TY - JOUR A1 - Wasmus, Christina A1 - Dudek, Jan T1 - Metabolic Alterations Caused by Defective Cardiolipin Remodeling in Inherited Cardiomyopathies JF - Life N2 - The heart is the most energy-consuming organ in the human body. In heart failure, the homeostasis of energy supply and demand is endangered by an increase in cardiomyocyte workload, or by an insufficiency in energy-providing processes. Energy metabolism is directly associated with mitochondrial redox homeostasis. The production of toxic reactive oxygen species (ROS) may overwhelm mitochondrial and cellular ROS defense mechanisms in case of heart failure. Mitochondria are essential cell organelles and provide 95% of the required energy in the heart. Metabolic remodeling, changes in mitochondrial structure or function, and alterations in mitochondrial calcium signaling diminish mitochondrial energy provision in many forms of cardiomyopathy. The mitochondrial respiratory chain creates a proton gradient across the inner mitochondrial membrane, which couples respiration with oxidative phosphorylation and the preservation of energy in the chemical bonds of ATP. Akin to other mitochondrial enzymes, the respiratory chain is integrated into the inner mitochondrial membrane. The tight association with the mitochondrial phospholipid cardiolipin (CL) ensures its structural integrity and coordinates enzymatic activity. This review focuses on how changes in mitochondrial CL may be associated with heart failure. Dysfunctional CL has been found in diabetic cardiomyopathy, ischemia reperfusion injury and the aging heart. Barth syndrome (BTHS) is caused by an inherited defect in the biosynthesis of cardiolipin. Moreover, a dysfunctional CL pool causes other types of rare inherited cardiomyopathies, such as Sengers syndrome and Dilated Cardiomyopathy with Ataxia (DCMA). Here we review the impact of cardiolipin deficiency on mitochondrial functions in cellular and animal models. We describe the molecular mechanisms concerning mitochondrial dysfunction as an incitement of cardiomyopathy and discuss potential therapeutic strategies. KW - cardiolipin KW - mitochondria KW - Barth syndrome KW - Sengers syndrome KW - respiratory chain KW - Dilated Cardiomyopathy with Ataxia KW - cardiomyopathy Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-219286 SN - 2075-1729 VL - 10 IS - 11 ER - TY - JOUR A1 - Wagner, Michael A1 - Bertero, Edoardo A1 - Nickel, Alexander A1 - Kohlhaas, Michael A1 - Gibson, Gary E. A1 - Heggermont, Ward A1 - Heymans, Stephane A1 - Maack, Christoph T1 - Selective NADH communication from α-ketoglutarate dehydrogenase to mitochondrial transhydrogenase prevents reactive oxygen species formation under reducing conditions in the heart JF - Basic Research in Cardiology N2 - In heart failure, a functional block of complex I of the respiratory chain provokes superoxide generation, which is transformed to H\(_2\)O\(_2\) by dismutation. The Krebs cycle produces NADH, which delivers electrons to complex I, and NADPH for H\(_2\)O\(_2\) elimination via isocitrate dehydrogenase and nicotinamide nucleotide transhydrogenase (NNT). At high NADH levels, α-ketoglutarate dehydrogenase (α-KGDH) is a major source of superoxide in skeletal muscle mitochondria with low NNT activity. Here, we analyzed how α-KGDH and NNT control H\(_2\)O\(_2\) emission in cardiac mitochondria. In cardiac mitochondria from NNT-competent BL/6N mice, H\(_2\)O\(_2\) emission is equally low with pyruvate/malate (P/M) or α-ketoglutarate (α-KG) as substrates. Complex I inhibition with rotenone increases H2O2 emission from P/M, but not α-KG respiring mitochondria, which is potentiated by depleting H\(_2\)O\(_2\)-eliminating capacity. Conversely, in NNT-deficient BL/6J mitochondria, H2O2 emission is higher with α-KG than with P/M as substrate, and further potentiated by complex I blockade. Prior depletion of H\(_2\)O\(_2\)-eliminating capacity increases H\(_2\)O\(_2\) emission from P/M, but not α-KG respiring mitochondria. In cardiac myocytes, downregulation of α-KGDH activity impaired dynamic mitochondrial redox adaptation during workload transitions, without increasing H\(_2\)O\(_2\) emission. In conclusion, NADH from α-KGDH selectively shuttles to NNT for NADPH formation rather than to complex I of the respiratory chain for ATP production. Therefore, α-KGDH plays a key role for H\(_2\)O\(_2\) elimination, but is not a relevant source of superoxide in heart. In heart failure, α-KGDH/NNT-dependent NADPH formation ameliorates oxidative stress imposed by complex I blockade. Downregulation of α-KGDH may, therefore, predispose to oxidative stress in heart failure. KW - mitochondria KW - α-Ketoglutarate dehydrogenase KW - reactive oxygen species KW - nicotinamide nucleotide transhydrogenase Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-234907 SN - 0300-8428 VL - 115 ER - TY - THES A1 - Schäfer, Ingo T1 - Fremdgenexpression in humanen Mitochondrien T1 - Artificial gene expression in human mitochondria N2 - Bei einer Vielzahl neuromuskulärer und neurodegenerativer Erkrankungen spielen Fehlfunktionen der Mitochondrien eine wichtige Rolle. Da die Proteine der Atmungsketten-komplexe sowohl durch die mitochondriale DNA als auch durch das Kerngenom codiert werden, können Mutationen in beiden Genomen die Auslöser dieser Erkrankungen darstellen. Veränderungen der mitochondrialen DNA lassen sich - im Gegensatz zum Kerngenom - bisher nicht korrigieren, weshalb bei einem großen Teil der Erkrankungen nur die Symptome und nicht die Auslöser behandelt werden können. Das grundlegende Problem stellt dabei der Transport der DNA in die Mitochondrien dar. Ziel dieser Arbeit war es, mit Hilfe von physikalischen Transfektionsmethoden exogene DNA in die Mitochondrien menschlicher Kulturzellen einzubringen. Dazu wurden unterschiedliche Vektoren hergestellt, die in Mitochondrien das an die Mitochondrien angepasste grün fluoreszierende mtEGFP exprimieren sollen. Die Expressionsfähigkeit und Prozessierung dieser Konstrukte konnte in in-vitro-Assays mit einem Mitochondrienextrakt nachgewiesen werden. Bei Transfektionsversuchen mit der Gene Gun gelang es erstmals, exogene Plasmid-DNA in die Mitochondrien menschlicher Zellen einzubringen. Das durch die transfizierten Vektoren exprimierte mtEGFP konnte am Fluoreszenzmikroskop eindeutig in den Mitochondrien der Zellen lokalisiert werden. Eine Transfektion mit Hilfe magnetischer Partikel erwies sich jedoch nicht als zielführend, da die die Partikel eine Eigenfluoreszenz aufwiesen, die eine Detektion der mtEGFP-Expression verhinderten. Eine wichtige Voraussetzung für die Transfektion von Mitochondrien durch mechanische Methoden wie die Mikroinjektion ist die reversible Induktion von Megamitochondrien, da sie erst in diesem Zustand penetriert werden können. Durch eine Ansäuerung des Kulturmediums mit Natriumacetat bzw. Essigsäure konnten Mitochondrien erzeugt werden, die beinahe die Größe des Zellkerns aufwiesen und somit ideale Bedingungen für die Mikroinjektion darstellen. Bei den anschließenden Mikroinjektionsversuchen mit den hergestellten mitochondrialen Expressionsvektoren wurden wiederum Zellen mit eindeutig grün fluoreszierenden Mitochondrien gefunden. Zusammenfassend wurden im Rahmen dieser Arbeit erstmalig menschliche Mitochondrien mit exogener DNA transfiziert. Dies stellt einen grundlegenden Schritt für die Entwicklung neuer Therapieformen bei mitochondrialen Myopathien dar. Zuvor müssen die Transfektionsmethoden jedoch noch weiter optimiert werden, um eine höhere Transfektionseffizienz zu erreichen. N2 - Mitochondrial dysfunctions play an important role in a variety of neuromuscular and neurodegenerative diseases. As the proteins of the respiratory chain complexes are encoded by the mitochondrial DNA as well as the nuclear genome, mutations in both could trigger solely the diseases. Up to now, changes of the mitochondrial DNA could not be corrected, hence, therapies were designed to decrease symptoms in patients. In this context, the limiting factor to cure these disease relies on the DNA transport into the mitochondria. The aim of this work was to insert exogenous DNA into the mitochondria of human cultured cells by physical transfection methods. A variety of different vectors was constructed to express the mitochondrially adapted green fluorescent mtEGFP within mitochondria. The ability of these constructs to be expressed and processed was proved by in vitro assays using a mitochrondrial extract. In the transfection experiments using the gene gun, we succeeded for the first time to introduce exogenous plasmid DNA into human mitochondria. The mtEGFP expressed by the transfected vectors could definitely be localized to the mitochondria of the cells. Transfections using magnetic particles as mediator could not be used, because the particles exhibit an autofluorescence which prevents a detection of the mtEGFP expression. An essential prerequisite for the transfection of mitochondria by mechanical methods like microinjection is the reversible induction of megamitochondria, since they could not be penetrated as small regular organelles. Acidification of the culture medium with sodium acetate or acetic acid led to mitochondria exhibiting almost the size of the nucleus, thus giving ideal conditions for microinjection. In the applied microinjection experiments using the mitochondrial expression vectors, cells displayed mitochondria with distinct green fluorescence. In summary, human mitochondria were transfected successfully for the first time with mitochondrial expression vectors. This is a fundamental step in the development of new therapies targeting mitochondrial myopathies. However, the transfection methods have to be optimized to achieve higher transfection efficiencies. KW - Mitochondrium KW - Heterologe Genexpression KW - Mitochondrien KW - mitochondria KW - gene expression KW - Transfektion KW - Mensch KW - Genexpression Y1 - 2011 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-85202 ER - TY - JOUR A1 - Schwemmlein, Julia A1 - Maack, Christoph A1 - Bertero, Edoardo T1 - Mitochondria as therapeutic targets in heart failure JF - Current Heart Failure Reports N2 - Purpose of Review We review therapeutic approaches aimed at restoring function of the failing heart by targeting mitochondrial reactive oxygen species (ROS), ion handling, and substrate utilization for adenosine triphosphate (ATP) production. Recent Findings Mitochondria-targeted therapies have been tested in animal models of and humans with heart failure (HF). Cardiac benefits of sodium/glucose cotransporter 2 inhibitors might be partly explained by their effects on ion handling and metabolism of cardiac myocytes. Summary The large energy requirements of the heart are met by oxidative phosphorylation in mitochondria, which is tightly regulated by the turnover of ATP that fuels cardiac contraction and relaxation. In heart failure (HF), this mechano-energetic coupling is disrupted, leading to bioenergetic mismatch and production of ROS that drive the progression of cardiac dysfunction. Furthermore, HF is accompanied by changes in substrate uptake and oxidation that are considered detrimental for mitochondrial oxidative metabolism and negatively affect cardiac efficiency. Mitochondria lie at the crossroads of metabolic and energetic dysfunction in HF and represent ideal therapeutic targets. KW - mitochondria KW - heart failure KW - reactive oxygen species KW - MitoQ KW - elamipretide KW - SGLT2 inhibitors KW - cardiac metabolism Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-324015 VL - 19 IS - 2 ER - TY - THES A1 - Schauß, Astrid Claudia T1 - Charakterisierung des mitochondrialen Teilungsproteins Dnm1p mittels quantitativer hochauflösender Lichtmikroskopie T1 - Characterization of the mitochondrial fission protein Dnm1p using quantitative high resolution light microscopy N2 - Mitochondrien verändern dynamisch durch ein balanciertes Verhältnis von Teilung und Fusion die Gestalt ihrer Netzwerke und reagieren so auf interne und externe Signale. Ein Schlülsselprotein der mitochondrialen Teilung ist die Dynamin-verwandte GTPase Dnm1p, die in dieser Arbeit charakterisiert wurde. Da Mitochondrien aufgrund ihres endosymbiontischen Ursprungs zwei Membranen besitzen, erfordert deren Teilung eine besondere Koordination. Unter Verwendung von photokonvertierbarem GFP wird in dieser Arbeit gezeigt, dass in S. cerevisiae die Teilung der inneren und äußeren Membran zeitlich eng gekoppelt verläuft. Dieser Prozess wird durch die GTPase Dnm1p, aber auch durch die Adaptor-Proteine Mdv1p und Caf4p sowie dem integralen Membrananker Fis1p v ermittelt. Dnm1p lagert sich zu Spiralen um den tubulären Strang an und trennt GTP-abhängig die Mitochondrien voneinander. Eine Voraussetzung für die Anlagerung dieser Spiralen stellen Matrix-Konstriktionen dar. In dieser Arbeit wird gezeigt, dass Dnm1p und auch Fis1p für die Ausbildung dieser mitochondrialen Einschnürungen nicht essentiell sind. Die Untersuchung der Verteilung, Orientierung und Größe der Epitop-markierten Dnm1p-Cluster bildet den Schwerpunkt der Arbeit. Weiterhin wird der Einfluss der Teilungsproteine Fis1p, Mdv1p und Caf4p auf diese Dnm1p-Charakteristika ermittelt. Die Analyse basiert auf quantitativen Konfokalmikroskopie-Aufnahmen, zusätzlich werden auch neue hochauflösende Lichtmikroskope (4Pi und STED) zur genauen Lokalisation und Größenbestimmung eingesetzt. Die Ergebnisse zeigen, dass im Wildtyp und in Mdv1p-Deletionsstämmen die Mehrheit der Cluster mit den Mitochondrien assoziiert ist, während in Fis1p- und Caf4p-Deletionszellen die Rekrutierung der Cluster zu den Mitochondrien gestört erscheint. Nur wenige Cluster bilden Spiralen um Matrix-Konstriktionen aus, die überwiegende Mehrheit der nicht an aktuellen Teilungsprozessen beteiligten Dnm1p-Aggregate weist dagegen im Wildtyp und in Mdv1p-Deletionszellen eine polare Orientierung Richtung Zellcortex auf. Die in dieser Arbeit zum ersten Mal beschriebene Polarität ist in Fis1p- und Caf4p-Deletionsstämmen aufgehoben, bleibt jedoch auch nach der Zerstörung des Aktin-Gerüstes aufrechterhalten. Die Ergebnisse der Arbeit deuten darauf hin, dass Dnm1p in einem Komplex mit Fis1p und Caf4p zusätzlich zu seiner Funktion als Teilungsprotein an der Anheftung der Mitochondrien an den Zellcortex beteiligt ist. Zudem scheinen die Adaptorproteine Mdv1p und Caf4p trotz molekularer Ähnlichkeit unterschiedliche Aufgaben in der Zelle zu erfüllen. N2 - Mitochondrial networks dynamically change their shape by balanced fission and fusion in response to internal and external signals. The key protein in mitochondrial fission, the dynamin-related GTPase Dnm1p, is characterised in this study. Because of their endosymbiotic origin mitochondria possess two membranes, whose separations must be coordinated. Using photoconvertable GFP, it is shown that the division of outer and inner membranes are tightly coupled in S. cerevisiae. This separation is due to the GTPase Dnm1p, but the adaptor proteins Mdv1p and Caf4p, as well as the membrane anchor Fis1p, are also involved in mitochondrial division in yeast. Dnm1p forms spirals around the mitochondrial tubes and separates them in a GTPase-dependant manner. Matrix constrictions are presumably one precondition for the formation of spirals. In this work it is shown that Dnm1p as well as Fis1p are not essential for the formation for this mitochondrial narrowing. The main focus of the work is the analysis of the distribution, orientation and size of the epitope-tagged Dnm1p clusters in yeast cells. Additionally, the influence of the other division proteins, Fis1p, Mdv1p and Caf4p, on these Dnm1p characteristics is determined. The analysis is based on both quantitative confocal images and high resolution 4Pi and STED microscopy, for better localization and determination of the cluster sizes. The results demonstrate that in wild type and Mdv1p deletion cells, the majority of clusters are associated with mitochondria, whereas the recruitment of Dnm1p-clusters is disturbed in Fis1p and Caf4p deletion cells. While just a few clusters form spirals around matrix constrictions, the overwhelming majority of clusters, which are not involved in an actual fission process, show a polar orientation towards the cell cortex in wild type and Mdv1p deletion cells. This polarity, described for the first time in this work, is abolished in Fis1 and Caf4p deletion cells, but is maintained after the destruction of the actin cytoskeleton. The results of this work point to an additional role of Dnm1p, together with Fis1p and Caf4p, in the attachment of mitochondria to the cell cortex. Furthermore it is shown that the adaptor proteins Mdv1p and Caf4p have different roles within the cell despite of their molecular similarity. KW - Hefeartige Pilze KW - Mitochondrium KW - Mikroskopie KW - Mitochondrien KW - Dynamik KW - Hefe KW - STED KW - 4Pi KW - mitochondria KW - dynamic KW - yeast KW - STED KW - 4Pi Y1 - 2006 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-17566 ER - TY - JOUR A1 - Sacchetto, Claudia A1 - Sequeira, Vasco A1 - Bertero, Edoardo A1 - Dudek, Jan A1 - Maack, Christoph A1 - Calore, Martina T1 - Metabolic Alterations in Inherited Cardiomyopathies JF - Journal of Clinical Medicine N2 - The normal function of the heart relies on a series of complex metabolic processes orchestrating the proper generation and use of energy. In this context, mitochondria serve a crucial role as a platform for energy transduction by supplying ATP to the varying demand of cardiomyocytes, involving an intricate network of pathways regulating the metabolic flux of substrates. The failure of these processes results in structural and functional deficiencies of the cardiac muscle, including inherited cardiomyopathies. These genetic diseases are characterized by cardiac structural and functional anomalies in the absence of abnormal conditions that can explain the observed myocardial abnormality, and are frequently associated with heart failure. Since their original description, major advances have been achieved in the genetic and phenotype knowledge, highlighting the involvement of metabolic abnormalities in their pathogenesis. This review provides a brief overview of the role of mitochondria in the energy metabolism in the heart and focuses on metabolic abnormalities, mitochondrial dysfunction, and storage diseases associated with inherited cardiomyopathies. KW - inherited cardiomyopathies KW - mitochondria KW - cardiac metabolism Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193806 SN - 2077-0383 VL - 8 IS - 12 ER - TY - JOUR A1 - Ruf, Dominik A1 - Brantl, Victor A1 - Wagener, Johannes T1 - Mitochondrial Fragmentation in \(Aspergillus\) \(fumigatus\) as Early Marker of Granulocyte Killing Activity JF - Frontiers in Cellular and Infection Microbiology N2 - The host's defense against invasive mold infections relies on diverse antimicrobial activities of innate immune cells. However, studying these mechanisms in vitro is complicated by the filamentous nature of such pathogens that typically form long, branched, multinucleated and compartmentalized hyphae. Here we describe a novel method that allows for the visualization and quantification of the antifungal killing activity exerted by human granulocytes against hyphae of the opportunistic pathogen Aspergillus fumigatus. The approach relies on the distinct impact of fungal cell death on the morphology of mitochondria that were visualized with green fluorescent protein (GFP). We show that oxidative stress induces complete fragmentation of the tubular mitochondrial network which correlates with cell death of affected hyphae. Live cell microscopy revealed a similar and non-reversible disruption of the mitochondrial morphology followed by fading of fluorescence in Aspergillus hyphae that were killed by human granulocytes. Quantitative microscopic analysis of fixed samples was subsequently used to estimate the antifungal activity. By utilizing this assay, we demonstrate that lipopolysaccharides as well as human serum significantly increase the killing efficacy of the granulocytes. Our results demonstrate that evaluation of the mitochondrial morphology can be utilized to assess the fungicidal activity of granulocytes against A. fumigatus hyphae. KW - Aspergillus fumigatus KW - killing KW - assay KW - PMNs KW - granulocytes KW - mitochondria KW - mitochondrial morphology KW - fungicidal activity Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-227133 VL - 8 IS - 128 ER - TY - JOUR A1 - Prinz, Johanna A1 - Karacivi, Aylin A1 - Stormanns, Eva R. A1 - Recks, Masha S. A1 - Kürten, Stefanie T1 - Time-Dependent Progression of Demyelination and Axonal Pathology in MP4-Induced Experimental Autoimmune Encephalomyelitis JF - PloS One N2 - Background Multiple sclerosis (MS) is an autoimmune disease of the central nervous system (CNS) characterized by inflammation, demyelination and axonal pathology. Myelin basic protein/proteolipid protein (MBP-PLP) fusion protein MP4 is capable of inducing chronic experimental autoimmune encephalomyelitis (EAE) in susceptible mouse strains mirroring diverse histopathological and immunological hallmarks of MS. Limited availability of human tissue underscores the importance of animal models to study the pathology of MS. Methods Twenty-two female C57BL/6 (B6) mice were immunized with MP4 and the clinical development of experimental autoimmune encephalomyelitis (EAE) was observed. Methylene blue-stained semi-thin and ultra-thin sections of the lumbar spinal cord were assessed at the peak of acute EAE, three months (chronic EAE) and six months after onset of EAE (long-term EAE). The extent of lesional area and inflammation were analyzed in semi-thin sections on a light microscopic level. The magnitude of demyelination and axonal damage were determined using electron microscopy. Emphasis was put on the ventrolateral tract (VLT) of the spinal cord. Results B6 mice demonstrated increasing demyelination and severe axonal pathology in the course of MP4-induced EAE. In addition, mitochondrial swelling and a decrease in the nearest neighbor neurofilament distance (NNND) as early signs of axonal damage were evident with the onset of EAE. In semi-thin sections we observed the maximum of lesional area in the chronic state of EAE while inflammation was found to a similar extent in acute and chronic EAE. In contrast to the well-established myelin oligodendrocyte glycoprotein (MOG) model, disease stages of MP4-induced EAE could not be distinguished by assessing the extent of parenchymal edema or the grade of inflammation. Conclusions Our results complement our previous ultrastructural studies of B6 EAE models and suggest that B6 mice immunized with different antigens constitute useful instruments to study the diverse histopathological aspects of MS. KW - Multiple sclerosis KW - spinal cord KW - central nervous system KW - nerve fibers KW - inflammatory diseases KW - axons KW - mitochondria KW - mouse models Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146651 VL - 10 IS - 12 ER - TY - THES A1 - Pedrotti, Lorenzo T1 - The SnRK1-C/S1-bZIPs network: a signaling hub in Arabidopsis energy metabolism regulation T1 - Das SnRK1-C/S1-bZIP-Netzwerk: ein Signalknoten in der Regulation des Arabidopsis Energie-Metabolismus N2 - The control of energy homeostasis is of pivotal importance for all living organisms. In the last years emerged the idea that many stress responses that are apparently unrelated, are actually united by a common increase of the cellular energy demand. Therefore, the so called energy signaling is activated by many kind of stresses and is responsible for the activation of the general stress response. In Arabidopsis thaliana the protein family SnF1- related protein kinases (SnRK1) is involved in the regulation of many physiological processes but is more known for its involvement in the regulation of the energy homeostasis in response to various stresses. To the SnRK1 protein family belong SnRK1.1 (also known as KIN10), SnRK1.2 (KIN11), and SnRK1.3 (KIN12). SnRK1 exerts its function regulating directly the activity of metabolic enzymes or those of key transcription factors (TFs). The only TFs regulated by SnRK1 identified so far is the basic leucine zipper (bZIP) 63. bZIP63 belongs to the C group of bZIPs (C-bZIPs) protein family together with bZIP9, bZIP10, and bZIP25. SnRK1.1 phosphorylates bZIP63 on three amino acids residues, serine (S) 29, S294, and S300. The phosphorylation of tbZIP63 is strongly related to the energy status of the plant, shifting from almost absent during the normal growth to strongly phosphorylated when the plant is exposed to extended dark. bZIPs normally bind the DNA as dimer in order to regulate the expression of their target genes. C-bZIPs preferentially form dimers with S1-bZIPs, constituting the so called C/S1- bZIPs network. The SnRk1 dependent phosphorylation of bZIP63 regulates its activation potential and its dimerization properties. In particular bZIP63 shift its dimerization preferences according to its phosphorylation status. The non-phosphorylated form of bZIP63 dimerize bZIP1, the phosphorylates ones, instead, forms dimer with bZIP1, bZIP11, and bZIP63 its self. Together with bZIP63, S1-bZIPs are important mediator of part of the huge transcriptional reprogramming induced by SnRK1 in response to extended dark. S1-bZIPs regulate, indeed, the expression of 4'000 of the 10'000 SnRK1-regulated genes in response to energy deprivation. In particular S1-bZIPs are very important for the regulation of many genes encoding for enzymes involved in the amino acid metabolism and for their use as alternative energy source. After the exposition for some hours to extended dark, indeed, the plant make use of every energy substrate and amino acids are considered an important energy source together with lipids and proteins. Interestingly, S1- bZIPs regulate the expression of ETFQO. ETFQO is a unique protein that convoglia the electrons provenienti from the branch chain amino acids catabolism into the mitochondrial electron transport chain. The dimer formed between bZIP63 and bZIP2 recruits SnRK1.1 directly on the chromatin of ETFQO promoter. The recruitment of SnRK1 on ETFQO promoter is associated with its acetylation on the lysine 14 of the histone protein 3 (K14H3). This chromatin modification is normally asociated with an euchromatic status of the DNA and therefore with its transcriptional activation. Beside the particular case of the regulation of ETFQO gene, S1-bZIPs are involved in the regulation of many other genes activated in response of different stresses. bZIP1 is for example an important mediator of the salt stress response. In particular bZIP1 regulates the primary C- and N-metabolism. The expression of bZIP1, in response of both salt ans energy stress seems to be regulated by SnRK1, as it is the expression of bZIP53 and bZIP63. Beside its involvement in the regulation of the energy stress response and salt response, SnRK1 is the primary activators of the lipids metabolism during see germination. SnRK1, indeed, controls the expression of CALEOSINs and OLEOSINs. Those proteins are very important for lipids remobilization from oil droplets. Without their expression seed germination and subsequent establishment do not take place because of the absence of fuel to sustain these highly energy costly processes, which entirely depend on the catabolism of seed storages. N2 - Die Kontrolle der Energiehomöostase ist für alle lebenden Organismen von großer Bedeutung. In den letzten Jahren kam die Idee auf, dass viele Stressantworten, die scheinbar unabhängig voneinander sind, durch den Energiebedarf doch miteinander verbunden sind. Das sogenannte Energie-Signaling wird von vielen verschiedenen Stress- Arten aktiviert und ist verantwortlich für die Aktivierung der allgemeinen Stressantwort. In Arabidopsis thaliana ist die Proteinfamilie der SnF1-verwandten Proteinkinasen (SnRK1) an der Regulation vieler physiologischer Prozesse beteiligt. Auch bei der Regulation der Energiehomöostase als Folge von Stress spielen SnRK1-Kinasen eine wichtige Rolle. Proteine aus der SnRK1-Familie sind SnRK1.1, auch als KIN10 bezeichnet, SnRK1.2 (KIN11) und SnRK1.3 (KIN12). SnRK1-Proteine können die Aktivität von metabolischen Enzyme oder bestimmten Transkriptionsfaktoren (TF) direkt regulieren. Bislang wurde nur für den basischen Leucin-Zipper (bZIP) TF bZIP63 die Regulation durch SnRK1 gezeigt. bZIP63 gehört zur Gruppe C der bZIP Proteinfamilie (C-bZIP). Ebenfalls zu Gruppe C werden bZIP9, bZIP10 und bZIP25 zugeordnet. SnRK1.1 phosphoryliert das bZIP63- Protein an Serin (S) 29, S294 und S300. Der Grad der Phosphorylierung von bZIP63 steht in direktem Zusammenhang mit dem Energiehaushalt der Pflanze. Unter normalen Bedingungen wird bZIP63 kaum phosphoryliert, während bei verlängerter Nacht bZIP63 stark phosphoryliert wird. bZIP TF bilden untereinander Dimere aus und binden so an die DNA um die Expression ihrer Zielgene zu regulieren. C-bZIP TF bilden bevorzugt Dimere mit bZIP TF der Gruppe S1, bekannt als das C/S1-bZIP-Netzwerk. Die SnRK1-abhängige Phosphorylierung von bZIP63 steuert das Aktivierungspotential und die Dimerisierungseigenschaften. Besonders bei bZIP63 ändern sich die Dimerisierungspartner in Abhängigkeit des Phosphorylierungsgrads. Nicht-phosphoryliert dimerisiert bZIP61 mit bZIP1, im phosphorylierten Zustand dagegen bildet bZIP63 Dimere neben bZIP1 auch mit bZIP11 und bZIP63. S1-bZIP TF sowie bZIP63 sind wichtige Regulatoren der transkriptionellen Reprogrammierung, die durch SnRK1 bei verlängerter Dunkelheit induziert wird. S1-bZIP TF regulieren die Expression von 4'000 der 10'000 durch SnRK1 regulierten Gene in der Energieverarmungsantwort. Besonders S1-bZIP TF sind sehr wichtig für die Regulation vieler Gene, die für Enzyme aus dem Aminosäuremetabolismus codieren und als alternative Energiequelle der Pflanze bekannt sind. Wird die Nacht für einige Stunden verlängert, greift die Pflanze auf jede mögliche Energiequelle zurück. Als Energiequelle werden besonders Aminosäuren, aber auch Lipiden und Proteinen herangezogen. Interessanterweise regulieren S1-bZIP TF die Expression von ETFQO. ETFQO ist ein besonderes Protein, das die Elektronen aus dem Metabolismus verzweigter Aminosäuren in die mitochondriale Elektronentransportkette steuert. Das Dimer aus bZIP63 und bZIP2 rekrutiert SnRK1.1 direkt an das Chromatin des ETFQO-Promotors. Dieser Rekrutierung folgt die Acetylierung des Histonproteins 3 (K14H3) am Lysin 14. Diese Modifikation des Chromatins führt normalerweise zu einem euchromatischen Status der DNA und der nachfolgenden transkriptionellen Aktivierung. Neben der Regulation des ETFQO-Gens sind S1-bZIP TF auch an der Regulation von vielen anderen Genen in Folge von verschiedenen Stressen beteiligt. bZIP1 ist beispielsweise ein wichtiger Regulator der Antwort auf Salz-Stress. Auch der primäre Kohlenstoff- und Stickstoffmetabolismus werden von bZIP1 reguliert. Es wird angenommen, dass die Expression von bZIP1 wie auch von bZIP53 und bZIP63 in der Antwort auf Salzstress und Energieverarmung durch SnRK1 gesteuert wird. Abgesehen von der Regulation der Antwort auf Energieverarmung und Salzstress spielen SnRK1-Proteine auch bei der Aktivierung des Lipidmetabolismus während der Keimung eine Rolle. SnRK1 kontrolliert die Expression von CALEOSINs und OLEOSINs. Diese beiden Proteine sind sehr wichtig für die Mobilisierung von Lipiden aus Öltröpfchen. In Abwesenheit von SnRK1 finden aufgrund von Energiemangel weder die Keimung noch die nachfolgende Entwicklung statt. KW - Ackerschmalwand KW - Homöostase KW - Proteinkinasen KW - Stress-Syndrom KW - SnRK1 KW - bZIPs KW - mitochondria KW - energy metabolism Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-116080 ER - TY - JOUR A1 - Palladino, Viola Stella A1 - Chiocchetti, Andreas G. A1 - Frank, Lukas A1 - Haslinger, Denise A1 - McNeill, Rhiannon A1 - Radtke, Franziska A1 - Till, Andreas A1 - Haupt, Simone A1 - Brüstle, Oliver A1 - Günther, Katharina A1 - Edenhofer, Frank A1 - Hoffmann, Per A1 - Reif, Andreas A1 - Kittel-Schneider, Sarah T1 - Energy metabolism disturbances in cell models of PARK2 CNV carriers with ADHD JF - Journal of Clinical Medicine N2 - The main goal of the present study was the identification of cellular phenotypes in attention-deficit-/hyperactivity disorder (ADHD) patient-derived cellular models from carriers of rare copy number variants (CNVs) in the PARK2 locus that have been previously associated with ADHD. Human-derived fibroblasts (HDF) were cultured and human-induced pluripotent stem cells (hiPSC) were reprogrammed and differentiated into dopaminergic neuronal cells (mDANs). A series of assays in baseline condition and in different stress paradigms (nutrient deprivation, carbonyl cyanide m-chlorophenyl hydrazine (CCCP)) focusing on mitochondrial function and energy metabolism (ATP production, basal oxygen consumption rates, reactive oxygen species (ROS) abundance) were performed and changes in mitochondrial network morphology evaluated. We found changes in PARK2 CNV deletion and duplication carriers with ADHD in PARK2 gene and protein expression, ATP production and basal oxygen consumption rates compared to healthy and ADHD wildtype control cell lines, partly differing between HDF and mDANs and to some extent enhanced in stress paradigms. The generation of ROS was not influenced by the genotype. Our preliminary work suggests an energy impairment in HDF and mDAN cells of PARK2 CNV deletion and duplication carriers with ADHD. The energy impairment could be associated with the role of PARK2 dysregulation in mitochondrial dynamics. KW - ADHD KW - hiPSC KW - PARK2 KW - mitochondria KW - disease modelling Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-220074 SN - 2077-0383 VL - 9 IS - 12 ER - TY - THES A1 - Ott, Christine Kornelia T1 - Diverse Aspects of the Sorting and Assembly Machinery in Human Mitochondria T1 - Diverse Aspekte der Sortierungs- und Assemblierungsmaschinerie in humanen Mitochondrien N2 - Mitochondria are organelles of endosymbiotic origin, which play many important roles in eukaryotic cells. Mitochondria are surrounded by two membranes and, considering that most of the mitochondrial proteins are produced in the cytosol, possess import machineries, which transport mitochondria-targeted proteins to their designated location. A special class of outer mitochondrial membrane (OMM) proteins, the β-barrel proteins, require the sorting and assembly machinery (SAM) for their OMM integration. Both mitochondrial β-barrel proteins and the central component of the SAM complex, Sam50, have homologs in gram-negative bacteria. In yeast mitochondria, bacterial β-barrel proteins can be imported and assembled into the OMM. Our group demonstrated that this, however, is not the case for human mitochondria, which import only neisserial β barrel proteins, but not those of Escherichia coli and Salmonella enterica. As a part of this study, I could demonstrate that β-barrel proteins such as Omp85 and PorB of different Neisseria species are targeted to human mitochondria. Interestingly, only proteins belonging to the neisserial Omp85 family were integrated into the OMM, whereas PorB was imported into mitochondria but not assembled. By exchanging parts of homologous neisserial Omp85 and E. coli BamA and, similarly, of neisserial PorB and E. coli OmpC, it could be demonstrated in this work that the mitochondrial import signal of bacterial β barrel proteins cannot be limited to one short linear sequence, but rather secondary structure and protein charge seem to play an important role, as well as specific residues in the last β-strand of Omp85. Omp85 possesses five conserved POTRA domains in its amino-terminal part. This work additionally demonstrated that in human mitochondria, at least two POTRA domains of Omp85 are necessary for membrane integration and functionality of Omp85. In the second part of this work, the influence of Sam50 on the mitochondrial cristae structure was investigated. This work contributed to a study performed by our group in which it was confirmed that Sam50 is present in a high molecular weight complex together with mitofilin, CHCHD3, CHCHD6, DnaJC11, metaxin 1 and metaxin 2. This connection between the inner and outer mitochondrial membrane was shown to be crucial for the maintenance of the mitochondrial cristae structure. In addition, a role of Sam50 in respiratory complex assembly, suggested by a SILAC experiment conducted in our group, could be confirmed by in vitro import studies. An influence of Sam50 not only on respiratory complexes but also on the recently described respiratory complex assembly factor TTC19 was demonstrated. It was shown that TTC19 not only plays a role in complex III assembly as published, but also influences the assembly of respiratory complex IV. Thus, in this part of the work a connection between the OMM protein Sam50 and maintenance of cristae structure, respiratory complex assembly and an assembly factor could be established. N2 - Mitochondrien sind Zellorganellen endosymbiotischen Ursprungs, die viele wichtige Funktionen in eukaryotischen Zellen haben. Mitochondrien sind von zwei Membranen umgeben, und da die meisten Mitochondrienproteine im Cytosol hergestellt werden, besitzen sie Importmaschinerien, die die für die Mitochondrien bestimmten Proteine zu ihrem jeweiligen Zielort transportieren. Eine besondere Klasse von Proteinen der äußeren Mitochondrienmembran (ÄMM), die β-Fassproteine, benötigen die Sortierungs- und Assemblierungsmaschinerie (SAM) für ihre Integration in die ÄMM. Sowohl mitochondriale β-Fassproteine als auch die zentrale Komponente des SAM-Komplexes, Sam50, haben Homologe in gramnegativen Bakterien. In Hefemitochondrien können bakterielle β Fassproteine importiert und in der ÄMM assembliert werden. Unsere Gruppe hat gezeigt, dass dies jedoch nicht auf humane Mitochondrien zutrifft, die nur neisserielle β-Fassproteine importieren, nicht aber diejenigen von Escherichia coli und Salmonella enterica. Im Rahmen dieser Studie konnte ich zeigen, dass β Fassproteine verschiedener Neisserienarten, wie Omp85 und PorB, in humane Mitochondrien aufgenommen werden. Interessanterweise wurden nur Proteine der neisseriellen Omp85-Familie in die ÄMM eingebaut, während PorB zwar importiert, jedoch nicht assembliert wurde. Durch das Austauschen von Teilen von homologem neisseriellen Omp85 und E.coli BamA und ebenso von neisseriellem PorB und E. coli OmpC konnte in dieser Arbeit gezeigt werden, dass das mitochondriale Importsignal bakterieller β-Fassproteine nicht auf eine kurze lineare Sequenz eingegrenzt werden kann, sondern dass die Sekundärstruktur und die Ladung des Proteins eine wichtige Rolle zu spielen scheinen, sowie im Fall von Omp85 einige bestimmte Aminosäurereste des letzten β-Stranges. Omp85 besitzt fünf konservierte POTRA-Domänen in seiner aminoterminalen Hälfte. In dieser Arbeit wurde zudem demonstriert, dass in humanen Mitochondrien mindestens zwei POTRA-Domänen von Omp85 für die Membranintegration und Funktionalität von Omp85 vorhanden sein müssen. Im zweiten Teil dieser Arbeit wurde der Einfluss von Sam50 auf die mitochondriale Cristaestruktur untersucht. Diese Arbeit hat zu einer von unserer Gruppe durchgeführten Studie beigetragen, in der bestätigt werden konnte, dass Sam50 in einem hochmolekularen Komplex mit Mitofilin, CHCHD3, CHCHD6, DnaJC11, Metaxin 1 und Metaxin 2 vorliegt. Es wurde gezeigt, dass diese Verbindung zwischen der inneren und äußeren Mitochondrienmembran unverzichtbar für die Aufrechterhaltung der mitochondrialen Cristaestruktur ist. Zudem konnte eine Rolle von Sam50 bei der Assemblierung von Atmungskettenkomplexen, die durch ein in unserem Labor durchgeführtes SILAC-Experiment nahegelegt worden war, durch in-vitro-Importstudien bestätigt werden. Weiterhin wurde ein Einfluss von Sam50 nicht nur auf Atmungskettenkomplexe, sondern auch auf einen vor kurzem beschriebenen Assemblierungsfaktor der Atmungskette, TTC19, demonstriert. Es wurde gezeigt, dass TTC19 nicht nur, wie veröffentlicht, eine Rolle bei der Assemblierung des Atmungskettenkomplexes III spielt, sondern auch die Assemblierung des Atmungskettenkomplexes IV beeinflusst. In diesem Teil der Arbeit konnte folglich eine Verbindung zwischen dem ÄMM-Protein Sam50 und der Organisation der Cristaestruktur, der Atmungskettenassemblierung und einem Assemblierungsfaktor nachgewiesen werden. KW - Mitochondrien KW - Mensch KW - Molekularbiologie KW - mitochondria KW - Import KW - Omp85 KW - beta-barrel-proteins KW - cristae KW - beta-Fassproteine KW - Cristaestruktur Y1 - 2013 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-85462 ER - TY - JOUR A1 - Ott, Christine A1 - Dorsch, Eva A1 - Fraunholz, Martin A1 - Straub, Sebastian A1 - Kozjak-Pavlovic, Vera T1 - Detailed Analysis of the Human Mitochondrial Contact Site Complex Indicate a Hierarchy of Subunits JF - PLoS One N2 - Mitochondrial inner membrane folds into cristae, which significantly increase its surface and are important for mitochondrial function. The stability of cristae depends on the mitochondrial contact site (MICOS) complex. In human mitochondria, the inner membrane MICOS complex interacts with the outer membrane sorting and assembly machinery (SAM) complex, to form the mitochondrial intermembrane space bridging complex (MIB). We have created knockdown cell lines of most of the MICOS and MIB components and have used them to study the importance of the individual subunits for the cristae formation and complex stability. We show that the most important subunits of the MIB complex in human mitochondria are Mic60/Mitofilin, Mic19/CHCHD3 and an outer membrane component Sam50. We provide additional proof that ApoO indeed is a subunit of the MICOS and MIB complexes and propose the name Mic23 for this protein. According to our results, Mic25/CHCHD6, Mic27/ApoOL and Mic23/ApoO appear to be periphery subunits of the MICOS complex, because their depletion does not affect cristae morphology or stability of other components. KW - co-immunoprecipitation KW - motor proteins KW - mitochondria KW - membrane potential KW - membrane proteins KW - protein complexes KW - mitochondrial membrane KW - outer membrane proteins Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125347 VL - 10 IS - 3 ER - TY - JOUR A1 - Niemann, Axel A1 - Huber, Nina A1 - Wagner, Konstanze M. A1 - Somandin, Christian A1 - Horn, Michael A1 - Lebrun-Julien, Frédéric A1 - Angst, Brigitte A1 - Pereira, Jorge A. A1 - Halfter, Hartmut A1 - Welzl, Hans A1 - Feltri, M. Laura A1 - Wrabetz, Lawrence A1 - Young, Peter A1 - Wessig, Carsten A1 - Toyka, Klaus V. A1 - Suter, Ueli T1 - The Gdap1 knockout mouse mechanistically links redox control to Charcot–Marie–Tooth disease JF - Brain N2 - The ganglioside-induced differentiation-associated protein 1 (GDAP1) is a mitochondrial fission factor and mutations in GDAP1 cause Charcot–Marie–Tooth disease. We found that Gdap1 knockout mice (\(Gdap1^{−/−}\)), mimicking genetic alterations of patients suffering from severe forms of Charcot–Marie–Tooth disease, develop an age-related, hypomyelinating peripheral neuropathy. Ablation of Gdap1 expression in Schwann cells recapitulates this phenotype. Additionally, intra-axonal mitochondria of peripheral neurons are larger in \(Gdap1^{−/−}\) mice and mitochondrial transport is impaired in cultured sensory neurons of \(Gdap1^{−/−}\) mice compared with controls. These changes in mitochondrial morphology and dynamics also influence mitochondrial biogenesis. We demonstrate that mitochondrial DNA biogenesis and content is increased in the peripheral nervous system but not in the central nervous system of \(Gdap1^{−/−}\) mice compared with control littermates. In search for a molecular mechanism we turned to the paralogue of GDAP1, GDAP1L1, which is mainly expressed in the unaffected central nervous system. GDAP1L1 responds to elevated levels of oxidized glutathione by translocating from the cytosol to mitochondria, where it inserts into the mitochondrial outer membrane. This translocation is necessary to substitute for loss of GDAP1 expression. Accordingly, more GDAP1L1 was associated with mitochondria in the spinal cord of aged \(Gdap1^{−/−}\) mice compared with controls. Our findings demonstrate that Charcot–Marie–Tooth disease caused by mutations in GDAP1 leads to mild, persistent oxidative stress in the peripheral nervous system, which can be compensated by GDAP1L1 in the unaffected central nervous system. We conclude that members of the GDAP1 family are responsive and protective against stress associated with increased levels of oxidized glutathione. KW - animal models KW - Charcot-Marie-Tooth disease KW - mitochondria KW - axonal transport KW - demyelinating disease Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-120731 VL - 137 IS - 3 ER - TY - JOUR A1 - Masic, Anita A1 - Valencia Hernandez, Ana Maria A1 - Hazra, Sudipta A1 - Glaser, Jan A1 - Holzgrabe, Ulrike A1 - Hazra, Banasri A1 - Schurigt, Uta T1 - Cinnamic Acid Bornyl Ester Derivatives from Valeriana wallichii Exhibit Antileishmanial In Vivo Activity in Leishmania major-Infected BALB/c Mice JF - PLoS One N2 - Human leishmaniasis covers a broad spectrum of clinical manifestations ranging from self-healing cutaneous leishmaniasis to severe and lethal visceral leishmaniasis caused among other species by Leishmania major or Leishmania donovani, respectively. Some drug candidates are in clinical trials to substitute current therapies, which are facing emerging drug-resistance accompanied with serious side effects. Here, two cinnamic acid bornyl ester derivatives (1 and 2) were assessed for their antileishmanial activity. Good selectivity and antileishmanial activity of bornyl 3-phenylpropanoate (2) in vitro prompted the antileishmanial assessment in vivo. For this purpose, BALB/c mice were infected with Leishmania major promastigotes and treated with three doses of 50 mg/kg/day of compound 2. The treatment prevented the characteristic swelling at the site of infection and correlated with reduced parasite burden. Transmitted light microscopy and transmission electron microscopy of Leishmania major promastigotes revealed that compounds 1 and 2 induce mitochondrial swelling. Subsequent studies on Leishmania major promastigotes showed the loss of mitochondrial transmembrane potential (ΔΨm) as a putative mode of action. As the cinnamic acid bornyl ester derivatives 1 and 2 had exhibited antileishmanial activity in vitro, and compound 2 in Leishmania major-infected BALB/c mice in vivo, they can be regarded as possible lead structures for the development of new antileishmanial therapeutic approaches. KW - leishmania major KW - promastigotes KW - apoptosis KW - mitochondria KW - parasitic diseases KW - leishmania KW - leishmaniasis KW - mouse models Y1 - 2015 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125354 VL - 10 IS - 11 ER - TY - JOUR A1 - Kunz, Tobias C. A1 - Götz, Ralph A1 - Gao, Shiqiang A1 - Sauer, Markus A1 - Kozjak-Pavlovic, Vera T1 - Using Expansion Microscopy to Visualize and Characterize the Morphology of Mitochondrial Cristae JF - Frontiers in Cell and Developmental Biology N2 - Mitochondria are double membrane bound organelles indispensable for biological processes such as apoptosis, cell signaling, and the production of many important metabolites, which includes ATP that is generated during the process known as oxidative phosphorylation (OXPHOS). The inner membrane contains folds called cristae, which increase the membrane surface and thus the amount of membrane-bound proteins necessary for the OXPHOS. These folds have been of great interest not only because of their importance for energy conversion, but also because changes in morphology have been linked to a broad range of diseases from cancer, diabetes, neurodegenerative diseases, to aging and infection. With a distance between opposing cristae membranes often below 100 nm, conventional fluorescence imaging cannot provide a resolution sufficient for resolving these structures. For this reason, various highly specialized super-resolution methods including dSTORM, PALM, STED, and SIM have been applied for cristae visualization. Expansion Microscopy (ExM) offers the possibility to perform super-resolution microscopy on conventional confocal microscopes by embedding the sample into a swellable hydrogel that is isotropically expanded by a factor of 4–4.5, improving the resolution to 60–70 nm on conventional confocal microscopes, which can be further increased to ∼ 30 nm laterally using SIM. Here, we demonstrate that the expression of the mitochondrial creatine kinase MtCK linked to marker protein GFP (MtCK-GFP), which localizes to the space between the outer and the inner mitochondrial membrane, can be used as a cristae marker. Applying ExM on mitochondria labeled with this construct enables visualization of morphological changes of cristae and localization studies of mitochondrial proteins relative to cristae without the need for specialized setups. For the first time we present the combination of specific mitochondrial intermembrane space labeling and ExM as a tool for studying internal structure of mitochondria. KW - Expansion microscopy KW - mitochondria KW - cristae KW - structured illumination microscope KW - ultrastructure Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-208296 SN - 2296-634X VL - 8 ER - TY - THES A1 - Kukat, Christian T1 - Fusion, Fission und Nucleoids in Megamitochondrien T1 - Fusion, fission and nucleoids in megamitochondria N2 - In rho0-Zellen, die über keine mitochondriale DNA (mtDNA) mehr verfügen, entstehen während der Kultivierung Megamitochondrien durch endogene Milchsäure-Azidifizierung des Kulturmediums. Diese Riesenorganellen bilden sich dabei durch mitochondriale Fusionsereignisse und/oder eine Hemmung der Fission. In Zellen mit mitochondrialem Genom ist es ebenso möglich Megamitochondrien durch artifizielles Ansäuern des Kulturmediums zu induzieren. Diese Erkenntnisse wurden im Rahmen dieser Arbeit als Werkzeug verwendet, um Einblicke in mitochondriale Fusions- und Fissionsereignisse zu erlangen. Zunächst wurde die Fusion mitochondrialer Matrixkompartimente mithilfe der photoaktivierbaren Variante des grünen fluoreszierenden Proteins (PA-GFP) untersucht. Hiermit konnte gezeigt werden, dass das Vermischen der Matrixkompartimente nach der Fusion ein sehr schneller Prozess ist. Die Analyse der Bildung und Rückbildung der Megamitochondrien erfolgte sowohl konfokal- als auch elektronenmikroskopisch, wobei sich zeigte, dass die Matrix der Riesenorganellen kaum mehr Cristae beinhaltet. Die Rückbildung der Megamitochondrien zum normalen Netzwerk ist ein sehr schneller Prozess, bei dem schon nach 15 min keine vergrößerten Organellen mehr sichtbar sind. Dies indiziert, dass der Rückbildungsprozess wahrscheinlich durch Veränderungen von verfügbaren Proteinen durchgeführt wird, ohne die Induzierung von Proteinneusynthese. Untersuchungen auf ultrastruktureller Ebene zeigten, dass es während der Rückbildung zur Formation von drei unterschiedlichen Mitochondrientypen kam, die sich in ihrer Morphologie stark unterschieden. Weiterhin wurden vergleichende Studien zur Bildung der Megamitochondrien durchgeführt, bei denen der Einfluss von Atmungsketten-Inhibitoren auf die Bildung von Milchsäure-induzierten Riesenorganellen untersucht wurde. Die Resultate deuten für die Megamitochondrieninduktion auf eine Abhängigkeit auf ein intaktes Membranpotential hin. Immunzytochemisch wurde die endogene Lokalisation der mitochondrialen Fusions- und Fissionsproteine Mitofusin 2, hFis1 und Drp1/DNM1L am Modellsystem der Megamitochondrieninduktion aufgeklärt. Es zeigte sich, dass diese Proteine punktförmig an der äußeren Membran der Riesenorganellen lokalisieren Um das Modellsystem an lebenden Zellen zu nutzen, wurden Vektoren konstruiert, die fluoreszenzmarkierte Proteine der mitochondrialen Fusions- und Fissionsmaschinerie exprimierten. Hiermit konnte einerseits die Lokalisation von Mitofusin 1, Mitofusin 2, hFis1 und Drp1/DNM1L in lebenden Zellen nach Induktion der Megamitochondrien analysiert werden und andererseits der Einfluss der Überexpression dieser Proteine auf die Bildung der Riesenorganellen dokumentiert werden. Die Ergebnisse machten deutlich, dass nur die Überepxression von hFis1 die Bildung der Megamitochondrien verhinderte. Ein weiterer Schwerpunkt der vorliegenden Arbeit lag in der Visualisierung und Dynamik mitochondrialer Nucleoids in lebenden Zellen. Nucleoids sind Protein-DNA-Komplexe, in denen mitochondriale Genome organisiert sind. Mit dem Farbstoff PicoGreen gelang es mtDNA in lebenden Zellen zu färben und Dynamikstudien der punktförmigen Strukturen mikroskopisch festzuhalten. Während sich mtDNA im mitochondrialen Netzwerk nur marginal aufgrund stattfindender Fusions- und Fissionsereignisse bewegte kam es in den Milchsäure-induzierten Megamitochondrien zu einer extensiven und extrem schnellen Bewegung von mitochondrialer DNA. In anschließenden Versuchen wurde der mitochondriale Transkriptions- und Verpackungsfaktor TFAM als fluoreszentes Fusionsprotein in Zellen transfiziert und Kolokalisationsstudien zeigten, dass das Fusionsprotein mit mtDNA kolokalisiert. In den Riesenorganellen präsentierten punktförmige TFAM-gefärbte Nucleoids ein sehr dynamisches Verhalten mit schneller Bewegung. In rho0-Zellen ohne mitochondriale DNA war die TFAM-Fluoreszenz hingegen gleichmäßig verteilt. Ein weiterer Nucleiodbestandteil ist das mitochondriale DNA-Einzelstrangbindeprotein SSBP1, welches in Megamitochondrien ebenso ein sehr dynamisches Verhalten aufwies. Eine mitochondrial-zielgesteuerte und EGFP-markierte Restriktionsendonuklease wies ebenfalls das typische, punktförmige Nucleoidmuster im mitochondrialen Netzwerk auf, was auf eine Interaktion mit der mtDNA schließen lässt. In rho0-Zellen ohne mtDNA kam es jedoch zur gleichmäßigen Verteilung des Konstruktes in den Mitochondrien. Zusammenfassend wurden in dieser Arbeit sowohl Einblicke in die Biologie der Megamitochondrien gewonnen, als auch Erkenntnisse über die Dynamik mitochondrialer Protein-DNA-Komplexe, wobei der Schwerpunkt hierbei auf einer Analyse mit Hilfe optischer Methoden lag. N2 - During the cultivation of rho0 cells, which are devoid of mitochondrial DNA (mtDNA), excessive endogenous lactic acid production during the fermentation process drives the development of megamitochondria. These giant organelles are formed by mitochondrial fusion events and/or the repression of fission. Megamitochondria formation is inducible in cells containing mtDNA by an artificial acidification of the culture medium by lactic acid. This work exploits these findings in order to investigate mitochondrial fusion and fission events. Fusion of mitochondrial matrix compartments was examined with the aid of the photoactivatable variant of the green fluorescent protein (PA-GFP), showing that the mixing of matrix components after fusion is an extremely fast process. Formation and reversion of megamitochondria was analyzed by confocal and electron microscopy, revealing that the matrix of giant organelles contains only rudiment structures of cristae organization. Reversion of the megamitochondria to a normal network displays fast kinetic characteristics. This indicates that the restoration process most likely is performed by alterations of novel protein expression. Additional assessment on an ultrastructural level displayed the occurrence of three different types of mitochondria during the reversion, which strongly differed in their morphology. To gain insights into the mechanism of megamitochondria formation and reversion comparative studies were performed with various inhibitors of the respiratory chain. The results indicated a dependence on an intact membrane potential for the induction of megamitochondria. Localization of the endogenous mitochondrial fusion and fission proteins mitofusin 1, hFis1 and Drp1/DNM1L were analyzed in megamitochondria by immunocytochemistry, demonstrating that these proteins localize foci-like to the outer membrane of the giant organelles. Fluorescently tagged proteins of the mitochondrial fusion and fission apparatus (mitofusin 1, mitofusin 2, hFis1 and Drp1/DNM1L) were used in localization and overexpression experiments in living cells by transient transfection. The results revealed that only the overexpression of hFis1 inhibited the formation of megamitochondria. Another main focus of this thesis was the visualization and dynamics of mitochondrial nucleoids in living cells. Nucleoids are protein-DNA complexes representing organizational units for the mitochondrial genomes The dye PicoGreen was used to stain mtDNA in living cells and the dynamics of nucleoid movement was analyzed by fluorescent and confocal microscopy. While mitochondrial DNA showed only marginal movements due to ongoing fusion and fission events in a mitochondrial network, an extensive and extremely fast movement in the lactic acid-induced megamitochondria could be observed. In subsequent experiments the mitochondrial transcription and packaging factor TFAM was fluorescently tagged and transfected into cells. Colocalization studies showed that this fusion protein colocalizes with mitochondrial DNA. In the giant organelles foci-like TFAM-stained nucleoids displayed a very dynamic performance with fast movement. However, in rho0 cells without mitochondrial DNA the TFAM-fluorescence was uniformly distributed. An additional nucleoid constituent and marker for mitochondrial DNA is the mitochondrial single-stranded DNA-binding protein SSBP1, and it could be shown that SSBP1 also exhibits very dynamic characteristics in megamitochondria. A mitochondrial-targeted and EGFP-tagged restriction endonuclease also exhibited the typical, punctual nucleoid pattern in the mitochondrial network, suggesting an mtDNA interaction. In rho0 cells, however, the construct was uniformly distributed in the mitochondrial matrix. In summary, in the present thesis optical and mechanistic insights into the biology of megamitochondria were obtained. This approach was further exploited to study the dynamics of mitochondrial protein-DNA complexes with optical methods. KW - Mitochondrium KW - Cytologie KW - Mitochondrien KW - mitochondria Y1 - 2008 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-30467 ER - TY - THES A1 - Kukat, Alexandra T1 - Mitochondriale Fusions- und Fissionsvorgänge am Modellsystem von Mega-Mitochondrien einer rho0-Zelllinie T1 - Mitochondrial fusion and fission on the model system of megamitochondria of a rho0 cell line N2 - Viele Funktionen der Mitochondrien basieren auf Prozessen, an denen sowohl mitochondriale wie auch kernkodierte Genprodukte beteiligt sind. Durch zahlreiche Interaktionen ist der Einfluss dieser Einzelkomponenten auf das zelluläre System oftmals nur schwierig erkennbar. Mit Hilfe von rho0 -Zellen, deren Mitochondrien über kein eigenes Genom mehr verfügen, kann die mitochondriale Genkomponente ausgeschlossen werden. Im Rahmen dieser Arbeit wurden zunächst die metabolischen, proliferativen und morphologischen Eigenschaften einer rho0-Zelllinie 143B.TK-K7 untersucht, welche durch die Expression einer mitochondrial zielgesteuerten Restriktionsendonuklease hergestellt wurde. Während der Kultivierung bilden sich im Zytoplasma der 143B.TK-K7-Zellen mit fortlaufender Kultivierungszeit und zunehmenden Azidifizierung des Mediums Mega-Mitochondrien. Diese entstehen sowohl durch zahlreiche Fusionsereignisse als auch einem Schwellen durch vermehrten Wassereinfluss in die Mitochondrienmatrix. Alle Mitochondrien liegen dann als große kugelförmige Strukturen in der Zelle vor und nehmen somit die geringste Oberfläche zu einem vorhandenen Volumen ein. Die Entstehung der Mega-Mitochondrien ist dabei abhängig von einer hohen Protonenkonzentration zusätzlich zu einer ausreichend großen Menge an Laktat im Medium (Milchsäure). Zudem zeigt sich, dass auch in Zellen, welche noch ein mitochondriales Genom besitzen, durch diese Bedingungen die Bildung von Mega-Mitochondrien induziert werden kann. Bei der Entstehung der Mega-Mitochondrien handelt es sich zunächst nicht um apoptotische Vorgänge, da durch den Austausch des aziden Mediums eine äußerst schnelle Rückbildung in ein, den rho0-Zellen ähnliches Mitochondriennetzwerk erfolgt. Metabolische Untersuchungen zeigen, dass für die Rückbildung der Mega-Mitochondrien zu einem Netzwerk ausschließlich die im Medium vorhandene Protonenkonzentration ausreichend gering sein muss. Durch immunzytochemische Untersuchungen wurde deutlich, dass sowohl das mitochondriale Fusionsprotein MFN2 wie auch das Fissionsprotein DNM1L während der Entstehung und auch Rückbildung der Mega-Mitochondrien in punktförmigen Bereichen an der äußeren Mitochondrienmembran lokalisieren. Um zu überprüfen, ob die Bildung der Mega-Mitochondrien durch einer Überexpression von Proteinen der Fissionsmaschinerie verhindert wird, wurden PAGFP- bzw. EGFP-Fusionsproteine mit hFis1 und DNM1L hergestellt und in die 143B.TK-K7-Zellen transfiziert. Dabei führt eine verstärkte Expression von hFis1 zu aggregierten Mitochondrien, welche zwar anschwellen, nach einem Mediumwechsel jedoch trotzdem bestehen bleiben. Eine Überexpression von DNM1L hat keinen Einfluss auf die Entstehung und Rückbildung der Mega-Mitochondrien. Durch Inhibierung des Tubulin- bzw. Aktin-Zytoskeletts, konnte gezeigt werden, dass eine Zerstörung des Tubulin-Zytoskeletts auf die Entstehung und Rückbildung der Mega-Mitochondrien keine Auswirkungen hat. Die Untersuchungen zu dem Einfluss des Aktin-Zytoskeletts zeigen, dass die Mega-Mitochondrien ringförmig von dem Aktin-Zytoskelett umgeben sind. Mit Hilfe von Fluoreszenzprotein-Markern für die äußere und innere Mitochondrienmembran wurden die Mega-Mitochondrien als Modellsystem für mitochondriale Fusions- und Fissionsstudien verwendet. Somit konnte in der vorliegenden Arbeit mitochondriale Fusion und Fission zum ersten Mal an lebenden Zellen direkt beobachtet werden und führte nachfolgend zu der Einteilung von Fusionsvorgängen der Mitochondrien in einen Modus 1, bei dem eine zeitlich gekoppelte vollständige Fusion von sowohl äußerer wie auch innerer Membran geschieht und einen Modus 2, bei dem die Fusion der äußeren Membranen ohne die Fusion der inneren Membranen erfolgt. In ähnlicher Weise kann die Fission von Mitochondrien unterteilt werden. In einem als Modus 1 bezeichneten Mechanismus beginnt die Rückbildung der Mega-Mitochondrien zunächst mit einer Tubulierung der Mitochondrien hin zu langen Mitochondrienschläuchen, die einen nur geringen Durchmesser besitzen. Erst dann treten vermehrt zeitlich sehr schnell ablaufende Fissionsvorgänge auf. Zusätzlich wurde ein Modus 2-Mechanismus der Fission beobachtet, welcher aus einer unvollständigen Fusion resultiert, bei dem die inneren Membranen noch nicht miteinander verschmolzen sind. Auf elektronenmikroskopischer Ebene finden während der Mega-Mitochondrien-Bildung drastische Veränderung von zwiebelringartigen Cristae hin zu einer Abnahme von inneren Membranstrukturen und der elektronendichte im Matrixraum statt. Somit ist im Rahmen dieser Arbeit zum ersten Mal eine optische Beobachtung sowohl dieser Bewegungen wie auch von Fusions- und Fissionsprozessen und deren zeitlich Auflösung in vivo mit Hilfe der Mega-Mitochondrien gelungen. N2 - A variety of mitochondrial features are based on processes involving mitochondrially encoded as well as nuclear encoded gene products. By means of these manifold interactions it is difficult to discern the influences of the single components. One effort to overcome these difficulties was the development of cells devoid of endogenous mtDNA (so called rho0 cells) and therefore to exclude the mitochondrial genetic component. The aim of this thesis was the investigation of the metabolic, proliferative and morphologic characteristics of a rho0 cell line (143B.TK-K7) based on a 143B.TK- background. This cell line was developed by the expression of a mitochondrially targeted restriction endonuclease. During the cultivation and proceeding acidification of the culture medium by lactic acid megamitochondria developed in the cytoplasm of the 143B.TK-K7 cells. These megamitochondria form both by multiple fusion events and an additional increase in water influx into the matrix. All mitochondria then exist as large spherical structures with diameters of up to 7 µm and therefore receive the smallest surface area to a given volume. The formation of megamitochondria is dependent on a high proton production level additional to a sufficient amount of lactate (lactic acid) in the medium. Furthermore it is possibly to induce megamitochondria in cells still possessing a mitochondrial genome by these conditions. The formation of megamitochondria is not a sign of apoptotic processes per se, because the back-formation of the megamitochondria into a rho0-like network can be induced very fast by the exchange of the acidulated medium. Initial deformations of the megamitochondria are followed by tubulation in progressive mitochondria tubules and numerous fission events. Metabolic analyses show that this backformation only depends on a sufficient low concentration of protons in the medium. When the given threshold is not being traversed the megamitochondria persist. Immunocytological investigations both of the fusion protein MFN2 and the protein of the fission machinery DNM1L demonstrate a constant mitochondrial distribution in focal regions of the outer mitochondrial membrane during formation as well as back-formation of megamitochondria. By overexpressing the fission proteins hFis1 and DNM1L respectively in 143B.TK-K7 cells, it should be tested whether or not megamitochondria develop. The enhanced expression of hFis1 led to the formation of aggregated mitochondria that indeed swell but persist after changing the medium. The overexpression of DNM1L has no influence on the formation as well as the back-formation of the megamitochondria. Incubation of the cells with inhibitors for the tubulin respectively actin cytoskeleton evidenced that the destruction of the tubulin cytoskeleton has no consequence for the formation and back-formation of megamitochondria. Unclear results were obtained with inhibitors of the actin cytoskeleton probably due to secondary effects of the inhibitors to the cells. However the findings showed that the megamitochondria are embedded into the actin cytoskeleton. Additionally the megamitochondria were used as a model system for mitochondrial fusion and fission events. For this purpose fluorescent protein markers for the inner and outer mitochondrial membrane were created. With these tools it was possible to observe directly mitochondrial fusion and fission in living cells by confocal microscopy. Furthermore this led to the classification of fusion processes of the mitochondria in a mode 1 with temporally coupled fusion of outer and inner membrane and a mode 2 where the fusion of outer membrane occurs independent of the inner membrane fusion. In a similar way the fission of mitochondria can be sub-classified: mode 1 is featured during the back-formation of megamitochondria by increasing tubulation events in long mitochondrial tubules with thin diameters. Only at this point very fast fission events could be observed. Furthermore in a fission mode 2 that results from an incomplete fusion of inner mitochondrial membranes, the outer membrane invaginates from one side along the unfused inner membranes until two separate mitochondrial units exist. During the megamitochondria formation on electron microscopic level drastic changes occur from fuzzy onion like structures to a decrease of inner membranes and electron density in the matrix. Additionally inversions and inclusions consisting of one membrane and also double membranes are evident. Comparisons with confocal microscopy images show that these inclusions apparently accomplish undirected movements with high velocity. In the present thesis it was possible to observe for the first time these movements as well as mitochondrial fusion and fission in living cells with an outstanding optical and temporal resolution. KW - Mitochondrium KW - Spaltung KW - Verschmelzung KW - Mitochondrien KW - rho0 KW - mitochondria KW - rho0 Y1 - 2007 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-26484 ER - TY - JOUR A1 - Janz, Anna A1 - Walz, Katharina A1 - Cirnu, Alexandra A1 - Surjanto, Jessica A1 - Urlaub, Daniela A1 - Leskien, Miriam A1 - Kohlhaas, Michael A1 - Nickel, Alexander A1 - Brand, Theresa A1 - Nose, Naoko A1 - Wörsdörfer, Philipp A1 - Wagner, Nicole A1 - Higuchi, Takahiro A1 - Maack, Christoph A1 - Dudek, Jan A1 - Lorenz, Kristina A1 - Klopocki, Eva A1 - Ergün, Süleyman A1 - Duff, Henry J. A1 - Gerull, Brenda T1 - Mutations in DNAJC19 cause altered mitochondrial structure and increased mitochondrial respiration in human iPSC-derived cardiomyocytes JF - Molecular Metabolism N2 - Highlights • Loss of DNAJC19's DnaJ domain disrupts cardiac mitochondrial structure, leading to abnormal cristae formation in iPSC-CMs. • Impaired mitochondrial structures lead to an increased mitochondrial respiration, ROS and an elevated membrane potential. • Mutant iPSC-CMs show sarcomere dysfunction and a trend to more arrhythmias, resembling DCMA-associated cardiomyopathy. Background Dilated cardiomyopathy with ataxia (DCMA) is an autosomal recessive disorder arising from truncating mutations in DNAJC19, which encodes an inner mitochondrial membrane protein. Clinical features include an early onset, often life-threatening, cardiomyopathy associated with other metabolic features. Here, we aim to understand the metabolic and pathophysiological mechanisms of mutant DNAJC19 for the development of cardiomyopathy. Methods We generated induced pluripotent stem cell-derived cardiomyocytes (iPSC-CMs) of two affected siblings with DCMA and a gene-edited truncation variant (tv) of DNAJC19 which all lack the conserved DnaJ interaction domain. The mutant iPSC-CMs and their respective control cells were subjected to various analyses, including assessments of morphology, metabolic function, and physiological consequences such as Ca\(^{2+}\) kinetics, contractility, and arrhythmic potential. Validation of respiration analysis was done in a gene-edited HeLa cell line (DNAJC19tv\(_{HeLa}\)). Results Structural analyses revealed mitochondrial fragmentation and abnormal cristae formation associated with an overall reduced mitochondrial protein expression in mutant iPSC-CMs. Morphological alterations were associated with higher oxygen consumption rates (OCRs) in all three mutant iPSC-CMs, indicating higher electron transport chain activity to meet cellular ATP demands. Additionally, increased extracellular acidification rates suggested an increase in overall metabolic flux, while radioactive tracer uptake studies revealed decreased fatty acid uptake and utilization of glucose. Mutant iPSC-CMs also showed increased reactive oxygen species (ROS) and an elevated mitochondrial membrane potential. Increased mitochondrial respiration with pyruvate and malate as substrates was observed in mutant DNAJC19tv HeLa cells in addition to an upregulation of respiratory chain complexes, while cellular ATP-levels remain the same. Moreover, mitochondrial alterations were associated with increased beating frequencies, elevated diastolic Ca\(^{2+}\) concentrations, reduced sarcomere shortening and an increased beat-to-beat rate variability in mutant cell lines in response to β-adrenergic stimulation. Conclusions Loss of the DnaJ domain disturbs cardiac mitochondrial structure with abnormal cristae formation and leads to mitochondrial dysfunction, suggesting that DNAJC19 plays an essential role in mitochondrial morphogenesis and biogenesis. Moreover, increased mitochondrial respiration, altered substrate utilization, increased ROS production and abnormal Ca\(^{2+}\) kinetics provide insights into the pathogenesis of DCMA-related cardiomyopathy. KW - cell biology KW - molecular biology KW - dilated cardiomyopathy with ataxia KW - genetics KW - metabolism KW - mitochondria KW - OXPHOS KW - ROS KW - contractility Y1 - 2024 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350393 SN - 2212-8778 VL - 79 ER - TY - INPR A1 - Hennig, Thomas A1 - Prusty, Archana B. A1 - Kaufer, Benedikt A1 - Whisnant, Adam W. A1 - Lodha, Manivel A1 - Enders, Antje A1 - Thomas, Julius A1 - Kasimir, Francesca A1 - Grothey, Arnhild A1 - Herb, Stefanie A1 - Jürges, Christopher A1 - Meister, Gunter A1 - Erhard, Florian A1 - Dölken, Lars A1 - Prusty, Bhupesh K. T1 - Selective inhibition of microRNA processing by a herpesvirus-encoded microRNA triggers virus reactivation from latency N2 - Herpesviruses have mastered host cell modulation and immune evasion to augment productive infection, life-long latency and reactivation thereof 1,2. A long appreciated, yet elusively defined relationship exists between the lytic-latent switch and viral non-coding RNAs 3,4. Here, we identify miRNA-mediated inhibition of miRNA processing as a novel cellular mechanism that human herpesvirus 6A (HHV-6A) exploits to disrupt mitochondrial architecture, evade intrinsic host defense and drive the latent-lytic switch. We demonstrate that virus-encoded miR-aU14 selectively inhibits the processing of multiple miR-30 family members by direct interaction with the respective pri-miRNA hairpin loops. Subsequent loss of miR-30 and activation of miR-30/p53/Drp1 axis triggers a profound disruption of mitochondrial architecture, which impairs induction of type I interferons and is necessary for both productive infection and virus reactivation. Ectopic expression of miR-aU14 was sufficient to trigger virus reactivation from latency thereby identifying it as a readily drugable master regulator of the herpesvirus latent-lytic switch. Our results show that miRNA-mediated inhibition of miRNA processing represents a generalized cellular mechanism that can be exploited to selectively target individual members of miRNA families. We anticipate that targeting miR-aU14 provides exciting therapeutic options for preventing herpesvirus reactivations in HHV-6-associated disorders like myalgic encephalitis/chronic fatigue syndrome (ME/CFS) and Long-COVID. KW - Herpesvirus KW - HHV-6 KW - miRNA processing KW - miR-30 KW - mitochondria KW - fusion and fission KW - type I interferon KW - latency KW - virus reactivation Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-267858 UR - https://doi.org/10.21203/rs.3.rs-820696/v1 ET - submitted version ER - TY - JOUR A1 - Goos, Carina A1 - Dejung, Mario A1 - Janzen, Christian J. A1 - Butter, Falk A1 - Kramer, Susanne T1 - The nuclear proteome of Trypanosoma brucei JF - PLoS ONE N2 - Trypanosoma brucei is a protozoan flagellate that is transmitted by tsetse flies into the mammalian bloodstream. The parasite has a huge impact on human health both directly by causing African sleeping sickness and indirectly, by infecting domestic cattle. The biology of trypanosomes involves some highly unusual, nuclear-localised processes. These include polycistronic transcription without classical promoters initiated from regions defined by histone variants, trans-splicing of all transcripts to the exon of a spliced leader RNA, transcription of some very abundant proteins by RNA polymerase I and antigenic variation, a switch in expression of the cell surface protein variants that allows the parasite to resist the immune system of its mammalian host. Here, we provide the nuclear proteome of procyclic Trypanosoma brucei, the stage that resides within the tsetse fly midgut. We have performed quantitative label-free mass spectrometry to score 764 significantly nuclear enriched proteins in comparison to whole cell lysates. A comparison with proteomes of several experimentally characterised nuclear and non-nuclear structures and pathways confirmed the high quality of the dataset: the proteome contains about 80% of all nuclear proteins and less than 2% false positives. Using motif enrichment, we found the amino acid sequence KRxR present in a large number of nuclear proteins. KRxR is a sub-motif of a classical eukaryotic monopartite nuclear localisation signal and could be responsible for nuclear localization of proteins in Kinetoplastida species. As a proof of principle, we have confirmed the nuclear localisation of six proteins with previously unknown localisation by expressing eYFP fusion proteins. While proteome data of several T. brucei organelles have been published, our nuclear proteome closes an important gap in knowledge to study trypanosome biology, in particular nuclear-related processes. KW - Trypanosoma KW - gambiense KW - Trypanosoma brucei KW - proteomes KW - yellow fluorescent protein KW - mitochondria KW - protein structure KW - histones Y1 - 2017 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158572 VL - 12 IS - 7 ER - TY - JOUR A1 - Dudek, Jan A1 - Maack, Christoph T1 - Mechano-energetic aspects of Barth syndrome JF - Journal of Inherited Metabolic Disease N2 - Energy-demanding organs like the heart are strongly dependent on oxidative phosphorylation in mitochondria. Oxidative phosphorylation is governed by the respiratory chain located in the inner mitochondrial membrane. The inner mitochondrial membrane is the only cellular membrane with significant amounts of the phospholipid cardiolipin, and cardiolipin was found to directly interact with a number of essential protein complexes, including respiratory chain complexes I to V. An inherited defect in the biogenesis of cardiolipin causes Barth syndrome, which is associated with cardiomyopathy, skeletal myopathy, neutropenia and growth retardation. Energy conversion is dependent on reducing equivalents, which are replenished by oxidative metabolism in the Krebs cycle. Cardiolipin deficiency in Barth syndrome also affects Krebs cycle activity, metabolite transport and mitochondrial morphology. During excitation-contraction coupling, calcium (Ca\(^{2+}\)) released from the sarcoplasmic reticulum drives sarcomeric contraction. At the same time, Ca\(^{2+}\) influx into mitochondria drives the activation of Krebs cycle dehydrogenases and the regeneration of reducing equivalents. Reducing equivalents are essential not only for energy conversion, but also for maintaining a redox buffer, which is required to detoxify reactive oxygen species (ROS). Defects in CL may also affect Ca\(^{2+}\) uptake into mitochondria and thereby hamper energy supply and demand matching, but also detoxification of ROS. Here, we review the impact of cardiolipin deficiency on mitochondrial function in Barth syndrome and discuss potential therapeutic strategies. KW - Barth syndrome KW - respiratory chain KW - reactive oxygen species KW - cardiolipin KW - mitochondria Y1 - 2022 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-257512 VL - 45 IS - 1 ER - TY - THES A1 - De Lira, Maria Nathalia T1 - The regulation of T cell metabolism by neutral sphingomyelinase 2 T1 - Die Regulation des T-Zell-Metabolismus durch Neutrale Sphingomyelinase 2 N2 - T cells play an essential role in the immune system. Engaging the T cell receptor (TCR) initiates a cascade of signaling events that activates the T cells. Neutral sphingomyelinase (NSM) is a member of a superfamily of enzymes responsible for the hydrolysis of sphingomyelin into phosphocholine and ceramide. Sphingolipids are essential mediators in signaling cascades involved in apoptosis, proliferation, stress responses, necrosis, inflammation, autophagy, senescence, and differentiation. Upon specific ablation of NSM2, T cells proved to be hyper-responsive to CD3/CD28 co-stimulation, indicating that the enzyme acts to dampen early overshooting activation of these cells. It remained unclear whether a deregulated metabolic activity supports the hyper-reactivity of NSM2 deficient T cells. This work demonstrates that the ablation of NSM2 activity affects the metabolism of the quiescent CD4+ T cells. These accumulate ATP in mitochondria and increase basal glycolytic activity by increasing the basal glucose uptake and GLUT1 receptor expression, which, altogether, raises intracellular ATP levels and boosts cellular respiration. The increased basal metabolic activity is associated with rapid phosphorylation of S6, a mTORC1 target, as well as enhanced elevation total ATP levels within the first hour after CD3/CD28 costimulation. Increased metabolic activity in resting NSM2 deficient T cells does, however, not support sustained stimulated responses. While elevated under steady-state conditions and elevated early after co-stimulation in NSM2 deficient CD4+ T cells, the mTORC1 pathway regulating mitochondria size, oxidative phosphorylation, and ATP production is impaired after 24 hours of stimulation. Taken together, the absence of NSM2 promotes a hyperactive metabolic state in unstimulated CD4+ T cells yet fails to support sustained T cell responses upon antigenic stimulation without affecting T cell survival. N2 - T-Zellen spielen eine wesentliche Rolle im Immunsystem. Die Aktivierung des T-Zell-Rezeptors (TCR) löst eine Kaskade von Signalereignissen aus, die die T-Zellen aktivieren. Neutrale Sphingomyelinase (NSM) gehört zu einer Superfamilie von Enzymen, die für die Aufspaltung von Sphingomyelin in Phosphocholin und Ceramid verantwortlich sind. Sphingolipide sind wesentliche Mediatoren in Signalkaskaden, die an Apoptose, Proliferation, Stressreaktionen, Nekrose, Entzündung, Autophagie, Seneszenz und Differenzierung beteiligt sind. NSM2-depletierte T-Zellen erwiesen sich als hyper-reaktiv gegenüber CD3/CD28-Kostimulation, was darauf hinweist, dass das Enzym eine überschießende Aktivierung dieser Zellen dämpft. Es blieb unklar, ob die Hyperreaktivität NSM2-defizienter T-Zellen durch eine deregulierte Stoffwechselaktivität unterstützt wird. Diese Arbeit zeigt, dass NSM2-Insuffizienz den Metabolismus ruhender CD4+-T-Zellen beeinflusst: Diese akkumulieren ATP in Mitochondrien und zeigen eine erhöhte basale glykolytische Aktivität, die auf einer erhöhten Glukoseaufnahme und Expression des GLUT1-Rezeptors beruht und mit einer Erhöhung intrazellulärer ATP-Werte und gesteigerten Zellrespiration einhergeht. Aufgrund ihrer bereits erhöhten basalen metabolische Aktivität zeigen NSM2 defiziente T Zellen eine im Vergleich zu Kontrollzellen schnellere, effizientere Aktivierung nach Kostimulation, die sich in Phosphorylierung von S6, eines mTORC1 Targets, sowie erhöhtem ATP Spiegel manifestiert. Dies kann jedoch nicht aufrechterhalten werden:Die mTORC1-Aktivierung, die die Größe der Mitochondrien, die oxidative Phosphorylierung und die ATP-Produktion reguliert, unter stationären Bedingungen in NSM2-defizienten CD4+-T-Zellen erhöht ist, ist nach 24-stündiger Kostimulation beeinträchtigt. Insgesamt scheint die NSM2-Aktivität wesentlich für die Regulation der basalen metabolischen Aktivität ruhender T-Zellen und der Vermeidung überschiessender Antworten nach Kostimulation zu sein, jedoch ebenso wichtig für die dauerhafte Aufrechterhaltung des Aktivierungssignals zu sein. KW - T zellen KW - metabolism KW - t cell KW - NSM2 KW - mitochondria Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-215673 ER - TY - THES A1 - Czisch, Michael T1 - Die Rolle von Bcl-2 bei der UV- und TRAIL-induzierten Keratinozytenapoptose T1 - The role of Bcl-2 in UV- and TRAIL-induced keratinocyte apoptosis N2 - In Keratinozyten wird sowohl durch UVB als auch durch PUVA-Bestrahlung Apoptose induziert. Wir untersuchten die in Keratinozyten durch UVB, PUVA, UVA und Todesliganden wie TRAIL ausgelösten Apoptosewege näher. UVB und PUVA, nicht aber UVA-Bestrahlung lösen in vitro Keratinozytenapoptose aus. 2-4 h nach UVB beobachteten wir die Aktivierung von Caspasen. Nach PUVA setzt die Aktivierung von Caspasen wesentlich später ein, nämlich erst 12 h nach Bestrahlung. Passend dazu, ist ein Verlust des mitochondrialen Transmembranpotentials 6-8 h nach UVB und 12-14 h nach PUVA detektierbar. Die Überexpression des Proteins Bcl-2 verhindert den Verlust des mitochondrialen Transmembranpotentials und die Caspase-Aktivierung nach UVB, und vermittelt auch einen klonogen Schutz, unabhängig von der Bildung reaktiver Sauerstoffradikale. Im Gegensatz dazu verzögert es den Verlust des Transmembranpotentials und die Caspase-Aktivierung nach PUVA nur und verhindert sie nicht. PUVA-bestrahlte Zellen können sich nicht weiter teilen, sind also durch Bcl-2 nicht klonogen geschützt. N2 - An important response of keratinocytes to UVB or PUVA irradiation is the induction of apoptosis. In order to understand the apoptotic responses of keratinocytes, we compared UVB, PUVA, UVA irradiated and TRAIL-treated keratinocytes for the activation of major apoptosis signalling pathways. UVB and PUVA, but not UVA irradiation induced keratinocyte apoptosis in vitro. Activation of caspases was detectable within 2 – 4 h after UVB irradiation. Interestingly, caspase activation following PUVA was delayed, beginning by 12 hours post irradiation. In line, mitochondrial transmembrane potential (MTP) decreased 6 – 8 hours after UVB, whereas PUVA mediated MTP loss started only 12 - 14h post irradiation. Interestingly, Bcl-2 overexpression protected against UVB induced early MTP loss and caspase activation. Moreover, Bcl-2 also protected clonogenic survival following UVB irradiation independent of the UV-induced generation of reactive oxygen species. In marked contrast, although Bcl-2 delayed PUVA induced MTP loss and caspase activation, Bcl-2 overexpressing keratinocytes failed to protect clonogenic survival following PUVA. Interestingly, similar levels of ROS were produced by UVA and PUVA irrespective of the expression of Bcl-2, suggesting that ROS generation does not have a major role in PUVA induced activation of apoptosis signalling. We conclude that distinct pathways independent of caspases are employed to exert the cell death program in PUVA and UVB induced apoptosis. While PUVA-induced cell death overcomes Bcl-2 protected mitochondrial pathways of apoptosis, UVB induced cell death is dose-dependently protected by Bcl-2. Our data suggest that PUVA-induced DNA damage rather than ROS generation plays the key role for PUVA induced apoptosis. KW - Bcl-2 KW - Apoptose KW - UV KW - UVB KW - UVA KW - PUVA KW - Keratinozyten KW - HaCaT KW - TRAIL KW - Zytochrom c KW - Caspasen KW - ROS KW - Mitochondrium KW - Bcl-2 KW - apoptosis KW - UV KW - UVB KW - UVA KW - PUVA KW - keratinocytes KW - HaCaT KW - TRAIL KW - cytochrome c KW - caspases KW - reactive oxygen species KW - mitochondria Y1 - 2004 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-10903 ER - TY - JOUR A1 - Chen, Shasha A1 - Lotz, Christopher A1 - Roewer, Norbert A1 - Broscheit, Jens-Albert T1 - Comparison of volatile anesthetic-induced preconditioning in cardiac and cerebral system: molecular mechanisms and clinical aspects JF - European Journal of Medical Research N2 - Volatile anesthetic-induced preconditioning ( APC) has shown to have cardiac and cerebral protective properties in both pre-clinical models and clinical trials. Interestingly, accumulating evidences demonstrate that, except from some specific characters, the underlying molecular mechanisms of APC-induced protective effects in myocytes and neurons are very similar; they share several major intracellular signaling pathways, including mediating mitochondrial function, release of inflammatory cytokines and cell apoptosis. Among all the experimental results, cortical spreading depolarization is a relative newly discovered cellular mechanism of APC, which, however, just exists in central nervous system. Applying volatile anesthetic preconditioning to clinical practice seems to be a promising cardio- and neuroprotective strategy. In this review, we also summarized and discussed the results of recent clinical research of APC. Despite all the positive experimental evidences, large-scale, long-term, more precisely controlled clinical trials focusing on the perioperative use of volatile anesthetics for organ protection are still needed. KW - APC KW - ischemia-reperfusion injury KW - mitochondria KW - apoptosis Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-175509 VL - 23 IS - 10 ER - TY - JOUR A1 - Boltze, Johannes A1 - Kleinschnitz, Christoph A1 - Reymann, Klaus G. A1 - Reiser, Georg A1 - Wagner, Daniel-Christoph A1 - Kranz, Alexander A1 - Michalski, Dominik T1 - Neurovascular pathophysiology in cerebral ischemia, dementia and the ageing brain – current trends in basic, translational and clinical research JF - Experimental & Translational Stroke Medicine N2 - The 7th International Symposium on Neuroprotection and Neurorepair was held from May 2nd to May 5th, 2012 in Potsdam, Germany. The symposium, which directly continues the successful Magdeburg meeting series, attracted over 330 colleagues from 29 countries to discuss recent findings and advances in the field. The focus of the 2012 symposium was widened from stroke and traumatic brain injury to neurodegenerative diseases, notably dementia, and more generally the ageing brain. Thereby, emphasis was given on neurovascular aspects of neurodegeneration and stroke including the blood–brain barrier, recent findings regarding the pathomechanism of Alzheimer’s disease, and brain imaging approaches. In addition, neurobiochemical aspects of neuroprotection, the role of astrogliosis, the clinical progress of cell-based approaches as well as translational hurdles and opportunities were discussed in-depth. This review summarizes some of the most stimulating discussions and reports from the meeting. KW - translational research KW - small vessel disease KW - Alzheimer’s disease KW - cerebral ischemia KW - neurorepair KW - neuroprotection KW - vascular dementia KW - mitochondria KW - astrogliosis KW - in vivo imaging Y1 - 2012 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126679 VL - 4 IS - 14 ER - TY - JOUR A1 - Bartel, Karin A1 - Pein, Helmut A1 - Popper, Bastian A1 - Schmitt, Sabine A1 - Janaki-Raman, Sudha A1 - Schulze, Almut A1 - Lengauer, Florian A1 - Koeberle, Andreas A1 - Werz, Oliver A1 - Zischka, Hans A1 - Müller, Rolf A1 - Vollmar, Angelika M. A1 - Schwarzenberg, Karin von T1 - Connecting lysosomes and mitochondria – a novel role for lipid metabolism in cancer cell death JF - Cell Communication and Signaling N2 - Background The understanding of lysosomes has been expanded in recent research way beyond their view as cellular trash can. Lysosomes are pivotal in regulating metabolism, endocytosis and autophagy and are implicated in cancer. Recently it was discovered that the lysosomal V-ATPase, which is known to induce apoptosis, interferes with lipid metabolism in cancer, yet the interplay between these organelles is poorly understood. Methods LC-MS/MS analysis was performed to investigate lipid distribution in cells. Cell survival and signaling pathways were analyzed by means of cell biological methods (qPCR, Western Blot, flow cytometry, CellTiter-Blue). Mitochondrial structure was analyzed by confocal imaging and electron microscopy, their function was determined by flow cytometry and seahorse measurements. Results Our data reveal that interfering with lysosomal function changes composition and subcellular localization of triacylglycerids accompanied by an upregulation of PGC1α and PPARα expression, master regulators of energy and lipid metabolism. Furthermore, cardiolipin content is reduced driving mitochondria into fission, accompanied by a loss of membrane potential and reduction in oxidative capacity, which leads to a deregulation in cellular ROS and induction of mitochondria-driven apoptosis. Additionally, cells undergo a metabolic shift to glutamine dependency, correlated with the fission phenotype and sensitivity to lysosomal inhibition, most prominent in Ras mutated cells. Conclusion This study sheds mechanistic light on a largely uninvestigated triangle between lysosomes, lipid metabolism and mitochondrial function. Insight into this organelle crosstalk increases our understanding of mitochondria-driven cell death. Our findings furthermore provide a first hint on a connection of Ras pathway mutations and sensitivity towards lysosomal inhibitors. KW - lysosome KW - V-ATPase KW - mitochondria KW - fission KW - apoptosis KW - lipid metabolism KW - cardiolipin Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-221524 VL - 17 ER -