H. pylori infection can cause chronic superficial gastritis and gastric duodenal ulcers, which is possibly linked to the development of gastric carcinoma and primary gastric lymphoma, especially of the mucosa-associated lymphoid tissue (MALT) type. It was recently defined as a class 1 carcinogen. The gastric inflammatory response to H. pylori infection is characterized by infiltration of the mucosa by neutrophils, T and B cells, plasma cells and macrophages. This reaction is initially induced by H. pylori attachment, followed by cytokine release by gastric epithelial cells. Epidemiological studies revealed that more than 50% of adults are infected with H. pylori all over the world. However, interestingly, only a subset of individuals develops serious H. pylori-related disease, while most infected individuals show no clinical symptoms. Gastric epithelial cells, like intestinal epithelial cells, express a subset of Toll-like receptors (TLRs) and similar pattern recognition receptors, which are important for the activation of the innate immune system. Bacterial components such as lipopeptides, peptidoglycan, LPS, flagellin, and CpG DNA are the ligands of TLRs. Thus, TLRs in gastric epithelial cells might be able to contribute to innate immune responses to H. pylori infection. However, there is scant knowledge about the mechanisms of innate immune response to acute and chronic H. pylori infection. This study is focused on host cell interaction with H. pylori flagellins, which are major components of the flagellar apparatus, and innate immune responses against them. The flagellins, which are essential for bacterial motility, are important for H. pylori to survive in the stomach mucus during the whole infectious cycle. Flagellins are known to act as the main determinant of many mucosal pathogenic bacteria that mediates proinflammatory signaling, including transcriptional factor NF-B activation via TLR5. In the first part of the study, we investigated the effects of H. pylori flagellins on TLR5 expression, NF-B activation and IL-8 production in various human intestinal and gastric epithelial cell lines by using Western blotting, semi-quantitative RT-PCR and ELISA. IL-8 is a potent neutrophil-activating chemokine expressed by gastric epithelial cells. When we stimulated the cells with the native form of or E. coli-expressed recombinant H. pylori flagellins, FlaA and FlaB, IL-8 was not induced in any case, while S. typhimurium flagellin (FliC) induced it significantly. H. pylori was able to modulate TLR5 protein expression and NF-B activation in epithelial cells regardless of the presence of flagellins. Having established the finding that H. pylori flagellins have unusually low immune-stimulatory properties, we further investigated to find out possible reasons why H. pylori flagellins are distinct from other flagellins of pathogenic bacteria in terms of immune-stimulatory activity. From amino acid sequence comparisons, we found that some regions in the terminal D0D1 protein domains of H. pylori flagellins are different from flagellins of other pathogenic bacteria. D0D1 is the domain which is known to interact with TLR5 in Salmonella FliC. To examine whether the differences endow H. pylori flagellins with low immune-stimulatory properties, we created several mutated H. pylori flagellins (FlaA and FlaB) by site-directed mutagenesis that contain one to four epitopes of Salmonella flagellin D0D1 domain amino acid sequences. The mutant flagellins expressed both in H. pylori and E. coli were used to determine their influence on TLR5-signaling mediators and cytokines, such as MAPkinases, (ERK, p38), NF-B, IL-8, and MIP-3. Salmonella FliC expressed in E. coli induced activation of p38, IB and NF-B leading to IL-8 and MIP-3 production in gastric epithelial cells. However, none of the H. pylori flagellin mutants activated MAP kinases or induced those cytokines. In a co-immunoprecipitation assay none of the recombinant wild type or mutated H. pylori flagellins showed any direct physical interaction with TLR5, while Salmonella FliC significantly co-precipitated with TLR5. Interestingly, we found H. pylori flagellins bind to the surface of gastric epithelial cells like FliC, although they do not bind to or stimulate TLR5. Based on the physical interaction of H. pylori flagellins and FliC with human gastric epithelial cells, we further analyzed transcriptional regulation by H. pylori flagellin in these host cells using microarray analysis. The result showed that H. pylori flagellins modulate host cell gene expression, and many of the identified regulation events overlap with the genes regulated by FliC. These findings imply that H. pylori flagellins do play a role in gene regulation of host cells probably through still unknown factors or receptors, although they do not trigger TLR5-related signaling pathways. The results of our study suggest that, in addition to the low immune-stimulatory activity of H. pylori LPS, the evolutionary reduction in stimulating activity of H. pylori flagellins on the local innate immune responses in the stomach in vivo might be a further strategy of this chronic mucosal pathogen to evade and minimize deleterious host responses, thereby promoting life-long persistence in the host, and possibly contributing to cancerogenesis.