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This thesis demonstrates the advancement of PELDOR spectroscopy beyond its original design of distance measurements in order to disentangle a maximum amount of information additionally encoded in the PELDOR data. In particular, the successful synthesis of novel polynitroxide radicals is described as well as the extraction of the relative orientation of spin labels, conformational flexibility and the separation of dipolar and exchange coupling via orientation selective PELDOR measurements in combination with PESIM based simulations. Moreover, the method of PELDOR "Spin Counting" was experimentally validated.
In dieser Arbeit werden Untersuchungen über die Anwendbarkeit von vier Methoden zur selektiven Einführung von Radikalen in DNA vorgestellt. Hierzu wurde die EPR-Spektroskopie (Elektronen-paramagnetische Resonanz) benutzt. Die selektive Einführung und Erzeugung von Radikalen in DNA ist nötig, um J-Kopplungen in DNA zu untersuchen. Vor dem Fernziel der Bestimmung der Austauschkopplungskonstanten J in biradikalischer DNA und deren Korrelation mit der charge-transfer-Geschwindigkeitskonstanten kCT stellen diese Untersuchungen einen wichtigen Ausgangspunkt dar. Stabile aromatische Nitroxide. Simulationen von Raumtemperatur-CW-X-Band-EPRSpektren fünf verschiedener aromatischer Nitroxide, welche potentielle DNA-Interkalatoren sind, wurden durchgeführt. Die aromatischen Nitroxide zeigen aufgelöste Hyperfeinkopplungen, welche zu dem Schluss führen, dass die Spindichte in hohem Maße delokalisiert ist, was die Verwendung dieser Verbindungen zur Messung von J-Kopplungen in biradikalischer DNA erlaubt. Transiente Guanin-Radikale. Transiente Guanin-Radikale werden in DNA selektiv durch die Flash-Quench-Technik erzeugt, bei der optisch anregbare Ruthenium-Interkalatoren verwendet werden. Transiente Thymyl-Radikale aus UV-bestrahltem 4'-Pivaloyl-Thymidin. Es werden photoinduzierte Prozesse untersucht, welche durch Bestrahlung von Thymin-Nukleosiden, die an der 4’-Position die optisch spaltbare Pivaloyl-Gruppe tragen, erzeugt werden. Dieses Nukleosid wurde speziell dafür entworfen, um Elektronenlöcher in DNA zu injizieren. In dieser Arbeit wird gezeigt, dass diese Verbindung benutzt werden kann, um selektiv eine Thymin-Base zu reduzieren. Transiente Thymyl-Radikale erzeugt durch ein neuartig modifiziertes Thymin nach UV-Bestrahlung. Photoinduzierte Prozesse, welche durch Bestrahlung eines ähnlichen Thymidin-Nukleosids erzeugt wurden, werden hier untersucht. Dieses Thymidin- Nukleosid wurde modifiziert, indem die optisch spaltbare Pivaloyl-Gruppe an eine Seitenkette angehängt wurde, welche an der C6-Position der Thymin-Base sitzt. Die Thymin-Base wurde speziell dafür entworfen, um Elektronen in DNA zu injizieren. In dieser Arbeit wurde bestätigt, dass ein Überschuss-Elektron selektiv auf eine Thymin-Base transferiert werden kann.
In the first part of the present work (Chapter 3), EPR spectroscopy at different microwave frequencies, namely at 9 GHz (X-band), 34 GHz (Q-band) and 180 GHz (G-band), was employed to resolve the g-values and the HFCs of a putative radical intermediate involved in the reduction of benzoyl-CoA catalyzed by benzoyl-CoA reductase. In particular, the effect of 33S-labeling on the EPR line shape was studied at X- and Q-band frequencies in order to gain further evidence for a sulfur centered radical proposed to be the electron donor in the reduction or the aromatic ring of BCoA [I]. The spectral components observed at X-, Q- and G-band were overall consistent and showed at least three overlapping EPR signals. The signal postulated to be due to a disulfide radical anion showed no resolved g-values and a relaxation behaviour faster than expected for such a radical species. These observations together with the simulations suggest that the signal could arise from a radical exchange coupled to an [4Fe-4S] cluster located nearby. In the future, pulsed EPR and ENDOR spectroscopy on the 57Fe-labeled enzyme could help to solve this question. The potential of high-field ENDOR in combination with 13C- and 31P-labeling for investigating the structure at the active site in proteins could be verified in the studies of the ligation sphere of the cofactor Mn2+ in Ras as reported in Chapter 4 [2]. Therein, high-field ENDOR performed at 94 GHz (W-band) was used to detect the hyperfine interactions between the electron spin mainly located on the metal ion and the phosphorous nuclei of the bound GDP and GppNHp as well as the carbon nuclei of bound amino acids in the wild-type Ras protein and its oncogenic mutant G12V. These studies aimed at searching for an additional free phosphate ion or amino acid ligand bound to the metal center in the wild type GDP-bound protein with respect to its oncogenic mutant. Rom the 13C- and 31P-ENDOR spectra, the hyperfine couplings of directly bound amino acids and the bound nucleotides were compatible with the hyperfine couplings obtained from DFT calculations based on the crystal structure data. No differences in the 13C- and 31P-ENDOR spectra could be found for the wild-type GDP-bound protein in comparison to its oncogenic mutant in frozen solution. Therefore, no evidence for binding of an additional free phosphate ion or amino acid ligand in the wild-type GDP-bound protein was found. The distances between the detected nuclei and the meta1 ion were in agreement with the ones extracted from crystal structures reported in the literature. Future 35C1-ENDOR studies could clarify whether a chloride ion from the buffer solution could be the ligand replacing one water molecule in the wild type GDP-bound Ras. In Chapter 5, the implementation of a high-field ENDOR setup into a homebuilt pulsed EPR spectrometer operating at 180 GHz is reported and its performance for 1H-ENDOR demonstrated on the model system BDPA. Mims and Davies ENDOR spectra were also obtained for Ras(wt).Mn2+.DP. The increased nuclear Zeeman resolution at 180 GHz may be further exploited in the future by extending the setup for studying hyperfine couplings of low-y nuclei such as 33S, 15N , 17O or 2H. In the present work, the advantages of performing EPR and ENDOR experiments at high fields and frequencies could be nicely demonstrated with the 94 GHz ENDOR studies of Ras. Furthermore, the complementing information obtained at X- and Q-band frequencies in the multifrequency EPR studies on BCR demonstrated that the analysis of EPR spectra can be greatly facilitated by simulating the spectra measured at different MW frequencies with the same set of parameters consistent with a proposed radical. Overall, it could be shown that the use of different experimental techniques at multiple fields and frequencies renders EPR spectroscopy a powerfull tool for structural studies in biological systems.
Pulsed electron-electron double resonance (PELDOR) is a pulsed EPR method that can reliably and precisely provide structural information regarding duplex RNAs and DNAs by measuring long-range distances (1.5-7 nm) utilizing distance-dependent magnetic dipole-dipole interaction between two nitroxide spin labels. In this thesis the application field of PELDOR spectroscopy has been expanded. For the first time the global architecture of tertiary folded RNA has been mapped in vitro. Moreover, the first application of PELDOR for determining structural aspects of RNA and DNA molecules inside cells has been presented. RNA has the central role in cellular processes and gene regulation. It can adopt complex three dimensional structures, which in combination with its conformational dynamics is essential for its function as biological catalyst, structural scaffold and regulator of gene expression. Riboswitches are cis-acting RNA segments that modulate gene expression by direct binding of small molecules with high affinity and specificity. Neomycin-responsive riboswitch is an engineered riboswitch developed by combination of in vitro selection and in vivo screening. Upon insertion into the 5‟ untranslated region of mRNA and binding the cognate ligand it is able to inhibit translational initiation in yeast. Using enzymatic probing the secondary structure had been postulated comprising global stem-loop architecture with a terminal and an internal loop. In the first part of this thesis, the global conformational arrangement of this 27 nucleotides long RNA element has been studied by means of site-directed spin labeling and PELDOR spectroscopy. Spin-labeled neomycin-responsive riboswitch mutants were synthesized via a Sonogashira cross-coupling reaction between 5-membered pyrroline ring based nitroxide radical (TPA) and 5-iodo-uridine. The labeling positions were chosen outside of the binding pocket and UV melting curves revealed that spin-labeling neither disturbs the secondary structure nor interferes with ligand binding. Efficient ligand binding was proven by thermal stabilization of 20.3±3.3 oC upon addition of neomycin, as well as by cw EPR spectra. PELDOR time traces with long observation time windows and with good signal to noise ratio and modulation depth were recorded for all double-labeled samples allowing a reliable data analysis. The fact that there were no shifts in the measured distances upon addition of neomycin implied the existence of a prearranged tertiary structure of the neomycin-sensing riboswitch without a significant global conformational change induced by ligand binding. Measured distances were in very good agreement with the NMR structure of the ligand-bound state of the riboswitch indicating the intrinsic propensity of the global RNA architecture toward its energetically favored ligand-bound form at low temperature. The results harvested in this work represent the first application of PELDOR for mapping the global structure of a tertiary folded RNA. In the second part of this thesis the possibility of applying PELDOR on nucleic acids (NAs) in cellular environment has been investigated. It was shown before that global NA structure depends on matrix conditions, such as concentration of ions and small molecules, molecular crowding, viscosity and interactions with proteins. Therefore, PELDOR spectroscopy on a double-labeled 12-base pair DNA duplex, the 14-mer cUUCGg tetraloop hairpin RNA and the 27-mer neomycin-sensing riboswitch has been used to obtain long-range distance constraints on such systems in Xenopus laevis oocytes and to compare them with in vitro measurements. The reduced lifetime of nitroxide spin labels under cellular conditions has been a major challenge in these measurements. Investigation of nitroxide reduction kinetics in-cell has revealed that the 5-membered pyrrolidine and pyrroline rings are significantly slower reduced compared to 6-membered piperidine ring based nitroxides. Due to prolonged lifetime of the TPA nitroxides covalently attached to NA molecules PELDOR signals could be measured with good signal-to-noise ratios up to 70 minutes of incubation time. The partial loss of coupled spin labels due to nitroxide reduction only led to a decrease in the modulation depth upon increasing the incubation time. No alterations in the measured distances between in vitro and in-cell experiments implies the existence of stable overall conformations of the 14-mer cUUCGg tetraloop hairpin RNA and the 27-mer neomycin-sensing riboswitch, whereas the 12-bp duplex DNA experiences stacking in-cell but retaining the secondary structure. Thus, for the first time nanometer distance measurements were performed inside cells, clearly laying a foundation for the application of PELDOR spectroscopy to study biological processes in cells, such as diffusion, interaction with proteins and other factors or chemical reactions.
Über lange Zeit wurden in der EPR-Spektroskopie hauptsächlich cw-Experimente bei einer Mikrowellenfrequenz von 9 GHz durchgeführt. In den letzten 10 bis 15 Jahren aber haben zwei verschiedene Entwicklungen immer stärkere Verbreitung gefunden. Dies sind zum einen die Verwendung von immer höheren Magnetfeldern und damit Mikrowellenfrequenzen, und zum anderen die Anwendung von Puls-Experimenten. Hochfeld-EPR bietet zwei wesentliche Vorteile gegenüber den klassisch verwendeten Magnetfeldstärken. Dies ist einerseits die erhöhte spektrale Auflösung bei Systemen mit anisotropen g-Tensoren, andererseits die höhere absolute Empfindlichkeit in Verbindung mit einem geringeren Probenvolumen. Puls-Experimente andererseits bieten die Möglichkeit, Informationen zu gewinnen, die mit cw-EPR Spektroskopie nicht oder nur sehr schwer zu erhalten sind. Die Kombination dieser beiden Weiterentwicklungen der EPR-Spektroskopie eröffnet die Möglichkeit, mittels mehrdimensionaler Spektroskopie detaillierte orientierungsabhängige Informationen zu erhalten. Im Rahmen dieser Arbeit wurde ein Puls EPR-Spektrometer aufgebaut, welches bei einer Mikrowellenfrequenz von 180 GHz und einem statischen Magnetfeld von 6,4 T arbeitet. 180 GHz ist derzeit weltweit die höchste Mikrowellenfrequenz, bei der routinemäßig ein zylindrischer Hohlraumresonator verwendet wird und bei der Puls EPR-Experimente durchgeführt werden. Da bei solchen Mikrowellenfrequenzen einige benötigte Bauteile nicht mehr in konventioneller Bauweise erhältlich sind, wurden quasioptische Elemente verwendet, um einen Zirkulator aufzubauen. Der Transport der Mikrowellenstrahlung von der Quelle zur Probe und von dort zurück zur Detektion geschieht mittels überdimensionierter Hohlleiter, um die Verluste zu minimieren. Ein zylindrischer Hohlraumresonator wird in einer fundamentalen Mode betrieben, um am Probenort die für Puls-Experimente notwendige Mikrowellenleistung zu erzeugen. Mit der erreichten Mikrowellenleistung und der Ankopplung des Resonators werden Pulslängen von ca. 60 bis 80 ns für Systeme mit S=1/2 erzielt. Die Eigenschaften des aufgebauten Spektrometers wie die Empfindlichkeit oder die Totzeit im Pulsbetrieb werden ausführlich dargestellt und diskutiert. Ebenso werden die Eigenschaften der implementierten Spektrometersteuerung, insbesondere im Hinblick auf das Zeitverhalten bei Puls-Experimenten, dargestellt und diskutiert. Im letzten Teil der Arbeit wird ein ausführliches Anwendungsbeispiel für Hochefeld-EPR diskutiert. Das Ras-Protein spielt eine wichtige Rolle in der intrazellulären Signalweiterleitung und reguliert solche Prozesse wie Zellwachstum, Differentiation und Apoptose. In ca. 30 % aller menschlicher Tumore werden Mutationen dieses Proteins gefunden, was die wichtige Rolle dieses Proteins demonstriert. Trotz dieser wichtigen Funktion ist der genaue Mechanismus des Aktivierungszykluses noch nicht im Detail aufgeklärt worden. Mittels cw-EPR Spektroskopie wurden die GDP-gebundenen inaktiven Proteinkomplexe verschiedener Mutanten untersucht. Durch Messungen in H217O-angereichertem Wasser konnte gezeigt werden, dass bei Raumtemperatur beim Wildtyp ein Wasserligand weniger am aktiven Zentrum der Proteinkomplexe vorliegt als bei einer onkogenen Mutante. Dieses Ergebnis widerspricht den bisher durch verschiedene Röntgenstrukturuntersuchungen gewonnen Erkenntnissen. Es wird ausführlich darüber diskutiert, dass diese unterschiedlichen Ergebnisse vermutlich auf Kristallbildungseffekte zurückzuführen sind.
Since the early 2000s, nucleic acid aptamers have gained considerable attention of life science communities. This is in particular due to the fact that aptamers are known to function as artificial riboswitches, which presents an efficient way to regulate gene expression. A promising candidate is the tetracycline-binding RNA aptamer (TC-aptamer) since the TC-aptamer is known to function in vivo and exhibits a very high affinity towards its ligand tetracycline (TC) (Kd = 800 pM at 10mM Mg2+). Although a highly resolved crystal structure exists in the ligand bound state, questions related to dynamics cannot be answered with X-ray crystallography. In this work, pulsed electron paramagnetic resonance (EPR) spectroscopy was used to study different biochemical and structural aspects of the TC-aptamer.
On the one hand, pulsed hyperfine spectroscopy was used to study the binding of TC via Mn2+ to the TC-aptamer at lower and thus more physiological divalent metal ion concentrations. In a first step, a protocol for the relatively new pulsed hyperfine technique electron-electron double resonance detected NMR (ELDORdetected NMR or just EDNMR) was developed for Q-band frequencies (34 GHz). After a successful verification of the EDNMR technique at Q-band frequencies on Mn2+ model complexes ([Mn(H2O)6]2+ and Mn-DOTA), two dimensional hyperfine techniques were used to confirm the formation of a ternary RNA-Mn2+- TC complex at physiological divalent metal ion concentrations. Correlation signals between 13C (13C-labeled TC) and 31P (from the RNA backbone) to the same Mn2+ electron spin were detected with 2D-EDNMR and triple hyperfine correlation spectroscopy (THYCOS).
On the other hand, pulsed electron-electron double resonance (PELDOR) spectroscopy on a doubly nitroxide-labeled TC-aptamer was used to investigate the conformational rearrangement upon ligand binding and how the conformational flexibility is affected by different Mg2+ concentrations. The Çm spin label was used as a nitroxide spin probe. Due to its rigidity and low degree of internal flexibility, the Çm spin label yields very narrow distance distributions and pronounced orientation selection (OS). As a consequence, the width of the distance distributions can be used to draw conclusions about the conformational flexibility of the spin-labeled helices. Analysis of the distance distributions showed that at high Mg2+ concentrations, the TC-aptamer is in its folded state, irrespective of the fact if TC is present or absent. Orientation selective PELDOR revealed that the orientation of the spin-labeled helices in frozen solution is the same as in the crystal structure. First Mn2+-nitroxide pulsed electron electron double resonance (PELDOR) measurements on a singly nitroxide-labeled and Mg2+/Mn2+-substituted TCaptamer at different Mn2+ concentrations in the presence and absence of TC gave insight into the affinities of the additional divalent metal ion binding sites of the TC-aptamer.
Ribonukleinsäure (ribonucleic acid, RNA) wirkt bei der Proteinbiosynthese nicht nur als Informationsüberträger, sondern kann auch beispielsweise durch sogenannten Riboschalter (auch Riboswitches) regulatorische Funktionen übernehmen. Riboschalter sind komplett aus RNA aufgebaut und man kann sie sich als molekulare Schalter vorstellen, die die Genexpression kontrollieren. Konzeptionell besteht ein Riboswitch aus zwei Untereinheiten, dem Aptamer und der Expressionsplattform. Das Aptamer bindet, üblicherweise sehr spezifisch, kleine organische Moleküle, aber auch Ionen. Diese Ligandenbindung induziert Änderungen in der Struktur des Riboswitches, welche wiederum die Expressionsplattform beeinflussen. Je nach Riboswitch ermöglicht oder verhindert dies schließlich die Genexpression. Die vorliegende Doktorarbeit beschäftigt sich mit der Entwicklung und Etablierung von Methoden der optischen Spektroskopie zur Aufklärung von RNA-Dynamiken und -Strukturen im Allgemeinen und der Erforschung von Aptamerbindungsmechanismen im Besonderen.
Eine der dazu verwendetet Methoden ist die FTIR-Spektroskopie. Hierfür wurden zunächst kritische Parameter wie verschiedenste Messeinstellungen oder die Probenpräparation ausgiebig an RNA-Modellsträngen getestet. Dabei war es möglich, eine kleine Spektrenbibliothek als internen Standard aufzubauen. Gleichzeitig konnte gezeigt werden, dass kleinere RNA-Oligonukleotide (< ca. 20 Nukleobasen) gut mittels FTIR-Methoden untersucht werden können. Anschließend wurde eine statische Bindungsstudie am adenosin- sowie am guanosinbindenden Aptamer vorgenommen.
Die zweite hier vorgestellte Methode zur Untersuchung von RNA-Molekülen ist die Fluoreszenzspektroskopie. Im Gegensatz zur FTIR-Spektroskopie ist dazu allerdings eine Modifizierung der RNA durch ein Fluoreszenzlabel nötig. Deshalb beschäftigt sich der Hauptteil dieser Doktorarbeit mit der Charakterisierung und der Anwendung des quasi bifunktionellen RNA-Markers (auch RNA-Labels) Çmf. So wurden zunächst die photophysikalischen und photochemischen Eigenschaften des Markers untersucht. Dabei konnte gezeigt werden, dass Çmf sich als lokale Sonde eignet, da es empfindlich auf Änderungen der Mikroumgebung in Lösung reagiert. Durch direkten Vergleich der optischen Eigenschaften von Çmf mit den entsprechenden Eigenschaften des Spinlabels Çm war es möglich, den starken Fluoreszenzlöschungseffekt (sog. quenching) des Çm aufzuklären. So kann davon ausgegangen werden, dass die Fluoreszenz des Çm durch eine sehr schnelle interne Konversion (IC) in einen dunklen Dublettzustand (D1) gelöscht wird.
Im nächsten Schritt wurde Çmf in RNA-Modellstränge eingebaut, um den Einfluss der RNA auf die Photochemie des Markers zu untersuchen. Dabei konnte gezeigt werden, dass sich dessen Fluoreszenzsignal abhängig von den direkten Nachbarbasen sowie abhängig vom Hybridisierungszustand signifikant ändert. Gleichzeitig konnte keine deutliche Veränderung der Stabilität der Modellstränge festgestellt werden. So konnte also nachgewiesen werden, dass sich Çmf sehr gut als lokale Sonde in RNA eignet. Im Speziellen wurde aus den Ergebnissen geschlossen, dass der Fluorophor für Ligandenbindungsstudien herangezogen werden kann.
Deshalb wurde Çmf schließlich an mehreren verschiedenen Stellen in das neomycinbindende Aptamer (N1) eingebaut, um dessen Bindungskinetik zu untersuchen. Mittels Stopped-Flow-Messungen war es möglich, die Bindungsdynamik des Aptamers zu beobachten. Anhand dieser transienten Daten konnte ein Zweischrittbindungsmodell abgeleitet werden. Dabei bindet Neomycin zunächst unspezifisch an das weitgehend vorgeformte Aptamer. Anschließend kommt es durch die Ausbildung von Wasserstoffbrücken zu einer spezifischen Bindung des Liganden am Aptamer.
Im dritten Teil dieser Arbeit geht es ebenfalls um die Entwicklung und Etablierung eines spektroskopischen Werkzeuges. Dabei stehen allerdings Rhodopsine im Mittelpunkt der Aufmerksamkeit. Hierbei handelt es sich um Membrantransportproteine, die nach optischer Anregung einen sehr schnellen Photozyklus mit mehreren Intermediaten durchlaufen. Es ist möglich, diese Intermediate dank transienter Absorptionsmessungen mit sehr guter zeitlicher und spektraler Auflösung zu beobachten. Allerdings besteht der Bedarf, diese Intermediate statisch zu präparieren, um sie näher charakterisieren und mit anderen Methoden, wie z.B. der Festkörper-NMR, vergleichen zu können.
Ein spektroskopisches Werkzeug zum Präparieren von frühen Photointermediaten ist kryogenes Einfangen (sog. Cryotrapping) dieser Intermediate. Im Rahmen dieser Arbeit wurden das Cryotrapping und die anschließende statische UV/vis-Absorptionsspektroskopie der fixierten (getrappten) Zustände optimiert und an einer Reihe von Rhodopsinen (ChR2, GPR) demonstriert.
Gepulste dipolare EPR-Spektroskopie ist eine wertvolle Methode, um Abstände von 1.5 bis 10 nm zwischen zwei Spinmarkern zu messen. Diese Information kann für Strukturbestimmungen hilfreich sein, wo traditionelle Methoden wie Kristallstrukturanalyse und NMR nicht angewendet werden können. Zusätzlich ist es möglich, Änderungen in Konformation und Flexibilität zu verfolgen. Für diese Studien haben sich stabile Nitroxidradikale als Spinmarker etabliert. Diese werden spezifisch durch die site-directed spin labelling Methode (SDSL) kovalent an das zu untersuchende Biomolekül gebunden. In den letzten Jahren wurden weitere Spinmarker für Abstandsbestimmungen mittels EPR-Spektroskopie entwickelt. Besonders interessant sind Triarylmethylradikale (im Folgenden abgekürzt als Trityl) und paramagnetische Metallzentren.
Im Vergleich zu Nitroxidradikalen hat das Tritylradikal einige Vorteile: Eine höhere Stabilität in einer reduzierenden Umgebung wie im Inneren von Zellen, längere Elektronenspin-Relaxationszeiten bei Raumtemperatur und ein schmaleres EPR-Spektrum. Deswegen ist dieses organische Radikal ein alternativer Spinmarker, der besonders gut für die Forschung von Biomolekülen in einer nativen Umgebung unter physiologischen Bedingungen geeignet ist. Auch paramagnetische Metallzentren sind weniger reduktionsempfindlich als Nitroxidradikale. Zusätzlich sind diese Spinmarker interessant in biologischen Fragestellungen. Zum Beispiel besitzen zahlreiche Enzyme paramagnetische Manganzentren als Cofaktoren. Zudem kann Magnesium, ein wesentlicher Cofaktor in Enzymen, Nukleinsäuren und Nukleotid-Bindungsdomänen der G- und Membranproteine, oft durch das paramagnetische Mangan ersetzt werden. Um Abstandsmessungen an Biomolekülen, die nur ein Metallzentrum besitzen, durchzuführen, können zusätzliche Spinmarker in Form eines Nitroxid-, Tritylradikals oder eines anderen paramagnetischen Metallkomplexes mithilfe der SDSL-Methode kovalent gebunden werden.
Nitroxidradikale, Tritylradikale und Metallzentren haben deutlich unterschiedliche EPR-spektroskopische Eigenschaften, welche oft als orthogonale Spinmarker bezeichnet werden. Solche Spinmarker sind nützlich für die Untersuchung von verschiedenen Untereinheiten bei makromolekularen Komplexen. Somit können die intramolekularen Abstände innerhalb einer Untereinheit sowie intermolekularen Abstände zwischen den unterschiedlichen Untereinheiten mit nur einer einzigen Probe bestimmt werden. Zusätzlich können die orthogonalen Marker sehr effektiv genutzt werden, um Metallzentren in Biomolekülen mithilfe der Trilateration-Strategie genau zu lokalisieren.
Die hier vorliegende Doktorarbeit beschäftigt sich mit der Nutzung dieser neuen Spinmarker für Abstandsmessungen. Solche Spinmarker sind noch kaum erforscht, obwohl sie für biologische Anwendungen eine große Rolle spielen könnten.
Das erste Ziel dieser Doktorarbeit war eine Studie über Tritylradikale mithilfe der dipolaren EPR-Spektroskopie. Zu diesem Zweck wurden sowohl double quantum coherence (DQC) und single frequency technique for refocussing dipolar couplings (SIFTER) Experimente als auch Hochfrequenz pulsed electron electron double resonance (PELDOR) Experimente mit einem Trityl-Modellsystem durchgeführt. Dabei wurden die Besonderheiten der unterschiedlichen dipolaren Spektroskopiemethoden mit diesem Spinmarker untersucht, um die Empfindlichkeit und Robustheit für die Abstandsmessungen zu optimieren.
Das zweite Ziel war eine Studie über den Einfluss der Hochspin-Multiplizität des Mangans auf die Abstandsbestimmungen. Für diesen Zweck wurde zuerst ein Modellsystem mit einem orthogonalen Mn2+ Ion und Nitroxidradikal mithilfe der PELDOR-Spektroskopie untersucht. Anschließend wurde ein weiteres Modellsystem mit zwei Mn2+-Ionen untersucht, um PELDOR und relaxation-induced dipolar modulation enhancement (RIDME) Experimente bezüglich ihrer Empfindlichkeit und Robustheit sowie Genauigkeit der Datenanalyse zu optimieren.
Das Trityl-Modellsystem wurde in der Arbeitsgruppe von Prof. Sigurdsson synthetisiert. Die EPR Messungen wurden bei zwei verschiedenen Mikrowellenfrequenzen (34 und 180 GHz) durchgeführt. Es wurde gezeigt, dass die Auswahl der optimalen Methode von den EPR-spektroskopischen Eigenschaften des Systems bei den jeweiligen Mikrowellenfrequenzen abhängig ist. Das EPR-Spektrum des Trityls ist bei 34 GHz so schmal, dass das ganze Spektrum von einem üblichen Mikrowellenpuls angeregt werden kann. In diesem Fall sind die DQC und SIFTER Experimente am besten geeignet. Der mit diesen Methoden bestimmte Abstand von 4.9 nm ist in guter Übereinstimmung mit Werten aus der Literatur. Es wurde festgestellt, dass die SIFTER Messung eine höhere Empfindlichkeit als DQC besitzt, da das Signal-zu-Rausch Verhältnis um den Faktor vier größer ist. Außerdem ist die SIFTER-Methode experimentell weniger anspruchsvoll, da ein deutlich kürzerer Phasenzyklus für die Mikrowellenpulse benötigt wird. ...
Pulsed Electron Paramagnetic Resonance (EPR) spectroscopy is the most powerful tool to investigate structural properties and dynamics of paramagnetic substances. Up to date the electron spin is almost exclusively manipulated by rectangular shaped microwave pulses generated with switches. These pulses are unselective which means they excite outside their nominal bandwidth which is in most cases shallow compared to the overall spectral width of the spin system. Shaped pulses which are widely applied in NMR promise higher bandwidth and selectivity. The use of amplitude and phase modulated pulses was not possible for EPR due to the three orders of magnitude faster timescale compared to NMR. In this work, for the first time, an AWG (arbitrary waveform generator) operating with a 1 ns time resolution and 14 bit amplitude resolution was implemented into a commercial Bruker pulsed EPR spectrometer.
First results were obtained with broadband excitation pulses derived by optimum control theory (OCT). The OCT-pulse used excites transverse magnetization with 98% efficiency over a more than four times larger bandwidth than common rectangular pulse generating the same 1 B field. The benefit of such a pulse was demonstrated for magnitude FT-EPR spectroscopy on organic radicals in liquid phase.
Due to Spectrometer deadtime an FID cannot be observed for most inhomogeneous spin systems. For that reason prefocused pulses have been evaluated for their applicability to EPR spectroscopy. OCT-derived prefocused pulses can be understood as a compact Hahn Echo sequence in one monolithic pulse. Here, two problems have been encountered. 1) The limited bandwidth of the active and passive microwave components in the excitation path as well as microwave resonator cause linear distortions of the pulse shape which results in inferior pulse performance. This could be circumvented by measuring the impulse response function of the whole spin excitation path and including this information in the pulse optimization procedure. 2) Anisotropic hyperfine interaction which was not taken into account during the pulse optimization also caused efficiency losses.
PELDOR spectroscopy is a valuable tool to measure distance distributions between two or more paramagnetic centers in the range from 2-8 nm. It is demonstrated that the S/N ratio of PELDOR experiments can be substantially increased by substituting the rectangular shaped pump pulse by an adiabatic inversion pulse. The damping of the dipolar oscillations introduced by the prolonged pump pulse towards shorter distances could be circumvented by introducing a second time reversed pump pulse.
By substituting the refocused echo of the well-known 4-pulse PELDOR with a CPMG sequence the dipolar evolution time and thus the validity of PELDOR experiments would be increased. To achieve the maximum dipolar evolution time in a CPMG PELDOR for each refocusing pulse one pump pulse has to be applied. This could only be achieved with the new adiabatic inversion pulses since multiple inversions with efficiency close to one are not possible with rectangular pulses. Even with adiabatic pump pulses a reduced efficiency was observed due to hardware limitations thus limiting the sequence to three refocusing pulses. An iterative method was developed to remove the residual dipolar signals attributed to the reduced inversion efficiency.
The new 7-pulse CPMG PELDOR sequence enabled measuring reliable distance distributions between the protomers of the trimeric betaine transporter BetP. With these it could be shown that the asymmetries found for the 2 and 3-dimensional crystal structures are even larger in frozen detergent.
Nuclear Magnetic Resonance ("NMR") is a powerful and versatile technique relying on nuclei that posses a spin. Since its discovery more than 6 decades ago, NMR and related techniques has become a tool with innumerable applications throughout the fields of Physics, Chemistry, Biology and Medicine. Numerous Nobel Prizes have been awarded for work in the field and a multi billion dollar industry has developed on its basis.
One of NMR's major shortcomings is its inherent lack of sensitivity. Because it relies on the Boltzmann populations of spin states with a minuscule Zeeman splitting, this is particularly true for room temperature experiments.
As a result, in an enormous technological effort to enlarge the Zeeman splitting NMR magnets have been moving to higher and higher magnetic fields. However, even for proton spins possessing the largest magnetic moment of all nuclei, the degree of polarization that can be achieved in the strongest spectroscopic magnets available today (~24 T) at room temperature is merely ~ 8*(10 exp (-5)). In other words, this low polarization theoretically allows a sensitivity enhancement of 104 towards full polarization.
Since Magnetic Resonance Imaging ("MRI") is based on the same principle, it shares this problem with NMR. Furthermore, for technical and physiological reasons full body MRI tomographs do not reach the magnetic field strengths of spectroscopic NMR magnets, making this even more of an issue for MRI.
In consequence, MRI is chiefly restricted to detecting protons, while both MRI and NMR detection of 13C (or other low nuclei) under physiological conditions, i.e. low natural abundance of 13C and a low concentration of the respective substance, suffer from long acquisitions times that are necessary to obtain adequate signal to noise ratios ("SNR").
However, this drawb of NMR can be overcome. The enormous potential sensitivity increase of four orders of magnitude can - at least partially - be exploited by several hyperpolarization techniques, creating entirely new applications and fields of research.
These hyperpolarization techniques comprise chemical approaches like Parahydrogen Induced Polarization ("PHIP") or Photochemically Induced Dynamic Nuclear Polarization ("Photo-CIDNP"), as well as physical techniques like optically pumped (noble) gases13, 14 or Dynamic Nuclear Polarization ("DNP"), which will be the focus of this work. A hyperpolarized substance will render a larger signal without being physically or chemically altered in any other way. It is therefore "marked" without any marker, making it an agent free contrast agent for MRI.
DNP is a technique, in which hyperpolarization of nuclear spins is achieved by microwave (\MW") irradiation of unpaired electron spins in radicals, which are coupled to these nuclei, e.g. 1H, 13C or 15N. The electron spin population is perturbed if the microwave irradiation is resonant with the electron spin transition, which affects the polarization of hyperfine-coupled close nuclei. For large microwave power (i.e. saturating the electron spin transition) the orders of magnitude larger thermal electron spin polarization is effectively transferred to these nuclear spins in the sample. For proton spins the maximum polarization gain amounts to 660, whereas for 13C the sensitivity gain can be as large as 2600. In contrast to e.g. PHIP, which is restricted to specific reaction precursors, DNP is not limited to specific nuclei or hyperpolarization target molecules, making it a very versatile technique. DNP has been first proposed by Overhauser in 1953,15 and experimentally observed shortly thereafter in metals16 and liquids,17 both being systems with mobile electrons. In the 1960s and 70s, DNP was used as a spectroscopic tool in liquids, thoroughly mapping the effect in the low field regime. As well, several other transfer mechanisms were discovered, which are active in the solid state with localized electrons, namely the solid effect the cross effect and thermal mixing. The theory for all three of these mechanisms predicts reduced transfer efficiencies at higher magnetic fields. This fact and the lack of high frequency microwave sources to excite electron spins at magnetic field strengths above 1 T, effectively relegated DNP to a position of an interesting scientifi curiosity.
In the early 1990s, DNP came to a renaissance, when DNP was performed at high field in solid state magic angle spinning ("MAS") experiments using high power gyrotron microwave sources. This pioneering work sparked a surge of new developments and applications.
As well, this success triggered attempts to investigate also the potential of DNP in the liquid state at high magnetic fields, e.g. at 3.4 T35{38 and 9.2 T. To date, DNP can be considered one of the "hot topics" in the field of magnetic resonance, bringing about special issue in magnetic resonance journals and DNP sections on magnetic resonance conferences.
This thesis deals with the development of an in-bore liquid state DNP polarizer for MRI applications operating in ow through mode at a magnetic field strength of 1.5 T. Following this introductory chapter, the theoretical background necessary to understand and interpret the experimental results is explained in chapter 2. Subsequently, chapter 3 deals with the issue of performing liquid state DNP at high magnetic fields and its challenges. The chapter comprises a quick overview of the necessary hardware, the experimental findings for various samples and the interpretation of these findings. along with the ramifications for the aim of this work. Chapter 4 deals with the issue of increasing sensitivity and contrast in MRI, in particular by means of DNP. The chapter illustrates the development of our polarizer by presenting the hardware that was developed and demonstrating its performance under various conditions. As well, several alternative approaches are introduced and compared to our approach. Finally, chapter 5 summarizes the findings and gives an outlook on further developments.
Structural biology often employs a combination of experimental and computational approaches to unravel the structure-function paradigm of biological macromolecules. This thesis aims to approach this combination by the application of Pulsed Electron-Electron Double Resonance (PELDOR/DEER) spectroscopy and structural modelling. In this respect, PELDOR spectroscopy in combination with site-directed spin labelling (SDSL) of proteins is frequently used to gain distance restraints in the range from 1.8 to 8 nm. The inter-spin distance and the flexibility of the spin labelled protein domains are encoded in the oscillation and the dampening of the PELDOR signal. The intrinsic flexibility of the commonly used MTSSL (1-Oxyl-2,2,5,5-tetramethylpyrroline-3-methyl) spin label itself can be an obstacle for structural modelling if the flexibility of the label is large compared to the flexibility of the protein domains. In this thesis the investigation of two multi-domain proteins by the 4-pulse PELDOR sequence is presented. At first, the N-terminal polypeptide transport-associated (POTRA) domains of anaOmp85, a rigid three domain protein, giving well-defined PELDOR distance restraints, is investigated. The experimental restraints are used for structure refinement of the X-ray structure and reveal a strong impact of the intrinsic flexibility of MTSSL on the accuracy of structural refinement. The second example, K48-linked diubiquitin, is a highly flexible multi-domain protein on which the flexibility of MTSSL is of minor impact on structural modelling. In this case, the distance restraints are utilized to determine conformational ensembles. Due to the high intrinsic flexibility already characterizing diubiquitin the recently developed 7-pulse Carr-Purcell (CP) PELDOR sequence was applied to investigate longer ubiquitin chains. This sequence enables to measure dipolar oscillations with an extended time window, allowing a good separation between inter- and intramolecular contributions even for long distance and broad conformational distributions, thereby providing an increased accuracy of the obtained distance distributions.
Functional dynamics of ribonucleic acids : development and application of spectroscopic tools
(2016)
Im Rahmen der vorliegenden Dissertation wird der Aufbau eines zeitaufgelösten Fluorimeters, die photophysikalische Grundcharakterisierung der drei 2-(Pyrenylethinyl)-Adenosine (PyAs) und das Wechselwirkungsgeflecht des tetracyclinbindenden Aptamers (TC-Aptamer) mit seinem Liganden Tetracycyclin (TC) und Mg2+ dargestellt.
Das zeitaufgelöste Fluorimeter basiert auf der experimentellen Technik des zeitkorrelierten Einzelphotonenzählens. Es verfügt über zwei Anregungsquellen: gepulste UV-LEDs und einen frequenzverdoppelten titandotierten Saphirlaser. Diese Quellen Decken einen Wellenlängenbereich von (310 - 550) nm ab. Das Spektrometer kann unter günstigen Umständen eine Zeitauflösung von 50 ps erreichen bei einer zeitlichen Messungenauigkeit von weniger als 0,02 %.
Die Leistungsfähigkeit des Aufbaus wird anhand einer umfangreichen Studie an den drei PyAs demonstriert.
Die drei PyAs 2-(1-Pyrenylethinyl)-Adenosine (1PyA), 2-(2-Pyrenylethinyl)-Adenosine (2PyA) und 2-(4-Pyrenylethinyl)-Adenosine (4PyA) sind eine Gruppe fluoreszierender RNA-Nukleosidanaloga, welche die Gesamtheit aller möglichen Konfigurations-isomere der Grundverbindung PyA umfassen. Ihre zeitabhängigen Fluoreszenzzerfallseigenschaften werden ergänzt von stationären Absorptions- und Fluoreszenzspektren, ultraschneller transienter Absorptionsspektroskopie und quantenchemischen Rechnungen. Die Fluoreszenz von 1PyA und 4PyA gehorchen der Regel von Kasha, wohingegen 2PyA einen triexponentiellen Zerfall mit ausgeprägter Abhängigkeit von der Anregungswellenlänge zeigt. Die transienten Absorptionsspektren aller drei Isomere weisen im gesamten Spektrum dominante, wenig strukturierte Absorptionsbanden des ersten angeregten Zustands auf, welche im nahen UV in unterschiedlichem Maße vom Grundzustandsbleichen und stimulierter Emission überlagert werden. 2PyA zeigt eine deutlich ausgeprägte Signatur für eine interne Umwandlung hin zum S1, wenn es in höhere angeregte Zustände angeregt wird.
Das Fluoreszenzverhalten von 2PyA wird mithilfe eines lokal angeregten (LE) und zweier intramolekularer Ladungstransferzustände, von denen einer der koplanaren Orientierung von Pyren und Adenin (MICT) und der andere einer um 90 ° verdrehten Orientierung (TICT) entspricht. Der LE-Zustand ist hierbei verknüpft mit dem S2 von 2PyA, welcher einer rein pyrenlokalisierten Anregung entspricht. Dieser Zustand existiert so in 1PyA und 4PyA nicht. Der verdrehte TICT-Zustand ist nur in 2PyA bevölkerbar, weil für 2PyA die Barriere zur Bildung von Rotameren am niedrigsten ist und das Molekül nach Anregung daher in diese Geometrie kommen kann und dann durch die stärkere elektrostatische Anziehung stabilisiert wird. 1PyA und 4PyA emittieren hingegen nur aus dem MICT-Zustand.
Die Komplexbildung des TC-Aptamers mit seinem Liganden TC in Lösung wird empfindlich beeinflusst durch die-Konzentration von Magnesiumkationen. Dies wird untersucht durch Bindungs- und Faltungs- und Denaturierungsstudien mit verschiedenen Mg- und Harnstoffkonzentrationen. Als experimentelle Observable dienen hierbei die konformationsabhängige Nukleobasenabsorption und ihr Zirkulardichroismus im fernen UV, die Fluoreszenz des Liganden TC und die freiwerdende Wärme der exothermen Bindungsreaktion des Aptamers mit Mg in An- und Abwesenheit von TC.
Ohne Mg ist eine Interaktion des TC-Aptamers mit TC nicht nachweisbar. Dies liegt daran, dass Mg die notwendige elektrostatische Abschirmung der negativen elektrischen Ladung am RNA-Rückgrat zur Verfügung stellt. Die Abschirmung erlaubt es dem Aptamer kompakte Strukturen mit tertiären Kontakten auszubilden. Wenn die Mg-Konzentration die Faltung des Aptamers vollständig unterstützt (> 1 mM), so befindet sich das Aptamer weitgehend in einer vorgefalteten Konformation, welche der bindungskompetenten stark ähnelt. In diesem Zustand kann das Aptamer seinen Liganden extrem schnell, nämlich annähernd diffusionslimitiert binden. Unter diesen Bedingungen hat TC kaum Einfluss auf die Konformation seines Aptamers.
Bei physiologischen Mg-Konzentrationen (0,2 - 0,8 mM) kann das Aptamer kompakte Konformationen mit tertiären Strukturen einnehmen. Diejenige Konformation, welche der bindenden sehr stark ähnelt, dominiert das konformationelle Gleichgewicht jedoch noch nicht vollständig, es ist lediglich eine Konformation von vielen möglichen. Daher eröffnen physiologische Mg-Konzentrationen dem TC-Aptamer Teile des Konformationsraumes, welche andernfalls nicht zugänglich wären und TC stabilisiert selektiv die native Konformation. Diese konformationelle Verschiebung liefert kann hierbei zur robusten Signalgebung für die Funktion als Riboschalter dienen.
Pulsed dipolar (PD) EPR spectroscopy is an established and reliable tool for the investigation of biomolecules. In terms of long distance and orientation measurements, it is one of the leading methods and further fields of application are constantly being explored. The distances that can be detected with PD EPR also correspond to the range in which almost all important biomolecule interactions occur. In the transition from in vitro spectroscopy to in-cell spectroscopy, the power of PD EPR spectroscopy is particularly evident. It is non-invasive, more sensitive than NMR, and does not exhibit background signals from diamagnetic molecules. In particular, the absence of background signals is of great importance given the high density of molecules within cellular environment. However, like any other spectroscopic method, PD EPR has certain limitations. Owing to the intrinsically fast electron spin echo dephasing at higher temperature, these experiments are commonly carried out in frozen solutions at about 50 K. This temperature is far away from the physiological conditions and the freezing additives used, e.g. glycols, can further influence the structure. To enable measurements with and within living organisms, it is therefore necessary to ascend from the cold depths of the frozen state. At the same time, one has to adapt the spin tags for the desired application. Established nitroxides commonly used for EPR studies are typically susceptible to reduction. Thus, for studies under physiological conditions, e.g. in the cell, one has to fight against the reductive environment in the cell and somehow protect the spin labels. Initial published in-cell experiments within the research group and investigations of homogeneously distributed labeled double-stranded (ds) ‐DNA samples in solid matrices showed promising results and enabled pulsed measurement in the temperature range of 50‐ 295 K. It could also be demonstrated that spherical shielded nitroxides have a significantly longer life span in cellular environments than non-protected ones and first nuclear acids were measured in cell. Based on these results, we have gone further to overcome the standing limitations and developed the use of PD EPR spectroscopy. This work addresses these challenges with the overall goal of advancing the applications of PD EPR spectroscopy for studying biomolecules under physiological conditions.
We have focused on four different approaches. The results of these studies were published in various publications. They are presented and discussed together with further studies and put into the context of research conducted before and after the authors' publications.
In approach 1, we fought against the two main obstacles for using pulsed dipolar spectroscopy at ambient conditions – minimizing phase memory time T2 and averaging of the anisotropic dipolar coupling by rotational diffusion. We focused on an immobilization approach, while using rigid spin labels at same time. Besidesto the distance information, the incorporated rigid spin labels will give additional angular constrains and information about the molecular dynamics.
In approach 2, we focused on the on-site and on-demand formation of nitroxide spin labels using light-sensitive alkyl protection groups. This a very mild and efficient procedure that will hardly interfere with sensitive functional groups present in oligonucleotides or peptides. By establishing this method and using coumarin protecting groups plus two-photon excitation, this property may offer the potential to generate spin labels with very high levels of spatial and temporal resolution.
For approach 3, we used paramagnetic Gd3+ -ions as intrinsically stable labels, which are not reducible within a cellular environment. Easy to mix and bound to encodable lanthanide binding tags within the molecule Interleucin 1β, we were able to measure distances between two tags with PELDOR spectroscopy. We tested the extent to which this system is suitable for in-cell measurements.
Finally, we focus on methods for easier labeling by using non-covalentlabeling techniques. One of these is the novel nitroxide G´ for site-directed spin labeling of nucleic acids, especially for RNA. This spin label is sterically hindered, easy to build and binding occurs in seconds by simply mixing the spin label with the target. For large RNAs, another easy-to-mix and noncovalent spin-labeling strategy will be experimentally accompanied and presented.
The approaches and results described here are intended to demonstrate that the study of the biological functions of biomolecules under physiological conditions by pulsed EPR spectroscopy is feasible and operational. In combination, they will enable the life sciences to make further and faster progress in the search for the molecular master plan.
Pulsed electron-electron double resonance (PELDOR), also called Double Electron-Electron Resonance, (DEER) is a pulsed EPR technique that can provide structural information of biomolecules, such as proteins or nucleic acids, complementary to other structure determination methods by measuring long distances (from 1.5 up to 10 nm) between two paramagnetic labels. Incorporation of the rigid Ç-label pairwise into DNA or RNA molecules enables the determination not only of the distance but also of the mutual orientation between the two Ç-labels by multi-frequency orientation-selective PELDOR data (X-, Q- and G-band frequencies). Thus, information about the orientation of secondary structure elements of nucleic acids can be revealed and used as additional angular information for structure determination. Since Ç does not have motion independent from the helix where it resides, the conformational flexibility of the nucleic acid molecule can be directly determined. This thesis demonstrates the advancement of PELDOR spectroscopy, beyond its original scope of distance measurements, to determine the mutual orientation between two rigid spin labels towards the characterization of the conformational space sampled by highly flexible nucleic acid molecules. Applications of the methodology are shown on two systems: a three-way junction, namely a cocaine aptamer in its bound-state, and a two-way junction, namely a bent DNA.
More in detail, the conformational changes of the cocaine aptamer upon cocaine binding were investigated by analysis of the distance distributions. The cocaine-bound and the unbound states could be differentiated by their conformational flexibility, which decreases in the presence of the ligand. Moreover, the obtained distance distributions revealed a small change in the mean distance between the two spin labels upon cocaine binding. This indicates a ligand-induced conformational change, which presumably originates at the junction where cocaine is known to bind. The investigation of the relative orientation between the two spin-labeled helices of the aptamer revealed further structural insights into the conformational dynamics of the cocaine-bound state. The angular information from the orientation-selective PELDOR data and the a priori knowledge about the secondary structure of the aptamer were helpful in obtaining a molecular model describing its global folding and flexibility. In spite of a large flexible aptamer, the kink angle between the Ç-labeled helices was found to be rather well-defined.
As for the bent DNA molecule, a two-step protocol was proposed to investigate the conformational flexibility. In the first step, a database with all the possible conformers was created, using available restraints from NMR and distance restraints derived from PELDOR. In a second step, a weighted ensemble of these conformers fitting the multi-frequency PELDOR data was built. The uniqueness of the obtained structural ensemble was checked by validation against an independent PELDOR data set recorded at a higher magnetic field strength. In addition, the kink and twist angle pairs were determined and the resulting structural ensemble was compared with the conformational space deduced both from FRET experiments and from the structure determined by the NMR restraints alone.
Overall, this thesis underlines the potential of using PELDOR spectroscopy combined with rigid spin labels in the context of structure determination of nucleic acids in order to determine the relative orientation between two helices, the conformational flexibility and the conformational changes of nucleic acid molecules upon ligand binding.
Metal ions as novel polarizing agents for dynamic nuclear polarization enhanced NMR spectroscopy
(2017)
High-spin complexes of Gd(III) and Mn(II) were introduced as polarizing agents (PAs) for solid-state dynamic nuclear polarization (DNP) in 2011. This dissertation was undertaken in 2013, with the intention of exploring these PAs further. Major goals of this work were to understand their DNP mechanism(s) and explore their application in biomolecular research. This cumulative thesis details the methods, advantages, and practical implications of using high-spin PAs for MAS DNP. Data from electron paramagnetic resonance (EPR) and NMR spectroscopy are discussed for a complete understanding of DNP mechanisms.
Out of the two main mechanisms − solid effect (SE) and cross effect (CE − active under experimental conditions of solid-state DNP, commonly used nitroxide PAs evoke CE owing to their broad EPR spectra. On the other hand, DNP mechanisms evoked by high-spin metal ions seem non-trivial due to additional features (originating from spin-orbit coupling or zero field splitting) in their EPR spectra. The features of the EPR signal generally influence the shape of enhancement profiles. Therefore, the metal ion with a simpler EPR signal i.e., Gd(III) , is chosen as the starting point for the investigation of DNP mechanisms. Varying concentrations (2, 10, 20 mM) of a water-soluble and stable complex Gd-DOTA was dissolved as the PA in a glycerol-water solution of 13C,15N - urea. Field profiles of DNP enhancement on each nuclear type (1H, 13C, and 15N) establishes SE as the active DNP mechanism at the smallest PA concentration (2 mM). This confirms the theoretical predictions that narrow line width of the Gd(III) EPR signal arising from the central transition (CT, ms = -1/2 +1/2) allows for resolved SE DNP. However, that is no longer the case at higher PA concentrations of 10 and 20 mM. At higher Gd(III) concentrations, the CE mechanism contributes significantly and varies with nuclear Larmor frequency (ωn) of the concerned nuclei. The enhancement maxima shifts towards the EPR resonance as the contribution from CE increases. This shift is evident in the field profiles of 15N and 13C, whereas that of 1H is least influenced. This observation can be explained by combining theoretical estimates with the experimental data; the CE is evoked by increased dipolar coupling (Dee) – a prerequisite for CE – between neighboring Gd(III) spins as the statistical inter-spin distance shortens at elevated concentrations. This finding is important because the knowledge of active DNP mechanisms is essential for accurate interpretation of results from DNP experiments.
From the experiments on Gd-DOTA it becomes clear that concentration, inter-spin distances, and hence induced Dee are intertwined. In order to explicitly address the influence of inter-spin distances on DNP mechanisms we started a collaboration with the group of Adelheid Godt (Bielefeld). In this collaborative project, bis-complexes of the type Gd(III)-spacer-Gd(III) with variable spacer lengths were investigated. These PAs provided an excellent model system where the influence of only inter-spin distances can be determined for a fixed Gd(III) concentration. A small PA concentration of 4 mM is used to ensure absence of significant inter-molecular dipolar interactions. A mono-Gd complex of similar geometry and chemistry is taken as a reference for SE DNP.
The mono-Gd complex yields enhancements arising from SE as expected from negligible inter-molecular Dee. The contribution of CE increases as the inter-spin distances between Gd(III) ions become shorter going from 3.4 nm 2.1 nm 1.4 nm 1.2 nm due to corresponding increase in Dee. The extent of CE on ωn follows the same trend as for Gd-DOTA. Highest CE contribution is observed on nuclei with the smallest ωn 15N because smaller ωn approaches the width of the EPR signal, this is an additional requirement for CE DNP.
The field position for maximum DNP enhancement corresponding to Gd-DOTA, is used for DNP experiments on Ubiquitin with an attached Gd-tag as PA. The success of DNP on this sample illustrates the possibility of site-directed DNP with metal ions tags as PAs. As a perspective Gd-tags can be used to examine change in conformation of a protein that would give higher enhancements due to CE if two Gd(III) labeled domains are closer in space. In a separate project, Mn(II) (s=5/2) bound to the divalent site of a hammerhead ribozyme was used as a PA which resulted in the first demonstration of intra-complex DNP using an intrinsically bound metal ion PA.
Transport mechanism of a multidrug resistance protein investigated by pulsed EPR spectroscopy
(2019)
In human several diseases result from malfunctions of ATP-binding cassette (ABC) systems, which form one of the largest transport system superfamily. Many ABC exporters contain asymmetric nucleotide-binding sites (NBSs) and some of them are inhibited by the transported substrate.1 For the active transport of diverse chemically substrates across biological membranes, ABC transport complexes use the energy of ATP binding and subsequent hydrolysis. In this thesis, the heterodimeric ABC exporter TmrAB2,3 from Thermus thermophilus, a functional homolog of the human antigen translocation complex TAP, was investigated by using pulsed electron-electron double resonance (PELDOR/DEER) spectroscopy. In the presence of ATP, TmrAB exists in an equilibrium between inward- and outward-facing conformations. This equilibrium can be modulated by changing the ATP concentration, showing asymmetric behaviour in the open-to-close equilibrium between the consensus and the degenerate NBSs. At the degenerate NBS the closed conformation is more preferred and closure of one of the NBSs is sufficient to open the periplasmic gate at the transmembrane domain (TMD).3 By determining the temperature dependence of this conformational equilibrium, the thermodynamics of the energy coupling during ATP-induced conformational changes in TmrAB were investigated. The results demonstrate that ATP-binding alone drives the global conformational switching to the outward-facing state and allows the determination of the entropy and enthalpy changes for this step. With this knowledge, the Gibbs free energy of this ATP induced transition was calculated. Furthermore, an excess of substrate, meaning trans-inhibition of the transporter is resulting mechanistically in a reverse transition from the outward-facing state to an occluded conformation predominantly.3 This work unravels the central role of the reversible conformational equilibrium in the function and regulation of an ABC exporter. For the first time it is shown that the conformational thermodynamics of a large membrane protein complex can be investigated. The presented experiments give new possibilities to investigate other related medically important transporters with asymmetric NBSs or other similar protein complexes.
Die Lebensfunktion der Zelle beruht unter anderem auf der Funktion und Wechselwirkung der Nukleinsäuren DNA (2’-Desoxyribonukleinsäure) und RNA (Ribonukleinsäure). Mit Hilfe von PDS (engl. ’pulsed dipolare spectroscopy’)-Techniken, basierend auf der EPR (engl. ’electron paramagnetic resonance’)-Spektroskopie, können Abstände in einem Bereich von 2-10 nm zwischen zwei markierten Positionen einer Nukleinsäure bestimmt werden. Daneben kann mit der Abstandsverteilung auf die Flexibilität des Moleküls geschlossen werden. Durch PDS-Messungen eröffnet sich die Möglichkeit, Bewegungen und Zustandsänderungen zu untersuchen. Die Messungen beruhen auf der dipolaren Kopplung von Radikalen (Spinlabel). Da die gemessenen dipolaren Kopplungen eine anisotrope Wechselwirkung sind, können an starren Systemen neben den Abstandsinformationen auch die Orientierungen der beiden Spinlabel zueinander bestimmt werden. Diese zusätzliche Information ermöglicht es, mittels orientierungsselektiver PDS-Messungen noch genauer die Geometrie und Flexibilität des Systems zu untersuchen. Klassischerweise werden alle Messungen mit der Doppelfrequenztechnik PELDOR (engl. ’pulsed electron-electron double resonance’) durchgeführt. Einzelfrequenzmethoden basieren dagegen auf Breitbandanregung, die mit den technischen Gegebenheiten l nge nicht möglich war. Eine solche Sequenz ist 2D-SIFTER.ImmRahmen dieser Arbeit von PELDOR ausgehende, weiterentwickelte Simulationsprozedur etabliert. Eine große Herausforderung ist die eindeutige Interpretation der sensitiven orientierungsselektiven PELDOR-Messungen. Sie mittels MD (Moleküldynamik)-Simulationen zu beschreiben war bisher nur qualitativ möglich. Allerdings wurden mehrere neue Kraftfelder publiziert. Mit einem quantitativen Vergleich mit orientierungsselektiven PELDOR-Daten kann sichergestellt werden, dass die Flexibilität des Systems durch Kraftfelder richtig beschrieben ist. PELDOR-Zeitspuren, gemessen bei Raumtemperatur und 50 K, unterscheiden sich besonders in ihrer Dämpfung. Der physikalische Unterschied beider Messungen konnte durch MD-Simulationen qualitativ nachvollzogen worden. Eine Schwierigkeit für speziell orientierungsselektive PELDOR-Messungen ist die aufwendige Synthese von mit dem starren Ç-Label markierten Nukleinsäuren. Als Alternative wurde in der Sigurdsson-Gruppe das halbstarre IMU-Label entwickelt. Die Analyse der orientierungsselektiven Daten ergab ein klares Bild der Dynamik dieses Labels. Ein weiterer interessanter Spinlabel ist der `G. Dieser Label ist nicht kovalent gebunden, sondern interkaliert in eine Stelle der Nukleinsäure, in der eine Guanin- Base fehlt. MD-Simulationen im quantitativen Vergleich mit orientierungsselektiven PELDOR-Messungen an verschiedenen Magnetfeldern haben eine hohe Übereinstimmung. Dabei konnte gezeigt werden, dass der Label, interkaliert in eine dsDNA, flippen kann, was zu einer Ausmittelung der Anisotropie führt, allerdings zu keiner Verbreiterung der Abstandsverteilung. Dagegen wird in der dsRNA dieses Flippen um die Einfachbindung sterisch gehindert, so dass neben dem Abstand auch die Orientierung des Labels bestimmt werden kann. Kurze dsRNA-Bausteine tendieren dazu, Oligomere zu bilden, was zu Multispineffekten führte. Zusätzlich beeinflusst diese Aggregation die Dynamik der einzelnen RNAs. Daher musste dieses ’end-to-end’-Stacking verhindert werden. Eine Nukleobasean einem Ende der dsRNA führt zu einer Dimerisierung, während eine Nukleobase an beiden Seiten dieses Stacking vollständig verhindert. Messungen mit unterschiedlichen Salzkonzentrationen konnten zusätzlich zeigen, dass die Interaktion zweier dsRNAs bei höheren Salzkonzentrationen zunimmt.
Pulsed electron–electron double resonance (PELDOR) spectroscopy is a powerful tool for measuring nanometer distances in spin-labeled systems and recently is increasingly applied to membrane proteins. However, after reconstitution of labeled proteins into liposomes, spin labels often exhibit a much faster transversal relaxation (Tm) than in detergent micelles, thus limiting application of the method in lipid bilayers. In the first part of the thesis, optimization of transversal relaxation in phospholipid membranes was systematically investigated by use of spin-labeled derivatives of stearic acid and phosphatidylcholine as well as spin-labeled derivatives of the channel-forming peptide gramicidin A under the conditions typically employed for PELDOR distance measurements. Our results clearly show that dephasing due to instantaneous diffusion that depends on dipolar interaction among electron spins is an important contributor to the fast echo decay in cases of high local concentrations of spin labels in membranes. The main difference between spin labels in detergent micelles and membranes is their local concentration. Consequently, avoiding spin aggregation and suppressing instantaneous diffusion is the key step for maximizing PELDOR sensitivity in lipid membranes. Even though proton spin diffusion is an important relaxation mechanism, only in samples with low local concentrations does deuteration of acyl chains and buffer significantly prolong Tm. In these cases, values of up to 7 μs have been achieved. Furthermore, our study revealed that membrane composition and labeling position in the membrane can also affect Tm, either by promoting the segregation of spin-labeled species or by altering their exposure to matrix protons. Effects of other experimental parameters including temperature (<50 K), presence of oxygen, and cryoprotectant type are negligible under our experimental conditions.
In the second part of the thesis, inhomogeneous distribution of spin-labels in detergent micelles has been studied. A common approach in PELDOR is measuring the distance between two covalently attached spin labels in a macromolecule or singly-labeled components of an oligomer. This situation has been described as a spin-cluster. The PELDOR signal, however, does not only contain the desired dipolar coupling between the spin-labels of the molecule or cluster under study. In samples of finite concentration the dipolar coupling between the spin-labels of the randomly distributed molecules or spin-clusters also contributes significantly. In homogeneous frozen solutions or lipid vesicle membranes this second contribution can be considered to be an exponential or stretched exponential decay, respectively. In this study, it is shown that this assumption is not valid in detergent micelles. Spin-labeled fatty acids that are randomly partitioned into different detergent micelles give rise to PELDOR time traces which clearly deviate from stretched exponential decays. As a main conclusion a PELDOR signal deviating from a stretched exponential decay does not necessarily prove the observation of specific distance information on the molecule or cluster. These results are important for the interpretation of PELDOR experiments on membrane proteins or lipophilic peptides solubilized in detergent micelles or small vesicles, which often do not show pronounced dipolar oscillations in their time traces.
In the third part, PELDOR has been utilized to study the structural flexibility of the Toc34 GTPase homodimer, a preprotein receptor of the translocon of the outer envelope of chloroplasts (TOC). Toc34 belongs to GAD subfamily of G-proteins that are regulated and activated by nucleotide-dependent dimerization. However, the function of Toc34 dimerization is not yet fully understood. Previous structural investigations of the Toc34 dimer yielded only marginal structural changes in response to different nucleotide loads. PELDOR revealed a nucleotide-dependent transition of the dimer flexibility from a tight GDP to a flexible GTP-loaded state. Substrate-binding stabilizes the dimer in the transition state mimicked by GDP-AlFx, but induces an opening in the GDP or GTP-loaded state. Thus, the structural dynamics of bona fide GTPases induced by GTP hydrolysis is replaced by substrate-dependent dimer flexibility, which represents the regulatory mode for dimerizing GTPases.
In the fourth part of the thesis, conformational flexibility and relative orientation of the N-terminal POTRA domains of a cyanobacterial Omp85 from Anabaena sp. PCC 7120, a key component of the outer membrane protein assembly machinery, were investigated by PELDOR spectroscopy. Membrane proteins of the Omp85-TpsB superfamily are composed of a C-terminal β-barrel and a different number of N-terminal POTRA domains, three in the case of cyanobacterial Omp85. It has been suggested that the N-terminal POTRA domains (P1 and P2) might have functions in substrate recognition. Molecular dynamics (MD) simulations predicted a fixed orientation for P2 and P3 and a flexible hinge between P1 and P2. The PELDOR distances measured between the P2 and P3 POTRA domains are in good agreement with the structure determined by X-ray, and compatible with the MD simulations suggesting a fixed orientation between these domains. PELDOR constraints between the P1 and P2 POTRA domains imply a rather rigid structure with a slightly different relative orientation of these domains compared with the X-ray structure. Moreover, the large mobility predicted from MD is not observed in the frozen solution. The PELDOR results further highlight the restricted relative orientation of the POTRA domains of the Omp85-TpsB proteins as a conserved characteristic feature that might be important for the processive sliding of the unfolded substrate towards the membrane.
An application of EPR spectroscopy that is becoming increasingly important is the measurement of distances between electron spins. Several EPR methods have been developed for this purpose, all based on measuring the dipolar coupling between two spins. Due to the specific nature of the sample, we applied dipolar relaxation enhancement measurements to study the geometry of a protein-protein complex. The paramagnetic centers in question had EPR spectra that were too broad and had such short relaxation time that they could not be studied using the more straightforward PELDOR technique. EPR spectral resolution can be increased appreciably by measuring at a frequency higher than conventional X-band (9 GHz) frequency. The spectra of many paramagnetic species can only be resolved at frequencies higher than 90 GHz. For accurate measurement of the orientation of the vector between two dipolar coupled spins with respect to the g-tensors of the spins, high spectral resolution is required. We therefore performed our EPR measurements at G-band (180 GHz) frequency. Dipolar relaxation measurements were applied to study the complex that is formed by the two electron-transfer proteins cytochrome c and cytochrome c oxidase (CcO) from the soil bacterium Paracoccus denitrificans. We were able to detect dipolar relaxation enhancement due to complex formation of soluble subunit II of P.d. CcO (CcOII) with two substrate cytochromes, which was practically absent in a mixture of CcOII with the negative control protein cytochrome c1. This complex formation was characterized by a pronounced temperature dependence that could be simulated using a home-written computer program. The G-band EPR measurements could not be simulated with a single complex geometry. This provided evidence for the hypothesis that electron-transfer protein complexes are short-lived and highly dynamic; they do not seem to form one specific electron-transfer conformation, but rather move around on each other’s binding surfaces and transfer an electron as soon as the distance between donor and acceptor is short enough. As a test of our simulation program, we also applied dipolar relaxation measurements to specially synthesized organic molecules that contained a nitroxide radical and a metal center. The transverse relaxation of Cu2+-OEP-TPA was compared to the relaxation of Ni2+-OEP-TPA at temperatures between 20 and 120 K. In this temperature range, the nitroxide relaxation was enhanced due to the presence of Cu2+, but not by Ni2+. Similarly, relaxation enhancement was found in the nitroxide-Mn2+ pair in Mn2+-terpyridine-TPA with respect to the terpyridine-TPA ligand. Due to the fast T2 relaxation of the nitroxide radical at high temperatures, the measurements were all performed in the low-temperature regime where the T1 relaxation rate of the metal ion was smaller than the dipolar coupling frequency. In this region, no structural information about the molecule can be deduced, since the dipolar relaxation enhancement is only determined by the T1 of the metal ion. The dipolar relaxation measurements we performed at high field indicated a difference in relaxation times between X-band and G-band frequencies. Extensive T1 - measurements of different paramagnetic centers (CuA, Cu2+) confirmed a strong dependence of T1 on magnetic field in the temperature range where the direct process is the dominating T1 relaxation process. This dependence is very strong (factor of 103 with respect to X-band), but does not follow the B04 dependence predicted in literature. The T1 relaxation of low-spin iron in cytochrome c at high magnetic field, estimated from dipolar relaxation data, is also in agreement with a larger contribution by the direct process (factor of 104). Dipolar relaxation enhancement was found to be a technique that is useful for measuring distances between paramagnetic centers, but only for systems where several important conditions are met, such as: the system exists in one certain static geometry, and the relaxation rate of the fast-relaxing spin is faster than the dipolar coupling frequency within the accessible temperature range. Additionally, it is a great advantage for the analysis of dipolar relaxation data if the procedure of dividing the relaxation trace of the dipolar-coupled slow-relaxing spin by the relaxation trace of the slow-relaxing spin in absence of dipolar coupling can be applied. Another useful application of dipolar relaxation enhancement measurements is the measurement of T1 relaxation of extremely fast-relaxing spins, or spins that are otherwise difficult to detect.
The mitochondrial respiratory chain consists of NADH:ubiquinone oxidoreductase (Complex-I), succinate:ubiquinone reductase (Complex-II), ubiquinol:cytochrome c reductase (Complex-III), cytochrome c oxidase (Complex-IV) and cytochrome c as an electron mediator between Complex-III and Complex-IV. Paracoccus denitrificans membranes were used as a model system for the association of the mitochondrial respiratory chain. More than 50 years ago, a model was given for a supercomplex assembly formed by stable associations between these complexes. This model gradually shifted by the model of random diffusion given by Hackenbrock et al. 1986 Different independent approaches were used to further analyze this situation in a native membrane environment, thus avoiding any perturbation caused by detergent solubilization: (a) measuring the distance and orientation of the different complexes by multi-frequency EPR Spectroscopy we started to analyze simple system, the interaction between CuA fragment derived from P. denitrificans and various c type cytochrome by Pulsed X band and G band (180 GHz) EPR. Partner proteins for the CuA (excess negative surface charge) were (i) horse heart cytochrome c which contain a large number of positive charges in heme crevice,(ii) the cytochrome c552 soluble fragment (physiological electron donor and have positive charges), and as a control (iii) the cytochrome c1 soluble fragment (negative surface potential, derived from bc1 complex) The measurements were performed at several magnetic field positions varying temperature between 5 to 30 K. Both the X band and the high-field measurements show the existence of a strong relaxation enhancement of the CuA by the specific binding of the P. denitrificans cytochrome c552 and horse heart cytochrome c. This relaxation enhancement is dependent on temperature and provides information about the distance and relative orientation of the two interacting spins within this protein-protein complex. (b) For quantitative information about lateral diffusion of cytochrome c oxidase in the native membrane Fluorescence Correlation Spectroscopy (FCS) was used. In this experiment, diffusion coefficients for oxidase differ in the case of supercomplex for wild type membrane and for two deletion mutants lacking either Complex-I or Complex-III. (c) The optical absorption spectroscopy at microsecond level resolution was tried for the translational mobility of oxidase in membrane vesicles. Due to the presence of different hemes in the native membrane, carbon monoxide (CO) used as a probe for the experiment. The optimization of the experimental conditions were carried out to get the optimal signal.
One of the most important tasks in chemistry and especially in structural biology has always been the elucidation of three-dimensional molecular structures - either of small molecules or large biopolymers. Among the (bio)physical methods to acquire structural data at atomic resolution electron paramagnetic resonance (EPR) spectroscopy is the most valuable technique for obtaining structural information about many different kinds of paramagnetic species. In biological systems, either paramagnetic metal ions/clusters, transient paramagnetic intermediates in electron transfer processes or artificially attached stable spin labels can be found. The usual approach to interpret EPR spectra is to perform simulations based on the so-called spin Hamiltonian (SH). This means that the well-defined numerical parameters (tensors) in the SH representing different types of interaction are obtained by fitting the experimental data. The SH parameters include electronic g-values, hyperfine coupling (HFC) and quadrupole coupling (&C) constants, zero-field splittings and constants to describe exchange and dipolar interactions between electron spin systems. However, since the SH only contains spin degrees of freedom, a direct translation of the SH EPR parameters into structural information is not straightforward. Therefore, methods to predict such SH interaction parameters starting from molecular structures are required. In this thesis it was investigated whether quantum chemical calculations of EPR parameters based on density functional theory (DFT) methods may be employed to overcome these problems thus enabling a correlation of experimental EPR data with molecular structure. It was the central goal of this work to point out the potential of a fruitful interplay between quantum chemistry and experiment and to study how both can benefit from each other. For this purpose DFT methods were applied to a variety of organic radical or transition metal systems to calculate different EPR parameters. Using the 'broken symmetry' formalism it was possible to compute the exchange coupling constant for a nitroxide biradical and furthermore decompose the exchange mechanism in different through-bond and through-space interactions. Spin density distributions, 14N and 1H HFC constants as well as dipole moments and polarizabilities were computed for a number of aromatic nitroxides to examine their properties and select promising candidates which may serve as DNA-intercalating spin labels. Systematic investigations of the influence of hydrogen bond geometry on the 14N QC parameters for imidazole-water and methylimidazole-benzosemiquinone complexes lead to the conclusion that especially the imidazole amino nitrogen &C parameters are very sensitive probes of the bond geometry, in particular of the hydrogen bond length. The results of this study may be applied to biological systems, e.g. to gain structural information about quinone binding sites. Moreover, quantum chemical methods were applied to elucidate the structure of a nitrogen-centered radical intermediate in the inhibition process of ribonucleotide reductase (RNR). It was possible to find a molecular structure in accordance with all experimentally available data, thus revealing the longsought structure of the No radical and providing evidence for the trapping of a 3'-ketonucleotide in the reduction process catalyzed by RNR. To test the capability of modern DFT methods to predict g- and molybdenum HFC tensors for MoV complexes, validation studies were carried out. Comparison of computed EPR parameters of a number of MoV compounds with corresponding experimental values showed that g- and HFC tensors could be predicted in good accuracy, although some systematic errors of the computational methods have to be considered for such heavy 4d1 transition meta1 systems. Furthermore, DFT calculations on a Mn2+ binding site model of the hammerhead ribozyme allowed to conclude that the structure of the binding site as studied by EPR spectroscopy in frozen solution is very likely to be identical to the site found occupied by Mn2+ in crystals. Finally, computational methods were employed to aid in the structural characterization of the Mn2+ binding site in Ras (rat sarcoma protein) by providing accurate starting parameters for spectral simulations and furthermore helping to interpret the experimental data. In conclusion, it was demonstrated in this thesis that the combination of sophisticated experimental and quantum chemical methods represents a powerful approach in the field of EPR spectroscopy and that it may be essential to employ EPR parameter computations to extract the full information content from EPR spectra. Therefore, great potential lies in future applications of DFT methods to the large number of systems where detailed and reliable experimental data is available but where an unequivocal correlation of these data with structural information is still lacking.
One of the central research topics in the field of biophysical chemistry is the structure and function of membrane proteins involved in energy transduction. Both, the aerobic and the anaerobic respiration include electron transfer and proton translocation across the mitochondrial and bacterial membranes. These electron transfer processes lead to changes in oxidation states of cofactors some of which are paramagnetic. Therefore, EPR spectroscopy is the method of choice to obtain electronic and structural information directly related to the function of the respiratory chain proteins. In this work, multifrequency continuous wave (CW) and pulsed EPR spectroscopy has been used to characterize the molybdenum active site of polysulfide reductase (Psr) from the anaerobic bacterium Wolinella succinogenes and the protein-protein complex between cytochrome c oxidase (CcO) and cytochrome c from the aerobic bacterium Paracoccus denitrificans. Molybdenum in Psr-Psr is an enzyme essential for the sulfur respiration of Wolinella succinogenes. Biochemical studies suggested that the active site of this enzyme contains a mononuclear Mo center, which catalyzes the reduction of the substrate polysulfide to sulfide. Until now there is no crystal structure available for Psr. Consequently, current characterizations of this enzyme have to rely on biochemical and spectroscopic investigations. Within the present work, CW and modern pulsed EPR techniques were applied to investigate its catalytically active site. In the first part of this thesis, different redox agents have been used to generate paramagnetic states of Psr. Multifrequency CW-EPR spectroscopy was applied to identify the Mo(V) states. Using simulations of the experimental spectra, three spectroscopically distinct states have been identified based on the Mo hyperfine- and g-tensor values. Comparison of their EPR parameters with those of related enzymes indicated five or six sulfur ligands at the Mo center depending on the state. The state generated by addition of polysulfide is suggested to be the catalytically active form, in which the Mo is coordinated by a sulfur of the polysulfide chain as the sixth ligand. 33S (I = 3/2) labeled polysulfide was prepared to probe the proximity of the polysulfide to the molybdenum center via its hyperfine coupling. 1D-ESEEM and 2D122 HYSCORE spectroscopy was used to detect these hyperfine and quadrupole interactions, which are too small to be observed in conventional CW EPR spectra. To date there has been only one pulsed-EPR study involving a 33S nucleus [Finazzo et.al. 2003]. The reasons are that this nucleus has a high nuclear spin of I = 3/2 and a large nuclear quadrupole moment in addition to the low Larmor frequency. All these make the detection of sulfur and the extraction of structural information demanding. However, analysis of the 2D-data led to a Mo(V) 33S distance in a range of about 2 to 2.5 Å. Mo-S distances found in molybdenum enzymes of the same family are in a range of 1.8 to 2.8 Å suggesting that the 33S is indeed the sixth ligand of the Mo(V) center and demonstrating that polysulfide is the actual substrate for this enzyme. Thus HYSCORE experiments have been proved to be a powerful technique to gain further insight into the active site structures of molybdenum enzymes and the trafficking of substrate atoms during catalysis. Density functional theory (DFT) calculations together with quantitative numerical simulations of the 2D-data will help to obtain more structural details about the molybdenum binding site in Psr. CcO:cytochrome c complex Protein-protein complex formation is an important step in energy conversion biological processes such as respiration and photosynthesis. These protein-protein complexes are involved in long range electron transfer reactions and are known to be of transient nature. Within the bacterial and mitochondrial respiratory electron transport chains such a complex is formed between CcO and cytochrome c. Upon complex formation cytochrome c donates the electrons required for the CcO catalyzed reduction of dioxygen to water. Here, the protein-protein complex formation between CcO and cytochrome c from Paracoccus denitrificans was investigated by pulsed EPR spectroscopy. The idea was to use the relaxation enhancement due to the distance and orientation dependent magnetic dipole-dipole interaction between the paramagnetic centers in the different CcO constructs and cytochromes. Two-pulse electron spin echo experiments were carried out on mixtures of the CuA containing soluble subunit II or the full size CcO with the physiological partner cytochrome c552 or horse heart cytochrome c. Significantly enhanced relaxation of CuA due to specific protein-protein complex formation has been observed in all four cases. In contrast the non-binding cytochrome c1 showed only a very weak relaxation enhancement due to unspecific protein-protein interactions. The echo decays of the slowly relaxing observer spin (CuA of CcO) measured in the absence and presence of the fast relaxing spin (Fe(III) of cytochrome c) permitted the extraction of the pure dipolar relaxation contributions for the different complexes. Measurements at different temperatures proved the dipolar nature of the relaxation enhancement. Furthermore, it was demonstrated experimentally that this approach also works for the full-size CcO, which contains four paramagnetic metal centers, in complex with cytochrome c. Quantitative simulations of the data suggest a broad distribution in distances (2 - 4 nm) and orientations between the CuA and Fe(III) in the complex between CcO and cytochrome c. High-field EPR spectroscopy will be useful to further analyze and prove these complex structures. Within the present work, it has been shown that pulsed relaxation enhancement experiments can be used to investigate the distance and relative orientation between paramagnetic metal centers. Furthermore, it has been demonstrated on a qualitative level, that this method can be used complimentary to other biophysical approaches to study transient electron transfer protein-protein complexes. Finally, within this work it has been proven that this method can be applied also to biological systems where more than two paramagnetic centers are present. This is particularly interesting for supercomplexes between membrane proteins.
Die Kernspinresonanz(NMR)-Spektroskopie ist ein leistungsstarkes analytisches Werkzeug. Allerdings ist ihre Empfindlichkeit aufgrund geringer Wechselwirkungs-energie zwischen den Kernspins und dem externen Magnetfeld begrenzt. Die dynamische Kernpolarisation (DNP) erhöht DNP die Empfindlichkeit der NMR, indem sie die Polarisation von ungepaarten Elektronenspins auf die benachbarten Kernspins überträgt. In den letzten Jahrzehnten hat die DNP bei hohen Magnetfeldern erneut an Aufmerksamkeit gewonnen, bedingt durch die Verfügbarkeit leistungsstarker Gyrotron-Mikrowellen(mw)-Quellen. Jedoch wurde die Anwendung von DNP für Flüssigkeiten im Vergleich zu Festkörperproben bei niedrigen Temperaturen (≈100 K) weit weniger erforscht. Zwei Gründe können dafür hauptsächlich benennt werden. Bei hohen Magnetfeldern (entsprechend hohen mw-Frequenzen) wird die mw-Strahlung sehr stark von Flüssigkeiten absorbiert, was zu einer starken Erwärmung führt. Darüber hinaus sind die Translations- und Rotationsdynamik der Radikale und Target-Molekülen nicht schnell genug, um Spectraldichten bei den hohen mw-Frequenzen zu erzeugen, die für eine Overhauser-Effekt (OE) DNP Verstärkung benötigt werden. In dieser Arbeit wird gezeigt, Flüssigzustands-DNP bei hohen Magnetfeldern, insbesondere bei 9,4 T, mit hocheffizienten DNP-Probenköpfen möglich ist.
Der von skalaren Hyperfein-Wechselwirkung (hfWW) angetriebene OE ist für Flüssigzustands-DNP-Forschungen von besonderem Interesse, da der von der Theorie vorhergesagte Mechanismus auch bei hohen Magnetfeldern noch effizient ist. In der vorliegenden Arbeit wurde eine Methode zur Vorabprüfung potenzieller DNP-Kandidaten durch Messungen ihrer paramagnetischen NMR-Verschiebungen vorgeschlagen und untersucht. Wir beobachtete signifikante 13C-skalare OE DNP-Verstärkungen bis zu 50 bei den ausgewählten kleinen Biomolekülen, einschließlich Imidazol, Indol, verschiedene Aminosäuren und Kohlenhydraten. Das Lösungssystem wurde auch von organischen Lösungsmitteln auf Wasser erweitert.
Im Kontext von dipolarer OE DNP haben wir den Beitrag der Rotation des Radikals neben der Translationsbewegung zwischen Radikal und Target-Molekül zur OE DNP-Effizienz systematisch untersucht, indem wir verschiedene Nitroxidderivate mit unterschiedlichen Ringgeometrien und Substituenten verwendet haben. Mithilfe eines Models, das eine 'out-sphere' Translationsbewegung und eine 'inner-sphere' Rotationsbewegung des Radikal-Lösungsmittel-Komplexes enthält, konnte unsere Beobachtungen quantitativ simuliert werden. Außerdem wurde ein anderes Model untersucht, das eine Translationsbewegung mit der Rotation von Radikalen, bei denen das ungepaarte Elektron nicht im Zentrum sitzt, kombiniert.
Eine weitere neue Entdeckung in der DNP bei hohen Magnetfeldern waren der beobachtete SE (Solid-Effekt) an Lipidmolekülen mit BDPA-Radikal oberhalb der Lipidphasen-übergangstemperatur. Die neue Anwendung von SE DNP bietet einen alternativen Mechanismus zur OE DNP in Flüssigkeiten bei hohen Magnetfeldern und könnte möglicherweise auf Makromoleküle mit relativ langsamer Rotationsbewegung angewendet werden.
Wir haben zusätzliche Untersuchungen an den Lipiddoppelschichten mit Nitroxid-radikale durchgeführt, basierend auf dem beobachteten 1H DNP-Verstärkungen in einer viskosen Lipidumgebung bei 9,4 T . Durch Messung des Feldprofils wurden DNP-Verstärkungen durch OE und SE in Abhängigkeit ihrer relativen Verschiebungen von der Elektronen-Larmor-Frequenz bestimmt. Die individuelle OE DNP-Effizienzen für Protonen des Wassers, der Lipid-Cholin-Kopfgruppen oder der Lipid-Acylketten wurde bestimmt. Dadurch wird ein quantitativer Vergleich mit MD-Simulationen ermöglicht. Obwohl die von der MD-Simulationen vorhergesagten DNP Kopplungsfaktoren noch deutliche Abweichungen von den experimentellen Beobachtungen aufweisen, wird die schnelle Dynamik nahe der Elektronen-Larmor-Frequenz, die für einen erfolgreichen OE DNP Transfer erforderlich ist, von den MD-Simulationen gut erfasst.
In der Arbeit wurden auch zwei unterschiedliche Dreifachresonanz-DNP-Experimente durchgeführt. Zum einen wurde 13C OE DNP unter 1H-Entkopplung in wässriger Natriumpyruvatlösung, und zum anderen 13C-NMR von Glycin, verstärkt durch SE DNP an 1H zusammen mit einem 1H-13C INEPT-Polarisationstransfer, im Rahmen dieser Doktorarbeit durchgeführt.
Ferroelektrische Strontium-Wismut-Tantalat- (SBT) Filme werden in der Mikroelektronik als nicht-flüchtige Speichermedien verwendet und weiterentwickelt. Informationen werden durch Polarisation des Materials gespeichert und bleiben ohne weiteren Energieaufwand über einen Zeitraum von Jahren in solchen Speichern erhalten – sogenannten FeRAMs (Ferroelectric Random Access Memories). Darüber hinaus können gespeicherte Daten innerhalb von wenigen Nanosekunden wieder ausgelesen werden. Zusammengefasst ist eine Langzeitspeicherung kombiniert mit niedrigem Energieverbrauch und schneller Informationsverarbeitung durch den Einzug ferroelektrischer Materialien in die Computertechnologie möglich geworden.
Da die fortschreitende Miniaturisierung in der Mikroelektronik von zentraler Bedeutung ist, sind zur Charakterisierung der verwendeten Materialien Untersuchungsmethoden mit hoher Ortsauflösung unverzichtbar. Das Rasterkraftmikroskop – engl. Atomic Force Microscope (AFM) – ist eine solche Technik, mit der im Submikrometerbereich die Topographie sowie physikalische Eigenschaften von Materialien abgebildet werden können. Die vorliegende Arbeit widmet sich der Untersuchung von SBT-Filmen mit solchen AFM-Methoden.
Besonders die Rauhigkeit der einzelnen Filme in schichtartig aufgebauten Mikrochips ist bei der Herstellung von Halbleiterbauelementen von großer Bedeutung, wobei möglichst glatte Filme favorisiert werden. Deshalb wurden zunächst verschiedene SBT-Filme auf ihre topographischen Merkmale hin charakterisiert. Die Rauhigkeiten von SBT Filmen verschiedener Herstellungsverfahren wie der Metal Organic Decomposition (MOD) und der Metal Organic Chemical Vapour Deposition (MOCVD) wurden gegenübergestellt. Außerdem ist der Einfluss der SBT-Schichtdicke sowie der des Ferro-Anneals untersucht worden – Ferro-Anneal ist ein Temperungs-Schritt während der Filmherstellung, der zur Bildung der ferroelektrischen Aurivillius-Phase durchgeführt werden muss. Zudem wurde das unterschiedliche Kurzschlussverhalten zweier SBT-Filme in Zusammenhang mit ihren verschiedenen RMS-Rauhigkeitsdaten gebracht.
Der größte Teil der Arbeit setzt sich mit einer Methode auseinander, mit der die Polarisationseigenschaften von ferroelektrischen SBT-Filmen charakterisiert werden sollen – dem AFM/EFM-Polarisationsexperiment – engl. Electrostatic Force Microscope (EFM). Die SBT-Filme werden dabei mit einer AFM-Spitze polarisiert und in einem zweiten Schritt die daraus resultierenden elektrostatischen Felder mit einem EFM über der Probe abgebildet. Es wurde dabei kritisch hinterfragt, in wieweit diese Methode als Beurteilungskriterium der Materialeigenschaften herangezogen werden kann. Zudem wurden Aufladungsphänomene bei dieser Versuchsführung dokumentiert.
Außerdem wurde das Leckstromverhalten von SBT-Filmen auf der Submikrometerskala mit einer relativ neuen Messmethode, dem conducting-AFM (C-AFM), untersucht.
Die Ergebnisse aller Untersuchungen sind im folgenden stichpunktartig dargestellt.
Topographieuntersuchungen:
• Die RMS-Rauhigkeit von MOD/SBT-Filmen ist größer als die der MOCVD/SBTFilme. Mit steigender Prozesstemperatur des Ferro-Anneals wird die Oberflächenrauhigkeit von SBT-Filmen erhöht.
• SBT-Filme, die mit niedrigen Prozesstemperaturen hergestellt wurden, hier als Niedrigtemperatur-Filme bezeichnet, erfahren mit zunehmender Schichtdicke eine Glättung. Sie ist auf die Einbettung der Kristallite in die verhältnismäßig glatte FluoritPhase zurückzuführen, die wegen der geringen Temperaturen während des FerroAnneal-Prozesses noch nicht vollständig in die rauere ferroelektrische AurivilliusPhase umgesetzt wurde.
• Die unterschiedliche Zusammensetzung der Filme SrxBi2.2Ta2O8,3+x mit X1 = 0.9 und X2 = 1,0, im Text als Sr0,9-Film und Sr1,0-Film bezeichnet, führte zu höheren Kurzschlussraten des Sr0,9-Films in fertiggestellten FeRAM-Kondensatoren. Die Ursache kann auf die höhere Oberflächenrauhigkeit des Sr0,9-Films zurückgeführt werden. EFM-Untersuchungen:
• Bei der Polarisation ferroelektrischer SBT-Filme mit einer elektrisch gepolten AFMSpitze werden Ladungen in undefinierbarer Anzahl auf die Oberflächen gebracht. Diese Ladungen sind mehr oder weniger auf den Oberflächen beweglich. Mit zunehmender Polarisierbarkeit des ferroelektrischen Films wird die Ladung stärker am Polarisationsort durch elektrostatische Anziehung zwischen den orientierten Dipolen und der Oberflächenladung fixiert.