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The human Long Interspersed Nuclear Element-1 (LINE-1, L1) is a member of the group of autonomous non-LTR retrotransposons found in almost every eukaryotic genome. L1 elements generate copies of themselves by reverse transcription of an RNA intermediate and integrate into the host genome by a process called Target Primed Reverse Transcription (TPRT). They are responsible for the generation of approximately 35% of the human genome, cover about 17% of the genome and represent the only group of active autonomous transposable elements in humans. L1 activity bears several risks for the integrity of the human genome, since the L1-encoded protein machinery generates DNA double-strand breaks (DSBs) and is capable of conducting numerous genome-destabilizing effects, e.g. causing deletions at insertion sites, disrupting or rearranging coding sequences and deregulating transcription of functional host genes. On the other side, L1 elements have had and still exert a great impact on human genome structure and evolution by increasing the genome size and rearranging and modulating gene expression. Furthermore, due to its endogenous and generally non-pathogenic nature, L1 is a promising candidate as vector for gene delivery in somatic gene therapy. The structure of the flanking regions between de novo L1 integrants and the genomic sequence suggests an involvement of cellular DSB repair pathways in L1 mobilization. To elucidate the role of DSB repair proteins in L1 retrotransposition, I disabled DSB repair factors ATM, ATR, DNA-PK, p53 and Ku70 by knock down (KD) using short hairpin RNA (shRNA) expression constructs. To inhibit the function of DSB repair factors PARP and Rad51, I used dominant negative (DN) PARP and Rad51 mutants. Applying a well established L1-retrotransposition reporter assay in HeLa cells, de novo retrotransposition events were launched in order to test L1 for its retrotransposition activity in the context of altered DSB repair conditions. I could show that L1 retrotransposition frequency after ATM KD had increased by 3-fold, while ATR and p53 KD reduced L1 retrotransposition by approximately one third. Unfortunately, the cytotoxic effects of the DNA-PK and Ku70 shRNA expression constructs were too strong to determine potential effects of DNA-PK and Ku70 KD on L1 retrotransposition. Inhibition of PARP function by expression of the DN mutant and overexpression of wild type PARP were found to increase L1 retrotransposition by 1.8 and 1.5, respectively, while Rad51 DN had no detectable effect. Interestingly, overexpression of wild type Rad51 seemed to roughly double L1 retrotransposition frequencies. Since in my experiments KD or expression of DN mutants was time-delayed to the onset of L1 retrotransposition after transfection into the cells, I developed a temporally controllable, tetracyclin transactivator (tTA)-dependent L1 retrotransposition reporter assay which will be of great value for future L1 retrotransposition studies that rely on temporally controllable retrotransposition. Due to a previously published hypothesis of L1 playing a role in brain development by contributing to somatic mosaicism in neuronal precursor cells, I generated a transgenic mouse (LORFUS) using the tTA-dependent L1 construct to further test this hypothesis. LORFUS harbors a bidirectional cassette driving simultaneous expression of a GFP-tagged L1 retrotransposition reporter and beta-galactosidase. It was bred to another transgenic mouse line expressing tTA in the forebrain. The double transgenic offspring was used to characterize L1 expression and retrotransposition patterns in the brain at postnatal day 15 (P15). General transgene expression indicated by beta-galactosidase activity was found in hippocampus, cortex and striatum, while retrotransposition events revealed by GFP expression were found in hippocampus, cortex, striatum, olfactory bulb and brainstem. These results suggested L1 retrotransposition in the granule layer of the dentate gyrus earlier than P15 and migration of cells carrying these events along the rostral migratory stream into the olfactory bulb. To facilitate the use of L1 as gene delivery tool in gene therapy or genetic engineering, I furthermore intended to manipulate the L1 target site recognition to allow the site-specific integration into defined genomic locations. To this end, I performed crystal structure-guided mutational analysis exchanging single amino acid residues within the endonuclease (EN) domain of L1 to identify residues influencing target site recognition. However, individual point mutations did not change the nicking pattern of L1-EN, but resulted in a reduction of endonucleolytic activity reflected by a reduced retrotransposition frequency. This suggests that additional factors other than the DNA nicking specificity of L1-EN contribute to the targeted integration of non-LTR retrotransposons in the host genomes.
This thesis primarily covers a systematic assessment of quantum chemical methods to predict accurate 19F NMR shifts for fluoroarenes and magnetic exchange coupling constant (J) in organic spin dimers which are basic building blocks for rational designing of organic magnetic materials.
One of the most important goals in chemistry is to design and synthesize molecules with optimum properties. This thesis is divided into two parts: the first part comprises of a systematic effort to find an inexpensive quantum chemical method to predict accurate 19F NMR chemical shifts (within an accuracy of 2 ppm) for perfluoraromatics. Essentially, these strenuous efforts have been devoted to find best DFT functional and basis set combination to predict accurate 19F shifts. In addition,the influence of geometrical parameters, solvents, chemical environment was also analyzed. Various correction approaches were tested to correct the calculated shifts. The influence of various functionals and basis sets was also analyzed on the correction efficiency of an individual scheme. All the NMR calculation methods already being used and correction approaches were verified to predict shifts of three different fluorine-substituted molecular sets. These structure sets include fluorobenzenes, substituted benzenes and fluorine substituted aromatic fused rings (e.g. fluorine substituted anthracene).
In the second part of this thesis, we investigated the accurate prediction of magnetic exchange couplings (J) for organic spin dimers using quantum chemical methods. We analyzed the performance of various DFT methods and various post-HF methods, such as the CASSCF, CASPT2, MSTDISD, DDCI1, DDCI2, DDCI3, and FCI to predict magnetic exchange couplings (J).
Overview of the Chapters:
Chapter 1, presents a brief theoretical introduction to the Schrödinger equation and its application in quantum mechanical calculations, the Hartree-Fock approximation, basis sets, electron correlation energy, and density functional theory (using pure and hybrid functionals).
In chapters 2 and 3, an introduction is given for quantum chemical approaches used to calculate NMR parameters and magnetic exchange coupling constants. We discuss an effective spin Hamiltonian, the Breit-Pauli Hamiltonian (BPH), chemical shielding tensor and total energy relationship, measuring of the NMR spectra, and different techniques to deal with gauge origin problem. In addition, the theoretical background of magnetic exchange coupling constant calculation for spin dimers, the Heisenberg-Dirac-van-Vleck Hamiltonian (HDVV) and the Noodelman's broken-symmetry approach for calculating J values are briefly discussed.
Chapter 4, presents a benchmark study of various DFT functionals and basis sets to calculate accurate C-F bond lengths and 19F chemical shifts. High-resolution NMR spectral data of complex molecules are often difficult to interpret. Great scientific efforts have been devoted to search for a computational approach to interpret experimental NMR data. Quantum chemical methods such as the CCSD(T) method offer high accuracy in calculation of NMR parameters but being computationally too demanding they cannot be applied to large chemical systems. On the other hand, density functional theory (DFT) is achieving a steady progress among diversity of computational techniques. An accuracy within 2 ppm deviation from the experimental values in 19F chemical shifts can be achieved if the NMR calculation is performed using accurate equilibrium geometries, GIAO is used to tackle gauge origin problem and electron correlation is properly treated by employing a high level of theory (e.g. CCSD (T)/cc-pVQZ). We found that the calculation of 19F shielding tensors with the density-functional theory does not provide any noticeable improvement over the HF method. Post-HF theory demands too much computational resources that makes them impossible to use for large systems [35] .
We found that a quantitative prediction of NMR shifts can be made as the errors introduced by theoretical methods are cancelled out while calculating shifts. Various benchmark studies in this thesis show that 19F chemical shifts calculated for perfluoraromatics with the M06-L, BHandH, BHandHLYP in combination with the 6-311+G (2d,p) basis set are within 4 ppm deviation from the experiments. Furthermore, we noted that NMR calculations on accurate
C-F (e.g. PBE/6-311G (d, p)) bond lengths does not show any improvement if the NMR calculation and optimization are performed at the same level of theory. A significant improvement can be achieved on calculated 19F NMR shifts, if some correction schemes are used.
In chapter 4 we discuss various correction schemes applied to correct the calculated 19F chemical shifts. A multi-standard approach (MSTD) was used to minimize the error that may occur due to the difference in the nature of the reference compound and test molecules [122]. We propose another approach to correct shielding constants which is the reference corrected approach. This approach makes a correction similar to the MSTD. We also tested a Linear Regression Correction Approach and we noted that this is the best approach amongst all. This is found to be less dependent on the theoretical method. We use conformation averaging corrections to correct the calculated shifts[126].
...
This thesis reports on the results obtained by expression photoactivatable adenylyl cyclase from Beggiatoa spp. (bPAC) in cholinergic neurons from Caenorhabditis elegans (C. elegans) and the characterization of the role of a single neuron, RIS, during locomotion in the adult animal.
Pharmacological activation of adenylyl cyclases through Forskolin is known to induce increased neuronal output in diverse model organisms through a protein kinase A (PKA) dependent mechanism. Nevertheless, pharmacological assays are not spatially restricted, do not allow for precise and acute activation nor to cessation of the signal. Thus, an optogenetic approach for was selected trough the expression of photoactivatable adenylyl cyclase from Beggiatoa spp. (bPAC) in cholinergic neurons of Caenorhabditis elegans (C. elegans). This model organism was chosen due to its transparency, ease of maintenance, fast generation cycles as well as for being an eutelic animal. Further, its genome has been fully sequenced and the connectome of the neuronal network is known, thus allowing for precise analysis of neuronal function. Furthermore, the molecular mechanisms governing neuronal functions are well conserved up to primates. Mainly two optogenetical tools were applied, bPAC and the light gated cation channel channelrhodopsin 2 (ChR2).
Behavioral assays of bPAC photostimulation in cholinergic neurons recapitulated previous work performed with the photoactivatable adenylyl cyclase from Euglena gracilis (EuPACa), in which swimming frequency and speed on solid substrate were increased. Electrophysiological recordings of body wall muscle (BWM) cells by Dr. Jana F. Liewald showed that bPAC photoactivation led to an increase in miniature postsynaptic current (mPSC) rate and, in contrast to ChR2 invoked depolarization, also amplitude. Analysis of mutants deficient in neuropeptidergic signaling (UNC- 31) via electrophysiology performed by Dr. Jana F. Liewald showed that the increase in mPSC amplitude due to bPAC photoactivation requires neuropeptide release. This was confirmed by co-expression of bPAC with the neuropeptide marker NLP-21::Venus and subsequent fluorescence analysis of release, exploiting the fact that released neuropeptides are ultimately degraded by scavenger cells (coelomocytes). These were enriched with NLP-21::Venus after bPAC photostimulation, but no fluorescence could be observed in the UNC-31 mutants.
Additional analysis of the electrophysiological data performed by myself showed no modulation of mPSC kinetics dues to neuropeptidergic release induced by bPAC. Hence, neuropeptide release and action sites were in the cholinergic neurons, the latter including cholinergic motoneurons.
Dr. Szi-chieh Yu provided electron microscopy images of high pressure frozen, bPAC or ChR2 expressing animals. These were tagged by myself for automatic analysis of ultrastructural properties of the cholinergic presynapse, also during photoactivation of both optogenetic tools. Photoactivation of both induced a reduction of synaptic vesicles, with ChR2 showing a more severe effect. In contrast to ChR2, though, bPAC also reduced the amount of dense core vesicles (DCV), the neuropeptide transporters. Additionally, long bPAC photoactivation as well as ChR2 photoactivation led to the appearance of large vesicles (LV), presumably in response to the increased SV fusion rate. bPAC photostimulation also induced an increase in SV size, not observed after ChR2 photostimulation. In UNC-31 mutants, bPAC photostimulation could not lead to the SV size increase, a further argument for the presynaptic effect of the released neuropeptide. Additional analysis of electrophysiology paired with pharmacology, performed by Dr. Jana F. Liewald, showed that mPSC amplitude increase requires the function of the vesicular acetylcholine transporter.
A further effect observed in the ultrastructure of bPAC photostimulated cholinergic presynapses was a shift in the distribution of SV regarding the dense projection. An analysis of cAMP pathway mutants showed that synapsin is required for bPAC induced behavior effects. Synapsin is known to mediate SV tethering to the cytoskeleton. Here, I show evidence for a new role of synapsin in controlling the availability of DCVs for fusion and thus, in neuropeptidergic signaling.
In the second part of my thesis I characterized the function of the GABAergic interneuron RIS in the neuronal network of C. elegans. RIS was shown to induce lethargus, a sleep-like state, during all larval molts, but its function in the adult animal was not yet described. Specific RIS expression of ChR2 achieved by a recombinase based system allowed to acutely depolarize the neuron during locomotion, which led to an acute behavioral stop. Diverse signal transduction pathway mutants were analyzed showing that the phenotype was induced by neuropeptidergic signaling. Through mutagenesis followed by whole genome sequencing data analysis as well as analysis of RIS specific RNA sequencing data further narrowed the signal transduction pathway to mediate the locomotion stop behavior. Since the neuropeptide and, to some extent, the neuron are conserved across nematodes, an argument is outlined in favor of the conservation of this sleep-like state.
In addition, since ChR2 could induce neuropeptidergic signaling from RIS, secretion of vesicles is regulated by variable pathways depending on the neuronal identity. Nevertheless, expression of bPAC in RIS allowed to optogenetically increase the probability of short stops, as observed by expression of a calcium sensor (GCaMP) in RIS and analysis of its intrinsic activity in the adult animal.
Die Etablierung der Festphasensynthese innerhalb der letzten Jahrzehnte macht hoch modifizierte Oligonukleotide verfügbar. Damit werden Methoden wie Einzelmolekül-aufgelöstes Tracking möglich, um beispielsweise den Weg einer einzelnen RNA von der Transkriptionsstelle im Nukleus bis zur Proteinbiosynthese im Cytoplasma verfolgen und kritische Stelle verstehen zu können. In den letzten Jahren entwickelten sich auch vermehrt Fragen zur lokalen Proteinsynthese. Dabei nimmt man besonders im Fall von polaren Zellen wie Neuronen an, dass die Proteinbiosynthese nicht global im Cytosol stattfindet, sondern es einen Transport der „ruhenden“ RNA bis zu dem Ort geben muss, an dem das entsprechende Protein lokal benötigt wird. In dieser vorliegenden Arbeit sollen nun in zwei Hauptprojekten molekulare Werkzeuge entwickelt werden, mit deren Hilfe oben genannte Fragestellungen in Zukunft beantwortet werden könnten. Im ersten Hauptprojekt wurde dazu eine neue Generation lichtaktivierbarer Molecular Beacons (von engl.: molekulare Leuchtfeuer) entwickelt. Dabei handelt es sich um Oligonukleotide, die komplementär zu einer intrazellulären RNA-Sequenz (Target-RNA) sind und mit Fluorophor und Fluoreszenz-Quencher modifiziert werden. Bei den lichtaktivierbaren Designs kann Fluoreszenz detektiert werden, wenn der Molecular Beacon an seine Targetsequenz gebunden und zusätzlich zuvor eine Lichtaktivierung stattgefunden hat. Im Gegensatz zu früheren Designs wurde bei diesem hier vorgestellten Molecular Beacon der Fluorophor mit Hilfe eines zweiten photoabspaltbaren Quenchers verbunden. Dadurch kann der Beacon an seine Targetsequenz binden, obwohl noch keine Lichtaktivierung stattgefunden hat. Fluoreszenz kann allerdings erst nach photoinduzierter Abspaltung des zusätzlichen Quenchers detektiert werden. In der vorliegenden Studie konnten dadurch extrem gute Signal-zu-Rausch-Verhältnisse von bis zu 170:1 erreicht werden. Zusätzlicher Vorteil dieses Designs ist die Tatsache, dass eine Vielzahl kommerziell erhältlicher Fluorophor-Quencher-Paare verwendet werden kann. Dabei ist es nicht relevant, ob der entsprechende Farbstoff co-synthetisch während der Festphasensynthese oder post-synthetisch durch die Modifikation funktioneller Gruppen angebracht wird. Nach anfänglichen in vitro Tests wurden die besten Molecular Beacons in vivo in der Zuckmücken-Art Chironomus tentans getestet. Dieser Organismus ist aufgrund seiner Polytänchromosomen, der sog. Balbiani Ringe, interessant. Dabei handelt es sich um ein Chromosom, das viele Chromatiden mit jeweils identischen Gensequenzen enthält. Diese Balbiani Ringe haben eine sehr charakteristische Struktur. Die Molecular Beacons wurden in den Zellkern injiziert und anschließend photoinduziert. Auch in den in vivo Messungen zeigte sich die Überlegenheit des neuen Design mit Signal-zu-Rausch-Verhältnissen von bis zu 80:1. Im zweiten Hauptprojekt war es das Ziel, lokale mikroRNA-Reifung in Neuronen nachzuweisen bzw. sichtbar zu machen. MikroRNA (kurz miRNA) ist einer der wichtigsten zellulären Werkzeuge, um Genregulation auf post-transkriptioneller Ebene zu ermöglichen. Für dieses Projekt wurde eine Sonde entwickelt, die den nativen miRNA-Vorläufer – die sog. prä-miRNA – nachbildet. Der enzymatische Reifungsprozess durch die RNase Dicer sollte durch Fluoreszenz nachweisbar sein. Dies gelang durch Modifikationen der Sequenz um die enzymatische Schnittstelle herum. Durch den Dicer-vermittelten, enzymatischen Verdau wurde ein Fluorophor von einem Quencher getrennt, wobei der fluoreszente Farbstoff an der reifen mikroRNA verblieb. Nach der Etablierung der in vitro Tests und Auswahl des optimalen Fluorophor-Quencher-Paars zeigte sich in einem Kontrollexperiment, dass bei Verwendung von neuronalen Ganglien aus Dicer-Knock-Out Mäusen kein Fluoreszenzanstieg zu beobachten war. Dieses Experiment bewies, dass bisher beobachtete Fluoreszenzanstiege Dicer-spezifisch waren. Im nächsten Schritt wurden in vivo Messungen durchgeführt. Es zeigte sich dabei, dass die sog. Patch Clamp Technik herkömmlichen Transfektionsmethoden überlegen war. Unter normalen Bedingungen zeigte sich sowohl im Soma als auch in den Dendriten ein Fluoreszenzanstieg. Durch Depolarisation des Neurons konnte dieser Effekt noch verstärkt werden, wobei das somatische Signal grundsätzlich als höher einzustufen war. Interessanterweise führte eine Blockade der NMDA-Rezeptoren auch bei gleichzeitiger Depolarisation zu einer verringerten Fluoreszenz. Dies lässt darauf schließen, dass die Reifung der untersuchten prä-miRNA in Dendriten von der Aktivität des NMDA-Rezeptors bzw. einem als Konsequenz ansteigenden Ca2+-Spiegels in der Zelle abhängig ist. In einem weiteren Experiment wurde nach „Beladung“ eines Neurons mit der prä-miRNA-Sonde Dendriten punktuell aktiviert. Dies konnte durch Licht-aktivierbares Glutamat erreicht werden. Im zentralen Nervensystem gilt Glutamat als der wichtigste aktivierende Neurotransmitter. Es konnte beobachtet werden, wie einerseits Fluoreszenz lokal an der aktivierten Stelle anstieg und gleichzeitig sog. dendritische Spines wuchsen. Zum Teil war auch ein Wachstum benachbarter Spines zu beobachten. Dabei handelt es sich um pilzförmige Aussackungen der Dendriten an Stellen, an denen Vernetzungen zu Synapsen anderer Neuronen existieren. Als Ergebnis kann geschlussfolgert werden, dass es eine lokale Reifung der untersuchten prä-miRNA durch Dicer in Dendriten gibt. Dieser Prozess kann sehr spezifisch und lokal durch die Aktivierung einzelner synaptischer Verbindungen initiiert werden.
Die vorliegende Arbeit beschäftigt sich mit der vergleichenden funktionalen Charakterisierung der E.coli Transporter LacY, FucP und XylE und des Glucose-Transporters GlcP aus Staphylococcus epidermidis sowie funktionsrelevanter Mutanten. Sie katalysieren in vivo den PMF-gekoppelten Zuckertransport und repräsentieren die major facilitator superfamily (MFS), einer der größten Transporter-Familien überhaupt. Die Studien wurden mithilfe einer elektrophysiologischen Methode auf Basis Festkörper-unterstützter Membranen (SSM) durchgeführt. Komplementär dazu wurden radioaktive Transportassays, fluorometrische Messungen, kinetische Simulationen und theoretische Berechnungen auf Basis der 3D-Strukturen durchgeführt. Experimentell bestimmte Zucker- und pH-Abhängigkeiten elektrogener steady-state und pre steady-state Reaktionen wurden verwendet, um ein allgemeingültiges kinetisches Modell aufzustellen.
Insgesamt konnten bei allen Transportern zwei elementare elektrogene Reaktionen identifiziert werden. Eine schnelle Zucker-induzierte Konformationsänderung wurde dem induced fit des Zuckermoleküls zugeordnet. Die Elektrogenität im steady-state wird dagegen durch den langsamen Transfer der negativ geladenen Protonenbindestelle bestimmt. Die für den Symport ratenlimitierende Reaktion ist abhängig von den äußeren Bedingungen wie pH-Werten, Zuckerkonzentrationen, Substrat-Spezies und Membranpotential meist die Konformationsänderung des leeren (P) oder des beladenen (PSH) Carriers, welche die Substratbindestellen im Zuge des Alternating Access über die Membran transferieren. Ein Wechsel zwischen hohen Protonenbindungs-pK-Werten und niedrigen Protonenfreisetzungs-pK-Werten durch weitere lokale Konformationsänderungen ist zentraler Bestandteil des Transportmechanismus. Ein weiterer wichtiger Aspekt ist die Kopplung zwischen Zucker- und Protonen-Translokation, die sich zwischen E.coli Transportern und GlcP strikt unterscheidet. In E.coli Transportern erfolgt eine kooperative Bindung von Zucker und Proton. Zudem erfolgt keine Konformationsänderung im Zucker-gebundenen, unprotonierten Carrier (PS). In GlcP ist die Kopplung erheblich reduziert. Der Transport-Modus selbst ist abhängig von den äußeren Bedingungen. So katalysiert GlcP abhängig vom pH-Gradienten Uniport, Symport oder Antiport.
Die vorliegende Arbeit leistet einen wichtigen Beitrag zum Verständnis des PMF-gekoppelten Zuckertransports und zeigt die Grenzen des für LacY formulierten 6-Zustands-Modells mit nur zwei Konformationsänderungen auf. Ein erweitertes 8-Zustands-Modell mit vier Konformationsänderungen, die unterschiedliche Ratenkonstanten aufweisen können, erklärt sowohl Symport, Antiport als auch Uniport und berücksichtigt zudem die zahlreichen Ergebnisse für LacY aus der Literatur.