Holistic improvement of image acquisition and reconstruction in fluorescence microscopy

Recent developments in microscopic imaging led to a better understanding of intra- and intercellular metabolic processes and, for example, to visualize structural properties of viral pathogens. In this thesis, the imaging process of widefield and confocal scanning microscopy techniques is treated holistically to highlight general strategies and maximise their information content. Poisson or shot noise is assumed to be the fundamental noise process for the given measurements. A stable focus position is a basic condition for e.g. long-term measurements in order to provide reliable information about potential changes inside the Field-of-view. While newer microscopy systems can be equipped with hardware autofocus, this is not yet the widespread standard. For image-based focus analysis, different metrics for ideal, noisy and aberrated, in case of spherical aberration and astigmatism, measurements are presented. A stable focus position is also relevant in the example of 2-photon confocal imaging and at the same time the situation is aggravated in the given example, the measurement of the retina in the living mouse. In addition to the natural drift of the focal position, which can be evaluated by means of previously introduced metrics, rhythmic heartbeat, respiration, unrhythmic muscle twitching and movement of the mouse kept in artificial sleep are added. A dejittering algorithm is presented for the measurement data obtained under these circumstances. Using the additional information about the sample distribution in ISM, a method for reconstructing 3D from 2D image data is presented in the form of thick slice unmixing. This method can further be used for suppression of light generated outside the focal layer of 3D data stacks and is compared to selective layer multi-view deconvolution. To reduce phototoxicity and save valuable measurement time for a 3D stack, the method of zLEAP is presented, by which omitted Z-planes are subsequently calculated and inserted

Dynamically Tunable Plasmonic Structural Color

Functional surfaces which can control light across the electromagnetic spectrum are highly desirable. With the aid of advanced modeling and fabrication techniques, researchers have demonstrated surfaces with near arbitrary tailoring of reflected/transmitted amplitude, phase and polarization - the applications for which are diverse as light itself. These systems often comprise of structured metals and dielectrics that, when combined, manifest resonances dependent on structural dimensions. This attribute provides a convenient and direct path to arbitrarily engineer the surface\u27s optical characteristics across many electromagnetic regimes. But while many of these plasmonic systems struggle to compete with the efficiency of pre-existing technologies, the ability to tune plamsonic structures post-fabrication is a distinct advantage which may lead to novel devices. In this work, I will summarize fundamental and applied aspects of tunable plasmonic systems as applied to the visible and infrared regimes. I will demonstrate how liquid crystal may be used to dynamically and reversibly tune the plasmonic resonances of metallic surfaces on a millisecond time scale. For the visible, this results in dynamic color-changing surfaces capable of covering the entire RGB color space and which is compatible with active addressing schemes. I will then show the application of these concepts to infrared absorbers through the use of liquid crystal and phase change materials. The later of these devices can find use in infrared data/image encoding, thermal management and camouflage. Together, these works explore the limits of tunable plasmonic systems and the novel devices they might lead to

Expression data dnalysis and regulatory network inference by means of correlation patterns

With the advance of high-throughput techniques, the amount of available data in the bio-molecular field is rapidly growing. It is now possible to measure genome-wide aspects of an entire biological system as a whole. Correlations that emerge due to internal dependency structures of these systems entail the formation of characteristic patterns in the corresponding data. The extraction of these patterns has become an integral part of computational biology. By triggering perturbations and interventions it is possible to induce an alteration of patterns, which may help to derive the dependency structures present in the system. In particular, differential expression experiments may yield alternate patterns that we can use to approximate the actual interplay of regulatory proteins and genetic elements, namely, the regulatory network of a cell. In this work, we examine the detection of correlation patterns from bio-molecular data and we evaluate their applicability in terms of protein contact prediction, experimental artifact removal, the discovery of unexpected expression patterns and genome-scale inference of regulatory networks. Correlation patterns are not limited to expression data. Their analysis in the context of conserved interfaces among proteins is useful to estimate whether these may have co-evolved. Patterns that hint on correlated mutations would then occur in the associated protein sequences as well. We employ a conceptually simple sampling strategy to decide whether or not two pathway elements share a conserved interface and are thus likely to be in physical contact. We successfully apply our method to a system of ABC-transporters and two-component systems from the phylum of Firmicute bacteria. For spatially resolved gene expression data like microarrays, the detection of artifacts, as opposed to noise, corresponds to the extraction of localized patterns that resemble outliers in a given region. We develop a method to detect and remove such artifacts using a sliding-window approach. Our method is very accurate and it is shown to adapt to other platforms like custom arrays as well. Further, we developed Padesco as a way to reveal unexpected expression patterns. We extract frequent and recurring patterns that are conserved across many experiments. For a specific experiment, we predict whether a gene deviates from its expected behaviour. We show that Padesco is an effective approach for selecting promising candidates from differential expression experiments. In Chapter 5, we then focus on the inference of genome-scale regulatory networks from expression data. Here, correlation patterns have proven useful for the data-driven estimation of regulatory interactions. We show that, for reliable eukaryotic network inference, the integration of prior networks is essential. We reveal that this integration leads to an over-estimate of network-wide quality estimates and suggest a corrective procedure, CoRe, to counterbalance this effect. CoRe drastically improves the false discovery rate of the originally predicted networks. We further suggest a consensus approach in combination with an extended set of topological features to obtain a more accurate estimate of the eukaryotic regulatory network for yeast. In the course of this work we show how correlation patterns can be detected and how they can be applied for various problem settings in computational molecular biology. We develop and discuss competitive approaches for the prediction of protein contacts, artifact repair, differential expression analysis, and network inference and show their applicability in practical setups.Mit der Weiterentwicklung von Hochdurchsatztechniken steigt die Anzahl verfügbarer Daten im Bereich der Molekularbiologie rapide an. Es ist heute möglich, genomweite Aspekte eines ganzen biologischen Systems komplett zu erfassen. Korrelationen, die aufgrund der internen Abhängigkeits-Strukturen dieser Systeme enstehen, führen zu charakteristischen Mustern in gemessenen Daten. Die Extraktion dieser Muster ist zum integralen Bestandteil der Bioinformatik geworden. Durch geplante Eingriffe in das System ist es möglich Muster-Änderungen auszulösen, die helfen, die Abhängigkeits-Strukturen des Systems abzuleiten. Speziell differentielle Expressions-Experimente können Muster-Wechsel bedingen, die wir verwenden können, um uns dem tatsächlichen Wechselspiel von regulatorischen Proteinen und genetischen Elementen anzunähern, also dem regulatorischen Netzwerk einer Zelle. In der vorliegenden Arbeit beschäftigen wir uns mit der Erkennung von Korrelations-Mustern in molekularbiologischen Daten und schätzen ihre praktische Nutzbarkeit ab, speziell im Kontext der Kontakt-Vorhersage von Proteinen, der Entfernung von experimentellen Artefakten, der Aufdeckung unerwarteter Expressions-Muster und der genomweiten Vorhersage regulatorischer Netzwerke. Korrelations-Muster sind nicht auf Expressions-Daten beschränkt. Ihre Analyse im Kontext konservierter Schnittstellen zwischen Proteinen liefert nützliche Hinweise auf deren Ko-Evolution. Muster die auf korrelierte Mutationen hinweisen, würden in diesem Fall auch in den entsprechenden Proteinsequenzen auftauchen. Wir nutzen eine einfache Sampling-Strategie, um zu entscheiden, ob zwei Elemente eines Pathways eine gemeinsame Schnittstelle teilen, berechnen also die Wahrscheinlichkeit für deren physikalischen Kontakt. Wir wenden unsere Methode mit Erfolg auf ein System von ABC-Transportern und Zwei-Komponenten-Systemen aus dem Firmicutes Bakterien-Stamm an. Für räumlich aufgelöste Expressions-Daten wie Microarrays enspricht die Detektion von Artefakten der Extraktion lokal begrenzter Muster. Im Gegensatz zur Erkennung von Rauschen stellen diese innerhalb einer definierten Region Ausreißer dar. Wir entwickeln eine Methodik, um mit Hilfe eines Sliding-Window-Verfahrens, solche Artefakte zu erkennen und zu entfernen. Das Verfahren erkennt diese sehr zuverlässig. Zudem kann es auf Daten diverser Plattformen, wie Custom-Arrays, eingesetzt werden. Als weitere Möglichkeit unerwartete Korrelations-Muster aufzudecken, entwickeln wir Padesco. Wir extrahieren häufige und wiederkehrende Muster, die über Experimente hinweg konserviert sind. Für ein bestimmtes Experiment sagen wir vorher, ob ein Gen von seinem erwarteten Verhalten abweicht. Wir zeigen, dass Padesco ein effektives Vorgehen ist, um vielversprechende Kandidaten eines differentiellen Expressions-Experiments auszuwählen. Wir konzentrieren uns in Kapitel 5 auf die Vorhersage genomweiter regulatorischer Netzwerke aus Expressions-Daten. Hierbei haben sich Korrelations-Muster als nützlich für die datenbasierte Abschätzung regulatorischer Interaktionen erwiesen. Wir zeigen, dass für die Inferenz eukaryotischer Systeme eine Integration zuvor bekannter Regulationen essentiell ist. Unsere Ergebnisse ergeben, dass diese Integration zur Überschätzung netzwerkübergreifender Qualitätsmaße führt und wir schlagen eine Prozedur - CoRe - zur Verbesserung vor, um diesen Effekt auszugleichen. CoRe verbessert die False Discovery Rate der ursprünglich vorhergesagten Netzwerke drastisch. Weiterhin schlagen wir einen Konsensus-Ansatz in Kombination mit einem erweiterten Satz topologischer Features vor, um eine präzisere Vorhersage für das eukaryotische Hefe-Netzwerk zu erhalten. Im Rahmen dieser Arbeit zeigen wir, wie Korrelations-Muster erkannt und wie sie auf verschiedene Problemstellungen der Bioinformatik angewandt werden können. Wir entwickeln und diskutieren Ansätze zur Vorhersage von Proteinkontakten, Behebung von Artefakten, differentiellen Analyse von Expressionsdaten und zur Vorhersage von Netzwerken und zeigen ihre Eignung im praktischen Einsatz