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RNA hat neben der Rolle als Informationsüberträger wichtige Aufgaben in regulatorischen Prozessen. Sie kann komplexe Strukturen ausbilden und ähnlich wie Proteine Liganden binden oder enzymatische Reaktionen katalysieren. Im Rahmen dieser Arbeit sollten zwei Beispiele von RNA-Liganden-Interaktionen untersucht werden. Im ersten Abschnitt wurde die Interaktion des TetR-bindenden Aptamers 12-1 mit dem Tetracyclin-Repressorprotein (TetR) biochemisch charakterisiert. Über Gelverzögerungs- experimente wurde gezeigt, dass das Aptamer 12-1K delta A TetR mit hoher Affinität und Spezifität bindet. Es wurde ein KD von 22 nM bestimmt. Die Bindung ist dabei ebenso stark wie die Bindung von TetR an die Operatorsequenz tetO. In Anwesenheit von Tetracyclin (Tc) nimmt die Affinität des TetR/Aptamer-Komplexes um das sechsfache ab. Des Weiteren konnten die Bindeepitope des Aptamers durch eine Analyse von verschiedenen TetR-Mutanten im DNA-Bindebereich bestimmt werden. Die Aminosäuren T27, N47 und K48 sind dabei essentiell für die RNA-Bindung und führen bei einem Austausch zum Verlust der RNA-Bindung. Der Bindebereich des Aptamers überlappt mit Aminosäureresten, die für die tetO-Bindung essentiell sind. Die Stöchiometrie der TetR/Aptamer-Bindung wurde durch LILBID-Messungen auf eine molare Verteilung von 2:1 festgelegt. Ein TetR-Dimer bindet dabei ein Aptamermolekül. Durch die umfassende biochemische Analyse der TetR/Aptamer-Bindung kann das Aptamer 12-1 nun als Expressionssonde für RNAs in bakteriellen Zellen genutzt werden. Des Weiteren kann das Aptamer als alternativer, artifizieller Transkriptionsregulator im tet on / tet off-System verwendet werden. Im zweiten Teil der Arbeit sollten miRNAs identifiziert werden, die an der posttrans- kriptionellen Regulation der 5-Lipoxygenase (5-LO) und der Cyclooxygenase-2 (COX-2) beteiligt sind. Mit bioinformatischen Vorhersageprogrammen wurden die 3’-UTR- Bereiche von 5-LO und COX-2 nach putativen Bindestellen abgesucht. Im Fall der 5-LO wurden durch eine zusätzliche Microarray-Expressionsanalyse miRNAs ausgewählt, welche in 5-LO positiven Zellen hoch exprimiert sind und Bindestellen im 3’-UTR aufweisen. Es konnten verschiedene miRNAs detektiert werden, jedoch keine Regulation der 5-LO Aktivität beobachtet werden. Für COX-2 wurde neben der Suche nach putativen miRNA-Bindestellen zudem die Stabilität des 3’-UTR untersucht. Mit Hilfe des auf Perl basierenden Programms SignificanceScoreAssignment (Florian Groher, Diplomarbeit 2011) konnte der 3’-UTR von COX-2 als generell destabilisierend analysiert werden. In Colonkarzinom- spezifischen HT-29-Zellen wurden miRNAs untersucht, welche Bindestellen im 3’-UTR von COX-2 aufweisen. In diesem Kontext sollte der Einfluss einer Interaktion von HT- 29-Zellen mit aktivierten Thrombozyten sowie daraus isolierten Bestandteilen wie Mikropartikeln und PDGF analysiert werden. MiR-16, miR-26b, miR-199a und miR- 199a* konnten in HT-29-Zellen nachgewiesen werden. Bei einer Stimulation von HT-29- Zellen mit PDGF-BB werden miR-16 und miR-26b konzentrationsabhängig stärker exprimiert, während die Expression von miR-199a und miR-199a* signifikant abnimmt. Eine direkte Regulation von COX-2 durch die untersuchten miRNAs konnte durch Überexpressions- und Reportergenanalysen jedoch nicht festgestellt werden. Die Analysen der 5-LO- und COX-2-Regulation durch miRNAs stellen Vorarbeiten dar. Die etablierten Methoden können nun für eine detaillierte Betrachtung weiterer miRNAs verwendet werden.
The balance between peripheral T-cell reactivity and self-tolerance is achieved during T-cell development in the thymus. During thymic development T-cell sensitivity to self-antigens drives their selection and is dynamically regulated via multiple mechanisms. The microRNA miR-181 has been implicated as a post-transcriptional modulator of T-cell sensitivity due to its suppression of several negative regulators of T-cell receptor (TCR) signalling. By tuning developing thymocytes to be exquisitely sensitive to signals transduced through their TCR, miR-181 has previously been shown to be essential for the agonist selection of invariant natural killer T (iNKT) cells. In this thesis, we extend the knowledge on the developmental control elicited by miR-181 in the thymus to cover mucosal-associated invariant T (MAIT), regulatory T (Treg) and conventional T cells. Using a germline knock-out of mature miR-181a/b-1, we could show that all agonist-selected T cell populations are critically dependant on miR-181a/b-1, noting an absence of MAIT and a reduction of thymic-derived Tregs in miR-181a/b-1-deficient mice. Furthermore, we provided evidence that miR-181 is also required for the negative selection of conventional T cells, with miR-181a/b-1-deficient mice presenting with a near absence of apoptotic markers. Therefore, by heightening the TCR sensitivity to self-antigens, miR-181a/b-1 aids in the detection and subsequent elimination of autoreactive thymocytes. In addition, we characterised the murine primary miR-181a/b-1 transcript, which surprisingly has a transcription start site (TSS) more than 70kB upstream of the mature miRNA sequences. This shall hopefully lead to future research aimed at deciphering the upstream regulatory networks that promote dynamic miR-181a/b-1 expression in developing thymocytes. In summary, we present here a single miRNA subset with broad implications in T-cell development. In disagreement with central dogma that individual miRNAs generally provide weak to moderate modulation over cellular pathways, we showcase the miR-181 family subset, miR-181a/b-1, as an efficient regulator of TCR signalling pathways. Due to the sensitive nature of TCR signalling during thymocyte selection, miR-181a/b-1 elicits gross effects, which are essential for agonist selection, central tolerance and generating a functional self-tolerant peripheral T cell repertoire. We therefore conclude that miR-181a/b-1 is fundamental in T-cell development as a whole.
MicroRNAs (miRNAs) have emerged as critical posttranscriptional regulators of the immune system, including function and development of regulatory T (Treg) cells. Although this critical role has been firmly demonstrated through genetic models, key mechanisms of miRNA function in vivo remain elusive. Here, we review the role of miRNAs in Treg cell development and function. In particular, we focus on the question what the study of miRNAs in this context reveals about miRNA biology in general, including context-dependent function and the role of individual targets vs. complex co-targeting networks. In addition, we highlight potential technical pitfalls and state-of-the-art approaches to improve the mechanistic understanding of miRNA biology in a physiological context.
A high incidence of thromboembolic events associated with high mortality has been reported in severe acute respiratory syndrome coronavirus type 2 (SARS-CoV-2) infections with respiratory failure. The present study characterized post-transcriptional gene regulation by global microRNA (miRNA) expression in relation to activated coagulation and inflammation in 21 critically ill SARS-CoV-2 patients. The cohort consisted of patients with moderate respiratory failure (n = 11) and severe respiratory failure (n = 10) at an acute stage (day 0–3) and in the later course of the disease (>7 days). All patients needed supplemental oxygen and severe patients were defined by the requirement of positive pressure ventilation (intubation). Levels of D-dimers, activated partial thromboplastin time (aPTT), C-reactive protein (CRP), and interleukin (IL)-6 were significantly higher in patients with severe compared with moderate respiratory failure. Concurrently, next generation sequencing (NGS) analysis demonstrated increased dysregulation of miRNA expression with progression of disease severity connected to extreme downregulation of miR-320a, miR-320b and miR-320c. Kyoto encyclopedia of genes and genomes (KEGG) pathway analysis revealed involvement in the Hippo signaling pathway, the transforming growth factor (TGF)-β signaling pathway and in the regulation of adherens junctions. The expression of all miR-320 family members was significantly correlated with CRP, IL-6, and D-dimer levels. In conclusion, our analysis underlines the importance of thromboembolic processes in patients with respiratory failure and emphasizes miRNA-320s as potential biomarkers for severe progressive SARS-CoV-2 infection.
Einleitung: Die Bronchiolitis obliterans ist eine seltene Lungenerkrankung unterschiedlicher Ätiologie, die mit einer chronischen Entzündung der kleinen Atemwege einhergeht. Mit der Identifizierung von Kandidaten-miRNA sollen Biomarker evaluiert werden, die in der Diagnostik der postinfektiösen Bronchiolitis obliterans (PIBO) herangezogen werden sowie in Zukunft eine mögliche Therapieoption darstellen können.
Material und Methoden: 19 Patientinnen und Patienten mit PIBO sowie 18 gesunde Kontrollen wurden in die Studie eingeschlossen. Nach Komplettsequenzierung wurden die miRNA-Profile der Patienten mit den Profilen der alters- und geschlechtsadaptierten gesunden Kontrollgruppe verglichen. Als Nebenzielgrößen wurden die Lungenfunktion und Sputum-Biomarker erfasst.
Ergebnisse: Die Patientenkohorte wies signifikant niedrigere Werte in der Lungenfunktionsdiagnostik (Patienten, Median: FVC (%) 76,3***, FEV1 (%) 59,8***, FEV1/FVC 0,68***, FEF75 (%) 25,1***, *p<0,05, **p<0,01, ***p<0,001) sowie eine signifikante Erhöhung der neutrophilen Granulozyten und der proinflammatorischen Zytokine IL-1β, IL-6 und IL-8 in der Sputumanalyse auf (Patienten, Median: Neutrophile (%) 82,5***, IL-1β (pg/ml) 1453,0**, IL-6 (pg/ml) 825,6**, IL-8 (pg/ml) 35368,0***). Die Analyse der miRNA-Expression ergab insgesamt 40 unterschiedlich regulierte miRNAs (padj ≤ 0,05). 22 miRNAs waren in der Patientenkohorte vermehrt exprimiert, 18 miRNAs waren vermindert exprimiert. Die vier miRNAs mit pbonf < 0,05 wurden in der weiteren Analyse berücksichtigt. Die miRNAs hsa-let-7b-3p und hsa-miR-146a-3p waren signifikant vermehrt exprimiert, wohingegen die miRNAs hsa-miR-1287-5p und hsa-miR-27b-3p signifikant vermindert exprimiert waren. Die identifizierten miRNAs spielen unter anderem eine Rolle im TGF-β- und Hippo-Signalweg.
Schlussfolgerung: Die Ergebnisse zeigen, dass das miRNA-Expressionsmuster bei Patienten, die an postinfektiöser Bronchiolitis obliterans erkrankt sind, alteriert ist. Die identifizierten miRNAs sind relevante Biomarker und können als potentielle Ziele von miRNA-Therapeutika in Betracht gezogen werden.
The adult heart has a limited capacity to replace or regenerate damaged cardiac tissue following severe myocardial injury. Thus, therapies facilitating the induction of cardiac regeneration holds great promise for the treatment of end-stage heart failure, and for pathologies invoking severe cardiac dysfunction as a result of cardiomyocyte death. Recently, a number of studies have demonstrated that cardiac regeneration can be achieved through modulation and/or reprogramming of cardiomyocyte proliferation, differentiation, and survival signaling. Non-coding RNAs (ncRNAs), including microRNAs (miRNAs), long non-coding RNAs (lncRNAs) and circular RNAs (circRNAs), are reported to play critical roles in regulating key aspects of cardiomyocyte physiologic and pathologic signaling, including the regulation of cardiac regeneration both in vitro and in vivo. In this review, we will explore and detail the current understanding of ncRNA function in cardiac regeneration, and highlight established and novel strategies for the treatment of heart failure through modulation of ncRNAs-driven cardiac regeneration.
The miRNA biogenesis is tightly regulated to avoid dysfunction and consequent disease development. Here, we describe modulation of miRNA processing as a novel noncanonical function of the 5-lipoxygenase (5-LO) enzyme in monocytic cells. In differentiated Mono Mac 6 (MM6) cells, we found an in situ interaction of 5-LO with Dicer, a key enzyme in miRNA biogenesis. RNA sequencing of small noncoding RNAs revealed a functional impact, knockout of 5-LO altered the expression profile of several miRNAs. Effects of 5-LO could be observed at two levels. qPCR analyses thus indicated that (a) 5-LO promotes the transcription of the evolutionarily conserved miR-99b/let-7e/miR-125a cluster and (b) the 5-LO-Dicer interaction downregulates the processing of pre-let-7e, resulting in an increase in miR-125a and miR-99b levels by 5-LO without concomitant changes in let-7e levels in differentiated MM6 cells. Our observations suggest that 5-LO regulates the miRNA profile by modulating the Dicer-mediated processing of distinct pre-miRNAs. 5-LO inhibits the formation of let-7e which is a well-known inducer of cell differentiation, but promotes the generation of miR-99b and miR-125a known to induce cell proliferation and the maintenance of leukemic stem cell functions.
Development of T cells in the thymus is tightly controlled to continually produce functional, but not autoreactive, T cells. miRNAs provide a layer of post-transcriptional gene regulation to this process, but the role of many individual miRNAs in T-cell development remains unclear. miR-21 is prominently expressed in immature thymocytes followed by a steep decline in more mature cells. We hypothesized that such a dynamic expression was indicative of a regulatory function in intrathymic T-cell development. To test this hypothesis, we analyzed T-cell development in miR-21-deficient mice at steady state and under competitive conditions in mixed bone-marrow chimeras. We complemented analysis of knock-out animals by employing over-expression in vivo. Finally, we assessed miR-21 function in negative selection in vivo as well as differentiation in co-cultures. Together, these experiments revealed that miR-21 is largely dispensable for physiologic T-cell development. Given that miR-21 has been implicated in regulation of cellular stress responses, we assessed a potential role of miR-21 in endogenous regeneration of the thymus after sublethal irradiation. Again, miR-21 was completely dispensable in this process. We concluded that, despite prominent and highly dynamic expression in thymocytes, miR-21 expression was not required for physiologic T-cell development or endogenous regeneration.
miR-142-3p expression is predictive for severe traumatic brain injury (TBI) in trauma patients
(2020)
Background: Predictive biomarkers in biofluids are the most commonly used diagnostic method, but established markers in trauma diagnostics lack accuracy. This study investigates promisingmicroRNAs(miRNA)releasedfromaffectedtissueafterseveretraumathathavepredictive values for the effects of the injury.
Methods: A retrospective analysis of prospectively collected data and blood samples of n = 33 trauma patients (ISS≥16) is provided. Levels of miR-9-5p, -124-3p, -142-3p, -219a-5p, -338-3pand-423-3p inseverelyinjuredpatients (PT)withouttraumatic braininjury (TBI) or with severe TBI (PT + TBI) and patients with isolated TBI (isTBI) were measured within 6 h after trauma.
Results: The highest miR-423-3p expression was detected in patients with severe isTBI, followed by patients with PT + TBI, and lowest levels were found in PT patients without TBI (2−∆∆Ct,p = 0.009). ApositivecorrelationbetweenmiR-423-3plevelandincreasingAIShead (p = 0.001) and risk of mortality (RISC II, p = 0.062) in trauma patients (n = 33) was found. ROC analysis of miR-423-3p levels revealed them as statistically significant to predict the severity of brain injury in trauma patients (p = 0.006). miR-124-3p was only found in patients with severe TBI, miR-338-3p was shown in all trauma groups. miR-9-5p, miR-142-3p and miR-219a-5p could not be detected in any of the four groups. Conclusion: miR-423-3p expression is significantly elevated after isolated traumatic braininjuryandpredictableforsevereTBIinthefirsthoursaftertrauma. miR-423-3pcouldrepresent a promising new biomarker to identify severe isolated TBI.
Malignant gliomas are intrinsic brain tumors with a dismal prognosis. They are well-adapted to hypoxic conditions and poorly immunogenic. NKG2D is one of the major activating receptors of natural killer (NK) cells and binds to several ligands (NKG2DL).
Here we evaluated the impact of miRNA on the expression of NKG2DL in glioma cells including stem-like glioma cells. Three of the candidate miRNA predicted to target NKG2DL were expressed in various glioma cell lines as well as in glioblastomas in vivo: miR-20a, miR-93 and miR-106b. LNA inhibitor-mediated miRNA silencing up-regulated cell surface NKG2DL expression, which translated into increased susceptibility to NK cell-mediated lysis. This effect was reversed by neutralizing NKG2D antibodies, confirming that enhanced lysis upon miRNA silencing was mediated through the NKG2D system. Hypoxia, a hallmark of glioblastomas in vivo, down-regulated the expression of NKG2DL on glioma cells, associated with reduced susceptibility to NK cell-mediated lysis. This process, however, was not mediated through any of the examined miRNA. Accordingly, both hypoxia and the expression of miRNA targeting NKG2DL may contribute to the immune evasion of glioma cells at the level of the NKG2D recognition pathway. Targeting miRNA may therefore represent a novel approach to increase the immunogenicity of glioblastoma.