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Dive into the research topics where Moritz Kreysing is active.

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Featured researches published by Moritz Kreysing.


Cell | 2009

Nuclear Architecture of Rod Photoreceptor Cells Adapts to Vision in Mammalian Evolution

Irina Solovei; Moritz Kreysing; Christian Lanctôt; Süleyman Kösem; Leo Peichl; Thomas Cremer; Jochen Guck; Boris Joffe

We show that the nuclear architecture of rod photoreceptor cells differs fundamentally in nocturnal and diurnal mammals. The rods of diurnal retinas possess the conventional architecture found in nearly all eukaryotic cells, with most heterochromatin situated at the nuclear periphery and euchromatin residing toward the nuclear interior. The rods of nocturnal retinas have a unique inverted pattern, where heterochromatin localizes in the nuclear center, whereas euchromatin, as well as nascent transcripts and splicing machinery, line the nuclear border. The inverted pattern forms by remodeling of the conventional one during terminal differentiation of rods. The inverted rod nuclei act as collecting lenses, and computer simulations indicate that columns of such nuclei channel light efficiently toward the light-sensing rod outer segments. Comparison of the two patterns suggests that the conventional architecture prevails in eukaryotic nuclei because it results in more flexible chromosome arrangements, facilitating positional regulation of nuclear functions.


Advanced Materials | 2013

Bio‐Inspired Band‐Gap Tunable Elastic Optical Multilayer Fibers

Mathias Kolle; Alfred Lethbridge; Moritz Kreysing; Jeremy J. Baumberg; Joanna Aizenberg; Peter Vukusic

The concentrically-layered photonic structure found in the tropical fruit Margaritaria nobilis serves as inspiration for photonic fibers with mechanically tunable band-gap. The fibers show the spectral filtering capabilities of a planar Bragg stack while the microscopic curvature decreases the strong directional chromaticity associated with flat multilayers. Elongation of the elastic fibers results in a shift of the reflection of over 200 nm.


Optics Express | 2008

The optical cell rotator

Moritz Kreysing; Tobias R Kießling; Anatol Fritsch; Christian Dietrich; Jochen Guck; Josef A. Käs

The optical cell rotator (OCR) is a modified dual-beam laser trap for the holding and controlled rotation of suspended dielectric microparticles, such as cells. In contrast to optical tweezers, OCR uses two counter-propagating divergent laser beams, which are shaped and delivered by optical fibers. The rotation of a trapped specimen is carried out by the rotation of a dual-mode fiber, emitting an asymmetric laser beam. Experiments were performed on human erythrocytes, promyelocytic leukemia cells (HL60), and cell clusters (MCF-7). Since OCR permits the rotation of cells around an axis perpendicular to the optical axis of any microscope and is fully decoupled from imaging optics, it could be a suitable and expedient tool for tomographic microscopy.


Nature Chemistry | 2015

Heat flux across an open pore enables the continuous replication and selection of oligonucleotides towards increasing length

Moritz Kreysing; Lorenz Keil; Simon Lanzmich; Dieter Braun

The replication of nucleic acids is central to the origin of life. On the early Earth, suitable non-equilibrium boundary conditions would have been required to surmount the effects of thermodynamic equilibrium such as the dilution and degradation of oligonucleotides. One particularly intractable experimental finding is that short genetic polymers replicate faster and outcompete longer ones, which leads to ever shorter sequences and the loss of genetic information. Here we show that a heat flux across an open pore in submerged rock concentrates replicating oligonucleotides from a constant feeding flow and selects for longer strands. Our experiments utilize the interplay of molecular thermophoresis and laminar convection, the latter driving strand separation and exponential replication. Strands of 75 nucleotides survive whereas strands half as long die out, which inverts the above dilemma of the survival of the shortest. The combined feeding, thermal cycling and positive length selection opens the door for a stable molecular evolution in the long-term microhabitat of heated porous rock.


Science | 2012

Photonic crystal light collectors in fish retina improve vision in turbid water.

Moritz Kreysing; Roland Pusch; Dorothee Haverkate; Meik Landsberger; Jacob Engelmann; Janina Ruiter; Carlos Mora-Ferrer; Elke Ulbricht; Jens Grosche; Kristian Franze; Stefan Streif; Sarah Schumacher; Felix Makarov; Johannes Kacza; Jochen Guck; Hartwig Wolburg; James K. Bowmaker; Gerhard von der Emde; Stefan Schuster; Hans-Joachim Wagner; Andreas Reichenbach; Mike Francke

Seeing in the Dark Elephantnose fish are known to use electrosensing to navigate their murky freshwater environment. However, unlike some other animals from dark environments, they have retained their eyes and some dependence on vision. While most vertebrate vision optimizes either photon catch (for increased light capture) or visual acuity, Kreysing et al. (p. 1700) show that the unique structures of the grouped retinae found in the eyes of this species matches rod and cone sensitivity, which allows for the simultaneous use of both types of photoreceptors over a large range of dim light intensities. Layering cones on top of rods allows the elephantnose fish to see low-contrast objects in a murky environment. Despite their diversity, vertebrate retinae are specialized to maximize either photon catch or visual acuity. Here, we describe a functional type that is optimized for neither purpose. In the retina of the elephantnose fish (Gnathonemus petersii), cone photoreceptors are grouped together within reflecting, photonic crystal–lined cups acting as macroreceptors, but rod photoreceptors are positioned behind these reflectors. This unusual arrangement matches rod and cone sensitivity for detecting color-mixed stimuli, whereas the photoreceptor grouping renders the fish insensitive to spatial noise; together, this enables more reliable flight reactions in the fish’s dim and turbid habitat as compared with fish lacking this retinal specialization.


Nature Communications | 2014

Dynamic operation of optical fibres beyond the single-mode regime facilitates the orientation of biological cells

Moritz Kreysing; Dino Ott; Michael J. Schmidberger; Oliver Otto; Mirjam Schürmann; Estela Martín-Badosa; Graeme Whyte; Jochen Guck

The classical purpose of optical fibres is delivery of either optical power, as for welding, or temporal information, as for telecommunication. Maximum performance in both cases is provided by the use of single-mode optical fibres. However, transmitting spatial information, which necessitates higher-order modes, is difficult because their dispersion relation leads to dephasing and a deterioration of the intensity distribution with propagation distance. Here we consciously exploit the fundamental cause of the beam deterioration—the dispersion relation of the underlying vectorial electromagnetic modes—by their selective excitation using adaptive optics. This allows us to produce output beams of high modal purity, which are well defined in three dimensions. The output beam distribution is even robust against significant bending of the fibre. The utility of this approach is exemplified by the controlled rotational manipulation of live cells in a dual-beam fibre-optical trap integrated into a modular lab-on-chip system.


Optics Express | 2014

Direct observation of light focusing by single photoreceptor cell nuclei

Zuzanna Błaszczak; Moritz Kreysing; Jochen Guck

The vertebrate retina is inverted with respect to its optical function, which requires light to pass through the entire tissue prior to detection. The last significant barrier for photons to overcome is the outer nuclear layer formed by photoreceptor cell (PRC) nuclei. Here we experimentally characterise the optical properties of PRC nuclei using bright-field defocusing microscopy to capture near-field intensity distributions behind individual nuclei. We find that some nuclei efficiently focus incident light confirming earlier predictions based on comparative studies of chromatin organisation in nocturnal and diurnal mammals. The emergence of light focusing during the development of mouse nuclei highlights the acquired nature of the observed lens-like behaviour. Optical characterisation of these nuclei is an important first step towards an improved understanding of how light transmission through the retina is influenced by its constituents.


Nature Cell Biology | 2018

Non-invasive perturbations of intracellular flow reveal physical principles of cell organization

Matthäus Mittasch; Peter Gross; Michael Nestler; Anatol Fritsch; Christiane Iserman; Mrityunjoy Kar; Matthias Munder; Axel Voigt; Simon Alberti; Stephan W. Grill; Moritz Kreysing

Recent advances in cell biology enable precise molecular perturbations. The spatiotemporal organization of cells and organisms, however, also depends on physical processes such as diffusion or cytoplasmic flows, and strategies to perturb physical transport inside cells are not yet available. Here, we demonstrate focused-light-induced cytoplasmic streaming (FLUCS). FLUCS is local, directional, dynamic, probe-free, physiological, and is even applicable through rigid egg shells or cell walls. We explain FLUCS via time-dependent modelling of thermoviscous flows. Using FLUCS, we demonstrate that cytoplasmic flows drive partitioning-defective protein (PAR) polarization in Caenorhabditis elegans zygotes, and that cortical flows are sufficient to transport PAR domains and invert PAR polarity. In addition, we find that asymmetric cell division is a binary decision based on gradually varying PAR polarization states. Furthermore, the use of FLUCS for active microrheology revealed a metabolically induced fluid-to-solid transition of the yeast cytoplasm. Our findings establish how a wide range of transport-dependent models of cellular organization become testable by FLUCS.Mittasch et al. show that controlling cytoplasmic flow via focused-light-induced cytoplasmic streaming (FLUCS), a non-invasive technique, can be used to invert asymmetric cell division in Caenorhabditis elegans zygotes.


PLOS Computational Biology | 2018

Biobeam—Multiplexed wave-optical simulations of light-sheet microscopy

Martin Weigert; Kaushikaram Subramanian; Sebastian T. Bundschuh; Eugene W. Myers; Moritz Kreysing

Sample-induced image-degradation remains an intricate wave-optical problem in light-sheet microscopy. Here we present biobeam, an open-source software package that enables simulation of operational light-sheet microscopes by combining data from 105–106 multiplexed and GPU-accelerated point-spread-function calculations. The wave-optical nature of these simulations leads to the faithful reproduction of spatially varying aberrations, diffraction artifacts, geometric image distortions, adaptive optics, and emergent wave-optical phenomena, and renders image-formation in light-sheet microscopy computationally tractable.


bioRxiv | 2018

Active gelation breaks time-reversal-symmetry of mitotic chromosome mechanics

Matthäus Mittasch; Anatol Fritsch; Michael Nestler; Juan M. Iglesias-Artola; Kaushikaram Subramanian; Heike Petzold; Mrityunjoy Kar; Axel Voigt; Moritz Kreysing

In cell division, mitosis is the phase in which duplicated sets of chromosomes are mechanically aligned to form the metaphase plate before being segregated in two daughter cells. Irreversibility is a hallmark of this process, despite the fundamental laws of Newtonian mechanics being time symmetric. Here we show experimentally that mitotic chromosomes receive the arrow of time by time-reversal-symmetry breaking of the underlying mechanics in prometaphase. By optically inducing hydrodynamic flows within prophase nuclei, we find that duplicated chromatid pairs initially form a fluid suspension in the nucleoplasm: although showing little motion on their own, condensed chromosomes are free to move through the nucleus in a time-reversible manner. Actively probing chromosome mobility further in time, we find that this viscous suspension of chromatin transitions into a gel after nuclear breakdown. This gel state, in which chromosomes cannot be moved by flows, persists even when chromosomes start moving to form the metaphase plate. Complemented by minimal reconstitution experiments, our active intra-nuclear micro-rheology reveals time-reversal-symmetry breaking of chromosome mechanics to be caused by the transition from a purely fluid suspension into an active gel. Graphical abstract One sentence summary Flows induced in living cell nuclei reveal the rheological changes that bring chromosomes under mechanical control during mitosis.

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Jochen Guck

Dresden University of Technology

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Mathias Kolle

Massachusetts Institute of Technology

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Axel Voigt

Dresden University of Technology

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Michael Nestler

Dresden University of Technology

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