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Electron microscopy (EM) demarcates itself from other structural biology techniques by its applicability to a large range of biological objects that spans from whole cells to individual macromolecules. In single-particle cryo-EM, frozen-hydrated samples, prepared by vitrification with liquid ethane, retain macromolecules in a medium that approximates their natural aqueous environment and that, in this way, preserves high-resolution structural information. Nonetheless, the sensitivity of biological specimens to the high-energy electron beam introduces restrictions on the total dose that can be used during imaging while avoiding significant radiation damage. Consequently, the signal-to-noise ratio attained in each individual image is very low, and structures with high-resolution detail must be recovered by averaging thousands of projections in random orientations. This is achieved through the use of image processing algorithms capable of aligning and classifying particle images through the evaluation of cross-correlation functions between each particle and a reference.
In recent years, several innovations took place in the field of single-particle cryo-EM, among which the development of direct electron detectors must be highlighted. Direct electron detectors have a better detective quantum efficiency (DQE) than both photographic film and CCD cameras, and offer a fast readout, compatible with the acquisition of movie stacks. Additionally, new image processing software has become available, with more sophisticated algorithms and designed to take advantage of the specific characteristics of the movies produced with direct electron detectors. These technological advances in both hardware and software catalyzed a revolution in single-particle cryo-EM, which is now routinely used for the determination of near-atomic structures. As a result, the range of macromolecules accessible to cryo-EM has increased drastically, as targets that were unsuitable before for imaging due to their small dimensions can now be adequately visualized and refined to high-resolution.
During my doctoral work, I have used single-particle cryo-EM to structurally characterize challenging membrane proteins, with a strong emphasis on protein complexes from aerobic respiratory chains. In chapter I of this thesis, I present my results on the bovine respirasome, a mitochondrial supercomplex composed of complexes I, III and IV. Chapter II is dedicated to the analysis of the structure of alternative complex III (ACIII) from Rhodothermus marinus, a bacterial quinol:cytochrome c/HiPIP oxidoreductase unrelated to the canonical cytochrome bc1 complex (complex III). In addition, in chapter III I describe the structure of KimA, a high-affinity potassium transporter that drives the transport of its substrate by using the energy stored in the form of a proton gradient. These three membrane proteins, with molecular weights ranging from 140 kDa to 1.7 MDa, illustrate the possibilities and limitations faced in single-particle cryo-EM.
The aerobic respiratory chain is responsible for the generation of a transmembrane difference of electrochemical potential that is then used by ATP synthase for the production of ATP or for driving solute transport over the membrane. They catalyze the transfer of electrons from a substrate, such as NADH or succinate, to molecular oxygen and use the chemical energy released in these redox reactions to drive the translocation of protons, or in some cases sodium ions, to the intermembrane space in mitochondria or the periplasm in bacteria.
In mitochondria, the respiratory chain is composed of four complexes: complex I (NADH:ubiquinone oxidoreductase), complex II (succinate dehydrogenase), complex III (cytochrome bc1 complex) and complex IV (cytochrome c oxidase). While it was for a long time believed that these complexes existed as single entities in the membrane, the use of milder procedures for protein purification and analysis revealed that respiratory complexes associate into well-ordered structures, known as supercomplexes. These have been proposed to offer different structural and functional advantages that are still controversial, including substrate channeling, stabilization of individual complexes and reduction of reactive oxygen species (ROS) production. The most thoroughly studied respiratory supercomplex has been the respirasome, conserved in higher eukaryotes and composed of one copy of complex I, a complex III dimer and one complex IV. By single-particle cryo-EM analysis, I retrieved a 9 Å map of the respirasome from Bos taurus, which allowed the accurate docking of atomic models of the three component complexes. The structure shows that complex III associates to the concave side of the membrane arm of complex I, while complex IV is located between the end of the complex I hydrophobic arm and complex III. Several defined protein-protein contacts are observed between the component complexes, which are mediated predominantly by supernumerary subunits and close to the membrane surfaces. The interactions established between complex I and complex III are extensive and may support the argument that the association of complex I into supercomplexes is required for the stabilization or even the biogenesis of this complex.
...
The universal biological energy currency adenosine triphosphate (ATP) is synthesized by the F1Fo-ATP synthase in most living organisms. The overall structure and function of F-type ATPases is conserved in the different organisms. The F1Fo-ATP synthase consist of two domains; the soluble F1 complex has the subunit stoichiometry α3β3γδε and the membrane embedded Fo complex consists of subunits ab2c10-15 in its simplest form found in bacteria. F1 and Fo both function as reversible rotary motors that are connected by a central stalk (γε) and a peripheral stalk (b2δ).
For ATP synthesis, the electrochemical energy formed by a proton or sodium ion gradient is required. The ion translocation across the Fo subcomplex induces torque in the motor part of the enzyme (cnγε), which causes conformational changes in the α3β3 domain leading to ATP synthesis from ADP and inorganic phosphate (Pi) catalyzed in the β-subunits. ATP hydrolysis causes a reverse torque in the Fo subcomplex triggering uphill ion translocation from cytoplasm to periplasm, and the enzyme functions as an ion pump.
The ATP synthesis mechanism is well understood, since several high-resolution structures of F1 are available. In contrast, the ion translocation mechanism across the membrane, mediated by the Fo subcomplex, is not understood in its structural detail.
Subunit a and the c-ring form an ion pathway, but subunit b is needed to form an active ion translocation pathway in both H+- and Na+-dependent systems. Several high-resolution structures of c-rings have provided insights in the ion translocation mechanism. The different ion translocation models based on biochemical, biophysical and structural analysis are in agreement in the fact that ions are translocated through a periplasmic ion access pathway in subunit a to the middle of the membrane and there to the binding site of a c-subunit. After almost a whole rotation of the c-ring the ion returns into the a-c interface, where it can be released to the cytoplasm. In the different models the cytoplasmic access pathway has been proposed to be located in subunit a, at the a-c interface or within the c-ring. The driving force of torque generation has been proposed to be the pH gradient or membrane potential. Several biochemical studies show that a conserved arginine in helix four of subunit a (R226 in Ilyobacter tartaricus or R210 in Escherichia coli)plays a critical role in the ion translocation. The arginine has been proposed to function as an electrostatic separator between the cytoplasmic and periplasmic pathways and as a mediator of the ion exchange into the c-ring ion-binding site.
Structural data of a related enzyme (V1Vo-ATPase from Thermus thermophilus) has provided insight into the helical arrangement of the ion translocating subunits I and Lring (related to subunit a and the c-ring). These structures indicated a small interface between subunit I and the L-ring, and two four-helix bundles in the N-terminal domain of subunit I were proposed to build the periplasmic and cytoplasmic ion pathways. To comprehend the ion-translocation and torque generation mechanism in F1Fo-ATP synthase, structural data of an intact a-c complex is needed.
The goal of this work was to obtain structural data of subunit a, most preferably in a complex with the c-ring or additionally with subunit b. Therefore, a new purification procedure for the I. tartaricus Fo-subcomplex, heterologously expressed in E. coli cells, was established. The purified Fo was characterized biochemically and by Laserinduced liquid bead ion desorption mass spectrometry (LILBID-MS). These analyses showed that pure and completely assembled Fo containing all its subunits in the correct stoichiometry (ab2c11) was obtained. The purified Fo complex was stable at 4°C for several months and at room temperature in the presence of lipids for several weeks. A lipid analysis was performed by thin-layer chromatography (TLC) to investigate the qualitative lipid composition of I. tartaricus whole lipid extract and various I. tartaricus F1Fo isolates. The whole lipid extract contained PC, PG and PE lipids and probably cardiolipin. PC, PG and PE lipids were bound to wild type I. tartaricus F1Fo, whereas recombinant I. tartaricus F1Fo did not have any bound lipids, but was able to bind the synthetic lipids POPC and POPG if they were provided during the purification.
For subsequent structural studies the purified Fo was subjected to two-dimensional (2D) crystallization trials. Vesicles and sheets tightly packed with protein and crystals with a rare plane group for I. tartaricus c11 (p121) were obtained. The c-ring was visible in the CCD images, and immunogold-labeling revealed the presence of the His-tagged a-subunit in the reconstituted vesicles. Furthermore, atomic force microscopy (AFM) imaging showed protein densities next to the c-rings, which protruded less from the membrane (0.4±0.1 nm) than the c-ring (0.7±0.1 nm). These protein densities presumably belonged to subunit a.
Cryo-electronmicroscopy (cryo-EM) was used to collect data of the p121 crystals and a merged projection density map was calculated to 7.0 Å resolution. The unit cell of the crystals (81 × 252 Å) contained two asymmetric units with three c-rings in each and next to the c11-rings new prominent densities were visible. In each extra density up to 7 transmembrane helices were visible, belonging to the stator subunit a and/or subunit b. To elucidate whether there are conserved elements in the three extra densities non-crystallographic averaging was applied using a single-particle approach.
Six possible arrangements for the c-rings and the extra densities were identified and used for the averaging. The extra densities were enhanced only in one of the possible arrangements. The average showed a four-helix bundle and a fifth helix in close proximity to the c-ring. Two more helices were present in each position but their position was ambivalent. The data obtained in this work provides the first insight in the helical arrangement in the a-c interface of F1Fo-ATP synthase.
During my thesis, I worked on two different membrane proteins. One is a bacterial secondary transporter and the second is a human mitochondrial calcium channel.
The first part of my thesis involves the structural and biochemical characterization of an L-carnitine/ γ-butyrobetaine antiporter from bacteria called CaiT. The aim of the project was to understand the Na+ independence of CaiT and to determine the crystal structures of CaiT in different conformations to expand the mechanistic understanding of substrate/ product antiport in CaiT.
The study revealed how a positively charged amino acid side chain (arginine 262) in CaiT could structurally and functionally mimic a sodium ion. Additionally, various crystal structures of CaiT obtained in this study demonstrate that the central substrate-binding site is highly dynamic and can accommodate the substrate in various orientations.
In the second part of my thesis, I was able to optimize the expression and purification conditions for the human mitochondrial calcium uniporter or the MCU. Understanding how this channel functions can help us unravel the mechanism of calcium uptake by mitochondria. Secondary structure prediction analysis in combination with mass spectrometry of degraded MCU products obtained during the purification of the full-length protein led to the identification of a stable MCU construct. This study resulted in the successful purification of milligram quantities of stable MCU protein for the first time. Further optimization may be required to obtain more homogenous protein that is amenable for crystallization.
In der vorliegenden Dissertation stand die Aufklärung der Funktion und Regulation von p21 in der Mitose im Mittelpunkt. p21 ist als Cdk-Inhibitor und Schlüsselregulator bekannt, der in viele fundamentale zelluläre Prozesse involviert ist: Zellzyklusregulation, Apoptose, Seneszenz, Zellmigration und Dynamik des Zytoskeletts, Transkription, Differenzierung sowie DNA-Reparatur, aber auch in die Umprogrammierung induzierter pluripotenter Stammzellen (Besson et al. 2008; Abbas und Dutta 2009; Jung et al. 2010).
Die unkontrollierte Proliferation von Zellen ist mit der Tumorgenese assoziiert und wird unter anderem durch die Fehlregulation von p21, aber auch durch die wichtigen mitotischen Kinasen Cdk1, im Komplex mit ihrer regulatorischen Untereinheit Cyclin B1, sowie Plk1 bedingt. Zudem ist das Fehlen von p21 oder die Fehllokalisation in das Zytoplasma mit einer schlechteren Prognose für den Patienten und Chemotherapie-Resistenz von Tumoren verbunden (Abukhdeir und Park 2008). Aufgrund der zunehmenden Inzidenz und Mortalität von Krebserkrankungen ist es daher von besonderem klinischem Interesse, die molekularen Ursachen für die Entstehung maligner Tumorerkrankungen aufzuklären. Bislang existieren kaum Studien über welche molekularen Mechanismen die Funktionen von p21, dem wichtigsten Cdk-Inhibitor, der zum Beispiel durch die Anwendung niedermolekularer Inhibitoren wie BI 2536, das sich bereits in klinischen Phase II Studien befindet (Strebhardt 2010), beeinflusst wird, während der Mitose reguliert werden.
In der vorliegenden Dissertation wurde daher die physiologische Rolle des Cdk-Inhibitors bzw. Regulators p21 während der Mitose untersucht und mit der Kinaseaktivität von Cdk1/Cyclin B1, wie auch Plk1 korreliert. Es konnte gezeigt werden, dass p21 während der Mitose stark exprimiert wird und dass mitotisches p21 in verschiedenen Krebszelllinien unabhängig von dem p53-Status in einer phosphorylierten Form vorkommt, welche mit der Aktivität von Cdk1 und weniger mit der von Cdk2 assoziiert ist. Durch Untersuchungen der isogenen HCT116-Zelllinien mit und ohne p21 wurde aufgezeigt, wie wichtig p21 für den ordnungsgemäßen Ablauf der Mitose ist. Ohne p21 sind sowohl die Anaphase wie auch die Zytokinese verlängert, die Zellen ordnen die Chromosomen fehlerhaft in der Metaphaseplatte an (congression Fehler), besitzen weitaus mehr lagging Chromosomen und fast 20 % der Zellen weisen im Versuchsverlauf Polyploidie auf. Durch den Verlust des Cdk-Regulators p21 kommt es zur Fehlregulation von Cdk1 und seiner Substrate (wie MCAK) und es treten die oben beschriebenen Probleme auf.
Weiterhin phosphoryliert Cdk1/Cyclin B1 p21 an Ser-130 in vitro und ex vivo in der frühen Phase der Mitose, der Prophase bzw. Prometaphase. Die nicht phosphorylierbare p21 Form S130A befindet sich hauptsächlich im Zellkern und führt zu vermehrtem Auftreten von congression Fehlern, während die S130D-Mutante, die die Phosphorylierung durch Cdk1 vortäuscht, schneller degradiert wird und zudem den Phänotyp der HCT116 p21-/- Zellen verstärkt. Zellen, die S130D exprimieren, benötigen mehr Zeit für das Durchlaufen der Mitose. Hier ist vor allem die Metaphase stark verlängert, aber auch Anaphase und Zytokinese. Dies führt zu congression Fehlern und zu Polyploidie. Diese Ergebnisse bestätigen, wie wichtig die zeitlich korrekte Phosphorylierung von p21 und die dadurch vermittelte Aktivierung von Cdk1/Cyclin B1 ist.
Darüber hinaus stabilisiert die Suppression von Plk1 das p21 Protein, was darauf hinweist, dass die Degradation von p21 während der Prometaphase von Plk1 kontrolliert wird. Dies wird von der Tatsache unterstützt, dass Ser-114, wie auch Ser116 von Plk1 in vitro phosphoryliert wird. Die Deregulation von p21 durch Plk1, SS114/116AA bzw. SS114/116DD induziert Chromosomenfehler, wodurch die molekularen Mechanismen, warum fehlreguliertes Plk1 die Tumorgenese fördert, hervorgehoben werden.
Nach Abschluss der bisherigen Untersuchungen steht fest, dass man sich von der starren Rolle von p21 als Tumorsuppressor und Akteur während der G1/S-Phase lösen muss. Der Cdk-Inhibitor p21 trägt entscheidend zur mitotischen Progression bei, vor allem bedingt durch die zeitlich ordnungsgemäße Inaktivierung bzw. Aktivierung von Cdk1/Cyclin B1, der Kinase, die wiederum zahlreiche für die Mitose essentielle Proteine reguliert. In Zukunft muss zum besseren Verständnis der Rolle von p21 in der Mitose die genaue Abfolge der Ereignisse unter Einbeziehung der Degradationsmechanismen eingehender untersucht werden.
Rhabdomyosarcoma is the most common paediatric soft-tissue sarcoma, and for tumour recurrence, the prognosis is still unfavourable. The current standard therapy consisting of surgery, radiation and combined chemotherapy does not consider the specific biology of this tumour.
Histone deacetylases (HDACs) and the Lysine-specific demethylase-1 (LSD1) are two epigenetic modifiers which are both part of repressor complexes leading to transcriptional silencing of target genes. Whereas HDACs lead to deacetylation of several lysine-residues within the histone tail, LSD1 is specific for demethylation of H3K4me2 and H3K4me1, as well as in a different context for H3K9me2. Rhabdomyosarcoma is reported to harbour high levels of LSD1, but the functional relevance is yet unclear. HDAC inhibition proved to be effective as single agent treatment, however, the proximity of HDAC1/2 and LSD1 in repressor complexes at the DNA implies a suitable rationale for a combination therapy potentially leading to cooperative effects on target gene transcription. In this study, we aimed to evaluate the potential of a combined LSD1 and HDAC inhibition for cell death induction in rhabdomyosarcoma cell lines. Whereas LSD1 inhibitors failed to induce cell death on their own, the combined inhibition of HDACs and LSD1 resulted in highly synergistic cell death induction. This effect extended to several combinations of LSD1 and HDAC inhibitors as well as to four different rhabdomyosarcoma cell lines, two of embryonal and two of alveolar histology.
With the use of the HDAC inhibitor JNJ-26481585 and the reversible LSD1 inhibitor GSK690, we demonstrated that the cell death induced by the combination matches with the details of intrinsic mitochondrial apoptosis. JNJ-26481585/GSK690-induced cell death is partially caspase-dependent and leads to caspase cleavage, followed by substrate cleavage as shown for PARP, as well as loss of the mitochondrial membrane potential.
Furthermore, JNJ-26481585 and GSK690 acted together to transcriptionally upregulate the proapoptotic proteins NOXA, BIM and BMF, which resulted in respective changes on protein level for both cell lines. However, the antiapoptotic BCL-2 family proteins BCL-2, MCL-1 and BCL-xL displayed only minor changes in protein levels upon treatment with GSK690 and JNJ-26481585, which did not rely on transcriptional activity. Therefore, the increase in proapoptotic proteins induces a shift towards proapoptotic signalling at the mitochondrial membrane. This shift is functionally relevant since knockdown of a proapoptotic protein or overexpression of one of the antiapoptotic proteins BCL-2 and MCL-1, as well as a stabilized mutant MCL-1, can significantly protect from GSK690/JNJ-26481585-induced cell death.
Knockdown of the mitochondrial membrane protein BAK, which is directly guarding the mitochondrial membrane integrity, potently protected from GSK690/JNJ-26481585- induced cell death, directly linking the shift in the BCL-2 family proteins to the observed loss of mitochondrial membrane potential and the further downstream activation of caspases. Furthermore, treatment with JNJ-26481585 and GSK690 resulted in a cell cycle arrest in G2/M phase, indicating additional effects on the tumour cells beside apoptosis induction. Taken together, the combined inhibition of LSD1 and HDACs is a promising strategy for rhabdomyosarcoma treatment.
Im Rahmen dieser Arbeit sollte untersucht werden, ob eine Zellzyklusabhängigkeit der CD95- vermittelten Apoptose besteht. Dazu wurde ein ecdysoninduzierbares Genexpressionsystem für die induzierte Überexpression der CDK-Inhibitoren p21 und p27 in RKO-Zellen (Kolonkarzinomzellen) zur Herbeiführung eines Zellzyklusarrests in der G1-Phase benutzt. Nach Induktion mit dem Ecdysonhomolog Muristeron wurde durch Zugabe von rekombinanten hCD95-Liganden Apoptose ausgelöst und anschließend untersucht. Die erzielten Ergebnisse zeigen, dass der Induktor Muristeron an sich und nicht die p21- bzw. p27-Überexpression die anti-apoptotische Akt-Kinase aktiviert, die Expression des anti-apoptotischen Bcl-xL erhöht, die Caspase-8-Aktivierung (entweder am CD95-DISC oder durch "Feedback"-Aktivierung durch Caspase-3) und die darauf folgenden Ereignisse verhindert und somit die hCD95L-induzierte Apoptose blockiert. Zusätzlich beeinflusst der Induktor auch das Genexpressionsmuster der behandelten Zellen, was ebenfalls für die Hemmung der Apoptose mit verantwortlich sein könnte. Somit ist das ecdysoninduzierbare Genexpressionsystem zur Apoptoseuntersuchung in RKO-Zellen nicht verwendbar. Mit der Untersuchung des Apoptoseverhaltens proliferierender RKO-Zellen konnte gezeigt werden, dass überlebende Zellen nach hCD95L-Behandlung vermehrt in der G0/G1-Zellzyklusphase nachweisbar sind, während apoptotische (Caspase-3-positive) Zellen aus der G2/M-Phase heraus sterben. Allerdings weisen die apoptotischen Zellen kaum Cyclin B1 auf, ein für die G2-Phase wichtiges und typisches Cyclin. Somit bleibt die genaue Verknüpfung von Zellzyklusregulation und Apoptose auch nach diesen Analysen ungeklärt. In einem dritten Ansatz - Zellzyklusarrest durch Dichtearretierung - konnte eine Hemmung der CD95- vermittelten Apoptose in der arretierten Zellpopulation nachgewiesen werden. Allerdings sekretieren RKO-Zellen einen anti-apoptotischen Faktor in ihr Medium, dessen Konzentration und Wirkung mit größerer Zelldichte zunimmt und somit für die Protektion, unabhängig von Zellzyklusarrest oder Proliferation, verantwortlich ist. Konfluente und auch mit konditioniertem Medium behandelte RKO-Zellen zeigen im Vergleich zu dünn ausgesäten RKO-Zellen Veränderungen, die denen sehr ähnlich sind die beim Übergang einer epithelverankerten Zelle zu einer migrierenden Einzelzelle (EMT) auftreten. Beispielsweise verändert sich die Zusammensetzung des Zytoskeletts, die Zellen verlieren den Zell-Zell-Kontakt und lösen sich ab, bleiben aber am Leben. Zusätzlich steigt die Sekretion von Zytokinen an, die Angiogenese, Migration und Invasion positiv beeinflussen. Sowohl konfluente als auch mit konditioniertem Medium behandelte sub-konfluente Zellen sind apoptoseresistent (hCD95L, TRAIL, UV, Staurosporin), woran u.a. die Kinasen PKC und PI3K, aber auch das anti-apoptotische Bcl-xL beteiligt sind. Die Zellen sterben interessanterweise, wenn ein agonistischer anti-CD95-Antikörper statt des rekombinanten CD95-Liganden verwendet wird, was vermuten lässt, dass eine mangelhafte Vernetzung der einzelnen DISC-Komplexe zur Apoptosehemmung führt, welche durch den Antikörper dann aber erzwungen wird. Zwar handelt es sich hierbei um ein reines Zellkulturmodell, dennoch könnte es bedeuten, dass die Umgebung in einer dichten RKO-Zellkultur vergleichbar ist mit der in größeren soliden Tumoren. Die Zellen brauchen Nährstoffe, versuchen über eine Neovaskularisierung Anschluss an ein Blutsystem zu finden und sekretieren Lockstoffe, Wachstumsfaktoren sowie Proteasen, um die Metastasierung zu erleichtern. PI3K, cPKCs und Bcl-xL tragen dabei zu einer Apoptoseresistenz bei, welche die Zellen zum einen resistent gegenüber Anoikis, Nährstoffmangel, aber auch gegen angreifende zytotoxische T-Zellen macht. Eine weitere Aufklärung der hier ablaufenden Prozesse würde es erleichtern, Möglichkeiten zu finden, in diese Signalwege einzugreifen, um die Apoptosesensitivität wieder herzustellen und die Metastasierung zu verhindern. Insbesondere ist die Identifizierung des für die Apoptoseprotektion verantwortlichen Zytokins das nächste wichtige Ziel bei der Fortsetzung dieser Arbeiten.
Biomoleküle, insbesondere Membranproteine (MPs), sind oftmals sehr sensitiv gegenüber ihrer chemischen Umgebung, wie pH-Wert, Puffer, Salzkonzentration und vielen weiteren Faktoren. MPs stabil und funktional in Lösung zu halten ist nicht trivial. Sie stellen deshalb eine besondere Herausforderung bei der Analyse von biologischen Systemen dar. Aus diesem Grund wurden und werden nach wie vor sogenannte membrane mimicking-(MM-) Systeme, wie beispielsweise Nanodiscs (NDs) oder styrene-maleic acid lipid particles (SMALPs), untersucht und entwickelt, um MPs eine naturähnliche Umgebung in Form einer Lipid-Doppelschicht zu bieten und sie so in ihrer natürlichen Konformation und natürlichen Funktionsweise/Aktivität in Lösung zu halten.
Laser induced liquid bead ion desorption (LILBID) Massenspektrometrie (MS) hat sich als hervorragende analytische Methode herausgestellt, um MPs in Kombination mit MM-Systemen zu untersuchen. LILBID-MS bietet nicht nur die Möglichkeit Proteine an sich zu identifizieren, sondern ermöglicht ebenfalls eine zerstörungsfreie Analyse von nicht-kovalent gebundenen Proteinkomplexen, sowie die Detektion einzelner Subkomplexe eines Proteinkomplexes. Auch die Analyse von Protein-Ligand-Wechselwirkungen ist möglich. Bei der LILBID-Ionisationsmethode werden kleine Tröpfchen erzeugt, die einen wässrig gelösten Analyt enthalten. Die Analyt-Tröpfchen werden anschließend mittels IR-Laser bestrahlt, wodurch der Analyt freigesetzt und massenspektrometrisch analysiert werden kann.
Diese Dissertation beschäftigt sich zum einen mit der Analyse des Lyse-Proteins ΦX174-E der Bakteriophage ΦX174, zum anderen mit Untersuchungen zur Histidinkinase SpaK aus B. subtilis in Kombination mit MMs. Weiterhin wird die Frage geklärt, ob und wie gut sich LILBID-MS zur Analyse von Saposin-Nanopartikel-(SapNPs)-solubilisierten MPs eignet. Darüber hinaus wird in dieser Dissertation die Darstellung von SapNP-solubilisierten MPs mittels zellfreier Proteinsynthese näher charakterisiert und untersucht welche Parameter aus präparativer Sicht optimiert werden können.
In vorausgegangenen Analysen von ND-solubilisierten MPs mittels LILBID-MS zeigte sich, dass manche in Verbindung mit NDs genutzten Lipide unerwünschte Signale im Spektrum zur Folge haben, die aus massiven Lipid-Anhaftungen am MSP oder dem Analyten resultieren. Überlappungen der m/z-Signale verschiedener Analyt- und/oder Komplexkomponenten mit diesen Lipid-Cluster-Signalen kann wiederum zum Verlust von Informationen führen. Daher beschäftigt sich ein weiterer Teil dieser Arbeit mit der Frage, ob durch den Einsatz von UV-schaltbaren Lipiden der Anwendungsbereich und/oder die Auflösung von LILBID-MS erweitert und verbessert werden kann.
Um biologische Prozesse zu verstehen ist es ebenfalls wichtig die zeitlichen/kinetischen Aspekte einer Reaktion zu untersuchen/kennen, sowie molekulare Prozesse gezielt zu kontrollieren. Licht hat sich hierbei als ein hervorragendes Werkzeug in der Analytik, sowie in der molekularen Prozesskontrolle etabliert. Licht bietet den Vorteil sehr selektiv eingesetzt werden zu können und sowohl orts- als auch zeitaufgelöst Informationen liefern zu können. Das gezielte Triggern einer Reaktion oder einer Protein-Protein-Interaktion kann beispielsweise durch sog. photo-cleaving von photolabilen Schutzgruppen ermöglicht werden. Bisweilen bietet die native MS nur wenig Möglichkeiten schnelle Reaktionen zu analysieren und kinetische Informationen zu gewinnen. Daher beschäftigt sich ein weiterer Teil dieser Dissertation damit zu untersuchen, ob und wie sich lichtgesteuerte Reaktionen im LILBID-Ionisationsprozess induzieren und gegebenenfalls auch zeitlich analysieren und charakterisieren lassen können.
Mitochondria are important for cellular health and their dysfunction is linked to a variety of diseases, especially neurodegeneration. Thus, the renewal and degradation of dysfunctional mitochondria is crucial for the well-being of organisms. The selective digestion of damaged mitochondria via the lysosome (mitophagy), is the main pathway to do so.
In my dissertational work, I investigated the connection between protein misfolding, protein import into mitochondria and the degradation of mitochondria via mitophagy. Here, I present a new model for the initiation of mitophagy without collapse of the membrane potential. This model provides the link between protein import into mitochondria, stress signal transduction to the cytosol and the mitochondrial stress sensor PINK1. To comprehensively examine how mitophagy can be triggered, I performed a genome-wide CRISPR knockout screen utilizing the mitophagy reporter mitochondrial mKEIMA. Thereby, I observed numerous novel gene deletions that induce mitophagy. Prominently, I identified an accumulation of gene deletions of the protein import and of protein quality control factors. I validated several of those and examined HSPA9 (mitochondrial HSP70) and LONP1 (a mitochondrial matrix AAA protease) in more detail, regarding their effect on mitophagy and protein import. For this, I used an established fluorescence-based, mitochondrial-targeted EGFP, as well as a newly-developed pulsed-SILAC mass spectrometry approach (mePRODmt). Depletions of both genes resulted in reduced protein import and PINK1-dependent mitophagy. Strikingly, I did not observe any loss of mitochondrial membrane potential, which was hitherto believed to be essential for activation of PINK1-mediated mitophagy. Literature shows that certain mitochondrial stressors can also induce mitophagy without mitochondrial membrane depolarization, which I confirmed with my assays. Next, I characterized the impact of LONP1 and HSPA9 depletion, which are involved in proteostasis maintenance, and the mtHSP90 inhibitor GTPP on mitochondrial protein folding in more detail. GTPP treatment and LONP1 depletion both resulted in the accumulation of an insoluble protein fraction, as judged by proteomic analysis. This insoluble protein fraction enriched several components of the presequence translocase-associated motor PAM, including TIMM44. TIMM44 acts as a link between the translocon, the import pore of the inner mitochondrial membrane (TIM) complex and the PAM complex. Thus, I hypothesized that TIMM44 dissociates from the TIM complex upon protein folding stress, when it becomes part of the insoluble protein fraction. To validate this model, I measured the TIMM44 interactome upon proteostasis disturbance using proximity labeling. Indeed, interaction of TIMM44 with the import pore was almost completely abolished, explaining the loss of matrix-targeted import upon protein folding stress. From these findings, I reasoned that an import reduction mediated by the PAM complex would likely also inhibit the degradation of PINK1. Consistent with this hypothesis, I observed that mitophagy induced by HSPA9 or LONP1 deletion was prevented when PINK1 was genetically deleted. In comparison, non-processed PINK1 was stabilized on mitochondria in wild type cells when mitochondrial protein import was impaired. On this basis, I drew the conclusion that the loss of mitochondrial import was the stress signal, which leads to the stabilization of PINK1, as it could not be processed anymore via the inner mitochondrial membrane protease PARL. PINK1 auto-activates itself upon accumulation and signals to the cytosol that this mitochondrion is damaged. Mitophagy is subsequently initiated by the ubiquitin kinase activity of PINK1. As a result, the autophagy apparatus gets activated, damaged mitochondria are engulfed by a double membrane and removed via lysosomal digestion. This proposed model is, to the best of my knowledge, the first to provide an explanation for protein folding stress-induced and protein import inhibition-triggered mitophagy without mitochondrial depolarization. The model thus extends the PINK1/PARKIN-dependent mitophagy pathway to milder stresses and clears some of the open questions in the field. Furthermore, this work is also important, because protein misfolding stress and dysfunctional mitochondria are two hallmarks of neurodegeneration. In particular, mitochondrial protein import inhibition during Parkinson’s and Huntington disease might be driver of mitochondrial dysfunction. Hence, I hope and anticipate that the newly developed protein import method, mePRODmt, and the proposed model will be beneficial to further characterize underlying processes and to establish which factors prevent or drive these disorders on molecular level.
Solute carrier (SLC) are related to various diseases in human and promising pharmaceutical targets but more structural and functional information on SLCs is required to expand their use for drug design and therapy. The 7-transmembrane segment inverted (7-TMIR) fold was identified for the SLC families 4, 23 and 26 in the last decade thus detailed analysis of the structure function relationship of one of these families might also yield insights for the other two. SVCT1 and SVCT2 from the SLC23 family are sodium dependent ascorbic acid transporters in human but structural analysis of the SLC23 family is exclusively based on two homologs – UraA from E. coli and UapA from A. nidulans – yielding two inward-facing and one occluded conformation. In combination with outward-facing conformations from SLC4 transporters, and additional information from the SLC26 family, an elevator transport mechanism for all 7-TMIR proteins was identified but detailed mechanistic features of the transport remain elusive due to the lack of multiple conformations from individual transporters.
To increase the understanding of 7-TMIR protein structure and function in this study, the transport mechanism of SLC23 transporters was analyzed by two strategies including selection of alpaca derived nanobodies and synthetic nanobodies against UraA as prokaryotic model protein of the SLC23 family. The second strategy involved mutagenesis of UraA at functional relevant positions regarding the conformational change during transport. Therefore, available structures of 7-TMIR proteins and less related elevator transporters were analyzed and a common motif identified – the alpha helical inter-domain linkers. The proposed rigid body movement for transport in combination with the characteristic alpha helical secondary structure of the linkers connecting both rigid bodies led to the hypothesis of functional relevance of the linkers and a conformational hinge being located in close proximity to the linkers. These positions were identified and used to modulate the biophysical properties of the transporter. Mutagenesis at three relevant positions led to loss of transport functionality and these UraA variants could be recombinantly produced and purified to further examine the underlying mechanistic effects. The variants UraAG320P and UraAP330G from the periplasmic inter-domain linker showed increased dimerization and thermal stability as well as substrate binding in solution. The substrate affinity of UraAG320P was identified to be 5-fold higher compared to the wildtype. The solvent accessibility of the substrate binding site in UraAG320P and UraAP330G revealed reduced open probability that indicated an altered conformational space compared to UraAWT. This phenomenon was analyzed in more detail by differential hydrogen-deuterium exchange mass spectrometry and the results supported the hypothesis of a reduced open probability and gave further insights into the impact of the two mutations in the periplasmic inter-domain linker in UraA.
This thesis further presents strategies for phage display selection of nanobodies with epitope bias and a post selection analysis pipeline to identify nanobodies with desired binding characteristics. Thereby, whole cell transport inhibition highlighted periplasmic epitope binders and conformational selectivity. A cytoplasmic epitope could be identified by pulldown with inside-out membrane vesicles for one cytoplasmic side binder. Thermal stabilization analysis of the target protein in differential scanning fluorometry was performed in presence of two different nanobodies to identify simultaneous binding by additional thermal stabilization respectively competition by intermediate melting temperatures. Combination of epitope information with simultaneous DSF could be used to identify the stabilization of different UraA conformations by a set of binders and presents a general nanobody selection strategy for other SLCs. Synthetic nanobodies (sybodies) were also included in the analysis pipeline and Sy45 identified as promising candidate for co-crystallization that gave rise to UraAWT crystals in several conditions in presence or absence of uracil. Similar crystals could be obtained in combination with UraAG320P that were further optimized to gain structural information on this mutant. The structure was solved by molecular replacement and the model refined at 3.1 Å resolution confirming the cytoplasmic epitope of Sy45 as predicted by the selection pipeline. The stabilized conformation was inward-facing similar to the reported UapA structure but significantly different to the previously reported inward-facing structure of UraA. The structure further confirmed the structural integrity of the UraA mutant G320P. Despite the monomeric state of UraA in the structure, the gate domain aligned reasonably well with the gate domain of the previously published dimeric UraA structure in the occluded conformation and allowed detailed analysis of the conformational transition in UraA from inward-facing to occluded by a single rigid body movement. Thereby little movement in the gate domain of UraA was observed in contrast to a previously reported transport mechanism. Core domain rotation around a rotation axis parallel to the substrate barrier was found to explain the major part of conformational transition from inward-facing to occluded and experimentally supported the hypothesized mechanism by Chang et al. (2017). Additionally, the conformational hinge around position G320 in UraA could be identified as well as the impact of the backbone rigidity introduced by the highly conserved proline residue at position 330 in UraA on the conformational transition. This position was found to serve as anchoring point the inter-domain linker and determines the coordinated movement of inter-domain linker and core domain. The functional analysis further highlighted the requirement of alpha helical secondary structure within the inter-domain linker that serves as amphipathic structural entity that can adjust to changed core-gate domain distances and angles during transport by extension/compression or bending while preserving the rigid linkage.
The applied strategies to modulate the conformational space of UraA by mutagenesis at the hinge positions in the inter-domain linkers is transferrable to other transporters and might facilitate their structural and functional characterization.
Further, this study discusses the conformational thermostabilization of UraA that is based on increased melting temperatures upon restriction of its conformational freedom. The term ‘conformational thermostabilization’ introduced by Serrano-Vega et al. (2007) could be experimentally supported and the direct correlation between the conformational freedom and thermostabilization was qualitatively analyzed for UraA. The concept of conformational thermostabilization might help in characterization of other dynamic transport systems as well.
Ubiquitination is regarded as one of the key post-translational modifications in nearly all biological processes, endowed with numerous layers of complexity. Deubiquitinating enzymes (DUBs) dynamically counterbalance ubiquitination events by deconjugating ubiquitin signals from substrates. Dysregulation of the ubiquitin code and its negative regulators drive various pathologies, such as neurological disorders and cancer.
The DUB ubiquitin-specific peptidase 22 (USP22) is well-known for its essential role in the human Spt-Ada-Gcn5 acetyltransferase (SAGA) complex, mediating the removal of monoubiquitination events from Histone 2A and 2B (H2A and -B), thereby regulating gene transcription. In cancer, USP22 was initially described as a part of an 11-gene expression signature profile, predicting tumor metastasis, reoccurrence and death after therapy in a wide range of tumor cells. However, novel roles for USP22 have emerged recently, accrediting USP22 essential roles in regulating tumor development as well as apoptotic cell death signaling.
One of the hallmarks of cancer is the evasion of cell death, especially apoptosis, a form of programmed cell death (PCD). Necroptosis, a regulated form of necrosis, is regarded as an attractive therapeutic strategy to overcome apoptosis-resistance in tumor cells, although a profound understanding of the exact signaling cascade still remains elusive. Nevertheless, several ubiquitination and deubiquitination events are described in fine-tuning necroptotic signaling.
In this study, we describe a novel role for USP22 in regulating necroptotic cell death signaling in human tumor cell lines. USP22 depletion significantly delayed TNFa/Smac mimetic/zVAD.fmk (TBZ)-induced necroptosis, without affecting TNFa-induced nuclear factor-kappa B (NF-KB) signaling or TNFa-mediated extrinsic apoptosis. Intriguingly, re-expression of USP22 wildtype in the USP22 knockout background could re-sensitize HT-29 cells to TBZ-induced necroptosis, whereas re-constitution with the catalytic inactive mutant USP22 Cys185Ser did not rescue susceptibility to TBZ-induced necroptosis, confirming the USP22 DUB-function a pivotal role in regulating necroptotic cell death. USP22 depletion facilitated ubiquitination and unexpectedly also phosphorylation of Receptor-interacting protein kinase 3 (RIPK3) during necroptosis induction, as shown by Tandem Ubiquitin Binding Entities (TUBE) pulldowns and in vivo (de)ubiquitination immunoprecipitations. To substantiate our findings, we performed mass-spectrometric ubiquitin remnant profiling and identified the three novel USP22-regulated RIPK3 ubiquitination sites Lysine (K) 42, K351 and K518 upon TBZ-induced necroptosis. Further assessment of these ubiquitination sites unraveled, that mutation of K518 in RIPK3 reduced necroptosis-associated RIPK3 ubiquitination and additionally affected RIPK3 phosphorylation upon necroptosis induction. At the same time, genetic knock-in of RIPK3 K518R sensitizes tumor cells to TNFa-induced necroptotic cell death and amplified necrosome formation.
In summary we identified USP22 as a new regulator of TBZ-induced necroptosis in various human tumor cell lines and further unraveled the distinctive role of DUBs and (de)ubiquitination events in controlling programmed cell death signaling.