@article{BellDabauvalleScheer1992,
author = {Bell, Peter and Dabauvalle, Marie-Christine and Scheer, Ulrich},
title = {In vitro assembly of prenucleolar bodies in Xenopus egg extract},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-34233},
year = {1992},
abstract = {Nuclei assembled in Xenopus egg extract from purified DNA or chromatin resemble their natural counterparts in a number of structural and functional features. However, the most obvious structural element of normal interphase nuclei, the nucleolus, is absent from the in vitro reconstituted nuclei. By EM, cytological silver staining, and immunofluorescence microscopy employing antibodies directed against various nucleolar components we show that nuclei assembled in vitro contain numerous distinct aggregates that resemble prenucleolar bodies (PNBs) by several criteria. Formation of these PNB-like structures requires pore complex-mediated nuclear transport of proteins but is independent of the genetic content of the in vitro nuclei as well as transcriptional and translational events. Our data indicate that nuclei assembled in vitro are capable of initiating early steps of nucleologenesis but that the resulting PNBs are unable to fuse with each other, probably due to the absence of a functional nucleolus organizer. With appropriate modifications, this experimental system should be useful to define and analyze conditions promoting the site-specific assembly of PNBs into a coherent nucleolar body.},
language = {en}
}
@phdthesis{Beliu2020,
author = {Beliu, Gerti},
title = {Bioorthogonale Tetrazin-Farbstoffe f{\"u}r die Lebendzell-Markierung und hochaufgel{\"o}ste Fluoreszenzmikroskopie},
doi = {10.25972/OPUS-18962},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-189628},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2020},
abstract = {Der genetische Code beschreibt die Ver- und Entschl{\"u}sselung der Erb-information f{\"u}r das universelle Prinzip der Proteinbiosynthese aus einzelnen Aminos{\"a}uren. Durch Erweiterung des genetischen Codes lassen sich unna-t{\"u}rliche Aminos{\"a}uren (uAA) mit einzigartigen biophysikalischen Eigenschaf-ten ortsspezifisch in Proteine einf{\"u}hren und erm{\"o}glichen die spezifische Ma-nipulation von Proteinen. Die Click-Reaktion zwischen der unnat{\"u}rlichen Aminos{\"a}ure TCO*-Lysin und Tetrazin besitzt eine außergew{\"o}hnliche Reaktionskinetik (≥800 M-1s-1) und erm{\"o}glicht eine spezifische und bioorthogonale Markierung von Bio- ¬molek{\"u}len unter physiologischen Bedingungen. Im Fokus dieser Arbeit stand zun{\"a}chst die Markierung von Membran- ¬rezeptoren durch Click-Chemie in lebenden Zellen sowie die Untersuchung der Wechselwirkung 22 bekannter und neuartiger Tetrazin-Farbstoff- Konjugate. Dar{\"u}ber hinaus wurde die Anwendbarkeit von bioorthogonalen Click-Reaktionen f{\"u}r die hochaufl{\"o}sende Fluoreszenzmikroskopie untersucht. Durch Erweiterung des genetischen Codes in Proteine aus der Klasse der ionotropen Glutamatrezeptoren (iGluR), TNF-Rezeptoren oder Mikrotubu-li-assoziierten Proteinen (MAP) wurde ortspezifisch die unnat{\"u}rliche Amino-s{\"a}ure TCO*-Lysin eingef{\"u}hrt und dadurch die Fluoreszenzmarkierung durch Tetrazin-Farbstoffe erm{\"o}glicht. Die direkte chemische Kopplung von TCO an Liganden wie Phalloidin und Docetaxel, welche spezifisch das Aktin-Zytoskelett bzw. Mikrotubuli-Filamente binden k{\"o}nnen, erm{\"o}glichte zudem die Click-F{\"a}rbungen von fixierten und lebenden Zellen ohne genetische Ver-{\"a}nderungen der Zielproteine. Des Weiteren wurden die spektroskopischen Eigenschaften von 22 Tetrazin-Farbstoffen, verteilt {\"u}ber den gesamten sichtbaren Wellenl{\"a}ngenbereich, untersucht. Ein charakteristisches Kennzeichen der Click-Reaktion mit Tet-razin-Farbstoffen ist dabei ihre Fluorogenit{\"a}t. Das Tetrazin fungiert nicht nur als reaktive Gruppe w{\"a}hrend der Click-Reaktion mit Alkenen, sondern f{\"u}hrt in vielen Tetrazin-Farbstoff-Konjugaten zur Fluoreszenzl{\"o}schung. W{\"a}hrend bei gr{\"u}n-absorbierenden Farbstoffe vor allem FRET-basierte L{\"o}schprozesse dominieren, konnte photoinduzierter Elektronentransfer (PET) vom angeregten Farbstoff zum Tetrazin als Hauptl{\"o}schmechanismus bei rot-absorbierenden Oxazin- und Rhodamin-Derivaten identifiziert werden. Die effiziente und spezifische Markierung aller untersuchten Tetrazin- Farbstoffe erm{\"o}glichte die Visualisierung von Aktin-Filamenten, Mikrotubuli und Membranrezeptoren sowohl durch konventionelle Fluoreszenzmikrosko-pie als auch durch hochaufl{\"o}sende Verfahren, wie z.B. dSTORM, auf Ein-zelmolek{\"u}lebene. Die unterschiedliche Zellpermeabilit{\"a}t von Tetrazin-Farbstoffen kann dabei vorteilhaft f{\"u}r die spezifische intra- und extrazellul{\"a}re Markierung von Proteinen in fixierten und lebenden Zellen genutzt werden.},
subject = {Hochaufgel{\"o}ste Fluoreszenzmikroskopie},
language = {de}
}
@article{BeisserGrohmeKopkaetal.2012,
author = {Beisser, Daniela and Grohme, Markus A. and Kopka, Joachim and Frohme, Marcus and Schill, Ralph O. and Hengherr, Steffen and Dandekar, Thomas and Klau, Gunnar W. and Dittrich, Marcus and M{\"u}ller, Tobias},
title = {Integrated pathway modules using time-course metabolic profiles and EST data from Milnesium tardigradum},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-75241},
year = {2012},
abstract = {Background: Tardigrades are multicellular organisms, resistant to extreme environmental changes such as heat, drought, radiation and freezing. They outlast these conditions in an inactive form (tun) to escape damage to cellular structures and cell death. Tardigrades are apparently able to prevent or repair such damage and are therefore a crucial model organism for stress tolerance. Cultures of the tardigrade Milnesium tardigradum were dehydrated by removing the surrounding water to induce tun formation. During this process and the subsequent rehydration, metabolites were measured in a time series by GC-MS. Additionally expressed sequence tags are available, especially libraries generated from the active and inactive state. The aim of this integrated analysis is to trace changes in tardigrade metabolism and identify pathways responsible for their extreme resistance against physical stress. Results: In this study we propose a novel integrative approach for the analysis of metabolic networks to identify modules of joint shifts on the transcriptomic and metabolic levels. We derive a tardigrade-specific metabolic network represented as an undirected graph with 3,658 nodes (metabolites) and 4,378 edges (reactions). Time course metabolite profiles are used to score the network nodes showing a significant change over time. The edges are scored according to information on enzymes from the EST data. Using this combined information, we identify a key subnetwork (functional module) of concerted changes in metabolic pathways, specific for de- and rehydration. The module is enriched in reactions showing significant changes in metabolite levels and enzyme abundance during the transition. It resembles the cessation of a measurablemetabolism (e.g. glycolysis and amino acid anabolism) during the tun formation, the production of storage metabolites and bioprotectants, such as DNA stabilizers, and the generation of amino acids and cellular components from monosaccharides as carbon and energy source during rehydration. Conclusions: The functional module identifies relationships among changed metabolites (e.g. spermidine) and reactions and provides first insights into important altered metabolic pathways. With sparse and diverse data available, the presented integrated metabolite network approach is suitable to integrate all existing data and analyse it in a combined manner.},
subject = {Milnesium tardigradum},
language = {en}
}
@phdthesis{Beisser2011,
author = {Beisser, Daniela},
title = {Integrated functional analysis of biological networks},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-70150},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2011},
abstract = {In recent years high-throughput experiments provided a vast amount of data from all areas of molecular biology, including genomics, transcriptomics, proteomics and metabolomics. Its analysis using bioinformatics methods has developed accordingly, towards a systematic approach to understand how genes and their resulting proteins give rise to biological form and function. They interact with each other and with other molecules in highly complex structures, which are explored in network biology. The in-depth knowledge of genes and proteins obtained from high-throughput experiments can be complemented by the architecture of molecular networks to gain a deeper understanding of biological processes. This thesis provides methods and statistical analyses for the integration of molecular data into biological networks and the identification of functional modules, as well as its application to distinct biological data. The integrated network approach is implemented as a software package, termed BioNet, for the statistical language R. The package includes the statistics for the integration of transcriptomic and functional data with biological networks, the scoring of nodes and edges of these networks as well as methods for subnetwork search and visualisation. The exact algorithm is extensively tested in a simulation study and outperforms existing heuristic methods for the calculation of this NP-hard problem in accuracy and robustness. The variability of the resulting solutions is assessed on perturbed data, mimicking random or biased factors that obscure the biological signal, generated for the integrated data and the network. An optimal, robust module can be calculated using a consensus approach, based on a resampling method. It summarizes optimally an ensemble of solutions in a robust consensus module with the estimated variability indicated by confidence values for the nodes and edges. The approach is subsequently applied to two gene expression data sets. The first application analyses gene expression data for acute lymphoblastic leukaemia (ALL) and differences between the subgroups with and without an oncogenic BCR/ABL gene fusion. In a second application gene expression and survival data from diffuse large B-cell lymphomas are examined. The identified modules include and extend already existing gene lists and signatures by further significant genes and their interactions. The most important novelty is that these genes are determined and visualised in the context of their interactions as a functional module and not as a list of independent and unrelated transcripts. In a third application the integrative network approach is used to trace changes in tardigrade metabolism to identify pathways responsible for their extreme resistance to environmental changes and endurance in an inactive tun state. For the first time a metabolic network approach is proposed to detect shifts in metabolic pathways, integrating transcriptome and metabolite data. Concluding, the presented integrated network approach is an adequate technique to unite high-throughput experimental data for single molecules and their intermolecular dependencies. It is flexible to apply on diverse data, ranging from gene expression changes over metabolite abundances to protein modifications in a combination with a suitable molecular network. The exact algorithm is accurate and robust in comparison to heuristic approaches and delivers an optimal, robust solution in form of a consensus module with confidence values. By the integration of diverse sources of information and a simultaneous inspection of a molecular event from different points of view, new and exhaustive insights into biological processes can be acquired.},
subject = {Bioinformatik},
language = {en}
}
@article{BeierGaetschenbergerAzzamietal.2013,
author = {Beier, Hildburg and G{\"a}tschenberger, Heike and Azzami, Klara and Tautz, J{\"u}rgen},
title = {Antibacterial Immune Competence of Honey Bees (Apis mellifera) Is Adapted to Different Life Stages and Environmental Risks},
series = {PLoS ONE},
journal = {PLoS ONE},
doi = {10.1371/journal.pone.0066415},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-96895},
year = {2013},
abstract = {The development of all honey bee castes proceeds through three different life stages all of which encounter microbial infections to a various extent. We have examined the immune strength of honey bees across all developmental stages with emphasis on the temporal expression of cellular and humoral immune responses upon artificial challenge with viable Escherichia coli bacteria. We employed a broad array of methods to investigate defence strategies of infected individuals: (a) fate of bacteria in the haemocoel; (b) nodule formation and (c) induction of antimicrobial peptides (AMPs). Newly emerged adult worker bees and drones were able to activate efficiently all examined immune reactions. The number of viable bacteria circulating in the haemocoel of infected bees declined rapidly by more than two orders of magnitude within the first 4-6 h post-injection (p.i.), coinciding with the occurrence of melanised nodules. Antimicrobial activity, on the other hand, became detectable only after the initial bacterial clearance. These two temporal patterns of defence reactions very likely represent the constitutive cellular and the induced humoral immune response. A unique feature of honey bees is that a fraction of worker bees survives the winter season in a cluster mostly engaged in thermoregulation. We show here that the overall immune strength of winter bees matches that of young summer bees although nodulation reactions are not initiated at all. As expected, high doses of injected viable E.coli bacteria caused no mortality in larvae or adults of each age. However, drone and worker pupae succumbed to challenge with E.coli even at low doses, accompanied by a premature darkening of the pupal body. In contrast to larvae and adults, we observed no fast clearance of viable bacteria and no induction of AMPs but a rapid proliferation of E.coli bacteria in the haemocoel of bee pupae ultimately leading to their death.},
language = {en}
}
@article{BeetzKrauselJundi2023,
author = {Beetz, M. Jerome and Kraus, Christian and el Jundi, Basil},
title = {Neural representation of goal direction in the monarch butterfly brain},
series = {Nature Communications},
volume = {14},
journal = {Nature Communications},
doi = {10.1038/s41467-023-41526-w},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-358073},
year = {2023},
abstract = {Neural processing of a desired moving direction requires the continuous comparison between the current heading and the goal direction. While the neural basis underlying the current heading is well-studied, the coding of the goal direction remains unclear in insects. Here, we used tetrode recordings in tethered flying monarch butterflies to unravel how a goal direction is represented in the insect brain. While recording, the butterflies maintained robust goal directions relative to a virtual sun. By resetting their goal directions, we found neurons whose spatial tuning was tightly linked to the goal directions. Importantly, their tuning was unaffected when the butterflies changed their heading after compass perturbations, showing that these neurons specifically encode the goal direction. Overall, we here discovered invertebrate goal-direction neurons that share functional similarities to goal-direction cells reported in mammals. Our results give insights into the evolutionarily conserved principles of goal-directed spatial orientation in animals.},
language = {en}
}
@article{BeetzHechavarria2022,
author = {Beetz, M. Jerome and Hechavarr{\´i}a, Julio C.},
title = {Neural processing of naturalistic echolocation signals in bats},
series = {Frontiers in Neural Circuits},
volume = {16},
journal = {Frontiers in Neural Circuits},
issn = {1662-5110},
doi = {10.3389/fncir.2022.899370},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-274605},
year = {2022},
abstract = {Echolocation behavior, a navigation strategy based on acoustic signals, allows scientists to explore neural processing of behaviorally relevant stimuli. For the purpose of orientation, bats broadcast echolocation calls and extract spatial information from the echoes. Because bats control call emission and thus the availability of spatial information, the behavioral relevance of these signals is undiscussable. While most neurophysiological studies, conducted in the past, used synthesized acoustic stimuli that mimic portions of the echolocation signals, recent progress has been made to understand how naturalistic echolocation signals are encoded in the bat brain. Here, we review how does stimulus history affect neural processing, how spatial information from multiple objects and how echolocation signals embedded in a naturalistic, noisy environment are processed in the bat brain. We end our review by discussing the huge potential that state-of-the-art recording techniques provide to gain a more complete picture on the neuroethology of echolocation behavior.},
language = {en}
}
@article{BeerSteffanDewenterHaerteletal.2016,
author = {Beer, Katharina and Steffan-Dewenter, Ingolf and H{\"a}rtel, Stephan and Helfrich-F{\"o}rster, Charlotte},
title = {A new device for monitoring individual activity rhythms of honey bees reveals critical effects of the social environment on behavior},
series = {Journal of Comparative Physiology A},
volume = {202},
journal = {Journal of Comparative Physiology A},
number = {8},
doi = {10.1007/s00359-016-1103-2},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-188030},
pages = {555-565},
year = {2016},
abstract = {Chronobiological studies of individual activity rhythms in social insects can be constrained by the artificial isolation of individuals from their social context. We present a new experimental set-up that simultaneously measures the temperature rhythm in a queen-less but brood raising mini colony and the walking activity rhythms of singly kept honey bees that have indirect social contact with it. Our approach enables monitoring of individual bees in the social context of a mini colony under controlled laboratory conditions. In a pilot experiment, we show that social contact with the mini colony improves the survival of monitored young individuals and affects locomotor activity patterns of young and old bees. When exposed to conflicting Zeitgebers consisting of a light-dark (LD) cycle that is phase-delayed with respect to the mini colony rhythm, rhythms of young and old bees are socially synchronized with the mini colony rhythm, whereas isolated bees synchronize to the LD cycle. We conclude that the social environment is a stronger Zeitgeber than the LD cycle and that our new experimental set-up is well suited for studying the mechanisms of social entrainment in honey bees.},
language = {en}
}
@article{BeerSchenkHelfrichFoersteretal.2019,
author = {Beer, Katharina and Schenk, Mariela and Helfrich-F{\"o}rster, Charlotte and Holzschuh, Andrea},
title = {The circadian clock uses different environmental time cues to synchronize emergence and locomotion of the solitary bee Osmia bicornis},
series = {Scientific Reports},
volume = {9},
journal = {Scientific Reports},
doi = {10.1038/s41598-019-54111-3},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-202721},
pages = {17748},
year = {2019},
abstract = {Life on earth adapted to the daily reoccurring changes in environment by evolving an endogenous circadian clock. Although the circadian clock has a crucial impact on survival and behavior of solitary bees, many aspects of solitary bee clock mechanisms remain unknown. Our study is the first to show that the circadian clock governs emergence in Osmia bicornis, a bee species which overwinters as adult inside its cocoon. Therefore, its eclosion from the pupal case is separated by an interjacent diapause from its emergence in spring. We show that this bee species synchronizes its emergence to the morning. The daily rhythms of emergence are triggered by temperature cycles but not by light cycles. In contrast to this, the bee's daily rhythms in locomotion are synchronized by light cycles. Thus, we show that the circadian clock of O. bicornis is set by either temperature or light, depending on what activity is timed. Light is a valuable cue for setting the circadian clock when bees have left the nest. However, for pre-emerged bees, temperature is the most important cue, which may represent an evolutionary adaptation of the circadian system to the cavity-nesting life style of O. bicornis.},
language = {en}
}
@article{BeerJoschinskiSastreetal.2017,
author = {Beer, Katharina and Joschinski, Jens and Sastre, Alazne Arrazola and Krauss, Jochen and Helfrich-F{\"o}rster, Charlotte},
title = {A damping circadian clock drives weak oscillations in metabolism and locomotor activity of aphids (Acyrthosiphon pisum)},
series = {Scientific Reports},
volume = {7},
journal = {Scientific Reports},
number = {14906},
doi = {10.1038/s41598-017-15014-3},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-170020},
year = {2017},
abstract = {Timing seasonal events, like reproduction or diapause, is crucial for the survival of many species. Global change causes phenologies worldwide to shift, which requires a mechanistic explanation of seasonal time measurement. Day length (photoperiod) is a reliable indicator of winter arrival, but it remains unclear how exactly species measure day length. A reference for time of day could be provided by a circadian clock, by an hourglass clock, or, as some newer models suggest, by a damped circadian clock. However, damping of clock outputs has so far been rarely observed. To study putative clock outputs of Acyrthosiphon pisum aphids, we raised individual nymphs on coloured artificial diet, and measured rhythms in metabolic activity in light-dark illumination cycles of 16:08 hours (LD) and constant conditions (DD). In addition, we kept individuals in a novel monitoring setup and measured locomotor activity. We found that A. pisum is day-active in LD, potentially with a bimodal distribution. In constant darkness rhythmicity of locomotor behaviour persisted in some individuals, but patterns were mostly complex with several predominant periods. Metabolic activity, on the other hand, damped quickly. A damped circadian clock, potentially driven by multiple oscillator populations, is the most likely explanation of our results.},
language = {en}
}
@article{BeerHaertelHelfrichFoerster2022,
author = {Beer, Katharina and H{\"a}rtel, Stephan and Helfrich-F{\"o}rster, Charlotte},
title = {The pigment-dispersing factor neuronal network systematically grows in developing honey bees},
series = {The Journal of Comparative Neurology},
volume = {530},
journal = {The Journal of Comparative Neurology},
number = {9},
doi = {10.1002/cne.25278},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-257300},
pages = {1321-1340},
year = {2022},
abstract = {The neuropeptide pigment-dispersing factor (PDF) plays a prominent role in the circadian clock of many insects including honey bees. In the honey bee brain, PDF is expressed in about 15 clock neurons per hemisphere that lie between the central brain and the optic lobes. As in other insects, the bee PDF neurons form wide arborizations in the brain, but certain differences are evident. For example, they arborize only sparsely in the accessory medulla (AME), which serves as important communication center of the circadian clock in cockroaches and flies. Furthermore, all bee PDF neurons cluster together, which makes it impossible to distinguish individual projections. Here, we investigated the developing bee PDF network and found that the first three PDF neurons arise in the third larval instar and form a dense network of varicose fibers at the base of the developing medulla that strongly resembles the AME of hemimetabolous insects. In addition, they send faint fibers toward the lateral superior protocerebrum. In last larval instar, PDF cells with larger somata appear and send fibers toward the distal medulla and the medial protocerebrum. In the dorsal part of the medulla serpentine layer, a small PDF knot evolves from which PDF fibers extend ventrally. This knot disappears during metamorphosis and the varicose arborizations in the putative AME become fainter. Instead, a new strongly stained PDF fiber hub appears in front of the lobula. Simultaneously, the number of PDF neurons increases and the PDF neuronal network in the brain gets continuously more complex.},
language = {en}
}
@article{BeerHelfrichFoerster2020,
author = {Beer, Katharina and Helfrich-F{\"o}rster, Charlotte},
title = {Model and Non-model Insects in Chronobiology},
series = {Frontiers in Behavioral Neuroscience},
volume = {14},
journal = {Frontiers in Behavioral Neuroscience},
issn = {1662-5153},
doi = {10.3389/fnbeh.2020.601676},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-218721},
year = {2020},
abstract = {The fruit fly Drosophila melanogaster is an established model organism in chronobiology, because genetic manipulation and breeding in the laboratory are easy. The circadian clock neuroanatomy in D. melanogaster is one of the best-known clock networks in insects and basic circadian behavior has been characterized in detail in this insect. Another model in chronobiology is the honey bee Apis mellifera, of which diurnal foraging behavior has been described already in the early twentieth century. A. mellifera hallmarks the research on the interplay between the clock and sociality and complex behaviors like sun compass navigation and time-place-learning. Nevertheless, there are aspects of clock structure and function, like for example the role of the clock in photoperiodism and diapause, which can be only insufficiently investigated in these two models. Unlike high-latitude flies such as Chymomyza costata or D. ezoana, cosmopolitan D. melanogaster flies do not display a photoperiodic diapause. Similarly, A. mellifera bees do not go into "real" diapause, but most solitary bee species exhibit an obligatory diapause. Furthermore, sociality evolved in different Hymenoptera independently, wherefore it might be misleading to study the social clock only in one social insect. Consequently, additional research on non-model insects is required to understand the circadian clock in Diptera and Hymenoptera. In this review, we introduce the two chronobiology model insects D. melanogaster and A. mellifera, compare them with other insects and show their advantages and limitations as general models for insect circadian clocks.},
language = {en}
}
@article{BeerHelfrichFoerster2020,
author = {Beer, Katharina and Helfrich-F{\"o}rster, Charlotte},
title = {Post-embryonic Development of the Circadian Clock Seems to Correlate With Social Life Style in Bees},
series = {Frontiers in Cell and Developmental Biology},
volume = {8},
journal = {Frontiers in Cell and Developmental Biology},
issn = {2296-634X},
doi = {10.3389/fcell.2020.581323},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-216450},
year = {2020},
abstract = {Social life style can influence many aspects of an animal's daily life, but it has not yet been clarified, whether development of the circadian clock in social and solitary living bees differs. In a comparative study, with the social honey bee, Apis mellifera, and the solitary mason bee, Osmia bicornis, we now found indications for a differentially timed clock development in social and solitary bees. Newly emerged solitary bees showed rhythmic locomotion right away and the number of neurons in the brain that produce the clock component pigment-dispersing factor (PDF) did not change during aging of the adult solitary bee. Honey bees on the other hand, showed no circadian locomotion directly after emergence and the neuronal clock network continued to grow after emergence. Social bees appear to emerge at an early developmental stage at which the circadian clock is still immature, but bees are already able to fulfill in-hive tasks.},
language = {en}
}
@phdthesis{Beer2021,
author = {Beer, Katharina},
title = {A Comparison of the circadian clock of highly social bees (\(Apis\) \(mellifera\)) and solitary bees (\(Osmia\) \(spec.\)): Circadian clock development, behavioral rhythms and neuroanatomical characterization of two central clock components (PER and PDF)},
doi = {10.25972/OPUS-15976},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-159765},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2021},
abstract = {Summary Bees, like many other organisms, evolved an endogenous circadian clock, which enables them to foresee daily environmental changes and exactly time foraging flights to periods of floral resource availability. The social lifestyle of a honey bee colony has been shown to influence circadian behavior in nurse bees, which do not exhibit rhythmic behavior when they are nursing. On the other hand, forager bees display strong circadian rhythms. Solitary bees, like the mason bee, do not nurse their offspring and do not live in hive communities, but face the same daily environmental changes as honey bees. Besides their lifestyle mason and honey bees differ in their development and life history, because mason bees overwinter after eclosion as adults in their cocoons until they emerge in spring. Honey bees do not undergo diapause and have a relatively short development of a few weeks until they emerge. In my thesis, I present a comparison of the circadian clock of social honey bees (Apis mellifera) and solitary mason bees (Osmia bicornis and Osmia cornuta) on the neuroanatomical level and behavioral output level. I firstly characterized in detail the localization of the circadian clock in the bee brain via the expression pattern of two clock components, namely the clock protein PERIOD (PER) and the neuropeptide Pigment Dispersing Factor (PDF), in the brain of honey bee and mason bee. PER is localized in lateral neuron clusters (which we called lateral neurons 1 and 2: LN1 and LN2) and dorsal neuron clusters (we called dorsal lateral neurons and dorsal neurons: DLN, DN), many glia cells and photoreceptor cells. This expression pattern is similar to the one in other insect species and indicates a common ground plan of clock cells among insects. In the LN2 neuron cluster with cell bodies located in the lateral brain, PER is co-expressed with PDF. These cells build a complex arborization network throughout the brain and provide the perfect structure to convey time information to brain centers, where complex behavior, e.g. sun-compass orientation and time memory, is controlled. The PDF arborizations centralize in a dense network (we named it anterio-lobular PDF hub: ALO) which is located in front of the lobula. In other insects, this fiber center is associated with the medulla (accessory medulla: AME). Few PDF cells build the ALO already in very early larval development and the cell number and complexity of the network grows throughout honey bee development. Thereby, dorsal regions are innervated first by PDF fibers and, in late larval development, the fibers grow laterally to the optic lobe and central brain. The overall expression pattern of PER and PDF are similar in adult social and solitary bees, but I found a few differences in the PDF network density in the posterior protocerebrum and the lamina, which may be associated with evolution of sociality in bees. Secondly, I monitored activity rhythms, for which I developed and established a device to monitor locomotor activity rhythms of individual honey bees with contact to a mini colony in the laboratory. This revealed new aspects of social synchronization and survival of young bees with indirect social contact to the mini colony (no trophalaxis was possible). For mason bees, I established a method to monitor emergence and locomotor activity rhythms and I could show that circadian emergence rhythms are entrainable by daily temperature cycles. Furthermore, I present the first locomotor activity rhythms of solitary bees, which show strong circadian rhythms in their behavior right after emergence. Honey bees needed several days to develop circadian locomotor rhythms in my experiments. I hypothesized that honey bees do not emerge with a fully matured circadian system in the hive, while solitary bees, without the protection of a colony, would need a fully matured circadian clock right away after emergence. Several indices in published work and preliminary studies support my hypothesis and future studies on PDF expression in different developmental stages in solitary bees may provide hard evidence.},
subject = {Chronobiologie},
language = {en}
}
@article{BeckerKucharskiRoessleretal.2016,
author = {Becker, Nils and Kucharski, Robert and R{\"o}ssler, Wolfgang and Maleszka, Ryszard},
title = {Age-dependent transcriptional and epigenomic responses to light exposure in the honey bee brain},
series = {FEBS Open Bio},
volume = {6},
journal = {FEBS Open Bio},
number = {7},
doi = {10.1002/2211-5463.12084},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-147080},
pages = {622-639},
year = {2016},
abstract = {Light is a powerful environmental stimulus of special importance in social honey bees that undergo a behavioral transition from in-hive to outdoor foraging duties. Our previous work has shown that light exposure induces structural neuronal plasticity in the mushroom bodies (MBs), a brain center implicated in processing inputs from sensory modalities. Here, we extended these analyses to the molecular level to unravel light-induced transcriptomic and epigenomic changes in the honey bee brain. We have compared gene expression in brain compartments of 1- and 7-day-old light-exposed honey bees with age-matched dark-kept individuals. We have found a number of differentially expressed genes (DEGs), both novel and conserved, including several genes with reported roles in neuronal plasticity. Most of the DEGs show age-related changes in the amplitude of light-induced expression and are likely to be both developmentally and environmentally regulated. Some of the DEGs are either known to be methylated or are implicated in epigenetic processes suggesting that responses to light exposure are at least partly regulated at the epigenome level. Consistent with this idea light alters the DNA methylation pattern of bgm, one of the DEGs affected by light exposure, and the expression of microRNA miR-932. This confirms the usefulness of our approach to identify candidate genes for neuronal plasticity and provides evidence for the role of epigenetic processes in driving the molecular responses to visual stimulation.},
language = {en}
}
@phdthesis{Becker2020,
author = {Becker, Mira Caroline},
title = {Principles of olfactory-visual integration to form a common percept in honeybees},
doi = {10.25972/OPUS-19919},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-199190},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2020},
abstract = {The honeybee is a well studied and important organism in neuroethology. The possibility to train them with a classical conditioning paradigm and their miniature brain provide a perfect requisite to investigate the neuronal principles of learning and memory. Honeybees use visual and olfactory cues to detect flowers during their foraging trips. Hence, the reward association of a nectar source is a multi-modal construct, which has at least two major components - olfactory and visual cues. It is still an open question, how both sensory components are converged in the mushroom body, which represent the multi-modal integration centre of the honeybee brain. The main goal of this study, is to investigate the processing of multiple modalities and how a reward association is formed. This includes, how and wether both sensory modalities interfere during learning. Thus, in this study stimulation with UV, blue and green light was used to evoke distinct photoreceptor activities in the compound eye. Furthermore, three different odours (Geraniol, Citronellol and Farnesol) were used. These stimuli were tested in three different experimental series. The first experiment involved classical differential conditioning of the single modalities - odour and colour. Honeybees showed high learning performances in differentiating olfactory stimuli and also reliable responses for visual conditioning. Furthermore, a temporal discrepancy in the stimulus length for best learning in the olfatcoty and visual cues was found. In the second series, it was tested how multi-modal compounds are perceived. This includes, unique cues (configural processing) or the sum of the single components of a compound (elemen- tal processing). This was tested by combining single odour components with monochromatic light in a positive (PP) and negative patterning (NP) experiment. During PP, the olfactory- visual compound was rewarded, whereas the single components were unrewarded. In contrast, during NP the single components were reinforced, but the compound was not. In addition, the ability to distinguish between two different light stimuli presented as a part of an olfactory-visual compound with the same odour component during acquisition was tested. In a memory test, the light stimuli were presented again as a compound and in addition as the single components. The results revealed that bees used elemental processing with compounds containing green and blue light. In contrast, when UV light was presented the bees used configural processing. Finally, a third experiment was conducted at the neuronal level. Multi-unit recordings were established to provide a suitable method to analyse extrinsic neurons at the mushroom body output region, the so called ventral lobe of the pedunculus. Here, three different odours (Geran- iol, Farnesol and Citronellol), two colours (green and blue) and two combined stimuli (colour + odour) were chosen as stimuli, to search for possible variations in processing stimuli with different modalities. Two units could be detected that responded mainly to visual stimuli.},
language = {en}
}
@article{BeckYuStrzelczykPaulsetal.2018,
author = {Beck, Sebastian and Yu-Strzelczyk, Jing and Pauls, Dennis and Constantin, Oana M. and Gee, Christine E. and Ehmann, Nadine and Kittel, Robert J. and Nagel, Georg and Gao, Shiqiang},
title = {Synthetic light-activated ion channels for optogenetic activation and inhibition},
series = {Frontiers in Neuroscience},
volume = {12},
journal = {Frontiers in Neuroscience},
number = {643},
doi = {10.3389/fnins.2018.00643},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-177520},
year = {2018},
abstract = {Optogenetic manipulation of cells or living organisms became widely used in neuroscience following the introduction of the light-gated ion channel channelrhodopsin-2 (ChR2). ChR2 is a non-selective cation channel, ideally suited to depolarize and evoke action potentials in neurons. However, its calcium (Ca2\(^{2+}\)) permeability and single channel conductance are low and for some applications longer-lasting increases in intracellular Ca\(^{2+}\) might be desirable. Moreover, there is need for an efficient light-gated potassium (K\(^{+}\)) channel that can rapidly inhibit spiking in targeted neurons. Considering the importance of Ca\(^{2+}\) and K\(^{+}\) in cell physiology, light-activated Ca\(^{2+}\)-permeant and K\(^{+}\)-specific channels would be welcome additions to the optogenetic toolbox. Here we describe the engineering of novel light-gated Ca\(^{2+}\)-permeant and K\(^{+}\)-specific channels by fusing a bacterial photoactivated adenylyl cyclase to cyclic nucleotide-gated channels with high permeability for Ca\(^{2+}\) or for K\(^{+}\), respectively. Optimized fusion constructs showed strong light-gated conductance in Xenopus laevis oocytes and in rat hippocampal neurons. These constructs could also be used to control the motility of Drosophila melanogaster larvae, when expressed in motoneurons. Illumination led to body contraction when motoneurons expressed the light-sensitive Ca\(^{2+}\)-permeant channel, and to body extension when expressing the light-sensitive K\(^{+}\) channel, both effectively and reversibly paralyzing the larvae. Further optimization of these constructs will be required for application in adult flies since both constructs led to eclosion failure when expressed in motoneurons.},
language = {en}
}
@article{BeckHovhanyanMenegazzietal.2018,
author = {Beck, Katherina and Hovhanyan, Anna and Menegazzi, Pamela and Helfrich-F{\"o}rster, Charlotte and Raabe, Thomas},
title = {Drosophila RSK Influences the Pace of the Circadian Clock by Negative Regulation of Protein Kinase Shaggy Activity},
series = {Frontiers in Molecular Neuroscience},
volume = {11},
journal = {Frontiers in Molecular Neuroscience},
number = {122},
issn = {1662-5099},
doi = {10.3389/fnmol.2018.00122},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-196034},
year = {2018},
abstract = {Endogenous molecular circadian clocks drive daily rhythmic changes at the cellular, physiological, and behavioral level for adaptation to and anticipation of environmental signals. The core molecular system consists of autoregulatory feedback loops, where clock proteins inhibit their own transcription. A complex and not fully understood interplay of regulatory proteins influences activity, localization and stability of clock proteins to set the pace of the clock. This study focuses on the molecular function of Ribosomal S6 Kinase (RSK) in the Drosophila melanogaster circadian clock. Mutations in the human rsk2 gene cause Coffin-Lowry syndrome, which is associated with severe mental disabilities. Knock-out studies with Drosophila ortholog rsk uncovered functions in synaptic processes, axonal transport and adult behavior including associative learning and circadian activity. However, the molecular targets of RSK remain elusive. Our experiments provide evidence that RSK acts in the key pace maker neurons as a negative regulator of Shaggy (SGG) kinase activity, which in turn determines timely nuclear entry of the clock proteins Period and Timeless to close the negative feedback loop. Phosphorylation of serine 9 in SGG is mediated by the C-terminal kinase domain of RSK, which is in agreement with previous genetic studies of RSK in the circadian clock but argues against the prevailing view that only the N-terminal kinase domain of RSK proteins carries the effector function. Our data provide a mechanistic explanation how RSK influences the molecular clock and imply SGG S9 phosphorylation by RSK and other kinases as a convergence point for diverse cellular and external stimuli.},
language = {en}
}
@phdthesis{Beck2016,
author = {Beck, Katherina},
title = {Einfluss von RSK auf die Aktivit{\"a}t von ERK, den axonalen Transport und die synaptische Funktion in Motoneuronen von \(Drosophila\) \(melanogaster\)},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-130717},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2016},
abstract = {In dieser Arbeit sollte die Funktion von RSK in Motoneuronen von Drosophila untersucht werden. Mutationen im RSK2-Gen verursachen das Coffin-Lowry-Syndrom (CLS), das durch mentale Retardierung charakterisiert ist. RSK2 ist haupts{\"a}chlich in Regionen des Gehirns exprimiert, in denen Lernen und Ged{\"a}chtnisbildung stattfinden. In M{\"a}usen und Drosophila, die als Modellorganismen f{\"u}r CLS dienen, konnten auf makroskopischer Ebene keine Ver{\"a}nderungen in den Hirnstrukturen gefunden werden, dennoch wurden in verschiedenen Verhaltensstudien Defekte im Lernen und der Ged{\"a}chtnisbildung beobachtet. Die synaptische Plastizit{\"a}t und die einhergehenden Ver{\"a}nderungen in den Eigenschaften der Synapse sind fundamental f{\"u}r adaptives Verhalten. Zur Analyse der synaptischen Plastizit{\"a}t eignet sich das neuromuskul{\"a}re System von Drosophila als Modell wegen des stereotypen Innervierungsmusters und der Verwendung ionotroper Glutamatrezeptoren, deren Untereinheiten homolog sind zu den Untereinheiten der Glutamatrezeptoren des AMPA-Typs aus S{\"a}ugern, die wesentlich f{\"u}r die Bildung von LTP im Hippocampus sind. Zun{\"a}chst konnte gezeigt werden, dass RSK in den Motoneuronen von Drosophila an der pr{\"a}synaptischen Seite lokalisiert ist, wodurch RSK eine Synapsen-spezifische Funktion aus{\"u}ben k{\"o}nnte. Morphologische Untersuchungen der Struktur der neuromuskul{\"a}ren Synapsen konnten aufzeigen, dass durch den Verlust von RSK die Gr{\"o}ße der neuromuskul{\"a}ren Synapse, der Boutons sowie der Aktiven Zonen und Glutamatrezeptorfelder reduziert ist. Obwohl mehr Boutons gebildet werden, sind weniger Aktive Zonen und Glutamatrezeptorfelder in der neuromuskul{\"a}ren Synapse enthalten. RSK reguliert die synaptische Transmission, indem es die postsynaptische Sensitivit{\"a}t, nicht aber die Freisetzung der Neurotransmitter an der pr{\"a}synaptischen Seite beeinflusst, obwohl in immunhistochemischen Analysen eine postsynaptische Lokalisierung von RSK nicht nachgewiesen werden konnte. RSK ist demnach an der Regulation der synaptischen Plastizit{\"a}t glutamaterger Synapsen beteiligt. Durch immunhistochemische Untersuchungen konnte erstmals gezeigt werden, dass aktiviertes ERK an der pr{\"a}synaptischen Seite lokalisiert ist und diese synaptische Lokalisierung von RSK reguliert wird. Dar{\"u}ber hinaus konnte in dieser Arbeit nachgewiesen werden, dass durch den Verlust von RSK hyperaktiviertes ERK in den Zellk{\"o}rpern der Motoneurone vorliegt. RSK wird durch den ERK/MAPK-Signalweg aktiviert und {\"u}bernimmt eine Funktion sowohl als Effektorkinase als auch in der Negativregulation des Signalwegs. Demnach dient RSK in den Zellk{\"o}rpern der Motoneurone als Negativregulator des ERK/MAPK-Signalwegs. Dar{\"u}ber hinaus k{\"o}nnte RSK die Verteilung von aktivem ERK in den Subkompartimenten der Motoneurone regulieren. Da in vorangegangenen Studien gezeigt werden konnte, dass ERK an der Regulation der synaptischen Plastizit{\"a}t beteiligt ist, indem es die Insertion der AMPA-Rezeptoren zur Bildung der LTP reguliert, sollte in dieser Arbeit aufgekl{\"a}rt werden, ob der Einfluss von RSK auf die synaptische Plastizit{\"a}t durch seine Funktion als Negativregulator von ERK zustande kommt. Untersuchungen der genetischen Interaktion von rsk und rolled, dem Homolog von ERK in Drosophila, zeigten, dass die durch den Verlust von RSK beobachtete reduzierte Gesamtzahl der Aktiven Zonen und Glutamatrezeptorfelder der neuromuskul{\"a}ren Synapse auf die Funktion von RSK als Negativregulator von ERK zur{\"u}ckzuf{\"u}hren ist. Die Gr{\"o}ße der neuromuskul{\"a}ren Synapse sowie die Gr{\"o}ße der Aktiven Zonen und Glutamatrezeptorfelder beeinflusst RSK allerdings durch seine Funktion als Effektorkinase des ERK/MAPK-Signalwegs. Studien des axonalen Transports von Mitochondrien zeigten, dass dieser in vielen neuropathologischen Erkrankungen beeintr{\"a}chtigt ist. Die durchgef{\"u}hrten Untersuchungen des axonalen Transports in Motoneuronen konnten eine neue Funktion von RSK in der Regulation des axonalen Transports aufdecken. In den Axonen der Motoneurone von RSK-Nullmutanten wurden BRP- und CSP-Agglomerate nachgewiesen. RSK k{\"o}nnte an der Regulation des axonalen Transports von pr{\"a}synaptischem Material beteiligt sein. Durch den Verlust von RSK wurden weniger Mitochondrien in anterograder Richtung entlang dem Axon transportiert, daf{\"u}r verweilten mehr Mitochondrien in station{\"a}ren Phasen. Diese Ergebnisse zeigen, dass auch der anterograde Transport von Mitochondrien durch den Verlust von RSK beeintr{\"a}chtigt ist.},
subject = {Taufliege},
language = {de}
}
@phdthesis{Beck2019,
author = {Beck, Katharina},
title = {Die nitrerge Neurotransmission im Gastrointestinaltrakt der Maus},
doi = {10.25972/OPUS-15989},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-159896},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2019},
abstract = {Die NO-sensitive Guanylyl-Cyclase (NO-GC) ist ein zentrales Enzym der NO/cGMP-Signalkaskade, das {\"u}ber die Aktivierung von NO zur Bildung des second messangers cGMP f{\"u}hrt. Die NO-GC setzt sich aus zwei Untereinheiten zusammen, sodass zwei Isoformen des Enzyms gebildet werden k{\"o}nnen (α1β1 und α2β1). Da die genaue Verteilung der beiden Isoformen im Colon nicht bekannt ist, wurde diese im ersten Teil dieser Arbeit charakterisiert. Immunhistochemie und In-situ-Hybridisierung zeigten die Expression beider Isoformen sowohl in der glatten Muskelschicht als auch in der Submukosa und Lamina propria. Dabei war die α1β1-Isoform ubiquit{\"a}r, die α2β1-Isoform dagegen haupts{\"a}chlich im Bereich des myenterischen Plexus vorzufinden. In der glatten Muskelschicht des Colons ist die NO-GC in glatten Muskelzellen (SMC), interstitiellen Zellen von Cajal (ICC) sowie Fibroblasten-{\"a}hnliche Zellen (FLC) exprimiert und haupts{\"a}chlich in die Modulation der gastrointestinalen Motilit{\"a}t involviert. Zur spezifischen Charakterisierung der Funktion der NO-GC in den einzelnen Zelltypen wurden Knockout-M{\"a}use generiert, denen die NO-GC global (GCKO) oder spezifisch in SMC (SMC-GCKO), ICC (ICC-GCKO) oder beiden Zelltypen (SMC/ICC-GCKO) fehlt. Anhand dieser Mausmodelle sollten im zweiten Teil dieser Arbeit die modulatorischen Effekte der NO-GC auf die spontanen Kontraktionen des Colons bestimmt werden. Zur Charakterisierung der spontanen Kontraktionen der zirkul{\"a}ren Muskelschicht wurden Myographiestudien mit 2,5 mm langen Colonringen durchgef{\"u}hrt. Hierbei konnten drei verschiedene Kontraktionen gemessen werden: Kleine, hochfrequente Ripples, mittlere Kontraktionen und große Kontraktionen. Die detaillierte Analyse der einzelnen Kontraktionen zeigte einerseits eine NO-unabh{\"a}ngige Regulation der Ripples, andererseits eine NO-abh{\"a}ngige Modulation der mittleren und großen Kontraktionen {\"u}ber die NO-GC in SMC und ICC. Die NO-GC in SMC beeinflusst die Kontraktionen vermutlich vor allem {\"u}ber die Regulation des Muskeltonus der zirkul{\"a}ren Muskelschicht. Die NO-GC in ICC dagegen modifiziert die spontanen Kontraktionen m{\"o}glicherweise {\"u}ber eine Ver{\"a}nderung der Schrittmacheraktivit{\"a}t. Allerdings f{\"u}hrt erst ein Funktionsverlust des NO/cGMP-Signalweges in beiden Zelltypen zu einem sichtbar ver{\"a}nderten Kontraktionsmuster, das dem von globalen Knockout-Tieren glich. Dies weist auf eine kompensatorische Wirkung der NO-GC im jeweils anderen Zelltyp hin. Zur Analyse der propulsiven Kontraktionen entlang des gesamten Colons wurden Videoaufnahmen der Darmbewegungen in Kontraktionsmusterkarten transformiert. Zudem wurde der Darm durchsp{\"u}lt und die Ausflusstropfen aufgezeichnet, um die Effektivit{\"a}t der Kontraktionen beurteilen zu k{\"o}nnen. Hierbei zeigte sich, dass eine Beeintr{\"a}chtigung des NO/cGMP-Signalweges eine verminderte Effektivit{\"a}t der Kontraktionen zur Folge hat und vermutlich durch eine beeintr{\"a}chtige Synchronisation der Kontraktionen erkl{\"a}rt werden kann. In diesem Regulationsmechanismus konnte vor allem der NO-GC in SMC eine {\"u}bergeordnete Rolle zugewiesen werden. Der dritte Teil der Arbeit thematisierte den Befund, dass SMC-GCKO-Tiere ca. 5 Monate nach Tamoxifen-Behandlung Entartungen der Mukosa entwickelten. Diese Entartung war lediglich in Tamoxifen-induzierten Knockout-Tieren vorzufinden. Histologische Analysen identifizierten die Entartungen als tubulovill{\"o}ses Adenom. Die Genexpressionsanalyse von Mukosafalten von SMC-GCKO- und heterozygoten Kontrolltieren zeigte eine Vielzahl von Genen, welche spezifisch bei colorectalem Karzinom differenziell exprimiert sind. Einer dieser Faktoren war der BMP-Antagonist Gremlin1. Dieser Faktor erschien von besonderem Interesse, da er in Zellen der Lamina muscularis mucosae und kryptennahen Myofibroblasten exprimiert wird. Immunhistochemische Analysen ließen vermuten, dass diese Zellen sowohl die NO-GC als auch die Cre-Rekombinase unter dem SMMHC-Promotor exprimieren. Diese Arbeit liefert demnach Hinweise darauf, dass die NO-GC einen wichtigen Regulator innerhalb der Stammzellnische bildet. Die Deletion der NO-GC f{\"u}hrt vermutlich zu einer verst{\"a}rkten Bildung bzw. Sekretion von Gremlin1, was die Hom{\"o}ostase der mukosalen Erneuerung st{\"o}rt und somit zur Entwicklung von Adenomen f{\"u}hrt.},
subject = {Gastrointestinaltrakt},
language = {de}
}
@phdthesis{Beck2005,
author = {Beck, Jan},
title = {The macroecology of Southeast-Asian hawkmoths (Lepidoptera: Sphingidae)},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-13001},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2005},
abstract = {This study investigates the abundance and geographic distribution of the hawkmoth species (Lepidoptera: Sphingidae) of Southeast-Asia and analyses the resulting patterns of biodiversity, biogeography and macroecology. Data on the distribution of species were retrieved from published and unpublished faunal lists and museum collections (in close cooperation with the Natural History Museum, London). Over 34,500 records of the global distribution of the 380 species that occur in Southeast-Asia (including New Guinea and the Solomon Islands) were used for a GIS-supported estimate of distributional ranges, which can be accessed at http://www.sphingidae-sea.biozentrum.uni-wuerzburg.de, an Internet site that also provides pictures of the species and checklists for 114 islands of the Malesian region. The abundance of species in local assemblages was assessed from nightly collections at artificial light sources. Using a compilation of own samples as well as published and unpublished data from other sources, local abundance data on 93 sites were used for analysis, covering 159 species or 17,676 specimens.},
language = {en}
}
@article{BecherAndresPonsRomanovetal.2018,
author = {Becher, Isabelle and Andr{\´e}s-Pons, Amparo and Romanov, Natalie and Stein, Frank and Schramm, Maike and Baudin, Florence and Helm, Dominic and Kurzawa, Nils and Mateus, Andr{\´e} and Mackmull, Marie-Therese and Typas, Athanasios and M{\"u}ller, Christoph W. and Bork, Peer and Beck, Martin and Savitski, Mikhail M.},
title = {Pervasive Protein Thermal Stability Variation during the Cell Cycle},
series = {Cell},
volume = {173},
journal = {Cell},
doi = {10.1016/j.cell.2018.03.053},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-221565},
pages = {1495-1507},
year = {2018},
abstract = {Quantitative mass spectrometry has established proteome-wide regulation of protein abundance and post-translational modifications in various biological processes. Here, we used quantitative mass spectrometry to systematically analyze the thermal stability and solubility of proteins on a proteome-wide scale during the eukaryotic cell cycle. We demonstrate pervasive variation of these biophysical parameters with most changes occurring in mitosis and G1. Various cellular pathways and components vary in thermal stability, such as cell-cycle factors, polymerases, and chromatin remodelers. We demonstrate that protein thermal stability serves as a proxy for enzyme activity, DNA binding, and complex formation in situ. Strikingly, a large cohort of intrinsically disordered and mitotically phosphorylated proteins is stabilized and solubilized in mitosis, suggesting a fundamental remodeling of the biophysical environment of the mitotic cell. Our data represent a rich resource for cell, structural, and systems biologists interested in proteome regulation during biological transitions.},
language = {en}
}
@article{BecamWalterBurgertetal.2017,
author = {Becam, J{\´e}r{\^o}me and Walter, Tim and Burgert, Anne and Schlegel, Jan and Sauer, Markus and Seibel, J{\"u}rgen and Schubert-Unkmeir, Alexandra},
title = {Antibacterial activity of ceramide and ceramide analogs against pathogenic Neisseria},
series = {Scientific Reports},
volume = {7},
journal = {Scientific Reports},
doi = {10.1038/s41598-017-18071-w},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-159367},
pages = {17627},
year = {2017},
abstract = {Certain fatty acids and sphingoid bases found at mucosal surfaces are known to have antibacterial activity and are thought to play a more direct role in innate immunity against bacterial infections. Herein, we analysed the antibacterial activity of sphingolipids, including the sphingoid base sphingosine as well as short-chain C\(_{6}\) and long-chain C\(_{16}\)-ceramides and azido-functionalized ceramide analogs against pathogenic Neisseriae. Determination of the minimal inhibitory concentration (MIC) and minimal bactericidal concentration (MBC) demonstrated that short-chain ceramides and a ω-azido-functionalized C\(_{6}\)-ceramide were active against Neisseria meningitidis and N. gonorrhoeae, whereas they were inactive against Escherichia coli and Staphylococcus aureus. Kinetic assays showed that killing of N. meningitidis occurred within 2 h with ω-azido-C\(_{6}\)-ceramide at 1 X the MIC. Of note, at a bactericidal concentration, ω-azido-C\(_{6}\)-ceramide had no significant toxic effect on host cells. Moreover, lipid uptake and localization was studied by flow cytometry and confocal laser scanning microscopy (CLSM) and revealed a rapid uptake by bacteria within 5 min. CLSM and super-resolution fluorescence imaging by direct stochastic optical reconstruction microscopy demonstrated homogeneous distribution of ceramide analogs in the bacterial membrane. Taken together, these data demonstrate the potent bactericidal activity of sphingosine and synthetic short-chain ceramide analogs against pathogenic Neisseriae.},
language = {en}
}
@article{BazihizinaBoehmMessereretal.2022,
author = {Bazihizina, Nadia and B{\"o}hm, Jennifer and Messerer, Maxim and Stigloher, Christian and M{\"u}ller, Heike M. and Cuin, Tracey Ann and Maierhofer, Tobias and Cabot, Joan and Mayer, Klaus F. X. and Fella, Christian and Huang, Shouguang and Al-Rasheid, Khaled A. S. and Alquraishi, Saleh and Breadmore, Michael and Mancuso, Stefano and Shabala, Sergey and Ache, Peter and Zhang, Heng and Zhu, Jian-Kang and Hedrich, Rainer and Scherzer, S{\"o}nke},
title = {Stalk cell polar ion transport provide for bladder-based salinity tolerance in Chenopodium quinoa},
series = {New Phytologist},
volume = {235},
journal = {New Phytologist},
number = {5},
doi = {10.1111/nph.18205},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-287222},
pages = {1822 -- 1835},
year = {2022},
abstract = {Chenopodium quinoa uses epidermal bladder cells (EBCs) to sequester excess salt. Each EBC complex consists of a leaf epidermal cell, a stalk cell, and the bladder. Under salt stress, sodium (Na\(^{+}\)), chloride (Cl\(^{-}\)), potassium (K\(^{+}\)) and various metabolites are shuttled from the leaf lamina to the bladders. Stalk cells operate as both a selectivity filter and a flux controller. In line with the nature of a transfer cell, advanced transmission electron tomography, electrophysiology, and fluorescent tracer flux studies revealed the stalk cell's polar organization and bladder-directed solute flow. RNA sequencing and cluster analysis revealed the gene expression profiles of the stalk cells. Among the stalk cell enriched genes, ion channels and carriers as well as sugar transporters were most pronounced. Based on their electrophysiological fingerprint and thermodynamic considerations, a model for stalk cell transcellular transport was derived.},
language = {en}
}
@phdthesis{Bausenwein2000,
author = {Bausenwein, Burkhard},
title = {Funktionelle Charakterisierung von Daughter of Sevenless},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-814},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2000},
abstract = {Ein Weg, der von Rezeptor-Tyrosin-Kinasen benutzt wird um Signale auf "downstream" gelegene Effektormolek{\"u}le zu {\"u}bertragen, erfolgt {\"u}ber Adaptorproteine, die Bindungsstellen f{\"u}r verschiedene Proteine zur Verf{\"u}gung stellen. Das daughter of sevenless (dos) Gen wurde in einem Screen nach Downstream-Komponenten der Sevenless (Sev) Rezeptor-Tyrosin-Kinase gefunden. Dos besitzt eine N-terminale PH-Dom{\"a}ne und mehrere Tyrosinreste in Konsensussequenzen f{\"u}r SH2-Dom{\"a}nen Bindungsstellen von verschiedenen Proteinen. Die strukturellen Merkmale von Dos und Experimente, die zeigten, daß Tyrosine im Dos Protein nach der Aktivierung von Sev phosphoryliert werden, legen den Schluß nahe, daß Dos zur Familie der Multi-Adaptor-Proteine geh{\"o}rt. Zu dieser Familie werden die Insulin-Rezeptor-Substrat (IRS) Proteine, Gab1 und Gab2 gerechnet. In dieser Arbeit wurde ein monoklonaler Maus anti-Dos Antik{\"o}rper etabliert. Das Epitop dieses Antik{\"o}rpers liegt im Bereich der C-terminalen 416 Aminos{\"a}uren des Dos Proteins. Mittels Westernblot Analysen wurde f{\"u}r Dos ein Molekulargewicht von 115 kD ermittelt. Antik{\"o}rperf{\"a}rbungen von wildtypischen Augenimaginalscheiben dritter Larven zeigten, daß das Dos Protein in Zellen in und posterior der morphogenetischen Furche exprimiert wird und in diesen Zellen apikal lokalisiert ist. Zur Charakterisierung des homozygot letalen dosR31 Allels, wurde der genomische Bereich sequenziert und die erhaltenen Daten mit der cDNA Sequenz verglichen. Die so etablierte Aminos{\"a}uresequenz f{\"u}r das DosR31 Protein hat sechs Aminos{\"a}uresubstitutionen, die m{\"o}glicherweise die Terti{\"a}rstruktur beeinflussen. Zus{\"a}tzlich wurde ein Stopcodon in Position 463 der Aminos{\"a}uresequenz gefunden. Bei dosR31 handelt es sich um ein "loss of function" Allel, das nicht in der Lage ist, die normale Dos Funktion zu erf{\"u}llen. Um die funktionelle Rolle der potentiellen SH2-Dom{\"a}nen Bindungsstellen f{\"u}r die Dos Funktion in der Rezeptor-Tyrosin-Kinasen vermittelten Signaltransduktion zu untersuchen, wurden mutierte dos Transgene in Fliegen exprimiert. Die potentiellen Bindungsstellen f{\"u}r die SH2-Dom{\"a}nen des SH2/SH3 Adaptorproteins Shc, der PhospholipaseC-g (PLCg), der regulatorische Untereinheit der Phosphatidylinositol-3-Kinase (PI3Kinase) und der Corkscrew (Csw) Tyrosin Phosphatase wurden durch den Austausch des f{\"u}r die Bindung wichtigen Tyrosins gegen ein Phenylalanin mutiert. Die ektopische Expression der mutierten Konstrukte ohne Bindungsstellen f{\"u}r die Shc, PLCg und PI3Kinasen SH2-Dom{\"a}nen konnte in Abwesenheit von endogenem Dos die fehlende Dos Funktion w{\"a}hrend der Entwicklung vollst{\"a}ndig ersetzen. Im Gegensatz dazu ist das Tyrosin 801 als nachgewiesene Bindungsstelle f{\"u}r Csw SH2-Dom{\"a}nen essentiell f{\"u}r die Funktion von Dos. Ektopische Expression von Transgene durch Hitzeschock kann zu ph{\"a}notypischen Effekten f{\"u}hren, die nicht auf das Transgen zur{\"u}ckzuf{\"u}hren sind. Um dieses Problem zu umgehen wurde das endogene dos Enhancer/Promotor Element kloniert, damit die Funktion von mutierten Transgenen auch im endogenen Expressionsmuster untersucht werden konnte. Das klonierte genE-dos Minigen war in der Lage, den Verlust von endogenem Dos in dosR31 und dosP115 Tieren vollst{\"a}ndig zu ersetzen und zeigte eine v{\"o}llig wildtypische Expression in Augenimaginalscheiben. Zur Untersuchung, welche Rolle die mutierten SH2-Dom{\"a}nen Bindungsstellen bei der Dos Funktion in der Augenentwicklung spielen, wurde ein neues in vivo Testsystem basierend auf der Flp/FRT Flipase Rekombinase Technik etabliert. Dieses klonale Testsystem erlaubt die Expression mutierter Transgene unter der Kontrolle der dos Enhancer/Promotor Sequenzen in Klonen von Zellen, denen die endogene Dos Funktion fehlt. Die klonale Analyse der mutierten Konstrukte konnte zeigen, daß das Tyrosin 801, als Bindungsstelle f{\"u}r eine Csw SH2-Dom{\"a}ne, eine essentielle Rolle f{\"u}r die Dos Funktion spielt. Die Tyrosinreste in den potentiellen SH2-Dom{\"a}nen Bindungsstellen f{\"u}r Shc, PLCg und PI3Kinase spielen hingegen keine essentielle Rolle f{\"u}r die Dos Funktion bei der Augenentwicklung. Das etablierte klonale Testsystem kann allgemein zur Untersuchung der in vivo Funktion von potentiellen Protein-Protein Interaktionsregionen im Dos Protein bei der Augenentwicklung eingesetzt werden unabh{\"a}ngig von deren Erfordernis f{\"u}r andere Entwicklungsprozesse.},
subject = {Taufliege},
language = {de}
}
@article{BaurRautenbergFaulstichetal.2014,
author = {Baur, Stefanie and Rautenberg, Maren and Faulstich, Manuela and Grau, Timo and Severin, Yannik and Unger, Clemens and Hoffmann, Wolfgang H. and Rudel, Thomas and Autenrieth, Ingo B. and Weidenmaier, Christopher},
title = {A Nasal Epithelial Receptor for Staphylococcus aureus WTA Governs Adhesion to Epithelial Cells and Modulates Nasal Colonization},
series = {PLOS PATHOGENS},
volume = {10},
journal = {PLOS PATHOGENS},
number = {5},
issn = {1553-7374},
doi = {10.1371/journal.ppat.1004089},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-116280},
pages = {e1004089},
year = {2014},
abstract = {Nasal colonization is a major risk factor for S. aureus infections. The mechanisms responsible for colonization are still not well understood and involve several factors on the host and the bacterial side. One key factor is the cell wall teichoic acid (WTA) of S. aureus, which governs direct interactions with nasal epithelial surfaces. We report here the first receptor for the cell wall glycopolymer WTA on nasal epithelial cells. In several assay systems this type F-scavenger receptor, termed SREC-I, bound WTA in a charge dependent manner and mediated adhesion to nasal epithelial cells in vitro. The impact of WTA and SREC-I interaction on epithelial adhesion was especially pronounced under shear stress, which resembles the conditions found in the nasal cavity. Most importantly, we demonstrate here a key role of the WTA-receptor interaction in a cotton rat model of nasal colonization. When we inhibited WTA mediated adhesion with a SREC-I antibody, nasal colonization in the animal model was strongly reduced at the early onset of colonization. More importantly, colonization stayed low over an extended period of 6 days. Therefore we propose targeting of this glycopolymer-receptor interaction as a novel strategy to prevent or control S. aureus nasal colonization.},
language = {en}
}
@article{BaurNietzerKunzetal.2020,
author = {Baur, Florentin and Nietzer, Sarah L. and Kunz, Meik and Saal, Fabian and Jeromin, Julian and Matschos, Stephanie and Linnebacher, Michael and Walles, Heike and Dandekar, Thomas and Dandekar, Gudrun},
title = {Connecting cancer pathways to tumor engines: a stratification tool for colorectal cancer combining human in vitro tissue models with boolean in silico models},
series = {Cancers},
volume = {12},
journal = {Cancers},
number = {1},
issn = {2072-6694},
doi = {10.3390/cancers12010028},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-193798},
pages = {28},
year = {2020},
abstract = {To improve and focus preclinical testing, we combine tumor models based on a decellularized tissue matrix with bioinformatics to stratify tumors according to stage-specific mutations that are linked to central cancer pathways. We generated tissue models with BRAF-mutant colorectal cancer (CRC) cells (HROC24 and HROC87) and compared treatment responses to two-dimensional (2D) cultures and xenografts. As the BRAF inhibitor vemurafenib is—in contrast to melanoma—not effective in CRC, we combined it with the EGFR inhibitor gefitinib. In general, our 3D models showed higher chemoresistance and in contrast to 2D a more active HGFR after gefitinib and combination-therapy. In xenograft models murine HGF could not activate the human HGFR, stressing the importance of the human microenvironment. In order to stratify patient groups for targeted treatment options in CRC, an in silico topology with different stages including mutations and changes in common signaling pathways was developed. We applied the established topology for in silico simulations to predict new therapeutic options for BRAF-mutated CRC patients in advanced stages. Our in silico tool connects genome information with a deeper understanding of tumor engines in clinically relevant signaling networks which goes beyond the consideration of single drivers to improve CRC patient stratification.},
language = {en}
}
@article{BatzkeBuechelHansenetal.2018,
author = {Batzke, Katharina and B{\"u}chel, Gabriele and Hansen, Wiebke and Schramm, Alexander},
title = {TrkB-target Galectin-1 impairs immune activation and radiation responses in neuroblastoma: implications for tumour therapy},
series = {International Journal of Molecular Sciences},
volume = {19},
journal = {International Journal of Molecular Sciences},
number = {3},
issn = {1422-0067},
doi = {10.3390/ijms19030718},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-285097},
year = {2018},
abstract = {Galectin-1 (Gal-1) has been described to promote tumour growth by inducing angiogenesis and to contribute to the tumour immune escape. We had previously identified up-regulation of Gal-1 in preclinical models of aggressive neuroblastoma (NB), the most common extracranial tumour of childhood. While Gal-1 did not confer a survival advantage in the absence of exogenous stressors, Gal-1 contributed to enhanced cell migratory and invasive properties. Here, we review these findings and extend them by analyzing Gal-1 mediated effects on immune cell regulation and radiation resistance. In line with previous results, cell autonomous effects as well as paracrine functions contribute to Gal-1 mediated pro-tumourigenic functions. Interfering with Gal-1 functions in vivo will add to a better understanding of the role of the Gal-1 axis in the complex tumour-host interaction during immune-, chemo- and radiotherapy of neuroblastoma.},
language = {en}
}
@phdthesis{Batzilla2011,
author = {Batzilla, Julia},
title = {Complete genome sequence of Yersinia enterocolitica subspecies palearctica serotype O:3: Identification of novel virulence-associated genes and evolutionary aspects},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-69668},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2011},
abstract = {Yersinia enterocolitica subsp. palearctica Serobiotyp O:3/4 ist verantwortlich f{\"u}r 80-90 \% aller Yersiniosen beim Menschen in Deutschland und Europa. Y. enterocolitica Infektionen zeigen vielf{\"a}ltige Krankheitsbilder wie Gastroenteritis, Lymphadenitis und verschiedene Sp{\"a}tkomplikationen wie reaktive Arthritis. Das wichtigste Tierreservoir stellt das Hausschwein dar. Rohes Schweinefleisch in Metzgereien in Deutschland und anderen Regionen in Nord-Ost Europa ist h{\"a}ufig mit Yersinien kontaminiert (Bayern: 25 \%). Da sich Serobiotyp O:3/4-St{\"a}mme geografisch und phylogenetisch deutlich von dem bisher sequenzierten Serobiotyp O:8/1B Stamm 8081 unterscheiden, wurde eine komplette Genomsequenzierung des europ{\"a}ischen Serobiotyp O:3/4 DSMZ Referenzstammes Y11 (aus Patientenstuhl isoliert) durchgef{\"u}hrt. Um einen genaueren Einblick in die Y. enterocolitica subsp. palearctica Gruppe zu erhalten, wurden zus{\"a}tzlich zwei weitere Serobiotyp O:3/4 Isolate (Stamm Y8265, Patientenisolat, und Stamm Y5307, mit reaktiver Arthritis assoziiertes Patientenisolat), sowie ein eng verwandtes Y. enterocolitica subsp. palearctica Serobiotyp O:5,27/3 Isolat, Stamm Y527P, und zwei Biotyp 1A Isolate (ein Isolat nosokomialer Herkunft (Serogruppe O:5) und ein Umwelt-Isolat (O:36)) unvollst{\"a}ndig sequenziert. Die nicht mausvirulenten St{\"a}mme wurden mit dem mausvirulenten Y. enterocolitica subsp. enterocolitica Serobiotyp O:8/1B Stamm 8081 verglichen, um genetische Besonderheiten von Stamm Y11 und der Y. enterocolitica subsp. palearctica Gruppe zu identifizieren. Besonderer Fokus lag hierbei auf dem pathogenen Potential von Stamm Y11, um neue potentielle Virulenz Faktoren und Fitnessfaktoren zu identifizieren, darunter vor allem solche, die eine Rolle bei der Wirtsspezifit{\"a}t von Serobiotyp O:3/4 spielen k{\"o}nnten. Y. enterocolitica subsp. palearctica Serobiotyp O:3/4 St{\"a}mmen fehlen einige der Charakteristika der mausvirulenten Gruppe Y. enterocolitica subsp. enterocolitica, beispielsweise die Yersiniabactin kodierende‚ High-Pathogenicity Island (HPI), das Yts1 Typ 2 Sekretionssystem und das Ysa Typ 3 Sekretionssystem. Die Serobiotyp O:3/4-St{\"a}mme haben ein anderes Repertoir von Virulenz Faktoren erworben, darunter Gene bzw. genomische Inseln f{\"u}r das Ysp Typ 3 Sekretionssystem, Rtx-{\"a}hnliches putatives Toxin, Insektizid-Toxine und ein funktionelles PTS System f{\"u}r die Aufnahme von N-acetyl-galactosamin, dem aga-Operon. Nach dem Transfer des aga-Operons in Y. enterocolitica subsp. enterocolitica O:8/1B konnte Wachstum auf N-acetyl-galactosamin festgestellt werden. Neben diesen Genen k{\"o}nnen m{\"o}glicherweise auch zwei Prophagen (PhiYep-2 und PhiYep-3) und eine asn tRNA assoziierte genomische Insel (GIYep-01) zur Pathoadaptation von Y. enterocolitica subsp. palearctica Serobiotyp O:3/4 beitragen. Der PhiYep-3 Prophage und die GIYep-01 Insel weisen Rekombinationsaktivit{\"a}t auf, und PhiYep-3 wurde nicht in allen untersuchten Serobiotyp O:3/4 St{\"a}mmen gefunden. Y. enterocolitica subsp. palearctica Serobiotyp O:5,27/3 Stamm Y527P ist genetisch eng verwandt zu allen Serobiotyp O:3/4 Isolaten, wohingegen die Biotyp 1A Isolate ein mehr Mosaik-artiges Genom aufweisen und potentielle Virulenzgene sowohl mit Serobiotyp O:8/1B als auch O:3/4 gemeinsam haben, was einen gemeinsamen Vorfahren impliziert. Neben dem pYV Virulenz-Plasmid fehlen den Biotyp 1A Isolaten klassische Virulenzmarker wie das Ail Adhesin, das YstA Enterotoxin und das Virulenz-assoziierte Protein C (VapC). Interessanterweise gibt es keine betr{\"a}chtlichen Unterschiede zwischen den bekannten Virulenzfaktoren des nosokomialen Isolats und dem Umweltisolat der Biotyp 1A-Gruppe, abgesehen von einem verk{\"u}rzten Rtx Toxin-{\"a}hnlichem Genkluster und {\"U}berresten eines P2-{\"a}hnlichen Phagen im Krankenhausisolat der Serogruppe O:5.},
subject = {Genanalyse},
language = {en}
}
@article{BatramJonesJanzenetal.2014,
author = {Batram, Christopher and Jones, Nivola G. and Janzen, Christian J. and Markert, Sebastian M. and Engstler, Markus},
title = {Expression site attenuation mechanistically links antigenic variation and development in Trypanosoma brucei},
series = {eLife},
volume = {3},
journal = {eLife},
number = {e02324},
issn = {2050-084X},
doi = {10.7554/eLife.02324},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-119727},
year = {2014},
abstract = {We have discovered a new mechanism of monoallelic gene expression that links antigenic variation, cell cycle, and development in the model parasite Trypanosoma brucei. African trypanosomes possess hundreds of variant surface glycoprotein (VSG) genes, but only one is expressed from a telomeric expression site (ES) at any given time. We found that the expression of a second VSG alone is sufficient to silence the active VSG gene and directionally attenuate the ES by disruptor of telomeric silencing-1B (DOT1B)-mediated histone methylation. Three conserved expression-site-associated genes (ESAGs) appear to serve as signal for ES attenuation. Their depletion causes G1-phase dormancy and reversible initiation of the slender-to-stumpy differentiation pathway. ES-attenuated slender bloodstream trypanosomes gain full developmental competence for transformation to the tsetse fly stage. This surprising connection between antigenic variation and developmental progression provides an unexpected point of attack against the deadly sleeping sickness.},
language = {en}
}
@article{BassetCizekCuenoudetal.2015,
author = {Basset, Yves and Cizek, Lukas and Cu{\´e}noud, Philippe and Didham, Raphael K. and Novotny, Vojtech and {\O}degaard, Frode and Roslin, Tomas and Tishechkin, Alexey K. and Schmidl, J{\"u}rgen and Winchester, Neville N. and Roubik, David W. and Aberlenc, Henri-Pierre and Bail, Johannes and Barrios, Hector and Bridle, Jonathan R. and Casta{\~n}o-Meneses, Gabriela and Corbara, Bruno and Curletti, Gianfranco and da Rocha, Wesley Duarte and De Bakker, Domir and Delabie, Jacques H. C. and Dejean, Alain and Fagan, Laura L. and Floren, Andreas and Kitching, Roger L. and Medianero, Enrique and de Oliveira, Evandro Gama and Orivel, Jerome and Pollet, Marc and Rapp, Mathieu and Ribeiro, Servio P. and Roisin, Yves and Schmidt, Jesper B. and S{\o}rensen, Line and Lewinsohn, Thomas M. and Leponce, Maurice},
title = {Arthropod Distribution in a Tropical Rainforest: Tackling a Four Dimensional Puzzle},
series = {PLoS ONE},
volume = {10},
journal = {PLoS ONE},
number = {12},
doi = {10.1371/journal.pone.0144110},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-136393},
pages = {e0144110},
year = {2015},
abstract = {Quantifying the spatio-temporal distribution of arthropods in tropical rainforests represents a first step towards scrutinizing the global distribution of biodiversity on Earth. To date most studies have focused on narrow taxonomic groups or lack a design that allows partitioning of the components of diversity. Here, we consider an exceptionally large dataset (113,952 individuals representing 5,858 species), obtained from the San Lorenzo forest in Panama, where the phylogenetic breadth of arthropod taxa was surveyed using 14 protocols targeting the soil, litter, understory, lower and upper canopy habitats, replicated across seasons in 2003 and 2004. This dataset is used to explore the relative influence of horizontal, vertical and seasonal drivers of arthropod distribution in this forest. We considered arthropod abundance, observed and estimated species richness, additive decomposition of species richness, multiplicative partitioning of species diversity, variation in species composition, species turnover and guild structure as components of diversity. At the scale of our study (2km of distance, 40m in height and 400 days), the effects related to the vertical and seasonal dimensions were most important. Most adult arthropods were collected from the soil/litter or the upper canopy and species richness was highest in the canopy. We compared the distribution of arthropods and trees within our study system. Effects related to the seasonal dimension were stronger for arthropods than for trees. We conclude that: (1) models of beta diversity developed for tropical trees are unlikely to be applicable to tropical arthropods; (2) it is imperative that estimates of global biodiversity derived from mass collecting of arthropods in tropical rainforests embrace the strong vertical and seasonal partitioning observed here; and (3) given the high species turnover observed between seasons, global climate change may have severe consequences for rainforest arthropods.},
language = {en}
}
@phdthesis{Basile2009,
author = {Basile, Rebecca},
title = {Thermoregulation and Resource Management in the Honeybee (Apis mellifera)},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-39793},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2009},
abstract = {Ein grundlegender Faktor, der f{\"u}r das {\"U}berleben einer Kolonie sozialer Insekten ausschlaggebend ist, liegt in der F{\"a}higkeit Nahrung durch sogenannte „Trophallaxis" auszutauschen. Diese F{\"u}tterungskontakte sorgen f{\"u}r die gleichm{\"a}ßige Verteilung der Nahrung innerhalb der Kolonie und werden als einer der Grundpfeiler der Sozialit{\"a}t der Staatenbildenden Insekten erachtet. Im Fall der Honigbienen finden diese Kontakte in vollkommener Dunkelheit statt. Damit es in dieser Situation {\"u}berhaupt zum Nahrungsaustausch kommen kann, sind die Antennen von großer Wichtigkeit. Ein erster Schritt in den Verhaltensweisen, die der Rezipient eines trophallaktischen Kontaktes zeigt, ist der Kontakt einer Antennenspitze mit den Mundwerkzeugen des Donoren, da sich dort die regurgitierte Nahrung befindet. Diese Ber{\"u}hrung hat aufgrund der gustatorischen Sensibilit{\"a}t der Antenne den Zweck, das angebotene Futter zu „erschmecken". Die rechte Antenne wird vom Rezipienten eines trophallaktischen Kontakts signifikant h{\"a}ufiger eingesetzt als die linke Antenne. Die Pr{\"a}ferenz f{\"u}r die rechte Antenne bleibt dabei auch erhalten, wenn ein Teil der Antennengeisel abgetrennt wurde, also die sensorischen F{\"a}higkeiten der rechten Antenne stark beeintr{\"a}chtigt wurden. Der Grund f{\"u}r die Pr{\"a}ferenz der rechten Antenne k{\"o}nnte ihrer erh{\"o}hten Sensibilit{\"a}t gegen{\"u}ber Zuckerwasser zugrunde liegen, da die rechte Antenne im Laborversuch signifikant st{\"a}rker auf Stimulationen mit Zuckerwasser verschiedener Konzentrationen reagierte als die linke. Trophallaktische Kontakte sichern Individuen innerhalb einer Kolonie den Zugang zur lebenswichtigen Nahrung. Im Beispiel der Honigbienen ist st{\"a}ndige Zugriff auf Nahrung besonders wichtig, da es sich um ein heterothermes Tier handelt, das die F{\"a}higkeit besitzt, aktiv seine K{\"o}rpertemperatur zu regulieren. Obgleich jedes Individuum in der Lage ist, seine K{\"o}rpertemperatur den eigenen Bed{\"u}rfnissen anzupassen, ist diese F{\"a}higkeit streng durch den in der Nahrung aufgenommenen Zucker reguliert. Im Gegensatz zu den S{\"a}ugetieren oder V{\"o}geln, die f{\"u}r eine Erh{\"o}hung des Blutzuckerspiegels auch auf Fett- oder Eiweißressourcen zur{\"u}ckgreifen k{\"o}nnen, ist die Honigbiene auf die Glucose aus der aufgenommenen Nahrung angewiesen. Die Ergebnisse dieser Untersuchung zeigen, dass der Zuckergehalt der aufgenommenen Nahrung positiv mit der Thoraxtemperatur der Bienen korreliert. Dieser Zusammenhang tritt auf, selbst wenn keine W{\"a}rmeerzeugung f{\"u}r die Brutpflege oder f{\"u}r das Erw{\"a}rmen der Wintertraube notwendig ist und die Tiere außerhalb des Stockes ohne eigentliche Notwendigkeit f{\"u}r die W{\"a}rmeerzeugung in einem K{\"a}fig gehalten werden. Die Ergebnisse der Untersuchung zeigen, dass die Rezipienten beim Nahrungsaustausch eine signifikant h{\"o}here Thoraxtemperatur haben als die Donoren. Außerdem zeigen die Rezipienten nach der F{\"u}tterung signifikant h{\"a}ufiger Brutw{\"a}rmeverhalten als die Donoren. Letztere haben eine signifikant niedrigere Thoraxtemperatur als die Rezipienten und zeigen eine Verhaltenstendenz, h{\"a}ufig zwischen Brutbereich und Honiglager hin- und her zu pendeln. Dabei nehmen sie im Honiglager Honig in ihren Kropf auf und f{\"u}ttern mit dieser Nahrung danach Bienen im Brutbereich. Außerdem zeigen die Ergebnisse, dass es einen w{\"a}rmegesteuerten Ausl{\"o}semechanismus gibt, der den Donoren und Rezipienten des trophallaktischen Kontakts dazu verhilft, trotz der Dunkelheit des Stocks praktisch verz{\"o}gerungsfreie Nahrungs{\"u}bertragung am Ort des h{\"o}chsten Energieverbrauchs zu gew{\"a}hrleisten. Das Hervorw{\"u}rgen von Nahrung angesichts einer W{\"a}rmequelle k{\"o}nnte seinen Ursprung in einer Beschwichtigungsgeste haben. Aggressive Tiere zeigen neben sichtbaren aggressiven Verhalten auch durch ihre erh{\"o}hte K{\"o}rpertemperatur, dass sie bereit sind sich auf einen Kampf einzulassen. Die Temperaturerh{\"o}hung eines aggressiven Tieres beruht dabei auf der erh{\"o}hten Muskelaktivit{\"a}t, die vor allem bei Insekten dazu n{\"o}tig ist, einen entsprechende Reaktion im Falle eines Kampfes oder der Flucht zeigen zu k{\"o}nnen. Wird ein Individuum mit Aggression konfrontiert, so bleibt ihm die Wahl sich auf einen Kampf einzulassen, zu fl{\"u}chten oder durch eine Beschwichtigungsgeste eine Deeskalation der Situation einzuleiten. Besonders h{\"a}ufig wird f{\"u}r diesen Zweck Nahrung regurgitiert und dem dominanteren Tier angeboten, um einem Konflikt aus dem Weg zu gehen. Die F{\"a}higkeit, Arbeiterinnen mit kleinen Portionen konzentrierter Nahrung zu versorgen tr{\"a}gt zu einer {\"o}konomischen Verteilung der Ressourcen bei, die mit den physiologischen Bed{\"u}rfnissen der Honigbienen konform geht und die {\"o}kologischen Erfordernisse des Stockes erf{\"u}llt. Das daraus resultierende Managementsystem, welches sparsam mit den Ressourcen haushaltet und auf die individuellen Bed{\"u}rfnisse jeder einzelnen Biene einzugehen vermag, k{\"o}nnte ein Grund f{\"u}r die F{\"a}higkeit der Honigbienen zur Entwicklung mehrj{\"a}hriger Kolonien sein, die, anders als Hummeln oder Wespen, auch den Winter in gem{\"a}ßigten Zonen als Gemeinschaft zu {\"u}berstehen verm{\"o}gen.},
subject = {Biene},
language = {en}
}
@phdthesis{Bartossek2018,
author = {Bartossek, Thomas},
title = {Structural and functional analysis of the trypanosomal variant surface glycoprotein using x-ray scattering techniques and fluorescence microscopy},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-144775},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2018},
abstract = {Trypanosoma brucei is an obligate parasite and causative agent of severe diseases affecting humans and livestock. The protist lives extracellularly in the bloodstream of the mammalian host, where it is prone to attacks by the host immune system. As a sophisticated means of defence against the immune response, the parasite's surface is coated in a dense layer of the variant surface glycoprotein (VSG), that reduces identification of invariant epitopes on the cell surface by the immune system to levels that prevent host immunity. The VSG has to form a coat that is both dense and mobile, to shield invariant surface proteins from detection and to allow quick recycling of the protective coat during immune evasion. This coat effectively protects the parasite from the harsh environment that is the mammalian bloodstream and leads to a persistent parasitemia if the infection remains untreated. The available treatment against African Trypanosomiasis involves the use of drugs that are themselves severely toxic and that can lead to the death of the patient. Most of the drugs used as treatment were developed in the early-to-mid 20th century, and while developments continue, they still represent the best medical means to fight the parasite. The discovery of a fluorescent VSG gave rise to speculations about a potential interaction between the VSG coat and components of the surrounding medium, that could also lead to a new approach in the treatment of African Trypanosomiasis that involves the VSG coat. The initially observed fluorescence signal was specific for a combination of a VSG called VSG'Y' and the triphenylmethane (TPM) dye phenol red. Exchanging this TPM to a bromo-derivative led to the observation of another fluorescence effect termed trypanicidal effect which killed the parasite independent of the expressed VSG and suggests a structurally conserved feature between VSGs that could function as a specific drug target against T. b. brucei. The work of this thesis aims to identify the mechanisms that govern the unique VSG'Y' fluorescence and the trypanocidal effect. Fluorescence experiments and protein mutagenesis of VSG'Y' as well as crystallographic trials with a range of different VSGs were utilized in the endeavour to identify the binding mechanisms between TPM compounds and VSGs, to find potentially conserved structural features between VSGs and to identify the working mechanisms of VSG fluorescence and the trypanocidal effect. These trials have the potential to lead to the formulation of highly specific drugs that target the parasites VSG coat. During the crystallographic trials of this thesis, the complete structure of a VSG was solved experimentally for the first time. This complete structure is a key component in furthering the understanding of the mechanisms governing VSG coat formation. X-ray scattering techniques, involving x-ray crystallography and small angle x-ray scattering were applied to elucidate the first complete VSG structures, which reveal high flexibility of the protein and supplies insight into the importance of this flexibility in the formation of a densely packed but highly mobile surface coat.},
subject = {Trypanosoma brucei brucei},
language = {en}
}
@article{BartomeusPottsSteffanDewenteretal.2014,
author = {Bartomeus, Ignasi and Potts, Simon G. and Steffan-Dewenter, Ingolf and Vaissiere, Bernard E. and Woyciechowski, Michal and Krewenka, Kristin M. and Tscheulin, Thomas and Roberts, Stuart P. M. and Szentgyoergyi, Hajnalka and Westphal, Catrin and Bommarco, Riccardo},
title = {Contribution of insect pollinators to crop yield and quality varies with agricultural intensification},
series = {PEERJ},
volume = {2},
journal = {PEERJ},
number = {e328},
issn = {2167-9843},
doi = {10.7717/peerj.328},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-116928},
year = {2014},
abstract = {Background. Up to 75\% of crop species benefit at least to some degree from animal pollination for fruit or seed set and yield. However, basic information on the level of pollinator dependence and pollinator contribution to yield is lacking for many crops. Even less is known about how insect pollination affects crop quality. Given that habitat loss and agricultural intensification are known to decrease pollinator richness and abundance, there is a need to assess the consequences for different components of crop production. Methods. We used pollination exclusion on flowers or inflorescences on a whole plant basis to assess the contribution of insect pollination to crop yield and quality in four flowering crops (spring oilseed rape, field bean, strawberry, and buckwheat) located in four regions of Europe. For each crop, we recorded abundance and species richness of flower visiting insects in ten fields located along a gradient from simple to heterogeneous landscapes. Results. Insect pollination enhanced average crop yield between 18 and 71\% depending on the crop. Yield quality was also enhanced in most crops. For instance, oilseed rape had higher oil and lower chlorophyll contents when adequately pollinated, the proportion of empty seeds decreased in buckwheat, and strawberries' commercial grade improved; however, we did not find higher nitrogen content in open pollinated field beans. Complex landscapes had a higher overall species richness of wild pollinators across crops, but visitation rates were only higher in complex landscapes for some crops. On the contrary, the overall yield was consistently enhanced by higher visitation rates, but not by higher pollinator richness. Discussion. For the four crops in this study, there is clear benefit delivered by pollinators on yield quantity and/or quality, but it is not maximized under current agricultural intensification. Honeybees, the most abundant pollinator, might partially compensate the loss of wild pollinators in some areas, but our results suggest the need of landscape-scale actions to enhance wild pollinator populations.},
language = {en}
}
@article{BartmannJanakiRamanFloeteretal.2018,
author = {Bartmann, Catharina and Janaki Raman, Sudha R. and Fl{\"o}ter, Jessica and Schulze, Almut and Bahlke, Katrin and Willingstorfer, Jana and Strunz, Maria and W{\"o}ckel, Achim and Klement, Rainer J. and Kapp, Michaela and Djuzenova, Cholpon S. and Otto, Christoph and K{\"a}mmerer, Ulrike},
title = {Beta-hydroxybutyrate (3-OHB) can influence the energetic phenotype of breast cancer cells, but does not impact their proliferation and the response to chemotherapy or radiation},
series = {Cancer \& Metabolism},
volume = {6},
journal = {Cancer \& Metabolism},
number = {8},
doi = {10.1186/s40170-018-0180-9},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-175607},
year = {2018},
abstract = {Background: Ketogenic diets (KDs) or short-term fasting are popular trends amongst supportive approaches for cancer patients. Beta-hydroxybutyrate (3-OHB) is the main physiological ketone body, whose concentration can reach plasma levels of 2-6 mM during KDs or fasting. The impact of 3-OHB on the biology of tumor cells described so far is contradictory. Therefore, we investigated the effect of a physiological concentration of 3 mM 3-OHB on metabolism, proliferation, and viability of breast cancer (BC) cells in vitro. Methods: Seven different human BC cell lines (BT20, BT474, HBL100, MCF-7, MDA-MB 231, MDA-MB 468, and T47D) were cultured in medium with 5 mM glucose in the presence of 3 mM 3-OHB at mild hypoxia (5\% oxygen) or normoxia (21\% oxygen). Metabolic profiling was performed by quantification of the turnover of glucose, lactate, and 3-OHB and by Seahorse metabolic flux analysis. Expression of key enzymes of ketolysis as well as the main monocarboxylic acid transporter MCT2 and the glucose-transporter GLUT1 was analyzed by RT-qPCR and Western blotting. The effect of 3-OHB on short- and long-term cell proliferation as well as chemo- and radiosensitivity were also analyzed. Results: 3-OHB significantly changed the oxygen consumption rate (OCR) and extracellular acidification rate (ECAR) in BT20 cells resulting in a more oxidative energetic phenotype. MCF-7 and MDA-MB 468 cells had increased ECAR only in response to 3-OHB, while the other three cell types remained uninfluenced. All cells expressed MCT2 and GLUT1, thus being able to uptake the metabolites. The consumption of 3-OHB was not strongly linked to mRNA overexpression of key enzymes of ketolysis and did not correlate with lactate production and glucose consumption. Neither 3-OHB nor acetoacetate did interfere with proliferation. Further, 3-OHB incubation did not modify the response of the tested BC cell lines to chemotherapy or radiation. Conclusions: We found that a physiological level of 3-OHB can change the energetic profile of some BC cell lines. However, 3-OHB failed to influence different biologic processes in these cells, e.g., cell proliferation and the response to common breast cancer chemotherapy and radiotherapy. Thus, we have no evidence that 3-OHB generally influences the biology of breast cancer cells in vitro.},
language = {en}
}
@phdthesis{Bartl2012,
author = {Bartl, Jasmin},
title = {Impairment of insulin signaling pathway in Alzheimer's disease},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-74197},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2012},
abstract = {The neurodegenerative disorder Alzheimer's disease (AD) is the cause of approximately 60\% of the world's 35 million patients suffering from dementia. Current research focuses here are on association with other diseases such as diabetes type 2 (T2DM), possible genetic markers, specific signal transduction pathways within the brain and potential protein modification, because the pathogenesis and etiology of AD are still not fully understood. Specifically association of T2DM with AD came to the focus with the so-called "Rotterdam study" in 1999, indicating that T2DM doubles the risk of developing AD. In the meantime, it is known that the prevalence rate in patients with T2DM is 30\%. Drugs commonly used in the treatment of T2DM such as peroxisome proliferator-activated receptors gamma (PPARγ) agonists show improvement of the cognitive abilities in patients with early stage of dementia, with potential therapeutically relevance. Therefore it is important not only to investigate a link between these diseases, but also to investigate the insulin signaling pathway in the brain of AD patients. In order to investigate this complex issue in more details and demonstrate additional links between T2DM and AD, the present study used several basic biological methods to clarify the question: "Is impaired insulin signaling pathway within the brain crucial for the development of AD?" from several points of view. The methods used in this work have been i) an analysis of single nucleotide (SNP) polymorphism of the insulin-degrading enzyme gene (IDE) in relation to risk of AD and / or of T2DM, ii) post-mortem histochemical studies of brain tissue of patients with only AD, with AD combined with T2DM and with only T2DM compared with an age-matched control group, and iii.) investigations of neurochemical pathways and gene/protein expression changes of a human cell culture as a consequences of amyloid β (Aβ) treatment. After analysis of the IDE SNP polymorphism in the selected VITA (Vienna Trans Danube Aging) cohort disease-specific effects were discovered. The upstream polymorphism (IDE2) was found to influence AD risk in a protective manner, while the downstream polymorphism (IDE7) modified the T2DM risk. Based on the SNP results, the presented study delineate the model that IDE promoter and 3‟ untranslated region/downstream variation can have different effects on IDE expression, maybe a relevant endophenotype with disorder-specific effects on AD and T2DM susceptibility. Furthermore, the human post-mortem studies could show that both AD as well as T2DM patients had a significantly lower density of the insulin receptor (IR) in the hippocampus, whereas a significantly increased density of inactive phosphorylated PPARγ has been found and this persisted even in patients with both diseases. Summarizing the histological study, it was possible to reveal common histological features of AD and T2DM, but no direct connection between the two diseases. Although AD is nowadays not only characterized by amyloid-containing plaque deposits and by the hyperphosphorylation of tau protein, the excessive Aβ42 presence in the brains of AD patients is still playing a key role. Up to date it is still not entirely clear which physical form of Aβ42 is responsible for the development of AD. The present work investigated, what impact has the state of aggregation of Aβ42 on genes and proteins of the insulin signaling pathway and the amyloid cascade. It could be shown that the oligomeric variant enhanced specifically the gene and protein expression of glycogen synthase kinase (GSK) 3β and also the enzyme activity was significantly increased, but has in turn strongly inhibited the IR gene and protein expression. Additionally, the effect of Aβ42 on monoamine oxidase B (MAO-B) was examined. An effect of both aggregated forms of Aβ42 had on enzyme activity was discovered. However, the fibrillar variants led to significantly increased activity of MAO-B while the oligomeric variants inhibited the enzyme activity. Several previous studies have demonstrated the involvement of increased MAO-B activity in AD, but the present work provides for the first time a direct link between the states of aggregation of Aβ42 to enzyme activity. Finally the results of the presented thesis can be summarized to following conclusion: Although AD and T2DM sharing some degrees of common features, still there is a lack of direct association, and therefore the diseases must be considered more independent rather than linked. But the impaired cerebral insulin signaling pathway seems to be another manifested hallmark of AD.},
subject = {Alzheimer-Krankheit},
language = {en}
}
@phdthesis{Barth2008,
author = {Barth, Enrico},
title = {Study of the properties of channel-forming proteins of the cell walls of different Corynebacteriae},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-36325},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2008},
abstract = {Die Gattung Corynebacterium geh{\"o}rt, neben Mycobacterium, Nocardia, Rhodococcus und weiteren nahverwandten Gattungen, dem unverwechselbaren, gattungs{\"u}bergreifenden Taxon Mycolata an. Viele Spezies aus dieser heterogenen Gruppe Mycols{\"a}ure-haltiger Actinomyceten sind entweder aufgrund ihrer medizinischen oder ihrer biotechnologischen Bedeutung bekannt. Beispielsweise z{\"a}hlen Mycobacterium tuberculosis, Mycobacterium leprae, Corynebacterium diphtheriae und Nocardia farcinica, welche weltweit Verursacher besonders gef{\"a}hrlicher bakterieller Infektionskrankheiten sind, zu dieser ungew{\"o}hnlichen Gruppe Gram-positiver Bakterien. Ebenso bedeutsam sind einige apathogene Mycolata-Arten, die industrielle Anwendung finden. Corynebacterium glutamicum und Corynebacterium efficiens sind leistungsf{\"a}hige Bakterien, die zum Beispiel in der Produktion des Geschmacksverst{\"a}rkers Glutamat und des Tierfuttermittelzusatzes Lysin eingesetzt werden, w{\"a}hrend verschiedene Rhodococcus Spezies Anwendung bei der Herstellung von Acryls{\"a}uren finden. Die Zellwand der Mycolata zeigt, verglichen mit der klassischer Gram-positiver Bakterien, eine außergew{\"o}hnliche Zusammensetzung und Struktur auf. Abgesehen von einem Arabinogalactan-Peptidoglycan-Komplex enth{\"a}lt die Zellwand der meisten Actinomyceten einen hohen Anteil an Mycols{\"a}uren. Diese langkettigen, verzweigten Fetts{\"a}uren formen eine, mit der {\"a}ußeren Membran Gram-negativer Bakterien vergleichbare, stark undurchl{\"a}ssige, hydrophobe {\"a}ußere H{\"u}lle, welche die Grundlage der außergew{\"o}hnlichen Medikamentenresistenz bei den Mycolata bildet. Wie die {\"a}ußere Membran Gram-negativer Bakterien enth{\"a}lt die Zellwand der Mycolata porenformende Proteine, die den Durchlass hydrophiler Substanzen gestatten. Indem sie eine Verbindung zwischen dem Zellinneren und der Umwelt, in der das Bakterium lebt, schaffen und einen kontrollierten Austausch zwischen beiden erm{\"o}glichen, tragen die Kanalproteine entscheidend zur Funktion der bakteriellen Zellh{\"u}lle bei. Das Ziel dieser Arbeit war das Wissen {\"u}ber Zellwandkan{\"a}le in Corynebakterien zu erweitern. Deshalb untersuchten wir PorA und PorH Proteine, die basierend auf fr{\"u}heren Studien Zellwandkan{\"a}len in C. glutamicum, C. efficiens und Corynebacterium callunae zugeordnet werden, um ungekl{\"a}rten Fragen nachzugehen und um Wissen {\"u}ber deren Struktur zu erlangen. Ferner inspizierten wir Zellw{\"a}nde pathogener Corynebakterien, genauer gesagt von Corynebacterium diphtheriae und Corynebacterium jeikeium, um herauszufinden, ob diese Spezies wie ihre harmlosen Verwandten Kanalproteine besitzen. In dieser Arbeit wiesen wir mit C. diphtheriae und C. jeikeium in zwei weiteren Corynebacterium-Arten offene, mit Wasser gef{\"u}llte Zellwandkan{\"a}le nach. Des Weiteren stellten wir fest, dass sich die Zellwandkan{\"a}le von C. glutamicum, C. efficiens und C. diphtheriae aus zwei Proteinen zusammensetzen, einem zugeh{\"o}rig zu der Gruppe der PorH Proteine und einem weiteren aus der Gruppe der PorA Proteine. Diese heteromere Struktur von Zellwandkan{\"a}len bei Corynebakterien stellt ein Novum f{\"u}r Zellwandkan{\"a}le bei den Mycolata dar. Indessen besteht der Zellwandkanal von C. jeikeium aus nur einem Protein, CjPorA, angeordnet zu einem Oligomer. Obgleich das Molekulargewicht dieses Proteins (4 kDa) mit dem von PorH und PorA Proteinen vergleichbar ist (5-7 kDa), weißt seine Prim{\"a}rsequenz keine eindeutige Homologie zu diesen auf. Dennoch deutet vieles auf eine Verwandtschaft zwischen CjPorA und PorH/PorA Proteinen hin, da das Gen jk0268, welches f{\"u}r CjPorA kodiert, sich in einer Region des C. jeikeium Chromosoms befindet, die der Genomregion entspricht in welcher die porH/porA Gene der anderen Corynebakterien lokalisiert sind. Dies l{\"a}sst vermuten, dass jk0268 (welches f{\"u}r den homomeren Zellwandkanal in C. jeikeium kodiert) und die porH/porA Gene von C. glutamicum, C. efficiens und C. diphtheriae (die einen heteromeren Zellwandkanal kodieren) wahrscheinlich Nachkommen eines gemeinsamen Vorl{\"a}ufergens sind. Phylogenetische Analysen der Gattung Corynebacterium unterst{\"u}tzen diese Annahme. Desweitern legen sie nahe, dass die hier untersuchten Zellwandkan{\"a}le innerhalb dieser Gattung wahrscheinlich weit verbreitet sind. Ein umfassendes Wissen {\"u}ber Zellwandkan{\"a}le, denen beim Transport gel{\"o}ster Stoffe {\"u}ber die {\"a}ußere Membran in Corynebakterien und anderen Mitgliedern der Mycolata eine entscheidende Rolle zukommt, k{\"o}nnte von großem wirtschaftlichem und medizinischem Nutzen sein.},
subject = {Zellwand},
language = {en}
}
@article{BartelPeinPopperetal.2019,
author = {Bartel, Karin and Pein, Helmut and Popper, Bastian and Schmitt, Sabine and Janaki-Raman, Sudha and Schulze, Almut and Lengauer, Florian and Koeberle, Andreas and Werz, Oliver and Zischka, Hans and M{\"u}ller, Rolf and Vollmar, Angelika M. and Schwarzenberg, Karin von},
title = {Connecting lysosomes and mitochondria - a novel role for lipid metabolism in cancer cell death},
series = {Cell Communication and Signaling},
volume = {17},
journal = {Cell Communication and Signaling},
doi = {10.1186/s12964-019-0399-2},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-221524},
year = {2019},
abstract = {Background The understanding of lysosomes has been expanded in recent research way beyond their view as cellular trash can. Lysosomes are pivotal in regulating metabolism, endocytosis and autophagy and are implicated in cancer. Recently it was discovered that the lysosomal V-ATPase, which is known to induce apoptosis, interferes with lipid metabolism in cancer, yet the interplay between these organelles is poorly understood. Methods LC-MS/MS analysis was performed to investigate lipid distribution in cells. Cell survival and signaling pathways were analyzed by means of cell biological methods (qPCR, Western Blot, flow cytometry, CellTiter-Blue). Mitochondrial structure was analyzed by confocal imaging and electron microscopy, their function was determined by flow cytometry and seahorse measurements. Results Our data reveal that interfering with lysosomal function changes composition and subcellular localization of triacylglycerids accompanied by an upregulation of PGC1α and PPARα expression, master regulators of energy and lipid metabolism. Furthermore, cardiolipin content is reduced driving mitochondria into fission, accompanied by a loss of membrane potential and reduction in oxidative capacity, which leads to a deregulation in cellular ROS and induction of mitochondria-driven apoptosis. Additionally, cells undergo a metabolic shift to glutamine dependency, correlated with the fission phenotype and sensitivity to lysosomal inhibition, most prominent in Ras mutated cells. Conclusion This study sheds mechanistic light on a largely uninvestigated triangle between lysosomes, lipid metabolism and mitochondrial function. Insight into this organelle crosstalk increases our understanding of mitochondria-driven cell death. Our findings furthermore provide a first hint on a connection of Ras pathway mutations and sensitivity towards lysosomal inhibitors.},
language = {en}
}
@article{BarnekowJahnSchartl1990,
author = {Barnekow, Angelika and Jahn, Reinhard and Schartl, Manfred},
title = {Synaptophysin: a substrate for the protein tyrosine kinase pp60c-src in intact synaptic vesicles},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-86168},
year = {1990},
abstract = {Expression of pp60 c-src, the first well defined proto-oncogene product, is developmentally regulated and tissue-specific, with neuronal tissues displaying high amounts of the c-src encoded pp60 c-src kinase activity. In the central nervous system pp60 s-src is preferentially expressed in regions characterized by a high content of grey matter and elevated density of nerve terminals. In this study we show for the first time a direct interaction between pp60 c-src and synaptophysin as a physiological target protein in neurons by demonstrating that endogenous pp60 c-src is able to phosphorylate synaptophysin (p38). p38 is a major constituent of the synaptic vesicle membrane protein and is thought to play a key role in the exocytosis of small synaptic vesicles and possibly small clear vesicles in neuroendocrine cells.},
subject = {Synaptophysin},
language = {en}
}
@article{BarnekowGessler1986,
author = {Barnekow, Angelika and Gessler, Manfred},
title = {Activation of the pp60\(^{c-src}\) kinase during differentiation of monomyelocytic cells in vitro},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-59278},
year = {1986},
abstract = {Tbe proto-oncogene c-src, the cellular homolog of the Rous sarcoma virus (RSV) transforming gene v-src, is expressed in a tissue-specific and age-dependent manner. Its physiological function, although still unknown, appears to be more closely related to differentiation processes than to proliferation processes. To obtain more information about the physiological role of the c-src gene in cells, we have studied differentiation-dependent alterations using the human HL-60 leukaemia cell line as a model system. Induction of monocytic and granulocytic differentiation of HL-60 cells by 12-0-tetradecanoylphorbol-13-acetate (TPA) and dimethylsulfoxide (DMSO) is associated with an activation of the pp60c-src tyrosine kinase, but not with increased c-src gene expression. Control experiments exclude an interaction of TPA and DMSO themselves with the pp60c-src kinase.},
subject = {Biochemie},
language = {en}
}
@article{BarnekowSchartlAndersetal.1982,
author = {Barnekow, A. and Schartl, Manfred and Anders, F. and Bauer, H.},
title = {Identification of a fish protein associated with a kinase activity and related to the Rous sarcoma virus transforming protein},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-61946},
year = {1982},
abstract = {No abstract available},
subject = {Physiologische Chemie},
language = {en}
}
@article{BarnekowSchartl1987,
author = {Barnekow, A. and Schartl, Manfred},
title = {Comparative studies on the src proto-oncogene and its gene product pp60\(^{c-src}\) in normal and neoplastic tissues of lower vertebrates},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-61869},
year = {1987},
abstract = {No abstract available},
subject = {Physiologische Chemie},
language = {en}
}
@article{BarnekowPaulSchartl1987,
author = {Barnekow, A. and Paul, E. and Schartl, Manfred},
title = {Expression of the c-src protooncogene in human skin tumors},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-61870},
year = {1987},
abstract = {No abstract available},
subject = {Physiologische Chemie},
language = {en}
}
@phdthesis{Bargul2018,
author = {Bargul, Joel Ltilitan},
title = {Characterization of motility and erythrocyte adherence as virulence factors in African trypanosomes},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-115053},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2018},
abstract = {Pathogens causing African animal trypanosomiasis (AAT), the major livestock disease in sub-Saharan Africa, belong to the salivarian group of the African trypanosomes, which are transmitted by the bite of the tsetse fly (Glossina spec.). T. vivax, T. congolense and T. brucei brucei are major pathogens of cattle in particular, causing nagana, with dramatic socio-economic consequences for the affected regions. The parasites additionally have a huge reservoir of other livestock and wild animal hosts. T. brucei, the species which also includes the subspecies pathogenic to humans causing sleeping sickness, has been extensively studied as the cultivatable model trypanosome. But less is known about the other salivarian species, which are not routinely held in culture, if at all possible. A hallmark of trypanosomal lifestyle is the protozoan flagellates incessant motility, which enables them to populate an enormous range of habitats in very diverse hosts. We were now able to characterize, for the first time with high spatiotemporal resolution microscopy, the swimming behaviour and mechanism of the most relevant salivarian species isolated directly from blood. We show the influence of viscosity on the motility of bloodstream form (BSF) cells and simulate their movement between erythrocytes, giving a clear picture of how all analyzed species move under varying environmental conditions. We show that although the basic mechanism of flagellar motility applies to all analyzed species, there are clear morphological differences that produce different reactions to the physical environment. We could define specific conditions for highly increased swimming persistence and speed for compared to the behaviour in standard culture. These results have important implications for the parasites survival strategies in the host, e.g. regarding the capacity for antibody clearance. Although we show all species to effectively remove antibodies from the cell surface, T. congolense differed markedly in its motility behaviour, which gives rise to interesting questions about this species behaviour in the bloodstream. Most of the T. congolense parasites (and to a lesser extent T. vivax) adhere to sheep erythrocytes. Further in vitro studies showed that T. congolense and T. vivax adhered to rabbit, goat, pig and cattle erythrocytes- but binding behaviour was absent in murine blood. Notably, both T. brucei and T. evansi lacked adherence to all studied host erythrocytes. Generally, attachment to blood cells caused reduction of swimming velocities. Judging from its cell architecture, as well as the motility studies in higher media viscosity and in micropillar arrays, T. congolense is not adapted to swim at high speeds in the mammalian bloodstream. Low swimming speeds could allow these purely intravascular parasites to remain bound to the host erythrocytes.},
subject = {Motili{\"a}t},
language = {en}
}
@article{BargulJungMcOdimbaetal.2016,
author = {Bargul, Joel L. and Jung, Jamin and McOdimba, Francis A. and Omogo, Collins O. and Adung'a, Vincent O. and Kr{\"u}ger, Timothy and Masiga, Daniel K. and Engstler, Markus},
title = {Species-Specific Adaptations of Trypanosome Morphology and Motility to the Mammalian Host},
series = {PLoS Pathogens},
volume = {12},
journal = {PLoS Pathogens},
number = {2},
doi = {10.1371/journal.ppat.1005448},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-146513},
pages = {e1005448},
year = {2016},
abstract = {African trypanosomes thrive in the bloodstream and tissue spaces of a wide range of mammalian hosts. Infections of cattle cause an enormous socio-economic burden in sub-Saharan Africa. A hallmark of the trypanosome lifestyle is the flagellate's incessant motion. This work details the cell motility behavior of the four livestock-parasites Trypanosoma vivax, T. brucei, T. evansi and T. congolense. The trypanosomes feature distinct swimming patterns, speeds and flagellar wave frequencies, although the basic mechanism of flagellar propulsion is conserved, as is shown by extended single flagellar beat analyses. Three-dimensional analyses of the trypanosomes expose a high degree of dynamic pleomorphism, typified by the 'cellular waveform'. This is a product of the flagellar oscillation, the chirality of the flagellum attachment and the stiffness of the trypanosome cell body. The waveforms are characteristic for each trypanosome species and are influenced by changes of the microenvironment, such as differences in viscosity and the presence of confining obstacles. The distinct cellular waveforms may be reflective of the actual anatomical niches the parasites populate within their mammalian host. T. vivax displays waveforms optimally aligned to the topology of the bloodstream, while the two subspecies T. brucei and T. evansi feature distinct cellular waveforms, both additionally adapted to motion in more confined environments such as tissue spaces. T. congolense reveals a small and stiff waveform, which makes these parasites weak swimmers and destined for cell adherence in low flow areas of the circulation. Thus, our experiments show that the differential dissemination and annidation of trypanosomes in their mammalian hosts may depend on the distinct swimming capabilities of the parasites.},
language = {en}
}
@phdthesis{Banaszek2013,
author = {Banaszek, Agnes},
title = {Dual Antigen-Restricted Complementation of a Two-Part Trispecific Antibody for Targeted Immunotherapy of Blood Cancer},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-90174},
school = {Universit{\"a}t W{\"u}rzburg},
year = {2013},
abstract = {Cancer cells frequently escape from immune surveillance by down-regulating two important components of the immune defence: antigen-presenting MHC and costimulatory molecules. Therefore several novel anti-tumour compounds that aim to assist the immune system in recognising and fighting cancer are currently under development. Recombinant bispecific antibodies represent one group of such novel therapeutics. They target two different antigens and recruit cytotoxic effector cells to tumour cells. For cancer immunotherapy, bispecific T cell-engaging antibodies are already well characterised. These antibodies target a tumour-associated antigen and CD3ε, the constant molecule of the T cell receptor complex. On the one hand, this study presents the development of a bispecific antibody targeting CD3ε and the rhabdomyosarcoma-associated fetal acetylcholine receptor. On the other hand, it describes a novel two-part trispecific antibody format for the treatment of leukaemia and other haematological malignancies in the context of haematopoietic stem cell transplantation (HSCT). For HSCT, an HLA-identical donor is preferred, but very rarely available. In an HLA-mismatched setting, the HLA disparity could be exploited for targeted cancer treatment. In the present study, a two-part trispecific HLA-A2 × CD45 × CD3 antibody was developed for potential cases in which the patient is HLA-A2-positive, but the donor is not. This holds true for about half the cases in Germany, since HLA-A2 is the most common HLA molecule found here. Combinatorial targeting of HLA-A2 and the leucocyte-common antigen CD45 allows for highly specific dual-antigen restricted tumour targeting. More precisely, two single-chain antibody constructs were developed: i) a single-chain variable fragment (scFv) specific for HLA-A2, and ii) a scFv against CD45, both linked to the VL and the VH domain of a CD3ε-specific antibody, respectively. It turned out that, after the concomitant binding of these constructs to the same HLA-A2- and CD45-expressing cell, the unpaired variable domains of a CD3ε-specific antibody assembled to a functional scFv. In a therapeutic situation, this assembly should exclusively occur on the recipient's blood cancer cells, leading to T cell-mediated cancer cell destruction. In this way, a relapse of disease might be prevented, and standard therapy (radiation and chemotherapy) might be omitted. For both approaches, the antibody constructs were periplasmically expressed in E. coli, purified via His tag, and biochemically characterised. Their binding to the respective targets was proven by flow cytometry. The stimulatory properties of the antibodies were assayed by measuring IL-2 release after incubation with T cells and antigen-expressing target cells. Both the bispecific antibody against rhabdomyosarcoma and the assembled trispecific antibody against blood cancer mediated T-cell activation in a concentration-dependent manner at nanomolar concentrations. For the trispecific antibody, this effect indeed proved to be dual antigen-restricted, as it could be blocked by prior incubation of either HLA-A2- or CD45-specific scFv and did not occur on single-positive (CD45+) or double-negative (HLA-A2- CD45-) target cells. Furthermore, antibodies from both approaches recruited T cells for tumour cell destruction in vitro.},
subject = {Immuntherapie},
language = {en}
}
@article{BaluapuriHofstetterDudvarskiStankovicetal.2019,
author = {Baluapuri, Apoorva and Hofstetter, Julia and Dudvarski Stankovic, Nevenka and Endres, Theresa and Bhandare, Pranjali and Vos, Seychelle Monique and Adhikari, Bikash and Schwarz, Jessica Denise and Narain, Ashwin and Vogt, Markus and Wang, Shuang-Yan and D{\"u}ster, Robert and Jung, Lisa Anna and Vanselow, Jens Thorsten and Wiegering, Armin and Geyer, Matthias and Maric, Hans Michael and Gallant, Peter and Walz, Susanne and Schlosser, Andreas and Cramer, Patrick and Eilers, Martin and Wolf, Elmar},
title = {MYC Recruits SPT5 to RNA Polymerase II to Promote Processive Transcription Elongation},
series = {Molecular Cell},
volume = {74},
journal = {Molecular Cell},
doi = {10.1016/j.molcel.2019.02.031},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-221438},
pages = {674-687},
year = {2019},
abstract = {The MYC oncoprotein binds to promoter-proximal regions of virtually all transcribed genes and enhances RNA polymerase II (Pol II) function, but its precise mode of action is poorly understood. Using mass spectrometry of both MYC and Pol II complexes, we show here that MYC controls the assembly of Pol II with a small set of transcription elongation factors that includes SPT5, a subunit of the elongation factor DSIF. MYC directly binds SPT5, recruits SPT5 to promoters, and enables the CDK7-dependent transfer of SPT5 onto Pol II. Consistent with known functions of SPT5, MYC is required for fast and processive transcription elongation. Intriguingly, the high levels of MYC that are expressed in tumors sequester SPT5 into non-functional complexes, thereby decreasing the expression of growth-suppressive genes. Altogether, these results argue that MYC controls the productive assembly of processive Pol II elongation complexes and provide insight into how oncogenic levels of MYC permit uncontrolled cellular growth.},
language = {en}
}
@article{BalkenholKaltdorfMammadovaBachetal.2020,
author = {Balkenhol, Johannes and Kaltdorf, Kristin V. and Mammadova-Bach, Elmina and Braun, Attila and Nieswandt, Bernhard and Dittrich, Marcus and Dandekar, Thomas},
title = {Comparison of the central human and mouse platelet signaling cascade by systems biological analysis},
series = {BMC Genomics},
volume = {21},
journal = {BMC Genomics},
doi = {10.1186/s12864-020-07215-4},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-230377},
year = {2020},
abstract = {Background Understanding the molecular mechanisms of platelet activation and aggregation is of high interest for basic and clinical hemostasis and thrombosis research. The central platelet protein interaction network is involved in major responses to exogenous factors. This is defined by systemsbiological pathway analysis as the central regulating signaling cascade of platelets (CC). Results The CC is systematically compared here between mouse and human and major differences were found. Genetic differences were analysed comparing orthologous human and mouse genes. We next analyzed different expression levels of mRNAs. Considering 4 mouse and 7 human high-quality proteome data sets, we identified then those major mRNA expression differences (81\%) which were supported by proteome data. CC is conserved regarding genetic completeness, but we observed major differences in mRNA and protein levels between both species. Looking at central interactors, human PLCB2, MMP9, BDNF, ITPR3 and SLC25A6 (always Entrez notation) show absence in all murine datasets. CC interactors GNG12, PRKCE and ADCY9 occur only in mice. Looking at the common proteins, TLN1, CALM3, PRKCB, APP, SOD2 and TIMP1 are higher abundant in human, whereas RASGRP2, ITGB2, MYL9, EIF4EBP1, ADAM17, ARRB2, CD9 and ZYX are higher abundant in mouse. Pivotal kinase SRC shows different regulation on mRNA and protein level as well as ADP receptor P2RY12. Conclusions Our results highlight species-specific differences in platelet signaling and points of specific fine-tuning in human platelets as well as murine-specific signaling differences.},
language = {en}
}
@article{BalakrishnanHemmenChoudhuryetal.2022,
author = {Balakrishnan, Ashwin and Hemmen, Katherina and Choudhury, Susobhan and Krohn, Jan-Hagen and Jansen, Kerstin and Friedrich, Mike and Beliu, Gerti and Sauer, Markus and Lohse, Martin J. and Heinze, Katrin G.},
title = {Unraveling the hidden temporal range of fast β2-adrenergic receptor mobility by time-resolved fluorescence},
series = {Communications Biology},
volume = {5},
journal = {Communications Biology},
number = {1},
doi = {10.1038/s42003-022-03106-4},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-301140},
year = {2022},
abstract = {G-protein-coupled receptors (GPCRs) are hypothesized to possess molecular mobility over a wide temporal range. Until now the temporal range has not been fully accessible due to the crucially limited temporal range of available methods. This in turn, may lead relevant dynamic constants to remain masked. Here, we expand this dynamic range by combining fluorescent techniques using a spot confocal setup. We decipher mobility constants of β\(_{2}\)-adrenergic receptor over a wide time range (nanosecond to second). Particularly, a translational mobility (10 µm\(^{2}\)/s), one order of magnitude faster than membrane associated lateral mobility that explains membrane protein turnover and suggests a wider picture of the GPCR availability on the plasma membrane. And a so far elusive rotational mobility (1-200 µs) which depicts a previously overlooked dynamic component that, despite all complexity, behaves largely as predicted by the Saffman-Delbr{\"u}ck model.},
language = {en}
}
@article{BakariSoaleIkengaScheibeetal.2021,
author = {Bakari-Soale, Majeed and Ikenga, Nonso Josephat and Scheibe, Marion and Butter, Falk and Jones, Nicola G. and Kramer, Susanne and Engstler, Markus},
title = {The nucleolar DExD/H protein Hel66 is involved in ribosome biogenesis in Trypanosoma brucei},
series = {Scientific Reports},
volume = {11},
journal = {Scientific Reports},
number = {1},
doi = {10.1038/s41598-021-97020-0},
url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-263872},
year = {2021},
abstract = {The biosynthesis of ribosomes is a complex cellular process involving ribosomal RNA, ribosomal proteins and several further trans-acting factors. DExD/H box proteins constitute the largest family of trans-acting protein factors involved in this process. Several members of this protein family have been directly implicated in ribosome biogenesis in yeast. In trypanosomes, ribosome biogenesis differs in several features from the process described in yeast. Here, we have identified the DExD/H box helicase Hel66 as being involved in ribosome biogenesis. The protein is unique to Kinetoplastida, localises to the nucleolus and its depletion via RNAi caused a severe growth defect. Loss of the protein resulted in a decrease of global translation and accumulation of rRNA processing intermediates for both the small and large ribosomal subunits. Only a few factors involved in trypanosome rRNA biogenesis have been described so far and our findings contribute to gaining a more comprehensive picture of this essential process.},
language = {en}
}