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Institute
- Julius-von-Sachs-Institut für Biowissenschaften (362) (remove)
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Bone morphogenetic proteins (BMPs) are involved in various aspects of cell-cell communication in complex life forms. They act as morphogens, help differentiate different cell types from different progenitor cells in development, and are involved in many instances of intercellular communication, from forming a body axis to healing bone fractures, from sugar metabolism to angiogenesis. If the same protein or protein family carries out many functions, there is a demand to regulate and fine-tune their biological activities, and BMPs are highly regulated to generate cell- and context-dependent outcomes.
Not all such instances can be explained yet. Growth/differentiation factor (GDF)5 (or BMP14) synergizes with BMP2 on chondrogenic ATDC5 cells, but antagonizes BMP2 on myoblastic C2C12 cells. Known regulators of BMP2/GDF5 signal transduction failed to explain this context-dependent difference, so a microarray was performed to identify new, cell-specific regulatory components. One identified candidate, the fibroblast growth factor receptor (FGFR)2, was analyzed as a potential new co-receptor to BMP ligands such as GDF5: It was shown that FGFR2 directly binds BMP2, GDF5, and other BMP ligands in vitro, and FGFR2 was able to positively influence BMP2/GDF5-mediated signaling outcome in cell-based assays. This effect was independent of FGFR2s kinase activity, and independent of the downstream mediators SMAD1/5/8, p42/p44, Akt, and p38. The elevated colocalization of BMP receptor type IA and FGFR2 in the presence of BMP2 or GDF5 suggests a signaling complex containing both receptors, akin to other known co-receptors of BMP ligands such as repulsive guidance molecules.
This unexpected direct interaction between FGF receptor and BMP ligands potentially opens a new category of BMP signal transduction regulation, as FGFR2 is the second receptor tyrosine kinase to be identified as BMP co-receptor, and more may follow. The integration of cell surface interactions between members of the FGF and BMP family especially may widen the knowledge of such cellular communication mechanisms which involve both growth factor families, including morphogen gradients and osteogenesis, and may in consequence help to improve treatment options in osteochodnral diseases.
Plants extract mineral nutrients from the soil, or from interactions with mutualistic soil microbes via their root systems. Adapting root architecture to nutrient availability enables efficient resource utilization, particularly in patchy and dynamic environments. Root growth responses to soil nitrogen levels are shoot-mediated, but the identity of shoot-derived mobile signals regulating root growth responses has remained enigmatic. Here we show that a shoot-derived micro RNA, miR2111, systemically steers lateral root initiation and nitrogen responsiveness through its root target TML (TOO MUCH LOVE) in the legume Lotus japonicus, where miR2111 and TML were previously shown to regulate symbiotic infections with nitrogen fixing bacteria. Intriguingly, systemic control of lateral root initiation by miR2111 and TML/HOLT (HOMOLOGUE OF LEGUME TML) was conserved in the nonsymbiotic ruderal Arabidopsis thaliana, which follows a distinct ecological strategy. Thus, the miR2111-TML/HOLT regulon emerges as an essential, conserved factor in adaptive shoot control of root architecture in dicots.
To fire action-potential-like electrical signals, the vacuole membrane requires the two-pore channel TPC1, formerly called SV channel. The TPC1/SV channel functions as a depolarization-stimulated, non-selective cation channel that is inhibited by luminal Ca\(^{2+}\). In our search for species-dependent functional TPC1 channel variants with different luminal Ca\(^{2+}\) sensitivity, we found in total three acidic residues present in Ca\(^{2+}\) sensor sites 2 and 3 of the Ca\(^{2+}\)-sensitive AtTPC1 channel from Arabidopsis thaliana that were neutral in its Vicia faba ortholog and also in those of many other Fabaceae. When expressed in the Arabidopsis AtTPC1-loss-of-function background, wild-type VfTPC1 was hypersensitive to vacuole depolarization and only weakly sensitive to blocking luminal Ca\(^{2+}\). When AtTPC1 was mutated for these VfTPC1-homologous polymorphic residues, two neutral substitutions in Ca\(^{2+}\) sensor site 3 alone were already sufficient for the Arabidopsis At-VfTPC1 channel mutant to gain VfTPC1-like voltage and luminal Ca\(^{2+}\) sensitivity that together rendered vacuoles hyperexcitable. Thus, natural TPC1 channel variants exist in plant families which may fine-tune vacuole excitability and adapt it to environmental settings of the particular ecological niche.
Interleukin-4 (IL-4) plays a key role in atopic diseases. It coordinates T-helper cell differentiation to subtype 2, thereby directing defense toward humoral immunity. Together with Interleukin-13, IL-4 further induces immunoglobulin class switch to IgE. Antibodies of this type activate mast cells and basophilic and eosinophilic granulocytes, which release pro-inflammatory mediators accounting for the typical symptoms of atopic diseases. IL-4 and IL-13 are thus major targets for pharmaceutical intervention strategies to treat atopic diseases. Besides neutralizing antibodies against IL-4, IL-13, or its receptors, IL-4 antagonists can present valuable alternatives. Pitrakinra, an Escherichia coli-derived IL-4 antagonist, has been evaluated in clinical trials for asthma treatment in the past; however, deficits such as short serum lifetime and potential immunogenicity among others stopped further development. To overcome such deficits, PEGylation of therapeutically important proteins has been used to increase the lifetime and proteolytic stability. As an alternative, glycoengineering is an emerging strategy used to improve pharmacokinetics of protein therapeutics. In this study, we have established different strategies to attach glycan moieties to defined positions in IL-4. Different chemical attachment strategies employing thiol chemistry were used to attach a glucose molecule at amino acid position 121, thereby converting IL-4 into a highly effective antagonist. To enhance the proteolytic stability of this IL-4 antagonist, additional glycan structures were introduced by glycoengineering utilizing eucaryotic expression. IL-4 antagonists with a combination of chemical and biosynthetic glycoengineering could be useful as therapeutic alternatives to IL-4 neutralizing antibodies already used to treat atopic diseases.
Young grapevines (Vitis vinifera) suffer and eventually can die from the crown gall disease caused by the plant pathogen Allorhizobium vitis (Rhizobiaceae). Virulent members of A. vitis harbor a tumor-inducing plasmid and induce formation of crown galls due to the oncogenes encoded on the transfer DNA. The expression of oncogenes in transformed host cells induces unregulated cell proliferation and metabolic and physiological changes. The crown gall produces opines uncommon to plants, which provide an important nutrient source for A. vitis harboring opine catabolism enzymes. Crown galls host a distinct bacterial community, and the mechanisms establishing a crown gall–specific bacterial community are currently unknown. Thus, we were interested in whether genes homologous to those of the tumor-inducing plasmid coexist in the genomes of the microbial species coexisting in crown galls. We isolated 8 bacterial strains from grapevine crown galls, sequenced their genomes, and tested their virulence and opine utilization ability in bioassays. In addition, the 8 genome sequences were compared with 34 published bacterial genomes, including closely related plant-associated bacteria not from crown galls. Homologous genes for virulence and opine anabolism were only present in the virulent Rhizobiaceae. In contrast, homologs of the opine catabolism genes were present in all strains including the nonvirulent members of the Rhizobiaceae and non-Rhizobiaceae. Gene neighborhood and sequence identity of the opine degradation cluster of virulent and nonvirulent strains together with the results of the opine utilization assay support the important role of opine utilization for cocolonization in crown galls, thereby shaping the crown gall community.
Modern lifestyle is often at odds with endogenously driven rhythmicity, which can lead to circadian disruption and metabolic syndrome. One signature for circadian disruption is a reduced or altered metabolite cycling in the circulating tissue reflecting the current metabolic status. Drosophila is a well-established model in chronobiology, but day-time dependent variations of transport metabolites in the fly circulation are poorly characterized. Here, we sampled fly hemolymph throughout the day and analyzed diacylglycerols (DGs), phosphoethanolamines (PEs) and phosphocholines (PCs) using LC-MS. In wild-type flies kept on sugar-only medium under a light-dark cycle, all transport lipid species showed a synchronized bimodal oscillation pattern with maxima at the beginning and end of the light phase which were impaired in period01 clock mutants. In wild-type flies under constant dark conditions, the oscillation became monophasic with a maximum in the middle of the subjective day. In strong support of clock-driven oscillations, levels of the targeted lipids peaked once in the middle of the light phase under time-restricted feeding independent of the time of food intake. When wild-type flies were reared on full standard medium, the rhythmic alterations of hemolymph lipid levels were greatly attenuated. Our data suggest that the circadian clock aligns daily oscillations of DGs, PEs, and PCs in the hemolymph to the anabolic siesta phase, with a strong influence of light on phase and modality.
Photosynthetic plants have a remarkable ability to modify their metabolism and development according to ever changing environmental conditions. The root system displays continuous growth of the primary root and formation of lateral roots enabling efficient water and nutrient uptake and anchorage of the plant in soil. With regard to lateral roots, development is post-embryonic, originating from the pericycle of the primary root. Coordinated activity of several molecular signalling pathways controlled by the hormone auxin is important throughout all stages of lateral root development.At first, two adjacent Xylem Pole Pericycle (XPP) cells are activated and the nuclei of these cells migrate towards a common cell wall.This is followed by XPP cells acquiring volume thus swelling up.The XPP cells then undergo anticlinal cell division, followed by a series of periclinal and anticlinal divisions,leading to lateral root primordia.These break through the radial cell layers and emerge out the primary root.
Although root system plasticity is well-described in response to environmental cues such as ion nutrition in the soil, little is known on how root development is shaped according to the endogenous energy status of the plant.In this study, we were able to connect limited perturbations in photosynthetic energy supply to lateral root development.We established two experimental systems – treatment with low light and unexpected darkness which led to short-term energy imbalance in the plant.These short perturbations administered, showed an increase in the emerged lateral root density and decrease in root hexose availability and activation of the low energy marker gene ASN1 (ASPARAGINE SYNTHETASE 1).Although not demonstrated, presumably, these disturbances in the plant energy homeo-stasis activates SnRK1 (SNF1 RELATED KINASE 1),an evolutionary conserved kinase mediat-ing metabolic and transcriptional responses towards low energy conditions. In A. thaliana, two catalytic α-subunits of this kinase (SnRK1.α1 and SnRK1.α2) are functionally active and form ternary complexes with the regulatory β- and γ- subunits. Whereas unexpected darkness results in an increase in emerged lateral root density, the snrk1.α1 loss-of-function mutant displayed decrease in emerged lateral root density. As this effect is not that pronounced in the snrk1.α2 loss-of-function mutant, the α1 catalytic subunit is important for the observed lateral root phenotype under short-term energy perturbations. Moreover, root expression patterns of SnRK1.α1:GFP supports a role of this catalytic subunit in lateral root development. Furthermore, the lateral root response during short-term perturbations requires the SnRK1 downstream transcriptional regulator bZIP63 (BASIC LEU-CINE ZIPPER 63), as demonstrated here by a loss-of-function approach. Phenotypic studies showed that in comparison to wild-type, bzip63 mutants displayed decreased lateral root density upon low-light and unexpected darkness conditions. Previous work has demonstrat-ed that SnRK1 directly phosphorylates bZIP63 at three serine residues. Alanine-exchange mutants of the SnRK1 dependent bZIP63 phosphorylation sites behave similarly to bzip63 loss-of-function mutants and do not display increased lateral root density upon short-term unexpected darkness. This data strongly supports an impact of SnRK1-bZIP63 signalling in mediating the observed lateral root density phenotype. Plants expressing a bZIP63:YFP fu-sion protein showed specific localization patterns in primary root and in all developmental stages of the lateral root. bzip63 loss-of-function mutant lines displayed reduced early stage lateral root initiation events under unexpected darkness as demonstrated by Differen-tial Interference Contrast microscopy (DIC) and the use of a GATA23 reporter line. This data supports a role of bZIP63 in early lateral root initiation.
Next, by employing Chromatin Immunoprecitation (ChIP) sequencing, we were able to iden-tify global binding targets of bZIP63, including the auxin-regulated transcription factor (TF) ARF19 (AUXIN RESPONSE FACTOR 19), a well-described central regulator of lateral root development. Additional ChIP experiments confirmed direct binding of bZIP63 to an ARF19 promoter region harboring a G-Box cis-element, a well-established bZIP63 binding site. We also observed that short-term energy perturbation upon unexpected darkness induced tran-scription of ARF19, which was impaired in the bzip63 loss-of-function mutant. These results propose that bZIP63 mediates lateral root development under short-term energy perturba-tion via ARF19.
In conclusion, this study provides a novel mechanistic link between energy homeostasis and plant development. By employing reverse genetics, confocal imaging and high-throughput sequencing strategies, we were able to propose a SnRK1-bZIP63-ARF19 signalling module in integrating energy signalling into lateral root developmental programs.
Optogenetics became successful in neuroscience with Channelrhodopsin-2 (ChR2), a light-gated cation channel from the green alga Chlamydomonas reinhardtii, as an easy applicable tool. The success of ChR2 inspired the development of various photosensory proteins as powerful actuators for optogenetic manipulation of biological activity. However, the current optogenetic toolbox is still not perfect and further improvements are desirable. In my thesis, I engineered and characterized several different optogenetic tools with new features.
(i) Although ChR2 is the most often used optogenetic actuator, its single-channel conductance and its Ca2+ permeability are relatively low. ChR2 variants with increased Ca2+ conductance were described recently but a further increase seemed possible. In addition, the H+ conductance of ChR2 may lead to cellular acidification and unintended pH-related side effects upon prolonged illumination. Through rational design, I developed several improved ChR2 variants with larger photocurrent, higher cation selectivity, and lower H+ conductance.
(ii) The light-activated inward chloride pump NpHR is a widely used optogenetic tool for neural silencing. However, pronounced inactivation upon long time illumination constrains its application for long-lasting neural inhibition. I found that the deprotonation of the Schiff base underlies the inactivation of NpHR. Through systematically exploring optimized illumination schemes, I found illumination with blue light alone could profoundly increase the temporal stability of the NpHR-mediated photocurrent. A combination of green and violet light eliminates the inactivation effect, similar to blue light, but leading to a higher photocurrent and therefore better light-induced inhibition.
(iii) Photoactivated adenylyl cyclases (PACs) were shown to be useful for light-manipulation of cellular cAMP levels. I developed a convenient in-vitro assay for soluble PACs that allows their reliable characterization. Comparison of different PACs revealed that bPAC from Beggiatoa is the best optogenetic tool for cAMP manipulation, due to its high efficiency and small size. However, a residual activity of bPAC in the dark is unwanted and the cytosolic localization prevents subcellular precise cAMP manipulation. I therefore introduced point mutations into bPAC to reduce its dark activity. Interestingly, I found that membrane targeting of bPAC with different linkers can remarkably alter its activity, in addition to its localization. Taken together, a set of PACs with different activity and subcellular localization were engineered for selection based on the intended usage. The membrane-bound PM-bPAC 2.0 with reduced dark activity is well-tolerated by hippocampal neurons and reliably evokes a transient photocurrent, when co-expression with a CNG channel.
(iv) Bidirectional manipulation of cell activity with light of different wavelengths is of great importance in dissecting neural networks in the brain. Selection of optimal tool pairs is the first and most important step for dual-color optogenetics. Through N- and C-terminal modifications, an improved ChR variant (i.e. vf-Chrimson 2.0) was engineered and selected as the red light-controlled actuator for excitation. Detailed comparison of three two-component potassium channels, composed of bPAC and the cAMP-activated potassium channel SthK, revealed the superior properties of SthK-bP. Combining vf-Chrimson 2.0 and improved SthK-bP “SthK(TV418)-bP” could reliably induce depolarization by red light and hyperpolarization by blue light. A residual tiny crosstalk between vf-Chrimson 2.0 and SthK(TV418)-bP, when applying blue light, can be minimized to a negligible level by applying light pulses or simply lowering the blue
light intensity.
Agrochemicals like systemic active ingredients (AI) need to penetrate the outermost barrier of the plant, known as the plant cuticle, to reach its right target site. Therefore, adjuvants are added to provide precise and efficient biodelivery by i.a. modifying the cuticular barrier and increasing the AI diffusion. This modification process is depicted as plasticization of the cuticular wax which mainly consists of very long-chain aliphatic (VLCA) and cyclic compounds. Plasticization of cuticular waxes is pictured as an increase of amorphous domains and/or a decrease of crystalline fractions, but comprehensive, experimental proof is lacking to date. Hence, the objective of this thesis was to i) elucidate the permeation barrier of the plant cuticle to AIs in terms of the different wax fractions and ii) holistically investigate the modification of this barrier using selected oil and surface active adjuvants, an aliphatic leaf wax and an artificial model wax. Therefore, the oil adjuvant methyl oleate (MeO) and other oil derivatives like methyl linolenate (MeLin), methyl stearate (MeSt) and oleic acid (OA) were selected. Three monodisperse, non-ionic alcohol ethoxylates with increasing ethylene oxide monomer (EO) number (C10E2, C10E5, C10E8) were chosen as representatives of the group of surface active agents (surfactants). Both adjuvant classes are commonly used as formulation aids for agrochemicals which are known for its penetration enhancing effect. The aliphatic leaf wax of Schefflera elegantissima was selected, as well as a model wax comprising the four most abundant cuticular wax compounds of this species. Permeation, transpiration and penetration studies were conducted using enzymatically isolated cuticles of Prunus laurocerasus and Garcinia xanthochymus.
Cuticular permeability to the three organic solutes theobromine, caffeine and azoxystrobin differing in lipophilicity was measured using a steady-state two-chamber system separated by the isolated leaf cuticles of the evergreen species P. laurocerasus and G. xanthochymus. Treating the isolated cuticles with methanol selectively removed the cyclic fraction, and membrane permeability to the organic compounds was not altered. In contrast, fully dewaxing the membranes using chloroform resulted in a statistically significant increase in permeance for all compounds and species, except caffeine with cuticles of G. xanthochymus due to a matrix-specific influence on the semi-hydrophilic compound. Crystalline regions may reduce the accessibility to the lipophilic pathway across the waxes and also block hydrophilic domains in the cuticle.
Knowing that the aliphatic wax fraction builds the cuticular diffusion barrier, the influence of the adjuvants on the phase behaviour of an aliphatic cuticular wax as well as the influence on the cuticular penetration of AIs were investigated. Differential scanning calorimetry (DSC) and Fourier-transform infrared spectroscopy (FTIR) were selected to investigate the phase behaviour and thus possible plasticization of pure Schefflera elegantissima leaf wax, its artificial model wax comprising the four most abundant compounds (n-nonacosane, n-hentriacontane, 1-triacontanol and 1-dotriacontanol) and wax adjuvant mixtures. DSC thermograms showed a shift of the melting ranges to lower temperatures and decreased absolute values of the total enthalpy of transition (EOT) for all adjuvant leaf wax blends at 50 % (w/w) adjuvant proportion. The highest decrease was found for C10E2 followed by MeO > OA and C10E8 > MeLin > MeSt. The aliphatic crystallinity determined by FTIR yielded declined values for the leaf and the artificial wax with 50 % MeO. All other adjuvant leaf wax blends did not show a significant decrease of crystallinity. As it is assumed that the cuticular wax is formed by crystalline domains which consist of aliphatic hydrocarbon chains and an amorphous fraction comprising aliphatic chain ends and functional groups, the plasticizers are depicted as wax disruptors influencing amorphization and/or crystallization. The adjuvants can increase crystalline domains using the aliphatic tail whereas their more hydrophilic head is embedded in the amorphous wax fraction. DSC and FTIR showed similar trends using the leaf wax and the model wax in combination with the adjuvants.
In general, cuticular transpiration increased after adding the pure adjuvants to the surface of isolated cuticles or leaf envelopes. As waxes build the cuticular permeation barrier not only to AIs but also to water, the adjuvant wax interaction might affect the cuticular barrier properties leading to increased transpiration. Direct evidence for increased AI penetration with the adjuvants was given using isolated cuticles of P. laurocerasus in combination with the non-steady-state setup simulation of foliar penetration (SOFP) and caffeine at relative humidity levels (RH) of 30, 50 and 80 %. The increase in caffeine penetration was much more pronounced using C10E5 and C10E8 than MeO but always independent of RH. Only C10E2 exhibited an increased penetration enhancing effect positively related to RH. The role of the molecular structure of adjuvants in terms of humectant and plasticizer properties are discussed.
Hence, the current work shows for the first time that the cuticular permeation barrier is associated with the VLCAs rather than the cyclic fraction and that adjuvants structurally influence this barrier resulting in penetration enhancing effects. Additionally, this work demonstrates that an artificial model wax is feasible to mimic the wax adjuvant interaction in conformity with a leaf wax, making it feasible for in-vitro experiments on a larger scale (e.g. screenings). This provides valuable knowledge about the cuticular barrier modification to enhance AI penetration which is a crucial factor concerning the optimization of AI formulations in agrochemistry.
Xylem hydraulic safety and efficiency are key traits determining tree fitness in a warmer and drier world. While numerous plant hydraulic studies have focused on branches, our understanding of root hydraulic functioning remains limited, although roots control water uptake, influence stomatal regulation and have commonly been considered as the most vulnerable organ along the hydraulic pathway.
We investigated 11 traits related to xylem safety and efficiency along the hydraulic pathway in four temperate broad-leaved tree species.
Continuous vessel tapering from coarse roots to stems and branches caused considerable reduction in hydraulic efficiency. Wood density was always lowest in roots, but did not decline linearly along the flow path. In contrast, xylem embolism resistance (P50) did not differ significantly between roots and branches, except for one species. The limited variation in xylem safety between organs did not adequately reflect the corresponding reductions in vessel diameter (by ~70%) and hydraulic efficiency (by ~85%). Although we did not observe any trade-off between xylem safety and specific conductivity, vessel diameter, vessel lumen fraction and wood density were related to embolism resistance, both across and partly within organs.
We conclude that coarse roots are not highly vulnerable to xylem embolism as commonly believed, indicating that hydraulic failure during soil drying might be restricted to fine roots.
The negative impact of juvenile undernourishment on adult behavior has been well reported for vertebrates, but relatively little is known about invertebrates. In honeybees, nutrition has long been known to affect task performance and timing of behavioral transitions. Whether and how a dietary restriction during larval development affects the task performance of adult honeybees is largely unknown. We raised honeybees in-vitro, varying the amount of a standardized diet (150 µl, 160 µl, 180 µl in total). Emerging adults were marked and inserted into established colonies. Behavioral performance of nurse bees and foragers was investigated and physiological factors known to be involved in the regulation of social organization were quantified. Surprisingly, adult honeybees raised under different feeding regimes did not differ in any of the behaviors observed. No differences were observed in physiological parameters apart from weight. Honeybees were lighter when undernourished (150 µl), while they were heavier under the overfed treatment (180 µl) compared to the control group raised under a normal diet (160 µl). These data suggest that dietary restrictions during larval development do not affect task performance or physiology in this social insect despite producing clear effects on adult weight. We speculate that possible effects of larval undernourishment might be compensated during the early period of adult life.
The recently observed consistent loss of β-diversity across ecosystems indicates increasingly homogeneous communities in patches of landscapes, mainly caused by increasing land-use intensity. Biodiversity is related to numerous ecosystem functions and stability. Therefore, decreasing β-diversity is also expected to reduce multifunctionality. To assess the impact of homogenization and to develop guidelines to reverse its potentially negative effects, we combine expertise from forest science, ecology, remote sensing, chemical ecology and statistics in a collaborative and experimental β-diversity approach. Specifically, we will address the question whether the Enhancement of Structural Beta Complexity (ESBC) in forests by silviculture or natural disturbances will increase biodiversity and multifunctionality in formerly homogeneously structured production forests. Our approach will identify potential mechanisms behind observed homogenization-diversity-relationships and show how these translate into effects on multifunctionality. At eleven forest sites throughout Germany, we selected two districts as two types of small ‘forest landscapes’. In one of these two districts, we established ESBC treatments (nine differently treated 50x50 m patches with a focus on canopy cover and deadwood features). In the second, the control district, we will establish nine patches without ESBC. By a comprehensive sampling, we will monitor 18 taxonomic groups and measure 21 ecosystem functions, including key functions in temperate forests, on all patches. The statistical framework will allow a comprehensive biodiversity assessment by quantifying the different aspects of multitrophic biodiversity (taxonomical, functional and phylogenetic diversity) on different levels of biodiversity (α-, β-, γ-diversity). To combine overall diversity, we will apply the concept of multidiversity across the 18 taxa. We will use and develop new approaches for quantification and partitioning of multifunctionality at α- and β- scales. Overall, our study will herald a new research avenue, namely by experimentally describing the link between β-diversity and multifunctionality. Furthermore, we will help to develop guidelines for improved silvicultural concepts and concepts for management of natural disturbances in temperate forests reversing past homogenization effects.
Plants do not have neurons but operate transmembrane ion channels and can get electrical excited by physical and chemical clues. Among them the Venus flytrap is characterized by its peculiar hapto-electric signaling. When insects collide with trigger hairs emerging the trap inner surface, the mechanical stimulus within the mechanosensory organ is translated into a calcium signal and an action potential (AP). Here we asked how the Ca\(^{2+}\) wave and AP is initiated in the trigger hair and how it is feed into systemic trap calcium-electrical networks. When Dionaea muscipula trigger hairs matures and develop hapto-electric excitability the mechanosensitive anion channel DmMSL10/FLYC1 and voltage dependent SKOR type Shaker K\(^{+}\) channel are expressed in the sheering stress sensitive podium. The podium of the trigger hair is interface to the flytrap’s prey capture and processing networks. In the excitable state touch stimulation of the trigger hair evokes a rise in the podium Ca2+ first and before the calcium signal together with an action potential travel all over the trap surface. In search for podium ion channels and pumps mediating touch induced Ca\(^{2+}\) transients, we, in mature trigger hairs firing fast Ca\(^{2+}\) signals and APs, found OSCA1.7 and GLR3.6 type Ca\(^{2+}\) channels and ACA2/10 Ca\(^{2+}\) pumps specifically expressed in the podium. Like trigger hair stimulation, glutamate application to the trap directly evoked a propagating Ca\(^{2+}\) and electrical event. Given that anesthetics affect K\(^+\) channels and glutamate receptors in the animal system we exposed flytraps to an ether atmosphere. As result propagation of touch and glutamate induced Ca\(^{2+}\) and AP long-distance signaling got suppressed, while the trap completely recovered excitability when ether was replaced by fresh air. In line with ether targeting a calcium channel addressing a Ca\(^{2+}\) activated anion channel the AP amplitude declined before the electrical signal ceased completely. Ether in the mechanosensory organ did neither prevent the touch induction of a calcium signal nor this post stimulus decay. This finding indicates that ether prevents the touch activated, glr3.6 expressing base of the trigger hair to excite the capture organ.
Pflanzen müssen sich während der Samenkeimung und Keimlingsentwicklung über eingelagerte Speicherstoffe heterotroph versorgen, bis sie, nach Etablierung ihres Photosyntheseapparats, einen autotrophen Lebensstil führen können.
Diese Arbeit geht von der Hypothese aus, dass der evolutionär konservierten zentral-metabolischen Kinase Snf1-RELATED PROTEIN KINASE 1 (SnRK1) eine besondere Rolle bei der Mobilisierung von Speicherstoffen während der Keimlingsentwicklung zukommt. Während die Bedeutung von SnRK1 als zentraler Regulator katabolischer Prozesse unter Energiemangel- und Stresssituationen bereits gezeigt wurde, war die Funktion von SnRK1 im Zusammenhang mit der Samenkeimung weitgehend ungeklärt. In dieser Arbeit konnte erstmals gezeigt werden, dass SnRK1 in Arabidopsis die Mobilisierung und Degradation von Speicherstoffen, insbesondere von Triacylglyceride (TAGs), Samenspeicherproteinen und Aminosäuren, steuert. Sowohl Studien zur Lokalisation von SnRK1:GFP-Fusionsproteinen als auch Kinaseaktivitätsassays unterstützen eine mögliche Funktion von SnRK1 während der Keimlingsentwicklung. Eine induzierbare snrk1-knockdown Mutante zeigt neben einem eingeschränkten Wurzel- und Hypokotylwachstum auch keine Ausbildung eines Photosyntheseapparats, was die zentrale Rolle der SnRK1 in diesem frühen Entwicklungsstadium untermauert. Durch Fütterungsexperimente mit Glukose konnte der Phänotyp einer snrk1 -Mutante in Keimlingen gerettet werden. Dies zeigt, dass der metabolische Block durch externe Gabe von Kohlenhydraten umgangen werden kann. Die zentrale Funktion von SnRK1 ist folgich der Abbau von Speicherstoffen und keine allgemeine Deregulation des pflanzlichen Stoffwechsels. Durch massenspektrometrische Untersuchungen von Keimlingen des Wildtyps und der snrk1-Mutante konnte gezeigt werden, dass TAGs in der Mutante in der spä- ten Keimlingsentwicklung ab Tag 4 langsamer abgebaut werden als im Wildtyp. Ebenso werden Samenspeicherproteine in der Mutante langsamer degradiert, wodurch die Verfügbarkeit von freien Aminosäuren in geringer ist. Entgegen der allgemeinen Annahme konnte gezeigt werden, dass während der Keimlingsentwicklung zumindest in Arabidopsis, einer ölhaltigen Pflanze, zunächst Kohlenhydrate in Form von Saccharose abgebaut werden, bevor die Degradation von TAGs und Aminosäuren beginnt. Diese Abbauprodukte können dann der Glukoneogenese zugeführt werden um daraus Glukose herzustellen. Mittels Transkriptom-Analysen konnten zentrale SnRK1-abhängige Gene in der Speicherstoffmobilisierung von TAG, beispielsweise PEROXISOMAL NAD-MALATE DEHYDROGENASE 2 (PMDH2) und ACYL-CoA-OXIDASE 4 (ACX4), und Aminosäuren identifiziert werden. Somit wurde ein Mechanismus der SnRK1-abhängigen Genregulation während der Samenkeimung in Arabidopsis gefunden. Bei der Degradation von Aminosäuren wird die cytosolische PYRUVATE ORTHOPHOSPHATE DIKINASE (cyPPDK), ein Schlüsselenzym beim Abbau bestimmter Aminosäuren und bei der Glukoneogenese, SnRK1-abhängig transkriptionell reguliert. Durch Koregulation konnte der Transkriptionsfaktor bZIP63 (BASIC LEUCINE ZIPPER 63) gefunden werden, dessen Transkription ebenfalls SnRK1-abhängig reguliert wird. Außerdem konnte die Transkription von cyPPDK in bzip63-Mutanten nur noch sehr schwach induziert werden. In Protoplasten konnte der cyPPDK-Promotor durch Aktivierungsexperimente mit bZIP63 und SnRK1α1 induziert werden. Durch Mutationskartierung und Chromatin-Immunopräzipitation (ChIP)PCR konnte mehrfach eine direkte Bindung von bZIP63 an den cyPPDK-Promotor nachgewiesen werden. Zusammenfassend ergibt sich ein mechanistisches Arbeitsmodell, in dem bZIP63 durch SnRK1 phosphoryliert wird und durch Bindung an regulatorische G-Box cis-Elemente im cyPPDK- Promotor dessen Transkription anschaltet. Infolgedessen werden Aminosäuren abgebaut und wird über die Glukoneogenese Glukose aufgebaut. Dieser Mechanismus ist essentiell für die Übergangsphase zwischen heterotropher und autotropher Lebensweise, und trägt dazu bei, die im Samen vorhandenen Ressourcen dem Keimling zum idealen Zeitpunkt zugänglich zu machen. Darüber hinaus werden Gene im Abbau von verzweigtkettigen Aminosäuren ebenfalls durch bZIP63 reguliert. Dabei wird dem Keimling Energie in Form von Adenosin-Triphosphat (ATP) zur Verfügung gestellt.
Zusammengefasst zeigen die Ergebnisse dieser Arbeit, dass die Mobilisierung von Speicherstoffen auch während der Keimlingsentwicklung direkt von SnRK1 abhängig ist. Die umfangreichen Datensätze der RNA-Seq-Analysen bieten zudem die Möglichkeit, weitere SnRK1-abhängige Gene der Speichermobilisierung zu identifizieren und somit einem besseren Verständnis der Keimlingsentwicklung beizutragen. Aufgrund der zentralen Bedeutung der SnRK1-Kinase in diesem entscheidenden Entwicklungsschritt ist davon auszugehen, dass diese Erkenntnisse mittelfristig auch für bessere Keimungsraten und somit bessere Erträge in der Landwirtschaft genutzt werden können.
The evolution of the internal water transport system was a prerequisite for high plant productivity. In times of climate change, understanding the dependency of juvenile growth on xylem hydraulic physiology is therefore of high importance. Here, we explored various wood anatomical, hydraulic, and leaf morphological traits related to hydraulic safety and efficiency in three temperate broadleaved tree species (Acer pseudoplatanus, Betula pendula, and Sorbus aucuparia). We took advantage of a severe natural heat wave that resulted in different climatic growing conditions for even-aged plants from the same seed source growing inside a greenhouse and outside. Inside the greenhouse, the daily maximum vapour pressure deficit was on average 36% higher than outside during the growing seasons. Because of the higher atmospheric moisture stress, the biomass production differed up to 5.6-fold between both groups. Except for one species, a high productivity was associated with a high hydraulic efficiency caused by large xylem vessels and a large, supported leaf area. Although no safety-efficiency trade-off was observed, productivity was significantly related to P\(_{50}\) in two of the tree species but without revealing any clear pattern. A considerable plasticity in given traits was observed between both groups, with safety-related traits being more static while efficiency-related traits revealed a higher intra-specific plasticity. This was associated with other wood anatomical and leaf morphological adjustments. We confirm that a high hydraulic efficiency seems to be a prerequisite for a high biomass production, while our controversial results on the growth–xylem safety relationship confirm that safety-efficiency traits are decoupled and that their relationship with juvenile growth and water regime is species-specific.
Die Fähigkeit sich an die Rotation der Erde und den daraus resultierenden Tag- und Nacht-Rhythmus anzupassen, basiert auf einer komplexen Regulation verschiedener physiologischer Prozesse. Auf molekularer Ebene liegt diesen Prozessen eine Orchestration von Uhr-Genen zugrunde – auch als innere Uhr bezeichnet – die einen aktivierenden bzw. reprimierenden Einfluss auf die Expression einer Vielzahl weiterer Gene hat. Ausgehend von dieser Regulation lassen sich auf unterschiedlichsten Ebenen tageszeitabhängige, wiederkehrende Rhythmen beobachten.
Während diese wiederkehrenden Rhythmen auf einigen Ebenen bereits gut erforscht und beschrieben sind, gibt es weitere Ebenen wie den Metabolismus, über die das Wissen bisher noch begrenzt ist.
So handelt es sich bei Drosophila beispielsweise um den Organismus, dessen innere Uhr auf molekularer Ebene wahrscheinlich mit am besten charakterisiert ist. Dennoch ist bisher nur wenig über Stoffklassen bekannt, deren Metabolismus durch die innere Uhr kontrolliert wird.
Zwar konnte bereits gezeigt werden, dass sich eine gestörte innere Uhr auf die Anlage der Energiespeicher auswirkt, inwiefern dies allerdings einen Einfluss auf dem intermediären Stoffwechsel hat, blieb bisher weitgehend unerforscht. Auch die Frage, welche Metaboliten wiederkehrende, tageszeitabhängige Rhythmen aufweisen, wurde bisher nur für eine begrenzte Anzahl Metaboliten untersucht.
Bei der hier durchgeführten Arbeit wurden deshalb zunächst die globalen Metabolit-Profile von Fliegen mit einer auf molekularer Ebene gestörten inneren Uhr (per01) mit Fliegen, die über eine funktionale Uhr verfügen (CantonS), zu zwei Zeitpunkten verglichen. Um die Anzahl der zeitgleich untersuchten Gewebe und somit die Komplexität der Probe zu reduzieren, wurden hierfür die Köpfe von den Körpern der Fliegen getrennt und separat analysiert. Beide Körperteile wurden sowohl auf kleine hydrophile als auch auf hydrophobe Metaboliten hin mittels UPLC-ESI-qTOF-MS untersucht. Die anschließend durchgeführte, statistische Analyse brachte hervor, dass sich Unterschiede zwischen den beiden Fliegenlinien besonders in den Spiegeln der essentiellen Aminosäuren, den Kynureninen, den Pterinaten sowie den Spiegeln der Glycero(phospho)lipiden und Fettsäureester zeigten. Bei den Lipiden zeigte sich, dass die Auswirkungen weniger ausgeprägt für die Anlage der Speicher- und Strukturlipide als für die Intermediate des Lipidabbaus, die Diacylglycerole (DAGs) sowie die Acylcarnitine (ACs), waren.
Um zu bestätigen, dass die inneren Uhr tatsächlich einen regulatorischen Einfluss auf die ausgemachten Stoffwechselwege hat, wurden anschließend die Spiegel aller Mitglieder darauf hin untersucht, ob diese wiederkehrende, tageszeitabhängige Schwankungen aufweisen. Hierfür wurden Proben alle zwei Stunden über drei aufeinanderfolgende Tage genommen und analysiert, bevor mittels JTK_CYCLE eine statistische Analyse der Daten durchgeführt und die Metaboliten herausgefiltert wurden, die ein rhythmisches Verhalten bei einer Periodenlänge von 24h zeigten. Hierbei bestätigte sich, dass besonders die Mitglieder des intermediären Lipidmetablismus hiervon betroffen waren. So konnten zwar auch für einige Aminosäuren robuste Rhythmen ausgemacht werden, besonders ausgeprägt waren diese jedoch erneut bei den DAGs und den ACs. Die abschließende Untersuchung letzterer unter Freilaufbedingungen (DD) sowie in per01 brachte hervor, dass die ausgemachten Rhythmen unter diesen Bedingungen entweder nicht mehr detektiert werden konnten oder deutlich abgeschwächt vorlagen. Lediglich zwei kurzkettige ACs zeigten auch unter DD-Bedingungen statistisch signifikante Rhythmen in ihren Spiegeln. Dies spricht dafür, dass neben der Regulation durch die innere Uhr weitere Faktoren, wie beispielsweise das Licht, eine entscheidende Rolle zu spielen scheinen.
A part of the plant kingdom consists of a variety of carnivorous plants. Some trap their prey
using sticky leaves, others have pitfall traps where prey cannot escape once it has fallen inside.
A rare trap type is the snap-trap: it appears only twice in the plant kingdom, in the genera
Aldrovanda and Dionaea. Even Charles Darwin himself described Dionaea muscipula, the
Venus flytrap, with the following words “This plant, commonly called Venus' fly-trap, from the
rapidity and force of its movements, is one of the most wonderful in the world”. For a long
time now, the mechanisms of Dionaea’s prey recognition, capture and utilization are of
interest for scientists and have been studied intensively.
Dionaea presents itself with traps wide-open, ready to catch insects upon contact. For this,
the insect has to touch the trigger hairs of the opened trap twice within about 20-30 seconds.
Once the prey is trapped, the trap lobes close tight, forming a hermetically sealed “green
stomach”.
Until lately, there was only limited knowledge about the molecular and hormonal mechanisms
which lead to prey capture and excretion of digestive fluids. It is known that the digestion
process is very water-consuming; therefore, the interplay of digestion-inducing and digestion inhibiting
substances was to be analyzed in this work, to elucidate the fine-tuning of the
digestive pathway. Special attention was given to the impact of phytohormones on mRNA
transcript levels of digestion-related proteins after various stimuli as well as their effect on
Dionaea’s physiological responses.
Jasmonic acid (JA) and its isoleucine-conjugated form, JA-Ile, are an important signal in the
jasmonate pathway. In the majority of non-carnivorous plants, jasmonates are critical for the
defense against herbivory and pathogens. In Dionaea, this defense mechanism has been
restructured towards offensive prey catching. One question in this work was how the
frequency of trigger hair bendings is related to the formation of jasmonates and the induction
of the digestion process. Upon contact of a prey with the trigger hairs in the inside of the trap,
the trap closes and jasmonates are produced biosynthetically. JA-Ile interacts with the COI1-
receptor, thereby activating the digestion pathway which leads to the secretion of digestive
fluid and production of transporters needed to take up prey-derived nutrients. In this work it
could be shown that the number of trigger hair bendings is positively correlated with the level
and duration of transcriptional induction of several digestive enzymes/hydrolases.
Abscisic acid (ABA) acts, along with many other functions, as the plant “drought stress
hormone”. It is synthesized either by roots as the primary sensor for water shortage or by
guard cells in the leaves. ABA affects a network of several thousand genes whose regulation
prepares the plant for drought and initiates protective measurements. It was known from
previous work that the application of ABA for 48 hours increased the required amount of
trigger hair bendings to achieve trap closure. As the digestion process is very water-intensive,
the question arose how exactly the interplay between the jasmonate- and the ABA-pathway
is organized, and if ABA could stop the running digestion process once it had been activated.
In the present work it could be shown that the application of ABA on intact traps prior to
mechanically stimulating the trigger hairs (mechanostimulation) already significantly reduced
the transcription of digestive enzymes for an incubation time as short as 4 h, showing that
already short-term exposure to ABA counteracts the effects of jasmonates when it comes to
initiating the digestion process, but does not inhibit trap closure. Incubation for 24 and 48
hours with 100 μM active ABA had no effect on trap reopening, only very high levels of 200
μM of active ABA inhibited trap reopening but also led to tissue necrosis. As the application
of ABA could reduce the transcription of digestive hydrolases, it is likely that Dionaea can stop
the digestion process, if corresponding external stimuli are received.
Another factor, which only emerged later, was the effect of the wounding-induced systemic
jasmonate burst. As efficient as ABA was in inhibiting marker hydrolase expression after
mechanostimulation in intact plants, the application of ABA on truncated traps was not able
to inhibit mechanostimulation-induced marker hydrolase expression. One reason might be
that the ABA-signal is perceived in the roots, and therefore truncated traps were not able to
react to it. Another reason might be that the wounding desensitized the tissue for the ABAsignal.
Further research is required at this point.
Inhibitors of the jasmonate pathway were also used to assess their effect on the regulation of
Dionaea´s hunting cycle. Coronatine-O-methyloxime proved to be a potent inhibitor of
mechanostimulation-induced expression of digestive enzymes, thus confirming the key
regulatory role of jasmonates for Dionaea´s prey consumption mechanism.
In a parallel project, the generation of in vitro cultures from sterilized seeds and single plant
parts proved successful, which may be important for stock-keeping of future transgenic lines.
Protoplasts were generated from leaf blade tissue and transiently transformed, expressing the
reporter protein YFP after 24 h of incubation. In the future this might be the starting point for
the generation of transgenic lines or the functional testing of DNA constructs.
Pivotal barrier properties of the hydrophobic plant cuticle covering aerial plant surfaces depend on its physicochemical composition. Among plant species and organs, compounds of this boundary layer between the plant interior and the environment vary considerably but cuticle-related studies comparing different organs from the same plant species are still scarce. Thus, this study focused on the cuticle profiles of Physalis peruviana, Physalis ixocarpa, Alkekengi officinarum, and Nicandra physalodes species. Inflated fruiting calyces enveloping fruits make Physalis, Alkekengi, and Nicandra highly recognizable genera among the Solanoideae subfamily. Although the inflation of fruiting calyces is well discussed in the literature still little is known about their post-floral functionalities. Cuticular composition, surface structure, and barrier function were examined and compared in fully expanded amphistomatous leaves, ripe astomatous fruits, and fully inflated hypostomatous fruiting calyces. Species- and organ-specific abundances of non-glandular and glandular trichomes revealed high structural diversity, covering not only abaxial and adaxial leaf surfaces but also fruiting calyx surfaces, whereas fruits were glabrous. Cuticular waxes, which limit non-stomatal transpiration, ranged from <1 μg cm\(^{−2}\) on P. peruviana fruiting calyces and N. physalodes fruits to 22 μg cm\(^{−2}\) on P. peruviana fruits. Very-long-chain aliphatic compounds, notably n-alkanes, iso-, and anteiso-branched alkanes, alkanols, alkanoic acids, and alkyl esters, dominated the cuticular wax coverages (≥86%). Diversity of cuticular wax patterns rose from leaves to fruiting calyces and peaked in fruits. The polymeric cutin matrix providing the structural framework for cuticular waxes was determined to range from 81 μg cm\(^{−2}\) for N. physalodes to 571 μg cm\(^{−2}\) for A. officinarum fruits. Cuticular transpiration barriers were highly efficient, with water permeabilities being ≤5 × 10\(^{−5}\) m s\(^{−1}\). Only the cuticular water permeability of N. physalodes fruits was 10 × 10\(^{−5}\) m s\(^{−1}\) leading to their early desiccation and fruits that easily split, whereas P. peruviana, P. ixocarpa, and A. officinarum bore fleshy fruits for extended periods after maturation. Regarding the functional significance, fruiting calyces establish a physicochemical shield that reduces water loss and enables fruit maturation within a protective microclimate, and promotes different seed dispersal strategies among plant species investigated.
Sphingolipid long-chain bases (LCBs) are building blocks for membrane-localized sphingolipids, and are involved in signal transduction pathways in plants. Elevated LCB levels are associated with the induction of programmed cell death and pathogen-derived toxin-induced cell death. Therefore, levels of free LCBs can determine survival of plant cells. To elucidate the contribution of metabolic pathways regulating high LCB levels, we applied the deuterium-labeled LCB D-erythro-sphinganine-d7 (D7-d18:0), the first LCB in sphingolipid biosynthesis, to Arabidopsis leaves and quantified labeled LCBs, LCB phosphates (LCB-Ps), and 14 abundant ceramide (Cer) species over time. We show that LCB D7-d18:0 is rapidly converted into the LCBs d18:0P, t18:0, and t18:0P. Deuterium-labeled ceramides were less abundant, but increased over time, with the highest levels detected for Cer(d18:0/16:0), Cer(d18:0/24:0), Cer(t18:0/16:0), and Cer(t18:0/22:0). A more than 50-fold increase of LCB-P levels after leaf incubation in LCB D7-d18:0 indicated that degradation of LCBs via LCB-Ps is important, and we hypothesized that LCB-P degradation could be a rate-limiting step to reduce high levels of LCBs. To functionally test this hypothesis, we constructed a transgenic line with dihydrosphingosine-1-phosphate lyase 1 (DPL1) under control of an inducible promotor. Higher expression of DPL1 significantly reduced elevated LCB-P and LCB levels induced by Fumonisin B1, and rendered plants more resistant against this fungal toxin. Taken together, we provide quantitative data on the contribution of major enzymatic pathways to reduce high LCB levels, which can trigger cell death. Specifically, we provide functional evidence that DPL1 can be a rate-limiting step in regulating high LCB levels.
For the treatment of large bone defects, the commonly used technique of autologous bone grafting presents several drawbacks and limitations. With the discovery of the bone-inducing capabilities of bone morphogenetic protein 2 (BMP2), several delivery techniques were developed and translated to clinical applications. Implantation of scaffolds containing adsorbed BMP2 showed promising results. However, off-label use of this protein-scaffold combination caused severe complications due to an uncontrolled release of the growth factor, which has to be applied in supraphysiological doses in order to induce bone formation. Here, we propose an alternative strategy that focuses on the covalent immobilization of an engineered BMP2 variant to biocompatible scaffolds. The new BMP2 variant harbors an artificial amino acid with a specific functional group, allowing a site-directed covalent scaffold functionalization. The introduced artificial amino acid does not alter BMP2′s bioactivity in vitro. When applied in vivo, the covalently coupled BMP2 variant induces the formation of bone tissue characterized by a structurally different morphology compared to that induced by the same scaffold containing ab-/adsorbed wild-type BMP2. Our results clearly show that this innovative technique comprises translational potential for the development of novel osteoinductive materials, improving safety for patients and reducing costs.
Xylem embolism resistance has been identified as a key trait with a causal relation to drought-induced tree mortality, but not much is known about its intra-specific trait variability (ITV) in dependence on environmental variation. We measured xylem safety and efficiency in 300 European beech (Fagus sylvatica L.) trees across 30 sites in Central Europe, covering a precipitation reduction from 886 to 522 mm year−1. A broad range of variables that might affect embolism resistance in mature trees, including climatic and soil water availability, competition, and branch age, were examined. The average P50 value varied by up to 1 MPa between sites. Neither climatic aridity nor structural variables had a significant influence on P50. However, P50 was less negative for trees with a higher soil water storage capacity, and positively related to branch age, while specific conductivity (Ks) was not significantly associated with either of these variables. The greatest part of the ITV for xylem safety and efficiency was attributed to random variability within populations. We conclude that the influence of site water availability on P50 and Ks is low in European beech, and that the high degree of within-population variability for P50, partly due to variation in branch age, hampers the identification of a clear environmental signal.
Flowering plants or angiosperms have developed a fertilization mechanism that involves a female egg and central cell, as well as two male sperm cells. A male gametophyte carries the two non-mobile sperm cells, as they need to be delivered to the female gametophyte, the embryo sac. This transport is initiated by a pollen grain that is transmitted onto the stigma of the angiosperm flower. Here it hydrates, germinates, and forms a pollen tube, which navigates through the female plant tissue towards the ovary. The pollen tube grows into an ovule through the funiculus and into one of the two synergid cells. There, growth arrests and the pollen tube bursts, releasing the two sperm cells. One of the sperm cells fuses with the egg cell, giving rise to the embryo, the other one fuses with the central cell, developing into the endosperm, which nourishes the embryo during its development. After a successful fertilization, each ovule develops into a seed and a fruit is formed. This usually consists of several fertilized ovules.
The directional growth of the pollen tube through the maternal tissues towards the ovule, as well as sperm cell release, requires a complex communication between the male and the female gametophyte to achieve reproductive success. Over the last years many studies have been performed, contributing to the understanding of cell-cell communication events between the two gametophytes, nevertheless still many aspects remain to be elucidated.
This work focused on two topics: i.) Analysis of biological processes affected by pollination and fertilization in the Nicotiana tabacum flower and identification of cysteine rich proteins (CRPs) expressed via isolating and sequencing RNA from the tissue and analyzing the resulting data. ii.) Identification of the defensin-like protein (DEFL) responsible for pollen tube attraction towards the ovule in tobacco.
First, tissue samples of pollen tubes and mature ovules were taken at different stages of the fertilization process (unpollinated ovules, after pollination, and after fertilization of the flower). RNA was then isolated and a transcriptome was created. The resulting reads were assembled and transcriptome data analysis was performed. Results showed that pollen tubes and mature ovules differ severely from each other, only sharing about 23 % of the transcripts, indicating that different biological processes are dominant in the two gametophytes. A MapMan analysis revealed that in the pollen tube the most relevant biological processes are related to the cell wall, signaling, and transport, which supports the fact that the pollen tube grows fast to reach the ovule. On the other hand, in the ovule the values of highest significance were obtained for processes related to protein synthesis and regulation. Upon comparing the transcripts in the ovule before and after pollination, as well as after fertilization, it showed that pollination of the flower causes a bigger alteration in the ovule on the transcriptomic level compared to the step from pollination to fertilization.
A total of 953 CRPs were identified in Nicotiana tabacum, including 116 DEFLs. Among those, the peptide responsible for pollen tube attraction towards the ovule should be found. Based on in-silico analysis four candidate peptides were chosen for further analysis, two of which had increased expression levels upon pollination and fertilization and the other two displayed an opposite expression. Quantitative real time PCR experiments were performed for the candidates, confirming the in-silico data in vivo.
The candidate transcripts were then expressed in a cell free system and applied to pollen tubes in order to test their effect on the growing cells. Positive controls were used, where pollen tubes grew towards freshly dissected ovules. The four candidates did not provoke a pollen tube attraction towards the peptide, leaving open the chance to work on the 112 remaining DEFLs in the future.
Reaktive elektrophile Spezies-Oxylipine (RES-Oxylipine) finden sich in Pflanzen- und Tierzellen und zeichnen sich durch eine für sie typische Anordnung von Atomen aus: einer α,β ungesättigten Carbonyl Gruppe. In Pflanzenzellen gehören unter anderem 2-(E)-Hexenal und die Vorstufe der Jasmonsäure 12-Oxophytodiensäure (OPDA) zu den RES-Oxylipinen, in Tierzellen z.B. Prostaglandin A1 (PGA). RES-Oxylipine üben Signalfunktionen aus, wie dies in Pflanzenzellen funktioniert ist jedoch noch nicht bekannt. Ziel dieser Arbeit ist dabei einen möglichen RES-Oxylipin Signalweg aufzuklären und die beteiligten Gene zu identifizieren. Es konnte aber gezeigt werden, dass die Expressionsrate von bestimmten Genen wie z.B. GST6 durch RES-Oxylipine spezifisch induziert wird. Zur Untersuchung des RES-Oxylipin Signalweges wurde der GST6 Promotor vor das Luciferase-Gen fusioniert, um so ein RES-Oxylipin spezifisches Reportersystem zu erhalten. Die Ethylmethansulfonat mutagenisierten Linien wurden auf geänderte Luciferase-Aktivität hin untersucht. Dabei wurden drei Mutanten isoliert, die in dieser Arbeit näher untersucht wurden. Eine zeigte basal erhöhte Luciferase-Aktivität (constitutive overexpresser 3 = coe3) und die anderen beiden erniedrigte Luciferase-Aktivität nach PGA Gabe (non responsive 1 und 2 = nr1 und nr2). In dieser Arbeit konnte gezeigt werden, dass die Phänotypen in allen 3 Mutanten rezessiv vererbt werden und die Mutanten nicht zueinander allel sind. Zudem war die veränderte Luciferase-Aktivität nicht durch geänderte Phytohormonspiegel oder durch Mutationen im GST6 Promotor erklärbar. Auf die Gabe von RES, wie Benzylisothiocyanat oder Sulforaphan, sowie auf endogene RES-Oxylipine, wie OPDA und Hexenal, reagierten die Mutanten auf ähnliche Weise, wie nach PGA Gabe. Weiterführende Untersuchungen zeigten, dass sich die drei Mutanten stark voneinander unterschieden. Das Transkriptom kontrollbehandelter coe3 Pflanzen unterschied sich stark von dem der GST6::LUC Pflanzen. Die Mutante war trockenstressresistenter zudem war sie sensibler gegenüber NaCl, was jedoch nicht von einer veränderten Reaktion auf Abscisinsäure herrührte. Des Weiteren war der Chlorophyllabbau bei dunkel inkubierten Blättern geringer. Bei der Lokalisierung der Mutation, die noch nicht abgeschlossen ist, konnten Chromosom 2 und 5 als die wahrscheinlichsten Kandidaten ermittelt werden. Weitere Analysen sind nötig um den Bereich weiter eingrenzen zu können. Die Mutante nr1, die sich durch verminderte Reaktion auf RES-Oxylipine auszeichnete, zeigte einen kleineren Wuchs und ein deutlich verzögertes Blühen. Außerdem wies die Mutante erhöhte Argininspiegel in ihren Blättern auf. Das Transkriptom unterschied sich sowohl bei kontrollbehandelten, als auch bei PGA behandelten nr1 Pflanzen massiv von denen der gleichbehandelten Kontrollen. Auch die nr1 schien trockenstressresistenter zu sein, sie war im Gegensatz zur coe3 aber robuster gegenüber höheren Konzentrationen an NaCl. Mit Hilfe eines „Next Generation Genome-Mappings“ war es möglich die Mutation am Ende von Chromosom 3 zu lokalisieren und auf fünf mögliche Gene einzugrenzen. Weitere Untersuchungen müssen nun klären, welches dieser Gene ursächlich für den Phänotyp der geänderten Luciferase-Aktivität ist. Die zweite Mutante mit einer reduzierten Reaktion auf RES-Oxylipine war die nr2. Überraschender Weise unterschied sich das Transkriptom kontrollbehandelter nr2 Pflanzen deutlich stärker von dem der gleichbehandelten GST6::LUC Pflanzen, als das nach PGA Gabe der Fall war. Sie reagierte nur mit sehr schwacher Luciferase-Aktivität auf Verwundung und war zudem deutlich sensibler gegenüber Trockenheit. Für eine zukünftige Lokalisation der ursächlichen Mutation wurden entsprechende Kreuzungen durchgeführt aus deren Samen jederzeit mit einer Selektionierung begonnen werden kann. Mit dieser Arbeit konnte ein erster großer Schritt in Richtung Identifikation der, für die geänderte Luciferase-Aktivität, verantwortlichen Mutation gemacht werden, sowie erste Reaktionen der Mutanten auf abiotische Stressfaktoren untersucht werden. Somit ist man der Entdeckung von Signaltransduktionsfaktoren, die RES-Oxylipinabhängig reguliert werden, einen wichtigen Schritt näher gekommen.
Design of novel IL-4 antagonists employing site-specific chemical and biosynthetic glycosylation
(2021)
The cytokines interleukin 4 (IL-4) and IL-13 are important mediators in the humoral immune response and play a crucial role in the pathogenesis of chronic inflammatory diseases, such as asthma, allergies, and atopic dermatitis. Hence, IL-4 and IL-13 are key targets for treatment of such atopic diseases.
For cell signalling IL-4 can use two transmembrane receptor assemblies, the type I receptor consisting of receptors IL-4R and γc, and type II receptor consisting of receptors IL-4R and IL-13R1. The type II receptor is also the functional receptor of IL-13, receptor sharing being the molecular basis for the partially overlapping effects of IL-4 and IL-13. Since both cytokines require the IL-4R receptor for signal transduction, this allows the dual inhibition of both IL-4 and IL-13 by specifically blocking the receptor IL-4R.
This study describes the design and synthesis of novel antagonistic variants of human IL-4. Chemical modification was used to target positions localized in IL-4 binding sites for γc and IL-13R1 but outside of the binding epitope for IL-4R. In contrast to existing studies, which used synthetic chemical compounds like polyethylene glycol for modification of IL-4, we employed glycan molecules as a natural alternative. Since glycosylation can improve important pharmacological parameters of protein therapeutics, such as immunogenicity and serum half-life, the introduced glycan molecules thus would not only confer a steric hindrance based inhibitory effect but simultaneously might improve the pharmacokinetic profile of the IL-4 antagonist.
For chemical conjugation of glycan molecules, IL-4 variants containing additional cysteine residues were produced employing prokaryotic, as well as eukaryotic expression systems. The thiol-groups of the engineered cysteines thereby allow highly specific modification. Different strategies were developed enabling site-directed coupling of amine- or thiol- functionalized monosaccharides to introduced cysteine residues in IL-4. A linker-based coupling procedure and an approach requiring phenylselenyl bromide activation of IL-4 thiol-groups were hampered by several drawbacks, limiting their feasibility. Surprisingly, a third strategy, which involved refolding of IL-4 cysteine variants in the presence of thiol- glycans, readily allowed synthesis of IL-4 glycoconjugates in form of mixed disulphides in milligram amount. This approach, therefore, has the potential for large-scale synthesis of IL-4 antagonists with highly defined glycosylation. Obtaining a homogenous glycoconjugate with exactly defined glycan pattern would allow using the attached glycan structures for fine-tuning of pharmacokinetic properties of the IL-4 antagonist, such as absorption and metabolic stability.
The IL-4 glycoconjugates generated in this work proved to be highly effective antagonists inhibiting IL-4 and/or IL-13 dependent responses in cell-based experiments and in in vitro binding studies. Glycoengineered IL-4 antagonists thus present valuable alternatives to IL-4 inhibitors used for treatment of atopic diseases such as the neutralizing anti-IL-4R antibody Dupilumab.
Arid environments cover almost one-third of the land over the world. Plant life in hot arid regions is prone to the water shortage and associated high temperatures. Drought-stressed plants close the stomata to reduce water loss. Under such conditions, the remaining water loss exclusively happens across the plant cuticle. The cuticular water permeability equals the minimum and inevitable water loss from the epidermal cells to the atmosphere under maximally stomatal closure. Thus, low cuticular water permeability is primordial for plant survival and viability under limited water source. The assumption that non-succulent xerophytes retard water loss due to the secretion of a heavier cuticle is often found in the literature. Intuitively, this seems to be plausible, but few studies have been conducted to evaluate the cuticular permeability of xerophilous plants. In chapter one, we investigated whether the cuticular permeability of Quercus coccifera L. grown in the aridest Mediterranean-subtype climate is indeed lower than that of individuals grown under temperate climate conditions. Also, the cuticular wax chemical compositions of plants grown in both habitats were qualitatively and quantitatively analysed by gas-chromatography. In few words, our findings showed that although the cuticular wax deposition increased in plants under Mediterranean climate, the cuticular permeability remained unaltered, regardless of habitat.
The associated high temperatures in arid regions can drastically increase the cuticular water permeability. Thereby, the thermal stability of the cuticular transpirational barrier is decisive for safeguarding non-succulent xerophytes against desiccation. The successful adaptation of plants to hot deserts might be based on finding different solutions to cope with water and heat stresses. Water-saver plants close the stomata before the leaf water potential drastically changes in order to prevent damage, whereas water-spender plants reduce the leaf water potential by opening the stomata, which allow them to extract water from the deep soil to compensate the high water loss by stomatal transpiration. In chapter two, we compare the thermal stability of the cuticular transpiration barrier of the desert water-saver Phoenix dactylifera L. and the water-spender Citrullus colocynthis (L.) Schrad. In short, the temperature-dependent increase of the cuticular permeability of P. dactylifera was linear over the whole temperature range (25-50°C), while that of C. colocynthis was biphasic with a steep increase at temperatures ≥ 40°C. This drastic increase of cuticular permeability indicates a thermally induced breakdown of the C. colocynthis cuticular transpiration barrier, which does not occur in P. dactylifera. We further discussed how the specific chemical composition of the cutin and cuticular waxes might contribute to the pronounced thermal resistance of the P. dactylifera cuticular transpiration barrier.
A multitude of morpho and physiological modifications, including photosynthetic thermal tolerance and traits related to water balance, led to the successful plant colonisation of hot arid regions over the globe. High evaporative demand and elevated temperatures very often go along together, thereby constraining the plant life in arid environments. In chapter 3, we surveyed cuticular permeability, leaf thermal tolerance, and cuticular wax chemical composition of 14 non-succulent plant species native from some of the hottest and driest biomes in South-America, Europe, and Asia. Our findings showed that xerophilous flowering plants present high variability for cuticular permeability and leaf thermal tolerance, but both physiological features could not be associated with the species original habitat. We also provide substantial evidence that non-succulent xerophytes with more efficient cuticular transpirational barrier have higher leaf thermal tolerance, which might indicate a potential coevolution of these features in hot arid biomes. We further discussed the efficiency of the cuticular transpiration barrier in function to the cuticular wax chemical composition in the general discussion section.
Die wahrscheinlich größten Probleme des 21. Jahrhunderts sind der Klimawandel und die Sicherstellung der Nahrungsmittelversorgung für eine steigende Zahl an Menschen. Durch die Zunahme von extremen Wetterbedingungen wie Trockenheit und Hitze wird der Anbau konventioneller, wenig toleranter Nutzpflanzen erschwert und die dadurch notwendige, steigende Bewässerung der Flächen führt darüber hinaus zu einer zusätzlichen Versalzung der Böden mit für Pflanzen toxischen Natrium- und Chlorid-Ionen. Kenntnisse über Anpassungsstrategien salztoleranter Pflanzen an Salzstress, aber auch detailliertes Wissen über die Steuerung der Transpiration und damit des Wasserverlusts von Pflanzen sind daher wichtig, um auch künftig ertragreiche Landwirtschaft betreiben zu können. In dieser Arbeit habe ich verschiedene Aspekte der pflanzlichen Stressphysiologie bearbeitet, die im Folgenden getrennt voneinander zusammengefasst werden.
I. Funktionelle Unterschiede der PYR/PYL-Rezeptoren von Schließzellen
Entscheidend für den Wasserstatus von Pflanzen ist die Kontrolle des Wasserverlusts durch Spaltöffnungen (Stomata), die von einem Paar Schließzellen gebildet werden. Externe Faktoren wie Licht, Luftfeuchtigkeit und CO2, sowie interne Faktoren wie das Phytohormon Abszisinsäure (ABA) regulieren über Signalkaskaden die Stomaweite und dadurch den Wasserverlust. Die zugrunde liegenden Signalkaskaden überlappen teilweise. Vor allem der Stomaschluss durch erhöhtes CO2 und ABA weisen viele Gemeinsamkeiten auf und die Identifizierung des Konvergenzpunktes beider Signale ist immer noch aktueller Gegenstand der Forschung. Von besonderem Interesse sind dabei die in Schließzellen exprimierten ABA-Rezeptoren der PYR/PYL-Familie. Denn obwohl bislang nicht nachgewiesen werden konnte, dass CO2 zu einem Anstieg des ABA-Gehalts von Schließzellen führt deuten einige Studien darauf hin, dass die ABA-Rezeptoren selbst am CO2-Signalweg beteiligt sind.
Durch Untersuchungen der Stomareaktion von Arabidopsis ABA-Rezeptormutanten konnte ich in dieser Arbeit zeigen, dass die in Schließzellen exprimierten ABA-Rezeptoren der PYR/PYL-Familie funktionale Unterschiede aufweisen. Fünffach-Verlustmutanten der ABA-Rezeptoren PYR1, PYL2, 4, 5 und 8 (12458) waren in ihrem ABA-induzierten Stomaschluss beeinträchtigt und nur die Komplementation mit PYL2 und in geringerem Maße PYR1 konnte die ABA-Sensitivität wiederherstellen. Die Stomata von 12458-Verlustmutanten waren außerdem insensitiv gegenüber erhöhtem CO2, was auf eine Beteiligung der ABA-Rezeptoren am CO2-induzierten Stomaschluss hindeutet und diese Sensitivität konnte nur durch die Komplementation mit PYL4 oder PYL5, nicht aber mit PYL2 wiederhergestellt werden. Somit konnten in dieser Arbeit erstmals funktionelle Unterschiede der PYR/PYLs beim Stoma-Schluss nachgewiesen werden.
Alle externen und internen Stomaschluss-Signale haben außerdem Einfluss auf die Genexpression der Schließzellen und führen zu individuellen expressionellen Adaptionen. In vorangegangenen Microarray Studien konnte gezeigt werden, dass jeder Stimulus auch die Expression eines distinkten Sets an ABA-Rezeptoren beeinflusst. Im Rahmen dieser Arbeit konnte ich außerdem zeigen, dass die Expression der ABA-Rezeptoren bereits auf kleine Änderungen der ABA-Konzentration der Schließzellen reagiert und dass diese sich außerdem in ihrer Sensitivität gegenüber ABA unterschieden. Geringe Änderungen der ABA-Konzentration von Schließzellen haben demnach Auswirkungen auf deren Rezeptor-zusammensetzung. Darüber hinaus konnte ich zeigen, dass die Rezeptoren die Expression unterschiedlicher nachgeschalteter Gene beeinflussen, was darauf hindeutet, dass Anpassungen des Rezeptorpools durch geringe Änderungen des ABA-Gehalts von Schließzellen schlussendlich auf genexpressioneller Ebene zur längerfristigen Adaption an externe Bedingungen führen und die Rezeptoren auch hier funktional verschieden sind.
II. Stomatäre Besonderheiten der toleranten Dattelpalme (Phoenix dactylifera)
Dattelpalmen kommen natürlicherweise an besonders trockenen und heißen Standorten vor, an denen es aufgrund der harschen Bedingungen nur sehr wenigen Pflanzen möglich ist überhaupt zu wachsen. Ein naheliegender Grund für die herausragende Toleranz dieser Art gegenüber wasserlimitierenden Bedingungen ist eine Anpassung der stomatären Regulation zu Gunsten des Wasserhaushalts.
In dieser Arbeit konnte ich durch vergleichende Untersuchungen der lichtabhängigen Transpiration sowie dem ABA-induzierten Stomaschluss grundlegende Unterschiede in der Stomaphysiologie der Dattelpalmen und der eher sensitiven Modellpflanze Arabidopsis thaliana nachweisen. Blattgaswechselmessungen zeigten, dass Dattelpalmen in der Lage sind die Spaltöffnungen bei niedrigen Lichtintensitäten, bei denen Arabidopsis bereits deutlich geöffnete Stomata aufwies, geschlossen zu halten. Der bedeutendste Unterschied in der Stomaphysiologie von Dattelpalmen und Arabidopsis lag aber im ABA-induzierten Stomaschluss. Während über die Petiole verabreichtes ABA bei Arabidopsis innerhalb von 15 Minuten zu einem vollständigen Stomaschluss führte, konnte ich in dieser Arbeit zeigen, dass der ABA-induzierte Stomaschluss der Datteln nitratabhängig ist. ABA allein führte nur zu einem sehr langsamen Stomaschluss der innerhalb einer Stunde nicht vollständig abgeschlossen war. Nur in Gegenwart von Nitrat führte die ABA-Gabe in den Transpirationsstrom der Fiederblätter der Datteln zu einem schnellen und vollständigen Stomaschluss. In Arabidopsis wird der in Schließzellen vorkommende Anionenkanal AtSLAC1 durch eine über den ABA-Signalweg vermittelte Phosphorylierung aktiviert, was schlussendlich zur Aktivierung spannungsabhängiger Kationenkanäle und zum Ausstrom von Kalium aus den Schließzellen führt. Es konnte gezeigt werden, dass die Nitratabhängigkeit der ABA-Antwort der Schließzellen von Dattelpalmen auf Eigenschaften von PdSLAC1 zurückzuführen ist und dieser Kanal nur in Anwesenheit von extrazellulärem Nitrat aktivierbar ist. Mittlerweile konnte, unter anderem basierend auf diesen Ergebnissen, eine Tandem-Aminosäuresequenz identifiziert werden, die die SLAC-Homologe monokotyler Pflanzen wie der Dattelpalme von der dikotyler Pflanzen unterscheidet und zumindest teilweise für die nitratabhängige Aktivierung des Stomaschlusses vieler monokotyler verantwortlich ist.
III. Die Salztoleranz von Phoenix dactylifera und Chenopodium quinoa
Sowohl Dattelpalmen als auch C. quinoa weisen, verglichen mit den meisten anderen Pflanzen, eine hohe Toleranz gegenüber NaCl-haltigen Böden auf. In dieser Arbeit habe ich die Salztoleranz beider Arten untersucht, um so Strategien zu identifizieren, die diesen Pflanzen diese gesteigerte Toleranz ermöglichen.
Dattelpalmen können natürlicherweise auf salzigen Böden wachsen. Makroskopisch weisen diese Pflanzen aber keine Anpassungen wie bspw. Salzdrüsen auf und bislang ist unklar wie Dattelpalmen mit dem NaCl aus dem Boden umgehen. In dieser Arbeit konnte ich zeigen, dass der Natriumgehalt der Fiederblätter der Datteln durch eine sechswöchige Bewässerung mit 600mM NaCl, was ungefähr der Konzentration von Meerwasser entspricht, nicht zunimmt. Demnach sind Datteln so genannte „Exkluder“, also Pflanzen, die eine übermäßige Natriumaufnahme in photosynthetisch aktives Gewebe vermeiden. Der Natriumgehalt der Wurzeln dagegen nahm unter Salzstress aber zu. Diese Zunahme war allerdings in unterschiedlichen Bereichen der Wurzeln verschieden stark. Flammenphotometrische Messungen ergaben einen vom Wurzelansatz ausgehenden graduellen Anstieg des Natriumgehalts, der an der Wurzelspitze am höchsten war. Darüber hinaus konnte eine Induktion von PdSOS1, einem putativen Na+/H+-Antiporter in diesen unteren, natriumhaltigen Bereichen nachgewiesen werden. Eine hohe SOS1-Aktivität gilt bereits in anderen toleranten Arten als Schlüsselmerkmal für deren Toleranz und die gesteigerte Expression von PdSOS1 deutet auf eine erhöhte Natrium-Exportrate aus der Wurzel zurück in den Boden in diesen unteren Bereichen hin, was schlussendlich den Ausschluss von Natrium vermitteln könnte.
In sensitiven Arten führt Salzstress häufig zu einer Abnahme der Kaliumkonzentration des Gewebes. Interessanterweise war dies weder für das Blatt- noch das Wurzelgewebe der Dattelpalmen der Fall. Der Kaliumgehalt beider Gewebe blieb trotz der Bewässerung der Pflanzen mit Salzwasser konstant. Auf expressioneller Ebene konnte ich darüber hinaus zeigen, dass PdHAK5, ein putativer hochaffiner Kaliumtransporter, der unter Kontrollbedingungen überwiegend in den oberen Wurzelabschnitten exprimiert wurde, durch den Salzstress dort reprimiert wurde. PdKT, ebenfalls ein putatives Kalium-Transportprotein dagegen, wurde nicht durch die Salzbehandlung beeinflusst, was zusammengenommen darauf hindeutet, dass das Aufrechterhalten des Kaliumgehalts bei Salzstress durch die differentielle Regulation verschiedener Kaliumaufnahmesysteme gewährleistet wird. Der effiziente Ausschluss von Natrium zusammen mit dem hohen K+/Na+-Verhältnis könnten demnach Schlüsselmerkmale für die hohe Salztoleranz von Phoenix dactylifera darstellen.
Quinoa ist, ähnlich wie die Dattelpalme, eine salztolerante Nutzpflanze. Im Gegensatz zu Dattelpalmen weist Quinoa allerdings besondere Strukturen auf der Epidermis auf, die so genannten epidermalen Blasenhaare (englisch: epidermal bladder cells, EBCs). Die Funktion dieser ballonartig vergrößerten Zellen als externe Salzspeicher wird seit längerem diskutiert.
Flammenphotometrische Messungen des Natriumgehalts von Quinoa unter Salzstressbedingungen ergaben, dass Quinoa anders als Dattelpalmen, Natrium in die oberirdischen, photosynthetisch aktiven Organe aufnimmt. Auch die Zunahme des Natriumgehalts der EBCs konnte ich nachweisen. Junge Blätter haben eine hohe Dichte an intakten EBCs, was deren Funktion als externe Salzspeicher besonders zum Schutz dieser jungen Blätter nahelegt. mRNA-Sequenzierungen ergaben darüber hinaus, dass die EBCs bereits unter Kontrollbedingungen viele in grundlegende Stoffwechselprozesse involvierte Gene sowie membranständige Transportproteine differentiell exprimieren. Diese Unterschiede im Transkriptom der EBCs zum Blattgewebe zeigen, dass katabole Stoffwechselwege nur eine untergeordnete Rolle in den hochspezialisierten EBCs spielen und deren Stoffwechsel auf dem Import energiereicher Zucker und Aminosäuren basiert.
Mittels qPCR-Messungen und RNA-Sequenzierungen konnte ich die gewebespezifische Expression verschiedener Transportproteine nachweisen, die eine gerichtete Aufnahme von Natrium in EBCs ermöglichen könnten. Besonders die differentielle Expression eines Natriumkanals der HKT1-Familie deutet auf dessen Beteiligung an der Natriumbeladung der EBCs hin. CqHKT1.2 wurde ausschließlich in EBCs exprimiert und die elektrophysiologische Charakterisierung dieses Transportproteins ergab eine spannungsabhängige Natriumleitfähigkeit. Dieser Natriumkanal kann demnach die Natriumaufnahme bei Membranspannungen nahe dem Ruhepotential in die EBCs vermitteln und die Deaktivierung des CqHKT1.2 bei depolarisierenden Membranspannungen kann darüber hinaus einen Efflux von Na+ aus den EBCs verhindern. Auch das Expressionsmuster eines putativen Na+/H+-Antiporters (CqSOS1) der nur sehr gering in EBCs aber deutlich höher in Blattgewebe exprimiert wurde, deutet auf eine indirekte Beteiligung dieses SOS1 an der Beladung der EBCs hin. Bereits charakterisierte SOS1-Proteine anderer Pflanzen zeigten unter physiologischen Bedingungen eine Natriumexport-Aktivität. CqSOS1 könnte demnach den Export von Natrium aus Mesophyll- und Epidermiszellen der Blätter in den Apoplasten vermitteln, welches dann über CqHKT1.2 in die EBCs aufgenommen wird.
Trotz der Natriumaufnahme in die oberirdischen Teile und die EBCs führte die Salzbehandlung ähnlich wie bei den Datteln nicht zu einer Abnahme des bemerkenswert hohen Kaliumgehalts. Mittels qPCR-Untersuchungen konnte ich die Expression verschiedener HAK-Orthologe nachweisen, deren Aktivität die Aufrechterhaltung des Kaliumgehalts unter Salzstress vermitteln könnten. Frühere Studien konnten zeigen, dass Salzstress bei Quinoa wie bei vielen salztoleranten Arten zu einem Anstieg der Konzentration von kompatiblen gelösten Substanzen und besonders von Prolin führt. In dieser Arbeit konnte ich die hohe Expression eines Prolintransporters in EBCs nachweisen, was eher auf einen importbasierten Anstieg der Prolinkonzentration als auf die Synthese innerhalb der EBCs schließen lässt.
Zusammengefasst ergaben der Anstieg des Natriumgehalts der EBCs in Verbindung mit den Ergebnissen der RNA-Sequenzierung und den ergänzenden qPCR Messungen, dass die EBCs von Quinoa bereits unter Kontrollbedingen für die Aufnahme von überschüssigen Ionen unter Salzstress spezialisierte Zellen sind, deren Spezialisierung auf dem Import von energiereichreichen Zucken und anderen Substanzen basiert.
The cytokine interleukin-5 (IL-5) is part of the TH2-mediated immune response. As a key regulator of eosinophilic granulocytes (eosinophils), IL-5 controls multiple aspects of eosinophil life. Eosinophils play a pathogenic role in the onset and progression of atopic diseases as well as hypereosinophilic syndrome (HES). Here, cytotoxic proteins and pro-inflammatory mediators stored in intracellular vesicles termed granula are released upon activation thereby causing local inflammation to fight the pathogen. However, if such inflammation persists, tissue damage and organ failure can occur. Due to the close relationship between eosinophils and IL-5 this cytokine has become a major pharmaceutical target for the treatment of atopic diseases or HES. As observed with other cytokines, IL-5 signals by assembling a heterodimeric receptor complex at the cell surface in a stepwise mechanism. In the first step IL-5 binds to its receptor IL-5Rα (CD125). This membrane-located complex then recruits the so-called common beta chain βc (CD131) into a ternary ligand receptor complex, which leads to activation of intracellular signaling cascades. Based on this mechanism various strategies targeting either IL-5 or IL-5Rα have been developed allowing to specifically abrogate IL-5 signaling. In addition to the classical approach of employing neutralizing antibodies against IL 5/IL-5Rα or antagonistic IL-5 variants, two groups comprising small 18 to 30mer peptides have been discovered, that bind to and block IL-5Rα from binding its activating ligand IL-5. Structure-function studies have provided detailed insights into the architecture and interaction of IL-5IL-5Rα and βc. However, structural information for the ternary IL-5 complex as well as IL-5 inhibiting peptides is still lacking.
In this thesis three areas were investigated. Firstly, to obtain insights into the second receptor activation step, i.e. formation of the ternary ligand-receptor complex IL-5•IL-5Rα•βc, a high-yield production for the extracellular domain of βc was established to facilitate structure determination of the ternary ligand receptor assembly by either X-ray crystallography or cryo-electron microscopy.
In a second project structure analysis of the ectodomain of IL-5Rα in its unbound conformation was attempted. Data on IL-5Rα in its ligand-free state would provide important information as to whether the wrench-like shaped ectodomain of IL-5Rα adopts a fixed preformed conformation or whether it is flexible to adapt to its ligand binding partner upon interaction. While crystallization of free IL-5Rα failed, as the crystals obtained did not diffract X rays to high resolution, functional analysis strongly points towards a selection fit binding mechanism for IL-5Rα instead of a rigid and fixed IL-5Rα structure. Hence IL-5 possibly binds to a partially open architecture, which then closes to the known wrench-like architecture. The latter is then stabilized by interactions within the D1-D2 interface resulting in the tight binding of IL-5.
In a third project X-ray structure analysis of a complex of the IL-5 inhibitory peptide AF17121 bound to the ectodomain of IL-5Rα was performed. This novel structure shows how the small cyclic 18mer peptide tightly binds into the wrench-like cleft formed by domains D1 and D2 of IL-5Rα. Due to the partial overlap of its binding site at IL-5Rα with the epitope for IL-5 binding, the peptide blocks IL-5 from access to key residues for binding explaining how the small peptide can effectively compete with the rather large ligand IL-5. While AF17121 and IL-5 seemingly bind to the same site at IL-5Rα, functional studies however showed that recognition and binding of both ligands differ. With the structure for the peptide-receptor complex at hand, peptide design and engineering could be performed to generate AF17121 analogies with enhanced receptor affinity. Several promising positions in the peptide AF17121 could be identified, which could improve inhibition capacity and might serve as a starting point for AF17121-based peptidomimetics that can yield either superior peptide based IL-5 antagonists or small-molecule-based pharmacophores for future therapies of atopic diseases or the hypereosinophilic syndrome.
Seit mehr als zwei Jahrzehnten ist bekannt, dass nicht nur der Tumor Nekrose Faktor-α (=TNF-α) sondern auch Lymphotoxin-α (=LTα) in Form von Trimeren an TNFR1 und TNFR2 binden kann. Durch diese Fähigkeit an beide Rezeptoren zu binden, haben diese zwei Liganden eine essentielle Rolle in der Entwicklung und dem Verlauf von Autoimmunerkrankungen. Bereits mit Beginn der 1990er Jahren wurde gezeigt, dass LTα nicht nur in Form von Homotrimeren vorliegt, sondern auch mit dem verwandten TNF-Superfamilie Liganden Lymphotoxin β (=LTβ) Heterotrimere bilden kann. Hierbei lagern sich LTα und LTβ in Form von LTα2β und LTαβ2 zusammen. Die initialen Experimente mit diesen Heterotrimeren zeigten bereits Unterschiede von LTα2β und LTαβ2. Während LTα2β wie LTα an den TNFR1 bindet, kann LTαβ2 weder an TNFR1 noch TNFR2 binden und interagiert mit einem eigenen Rezeptor namens Lymphotoxin β Rezeptor (=LTβR). Da bereits zwei Liganden (TNF und LTα) für TNFR1 und TNFR2 bekannt waren, wurde LTα2β bis heute nicht weiter charakterisiert. LTαβ2 hingegen war lange Zeit der einzige bekannte Ligand für den LTβR, weshalb die LTαβ2-LTβR-Interaktion ausführlich untersucht wurde.
Diese Arbeit fokusiert sich auf die Charakterisierung von LTα2β. Hierfür wurde die einzige bekannte Eigenschaft aus den 90er Jahren von LTα2β nämlich die Bindung an TNFR1 aufgegriffen und um die Rezeptoren TNFR2 und LTβR erweitert. Diese Arbeit zeigt, dass LTα2β nicht nur an den TNFR1, sondern auch an TNFR2 und schwach an LTβR bindet. Trotz der asymmetrischen Bindestellen kann membrangebundenes LTα2β TNFR1 und TNFR2 nicht nur binden, sondern ist auch in der Lage diese zu aktivieren. Diese Arbeit gibt erste Einblicke in die Komplexizität dieses Heterotrimers indem gezeigt wird, dass LTα2β sowohl in seiner löslichen als auch in seiner membrangebundenen Form den TNFR1 aktivieren kann, während der TNFR2 nur durch das membranständige LTα2β aktiviert wird. Aufgrund der aktivierenden Eigenschaften von membranständigem LTα2β und LTαβ2 auf die murine (=mu) Panc02-Zelllinie wird ein ersten Ausblick auf mögliche weitergehende Experimente in mausbasierten Modellen gegeben. Die erzielten Ergebnisse zeigen, dass mit membranständigem LTα2β ein neuer TNFR2 Agonist gefunden wurde.
Soil salinity is an increasingly global problem which hampers plant growth and crop yield. Plant productivity depends on optimal water-use efficiency and photosynthetic capacity balanced by stomatal conductance. Whether and how stomatal behavior contributes to salt sensitivity or tolerance is currently unknown. This work identifies guard cell-specific signaling networks exerted by a salt-sensitive and salt-tolerant plant under ionic and osmotic stress conditions accompanied by increasing NaCl loads.
We challenged soil-grown Arabidopsis thaliana and Thellungiella salsuginea plants with short- and long-term salinity stress and monitored genome-wide gene expression and signals of guard cells that determine their function.
Arabidopsis plants suffered from both salt regimes and showed reduced stomatal conductance while Thellungiella displayed no obvious stress symptoms. The salt-dependent gene expression changes of guard cells supported the ability of the halophyte to maintain high potassium to sodium ratios and to attenuate the abscisic acid (ABA) signaling pathway which the glycophyte kept activated despite fading ABA concentrations.
Our study shows that salinity stress and even the different tolerances are manifested on a single cell level. Halophytic guard cells are less sensitive than glycophytic guard cells, providing opportunities to manipulate stomatal behavior and improve plant productivity.
The role of lipid transfer proteins (LTPs) during the fertilization process in Arabidopsis thaliana
(2021)
Double fertilization is a defining characteristic of flowering plants (angiosperms). As the sperm cells of higher plants are non-motile, they need to be transported to the female gametophyte via the growing pollen tube. The pollen-tube journey through the female tissues represents a highly complex process. To provide for successful reproduction it demands intricate communication between the cells of the two haploid gametophytes - the polar growing pollen tube (carrying the two non-motile sperm cells) and the ovule (hosting the egg cell/synergid cells). The polar growth of the pollen tube towards the female gamete is guided by different signaling molecules, including sugars, amino acids and peptides. Some of these belong to the family of lipid transfer proteins (LTPs), which are secreted cysteine-rich peptides. Depending on the plant species several lines of evidence have also suggested potential roles for LTPs during pollen germination or pollen-tube guidance. Although Arabidopsis thaliana has 49 annotated genes for LTPs, several of which are involved in plant immunity and cell-to-cell communication, the role of most members of this family during fertilization is unknown.
The aim of this project was therefore to systematically identify LTPs which play a role in the fertilization process in A. thaliana, particularly during pollen tube guidance. To identify candidate proteins, the expression profile of LTPs in reproductive tissue was investigated. This was accomplished by in-silico bioinformatic analysis using different expression databases. Following confirmion of these results by qRT-PCR analysis, seven Type-I nsLTPs (LTP1, LTP2, LTP3, LTP4, LTP5, LTP6 and LTP12) were found to be exclusively expressed in pistils. Except for LTP12, all other pistil expressed LTPs were transcriptionally induced upon pollination. Using reporter-based transcriptional and translational fusions the temporal and spatial expression patterns together with protein localizations for LTP2, 3, 4, 5, 6, and 12 were determined in planta. Stable transgenic plants carrying PromLTP::GUS constructs of the six different LTP candidates showed that most of LTPs were expressed in the stigma/stylar region and were induced upon pollination. With respect to protein localization on the cellular level, they split into two categories: LTP2, LTP5 and LTP6 were localized in the cell wall, while LTP3, LTP4 and LTP12 were specifically targeted to the plasma membrane.
For the functional characterization of the candidate LTPs, several T-DNA insertion mutant plant lines were investigated for phenotypes affecting the fertilization process. Pollen development and quality as well as their in-vitro germination rate did not differ between the different single ltp mutant lines and wildtype plants. Moreover, in-vivo cross pollination experiments revealed that tube growth and fertilization rate of the mutant plants were similar to wildtype plants. Altogether, no discernible phenotype was evident in other floral and vegetative parts between different single ltp mutant lines and wildtype plants. As there was no distinguishable phenotype observed for single ltp-ko plants, double knock out plants of the two highly homologous genes LTP2 (expressed in the female stigma, style and transmitting tract) and LTP5 (expressed in the stigma, style, pollen pollen-tube and transmitting tract) were generated using the EPCCRISPR-Cas9 genome editing technique. Two ltp2ltp5 mutant transgenic-lines (#P31-P2 and #P31-P3) with frameshift mutations in both the genes could be established. Further experiments showed, that the CRISPR/Cas9-mediated knock-out of LTP2/LTP5 resulted in significantly reduced fertilization success. Cell biological analyses revealed that the ltp2ltp5 double mutant was impaired in pollen tube guidance towards the ovules and that this phenotype correlated with aberrant callose depositions in the micropylar region during ovule development. Detailed analysis of in-vivo pollen-tube growth and reciprocal cross pollination assay suggested that, the severely compromised fertility was not caused by any defect in development of the pollen grains, but was due to the abnormal callose deposition in the embryo sac primarily concentrated at the synergid cell near the micropylar end. Aberrant callose deposition in ltp2ltp5 ovules pose a complete blockage for the growing pollen tube to change its polarity to enter the funiculus indicating funicular and micropylar defects in pollen tube guidance causing fertilization failure.
Our finding suggests that female gametophyte expressed LTP2 and LTP5 play a crucial role in mediating pollen tube guidance process and ultimately having an effect on the fertilization success. In line with the existence of a N-terminal signal peptide, secreted LTPs might represent a well-suited mobile signal carrier in the plant’s extracellular matrix. Previous reports suggested that, LTPs could act as chemoattractant peptide, imparting competence to the growing pollen tube, but the molecular mechanism is still obscure. The results obtained in this thesis further provide strong evidence, that LTP2/5 together regulate callose homeostasis and testable models are discussed. Future work is now required to elucidate the detailed molecular link between these LTPs and their potential interacting partners or receptors expressed in pollen and synergid cells, which should provide deeper insight into their functional role as regulatory molecules in the pollen tube guidance mechanism.
The cuticle is constituted of the biopolymer cutin and intra- and epicuticular waxes. In some cases, it has epicuticular wax crystals, protruding from the epicuticular wax film. One of the most important tasks is protection against desiccation. Many investigations were conducted to find the transport limiting component of the cuticle. It is evidentially confirmed that the waxes form this barrier. These waxes are multifactorial blends made of very-long-chain aliphatic (VLCA) compounds and triterpenoids (TRP). The VLCAs were proposed to constitute the transpiration barrier to water. However, experimental confirmation was lacking so far. The present study focuses on the development of a method to selectively extract TRPs from the cuticle and the impact of the removal on the transpiration barrier.
The plants deployed in this study exhibited several features. They had no epicuticular crystals on their surfaces, were astomatous, had a rather durable and possibly isolatable cuticle. A broad range of wax compositions was covered from plants with no TRP content and low wax load like Hedera helix and Zamioculcas zamiifolia to plants with high TRP content and high wax load like Nerium oleander. The selective extraction was conducted using a sequence of solvents. TRPs were extracted almost exhaustively from CMs with the first MeOH extract. Only a minor amount of shorter chained VLCAs was obtained. The remaining waxes, consisting mostly of VLCAs and some remnant TRPs, were removed with the following TCM extract.
After the extractions, the water permeance of native cuticular membranes (CM), MeOH extracted (M) and dewaxed cuticular discs (MX) was investigated gravimetrically. Compared to the water permeance of CMs, Ms showed no or only a small increase in water conductance. MXs, however, always showed strongly increased values.
The knowledge about the wax compounds constituting the transport-limiting properties is vital for different projects. For various issues, it would be favourable to have a standardized wax mixture as an initial point of research. It could be used to develop screening procedures to investigate the impact of adjuvants on cuticular waxes or the influence of wax constituents on the properties of cuticular waxes. This work concentrated on the development of an artificial wax mixture, which mimics the physical properties of a plant leaf wax sufficiently.
As target wax, the leaf wax of Schefflera elegantissima was chosen. The wax of this plant species consisted almost exclusively of VLCAs, had a rather simple composition regarding compound classes and chain length distribution and CMs could be isolated. Artificial binary, ternary and quaternary waxes corresponding to the conditions within the plant wax were investigated using differential scanning calorimetry (DSC), X-ray diffraction (XRD) techniques and Fourier-transform infrared (FTIR) spectroscopy. Phase diagrams were mapped out for a series of binary, ternary and quaternary wax mixtures. FTIR experiments were conducted using, ternary and a quaternary artificial wax blends. The blends were chosen to represent the conditions within the wax of the adaxial CM plant wax. The FTIR experiments exhibited an increasing resemblance of the artificial wax to the plant wax (adaxial CM wax) with an increasing number of compounds in the artificial wax. The same trend was found for DSC thermograms. Thermograms of ternary and quaternary blends exhibited more overlapping peaks and occurred in a temperature range more similar to the range of the whole leaf plant wax. The XRD spectrum at room temperature showed good conformity with the quaternary blend.
The current work illustrates a method for selective extraction of TRPs from isolated CMs. It gives direct experimental proof of the association of the water permeance barrier with the VLCA rather than to the TRPs. Furthermore, the possibility to mimic cuticular waxes using commercially available wax compounds is investigated. The results show promising feasibility for its viability, enabling it to perform as a standardized initial point for further research (e.g. to examine the influence of different constituents on waxes), revealing valuable knowledge about the structure and the chemistry-function relationship of cuticular waxes.
In vitro rearing of honeybee larvae is an established method that enables exact control and monitoring of developmental factors and allows controlled application of pesticides or pathogens. However, only a few studies have investigated how the rearing method itself affects the behavior of the resulting adult honeybees. We raised honeybees in vitro according to a standardized protocol: marking the emerging honeybees individually and inserting them into established colonies. Subsequently, we investigated the behavioral performance of nurse bees and foragers and quantified the physiological factors underlying the social organization. Adult honeybees raised in vitro differed from naturally reared honeybees in their probability of performing social tasks. Further, in vitro-reared bees foraged for a shorter duration in their life and performed fewer foraging trips. Nursing behavior appeared to be unaffected by rearing condition. Weight was also unaffected by rearing condition. Interestingly, juvenile hormone titers, which normally increase strongly around the time when a honeybee becomes a forager, were significantly lower in three- and four-week-old in vitro bees. The effects of the rearing environment on individual sucrose responsiveness and lipid levels were rather minor. These data suggest that larval rearing conditions can affect the task performance and physiology of adult bees despite equal weight, pointing to an important role of the colony environment for these factors. Our observations of behavior and metabolic pathways offer important novel insight into how the rearing environment affects adult honeybees.
Farmland tree cultivation is considered an important option for enhancing wood production. In South India, the native leaf-deciduous tree species Melia dubia is popular for short-rotation plantations. Across a rainfall gradient from 420 to 2170 mm year\(^{–1}\), we studied 186 farmland woodlots between one and nine years in age. The objectives were to identify the main factors controlling aboveground biomass (AGB) and growth rates. A power-law growth model predicts an average stand-level AGB of 93.8 Mg ha\(^{–1}\) for nine-year-old woodlots. The resulting average annual AGB increment over the length of the rotation cycle is 10.4 Mg ha\(^{–1}\) year\(^{–1}\), which falls within the range reported for other tropical tree plantations. When expressing the parameters of the growth model as functions of management, climate and soil variables, it explains 65% of the variance in AGB. The results indicate that water availability is the main driver of the growth of M. dubia. Compared to the effects of water availability, the effects of soil nutrients are 26% to 60% smaller. We conclude that because of its high biomass accumulation rates in farm forestry, M. dubia is a promising candidate for short-rotation plantations in South India and beyond.
Protein purification is the vital basis to study the function, structure and interaction of proteins. Widely used methods are affinity chromatography-based purifications, which require different chromatography columns and harsh conditions, such as acidic pH and/or adding imidazole or high salt concentration, to elute and collect the purified proteins. Here we established an easy and fast purification method for soluble proteins under mild conditions, based on the light-induced protein dimerization system improved light-induced dimer (iLID), which regulates protein binding and release with light. We utilize the biological membrane, which can be easily separated by centrifugation, as the port to anchor the target proteins. In Xenopus laevis oocyte and Escherichia coli, the blue light-sensitive part of iLID, AsLOV2-SsrA, was targeted to the plasma membrane by different membrane anchors. The other part of iLID, SspB, was fused with the protein of interest (POI) and expressed in the cytosol. The SspB-POI can be captured to the membrane fraction through light-induced binding to AsLOV2-SsrA and then released purely to fresh buffer in the dark after simple centrifugation and washing. This method, named mem-iLID, is very flexible in scale and economic. We demonstrate the quickly obtained yield of two pure and fully functional enzymes: a DNA polymerase and a light-activated adenylyl cyclase. Furthermore, we also designed a new SspB mutant for better dissociation and less interference with the POI, which could potentially facilitate other optogenetic manipulations of protein–protein interaction.
The technique to manipulate cells or living animals by illumination after gene transfer of light-sensitive proteins is called optogenetics. Successful optogenetics started with the use of the light-gated cation channel channelrhodopsin-2 (ChR2). After early demonstrations of the power of ChR2, further light-sensitive ion channels and ion pumps were recruited to the optogenetic toolbox. Furthermore, mutations and chimera of ChR2 improved its versatility.
However, there is still a need for improved optogenetic tools, e.g. with higher permeability for calcium or better expression in the plasma membrane. In this thesis, my work focuses on the design of highly functional channelrhodopsins with enhanced Na+ and Ca2+ conductance.
First, I tested different N-terminal signal peptides to improve the plasma membrane targeting of Channelrhodopsins. We found that a N-terminal peptide, named LR, could improve the plasma membrane targeting of many rhodopsins. Modification with LR contributed to three to ten-fold larger photocurrents (than that of the original version) of multiple channelrhodopsins, like ChR2 from C. reinhardtii (CrChR2), PsChR, Chrimson, CheRiff, CeChR, ACRs, and the light-activated pump rhodopsins KR2, Jaw, HR.
Second, by introducing point mutation, I could further improve the light sensitivity and photocurrent of different channelrhodopsins. For instance, ChR2-XXM 2.0, ChR2-XXL 2.0 and PsChR D139H 2.0 exhibited hundred times larger photocurrents than wild type ChR2 and they show high light sensitivity. Also, the Ca2+ permeable channelrhodopsins PsCatCh 2.0f and PsCatCh 2.0e show very large photocurrents and fast kinetics. In addition, I also characterized a novel bi-stable CeChR (from the acidophilic green alga Chlamydomonas eustigma) with a much longer closing time.
Third, I analysed the ion selectivity of different ChRs, which provides a basis for rational selection of channelrhodopsins for different experimental purposes. I demonstrate that ChR2, Chronos, Chrimson, CheRiff and CeChR are highly proton conductive, compared with wild type PsChR. Interestingly, Chronos has the lowest potassium conductance among these channelrhodopsins. Furthermore, I found that mutation of an aspartate in TM4 of ChR2 (D156) and PsChR (D139) to histidine obviously increased both the sodium and calcium permeability while proton conductance was reduced. PsChR D139H 2.0 has the largest sodium conductance of any published channelrhodopsin variants. Additionally, I generated PsCatCh 2.0e which exhibits a ten-fold larger calcium current than the previously reported Ca2+ transporting CrChR2 mutant CatCh.
In summary, my research work
1.) described strategies for improving plasma membrane trafficking efficiency of opsins;
2.) yielded channelrhodopsins with fast kinetics or high light sensitivity;
3.) provided optogenetic tools with improved calcium and sodium conductance.
We could also improve the performance of channelrhodopsins with distinct action spectra, which will facilitate two-color neural excitation, both in-vitro and in-vivo.
Ants belong to the most successful insects living on our planet earth. One criterion of their tremendous success is the division of labor among workers that can be related to age (age¬– or temporal polyethism) and/ or body size (size–related polymorphism). Young ants care for the queen and brood in the nest interior and switch to foraging tasks in the outside environment with ongoing age. This highly flexible interior–exterior transition probably allows the ant workers to properly match the colony needs and is one of the most impressive behaviors a single worker undergoes during its life. As environmental stimuli are changing with this transition, workers are required to perform a new behavioral repertoire. This requires significant adaptions in sensory and higher¬–order integration centers in the brain, like the mushroom bodies. Furthermore, foragers need proper time measuring mechanisms to cope with daily environmental changes and to adapt their own mode of life. Therefore, they possess a functional endogenous clock that generates rhythms with a period length of approximately 24 hours. The species–rich genus of Camponotus ants constitute a rewarding model to study how behavioral duties of division of labor were performed and modulated within the colony and how synaptic plasticity in the brain is processed, as they can divide their labor to both, age and body size, simultaneously.
In my PhD thesis, I started to investigate the behavioral repertoire (like foraging and locomotor activity) of two sympatric Camponotus species, C. mus and C. rufipes workers under natural and under controlled conditions. Furthermore, I focused on the division of labor in C. rufipes workers and started to examine structural and ultrastructural changes of neuronal architectures in the brain that are accompanied by the interior–exterior transition of C. rufipes ants.
In the first part of my thesis, I started to analyze the temporal organization of task allocation throughout the life of single C. rufipes workers. Constant video–tracking of individually labeled workers for up to 11 weeks, revealed an age–related division of labor of interior and exterior workers. After emergence, young individuals are tended to by older ones within the first 48 hours of their lives before they themselves start nurturing larvae and pupae. Around 52% switch to foraging duties at an age of 14–20 days. The workers that switched to foraging
tasks are mainly media–sized workers and seem to be more specialized than nurses. Variations in proportion and the age of switching workers between and within different subcolonies indicate how highly flexible and plastic the age–related division of labor occurs in this ant species. Most of the observed workers were engaged in foraging tasks exclusively during nighttime. As the experiments were conducted in the laboratory, they are completely lacking environmental stimuli of the ants´ natural habitat.
I therefore asked in a second study, how workers of the two closely related Camponotus species, C. rufipes and C. mus, adapt their daily activity patterns (foraging and locomotor activity) under natural (in Uruguay, South America) and controlled (in the laboratory) conditions to changing thermal conditions. Monitoring the foraging activity of both Camponotus species in a field experiment revealed, that C. mus workers are exclusively diurnal, whereas C. rufipes foragers are predominantly nocturnal. However, some nests showed an elevated daytime activity, which could be an adaption to seasonally cold night temperatures. To further investigate the impact of temperature and light on the differing foraging activity patterns in the field, workers of both Camponotus species were artificially exposed to different thermal regimes in the laboratory, simulating local winter and summer conditions. Here again, C. mus workers display solely diurnal locomotor activity, whereas workers of C. rufipes shifted their locomotor activity from diurnal under thermal winter conditions to nocturnal under thermal summer conditions. Hence, the combination of both, field work and laboratory studies, shows that daily activity is mostly shaped by thermal conditions and that temperature cycles are not just limiting foraging activity but can be used as zeitgeber to schedule the outside activities of the nests.
Once an individual worker switches from indoor duties to exterior foraging tasks, it is confronted with an entirely new set of sensory information. To cope with changes of the environmental conditions and to facilitate the behavioral switch, workers need a highly flexible and plastic neuronal system. Hence, my thesis further focuses on the underlying neuronal adaptations of the visual system, including the optic lobes as the primary visual neuropil and the mushroom bodies as secondary visual brain neuropil, that are accompanied with the behavioral switch from nursing to foraging. The optic lobes as well as the mushroom bodies of light–deprived workers show an `experience–independent´ volume increase during the first two weeks of adulthood. An additional light exposure for 4 days induces an `experience–dependent´ decrease of synaptic complexes in the mushroom body collar,
followed by an increase after extended light exposure for 14 days. I therefore conclude, that the plasticity of the central visual system represents important components for the optimal timing of the interior–exterior transitions and flexibility of the age–related division of labor. These remarkable structural changes of synaptic complexes suggest an active involvement of the mushroom body neuropil in the lifetime plasticity that promotes the interior–exterior transition of Camponotus rufipes ants. Beside these investigations of neuronal plasticity of synaptic complexes in the mushroom bodies on a structural level, I further started to examine mushroom body synaptic structures at the ultrastructural level. Until recently, the detection of synaptic components in projection neuron axonal boutons were below resolution using classical Transmission Electron Microscopy. Therefore, I started to implement Electron Tomography to increase the synaptic resolution to understand architectural changes in neuronal plasticity process. By acquiring double tilt series and consecutive computation of the acquired tilt information, I am now able to resolve individual clear–core and dense–core vesicles within the projection neuron cytoplasm of C. rufipes ants. I additionally was able to reveal single postsynaptic Kenyon cell dendritic spines (~62) that surround one individual projection neuron bouton. With this, I could reveal first insights into the complex neuronal architecture of single projection neuron boutons in the olfactory mushroom body lip region. The high resolution images of synaptic architectures at the ultrastructural level, received with Electron Tomography would promote the understanding of architectural changes in neuronal plasticity.
In my PhD thesis, I demonstrate that the temporal organization within Camponotus colonies involves the perfect timing of different tasks. Temperature seems to be the most scheduling abiotic factors of foraging and locomotor activity. The ants do not only need to adapt their behavioral repertoire in accordance to the interior–exterior switch, also the parts in the peripheral and central that process visual information need to adapt to the new sensory environment.
Water transport through the water channels, aquaporins (AQPs), is involved in epithelial fluid secretion and absorption, cell migration, brain edema, adipocyte metabolism, and other physiological or pathological functions. Modulation of AQP function has therapeutic potential in edema, cancer, obesity, brain injury, glaucoma, etc. The function of AQPs is in response to the osmotic gradient that is formed by the concentration differences of ions or small molecules. In terms of brain edema, it is a pathophysiological condition, resulting from dysfunction of the plasma membrane that causes a disorder of intracellular ion homeostasis and thus increases intracellular fluid content. Optogenetics can be used to regulate ion transport easily by light with temporal and spatial precision. Therefore, if we control the cell ion influx, boosting the water transport through AQPs, this will help to investigate the pathological mechanisms in e.g. brain edema. To this end, I investigated the possibility for optogenetic manipulating water transport in Xenopus oocytes. The main ions in Xenopus oocyte cytoplasm are ~10 mM Na+, ~50 mM Cl- and ~100 mM K+, similar to the mammalian cell physiological condition. Three light-gated channels, ChR2-XXM 2.0 (light-gated cation channel), GtACR1 (light-gated anion channel) and SthK-bPAC (light-gated potassium channel), were used in my study to regulate ion transport by light and thus manipulate the osmotic gradient and water transport. To increase water flow, I also used coexpression of AQP1. When expressing ChR2-XXM 2.0 and GtACR1 together, mainly Na+ influx was triggered by ChR2-XXM2.0 under blue light illumination, which then made the membrane potential more positive and facilitated Cl- influx by GtACR1. Due to this inward movement of Na+ and Cl-, the osmotic gradient was formed to trigger water influx through AQP1. Large amounts of water uptake can speedily increase the oocyte volume until membrane rupture. Next, when co-expressing GtACR1 and SthK-bPAC, water efflux will be triggered with blue light because of the light-gated KCl efflux and then oocyte shrinking could be observed.
I also developed an optogenetic protein purification method based on a light-induced protein interactive system. Currently, the most common protein purification method is based on affinity chromatography, which requires different chromatography columns and harsh conditions, such as acidic pH 4.5 - 6 and/or adding imidazole or high salt concentration, to elute and collect the purified proteins. The change in conditions could influence the activity of target proteins. So, an easy and flexible protein purification method based on the photo-induced protein interactive system iLID was designed, which regulates protein binding with light in mild conditions and does not require a change of solution composition. For expression in E. coli, the blue light-sensitive part of iLID, the LOV2 domain, was fused with a membrane anchor and expressed in the plasma membrane, and the other binding partner, SspB, was fused with the protein of interest (POI), expressed in the cytosol. The plasma membrane fraction and the soluble cytosolic fraction of E. coli can be easily separated by centrifugation. The SspB-POI can be then captured to the membrane fraction by light stimulation and released to clean buffer in the dark after washing. This method does not require any specific column and functions in mild conditions, which are very flexible at scale and will facilitate extensive protein engineering and purification of proteins, sensitive to changed buffer conditions.
Stomata sind kleine Poren in der Blattoberfläche, die Pflanzen eine Anpassung ihres Wasserhaushalts an sich ändernde Umweltbedingungen ermöglichen. Die Öffnungsweite der Stomata wird durch den Turgordruck der Schließzellen bestimmt, der wiederum durch Ionenflüsse über die Membranen der Zelle reguliert wird. Ein Netzwerk von Signaltransduktionswegen sorgt dafür, dass Pflanzen die Stomabewegungen an die Umgebungsbedingungen anpassen können. Viele molekulare Komponenten dieser Signaltransduktionketten in Schließzellen von Angiospermen sind inzwischen bekannt und Calcium spielt darin als Signalmolekül eine wichtige Rolle. Weitgehend unbekannt sind dagegen die Mechanismen, die zur Erzeugung von transienten Erhöhungen der Calciumkonzentration führen. Auch die molekularen Grundlagen der Regulierung der Stomaweite in Nicht-Angiospermen-Arten sind bisher nur wenig verstanden. Um zur Aufklärung dieser Fragestellungen
beizutragen, wurden in dieser Arbeit Mechanismen zur Erhöhungen der cytosolischen Calciumkonzentration sowie elektrophysiologische Eigenschaften von Schließzellen untersucht. Der Fokus lag hierbei insbesondere auf der Visualisierung cytosolischer Calciumsignale in Schließzellen. Im ersten Teil der Arbeit wurde durch die Applikation hyperpolarisierender Spannungspulse mittels TEVC (Two Electrode Voltage Clamp) gezielt eine Erhöhung der cytosolischen Calciumkonzentration in einzelnen Schließzellen von Nicotiana tabacum ausgelöst. Um die Dynamik der cytosolischen Calciumkonzentration dabei zeitlich und räumlich hoch aufgelöst zu visualisieren, wurde simultan zu den elektrophysiologischen Messungen ein
Spinning-Disc-System für konfokale Aufnahmen eingesetzt. Während der Applikation
hyperpolarisierender Spannungspulse wurde eine transiente Vergrößerung des cytosolischen Volumens beobachtet. Diese lässt sich durch einen osmotisch getriebenen Wasserfluss erklären, der durch die Veränderung der Ionenkonzentration im Cytosol verursacht wird. Diese wiederum wird durch die spannungsabhängige Aktivierung einwärtsgleichrichtender Kaliumkanäle in der Plasmamembran der Schließzellen und durch den Kompensationsstrom der eingestochenen Mikroelektrode hervorgerufen. Mit Hilfe des calciumsensitiven Farbstoffs Fura-2 konnte gezeigt werden, dass die Erhöhung der freien cytosolischen Calciumkonzentration während der Applikation hyperpolarisierender Spannungspulse durch zwei Mechanismen verursacht wird. Der erste Mechanismus ist die Aktivierung hyperpolarisationsaktivierter, calciumpermeabler Kanäle (HACCs) in der Plasmamembran, die schon 1998 von Grabov & Blatt beschrieben wurde. Zusätzlich zu diesem Mechanismus der Calciumfreisetzung, konnte ein zweiter bislang unbekannter Mechanismus aufgedeckt werden, bei dem Calcium aus intrazellulären Speichern in das Cytosol freigesetzt wird. Dieser Mechanismus hängt mit der oben beschriebenen Vergrößerung des cytosolischen Volumens zusammen und ist wahrscheinlich durch die Änderungen der mechanischen Spannung der Membran bzw. der Osmolarität innerhalb der Zelle bedingt. Diese könnten zu einer Aktivierung mechanosensitiver, calciumpermeabler Kanäle führen.
Der zweite Teil der Arbeit beschäftigt sich mit den molekularen Grundlagen der Regulierung von Stomata in Nicht-Angiospermen. In Schließzellen von Polypodium vulgare konnten durch die Anwendung der TEVC-Technik ähnliche spannungsabhängige Ströme über die Plasmamembran gemessen werden wie in Angiospermen. Ebenso wurden durch die Applikation hyperpolarisierender Spannungspulse an Schließzellen von Polypodium und Asplenium Erhöhungen der cytosolischen Calciumkonzentration ausgelöst, die auf die Existenz spannungsabhängiger, calciumpermeabler Kanäle in der Plasmamembran
hinweisen. Die Diffusion von Fluoreszenzfarbstoffen in die Nachbarschließzellen nach der iontophoretischen Beladung in Polypodium, Asplenium, Ceratopteris und Selaginella zeigte, dass in diesen Arten eine symplastische Verbindung zwischen benachbarten Schließzellen besteht, die an Schließzellen von Angiospermen bisher nicht beobachtet werden konnte. Anhand elektronenmikroskopischer Aufnahmen von Polypodium glycyrrhiza Schließzellen konnte gezeigt werden, dass diese Verbindung wahrscheinlich durch Plasmodesmata zwischen benachbarten Schließzellen gebildet wird. Durch die Analyse der Calciumdynamik in benachbarten Schließzellen nach hyperpolarisierenden Spannungspulsen stellte sich heraus, dass die Calciumhomöostase trotz symplastischer Verbindung in beiden Schließzellen unabhängig voneinander reguliert zu werden scheint. Im Rahmen der Untersuchungen an Farnschließzellen wurde desweiteren eine Methode zur Applikation von ABA etabliert, die es erlaubt mithilfe von Mikroelektroden das Phytohormon iontophoretisch in den Apoplasten zu laden. Im Gegensatz zu den Schließzellen von Nicotiana tabacum, die auf eine so durchgeführte ABA-Applikation mit dem Stomaschluss reagierten, wurde in Polypodium vulgare auf diese Weise kein Stomaschluss ausgelöst. Da die ABA-Antwort der Farnstomata aber auch von anderen Faktoren wie Wachstumsbedingungen abhängig ist (Hõrak et al., 2017), kann eine ABA-Responsivität in dieser Farnart trotzdem nicht vollkommen ausgeschlossen werden.
Die Freisetzung von Calcium aus intrazellulären Speichern, wie sie in dieser Arbeit gezeigt wurde, könnte eine wichtige Rolle bei der Regulierung der Stomaweite spielen. Zur Aufklärung dieser Fragestellung wäre die Identifizierung der Kanäle, die an der osmotisch/mechanisch induzierten Calciumfreisetzung aus internen Speichern beteiligt sind, von großem Interesse. Weiterführende Studien an Schließzellen von Farnen könnten die physiologische Bedeutung der aus Angiospermen bekannten Ionenkanäle für die Stomabewegungen in evolutionär älteren Landpflanzen aufklären und so maßgeblich zum Verständnis der Evolution der Regulierunsgmechanismen von Stomata beitragen. Außerdem stellt sich die Frage, welche Rolle die hier gezeigte symplastische Verbindung der Nachbarschließzellen durch Plasmodesmata für die Funktion der Stomata spielt.
Optogenetics was developed in the field of neuroscience and is most commonly using light-sensitive rhodopsins to control the neural activities. Lately, we have expanded this technique into plant science by co-expression of a chloroplast-targeted β-carotene dioxygenase and an improved anion channelrhodopsin GtACR1 from the green alga Guillardia theta. The growth of Nicotiana tabacum pollen tube can then be manipulated by localized green light illumination. To extend the application of analogous optogenetic tools in the pollen tube system, we engineered another two ACRs, GtACR2, and ZipACR, which have different action spectra, light sensitivity and kinetic features, and characterized them in Xenopus laevis oocytes, Nicotiana benthamiana leaves and N. tabacum pollen tubes. We found that the similar molecular engineering method used to improve GtACR1 also enhanced GtACR2 and ZipACR performance in Xenopus laevis oocytes. The ZipACR1 performed in N. benthamiana mesophyll cells and N. tabacum pollen tubes with faster kinetics and reduced light sensitivity, allowing for optogenetic control of anion fluxes with better temporal resolution. The reduced light sensitivity would potentially facilitate future application in plants, grown under low ambient white light, combined with an optogenetic manipulation triggered by stronger green light.
Background
Microbial rhodopsins vary in their chemical properties, from light sensitive ion transport to different enzymatic activities. Recently, a novel family of two-component Cyclase (rhod)opsins (2c-Cyclop) from the green algae Chlamydomonas reinhardtii and Volvox carteri was characterized, revealing a light-inhibited guanylyl cyclase (GC) activity. More genes similar to 2c-Cyclop exist in algal genomes, but their molecular and physiological functions remained uncharacterized.
Results
Chlamyopsin-5 (Cop5) from C. reinhardtii is related to Cr2c-Cyclop1 (Cop6) and can be expressed in Xenopus laevis oocytes, but shows no GC activity. Here, we exchanged parts of Cop5 with the corresponding ones of Cr2c-Cyclop1. When exchanging the opsin part of Cr2c-Cyclop1 with that of Cop5, we obtained a bi-stable guanylyl cyclase (switch-Cyclop1) whose activity can be switched by short light flashes. The GC activity of switch-Cyclop1 is increased for hours by a short 380 nm illumination and switched off (20-fold decreased) by blue or green light. switch-Cyclop1 is very light-sensitive and can half-maximally be activated by ~ 150 photons/nm2 of 380 nm (~ 73 J/m2) or inhibited by ~ 40 photons/nm\(^2\) of 473 nm (~ 18 J/m\(^2\)).
Conclusions
This engineered guanylyl cyclase is the first light-switchable enzyme for cGMP level regulation. Light-regulated cGMP production with high light-sensitivity is a promising technique for the non-invasive investigation of the effects of cGMP signaling in many different tissues.
Whereas the role of calcium ions (Ca\(^{2+}\)) in plant signaling is well studied, the physiological significance of pH‐changes remains largely undefined.
Here we developed CapHensor, an optimized dual‐reporter for simultaneous Ca\(^{2+}\) and pH ratio‐imaging and studied signaling events in pollen tubes (PTs), guard cells (GCs), and mesophyll cells (MCs). Monitoring spatio‐temporal relationships between membrane voltage, Ca\(^{2+}\)‐ and pH‐dynamics revealed interconnections previously not described.
In tobacco PTs, we demonstrated Ca\(^{2+}\)‐dynamics lag behind pH‐dynamics during oscillatory growth, and pH correlates more with growth than Ca\(^{2+}\). In GCs, we demonstrated abscisic acid (ABA) to initiate stomatal closure via rapid cytosolic alkalization followed by Ca2+ elevation. Preventing the alkalization blocked GC ABA‐responses and even opened stomata in the presence of ABA, disclosing an important pH‐dependent GC signaling node. In MCs, a flg22‐induced membrane depolarization preceded Ca2+‐increases and cytosolic acidification by c. 2 min, suggesting a Ca\(^{2+}\)/pH‐independent early pathogen signaling step. Imaging Ca2+ and pH resolved similar cytosol and nuclear signals and demonstrated flg22, but not ABA and hydrogen peroxide to initiate rapid membrane voltage‐, Ca\(^{2+}\)‐ and pH‐responses.
We propose close interrelation in Ca\(^{2+}\)‐ and pH‐signaling that is cell type‐ and stimulus‐specific and the pH having crucial roles in regulating PT growth and stomata movement.
Plant stress signalling involves bursts of reactive oxygen species (ROS), which can be mimicked by the application of acute pulses of ozone. Such ozone-pulses inhibit photosynthesis and trigger stomatal closure in a few minutes, but the signalling that underlies these responses remains largely unknown.
We measured changes in Arabidopsis thaliana gas exchange after treatment with acute pulses of ozone and set up a system for simultaneous measurement of membrane potential and cytosolic calcium with the fluorescent reporter R-GECO1.
We show that within 1 min, prior to stomatal closure, O\(_{3}\) triggered a drop in whole-plant CO\(_{2}\) uptake. Within this early phase, O\(_{3}\) pulses (200–1000 ppb) elicited simultaneous membrane depolarization and cytosolic calcium increase, whereas these pulses had no long-term effect on either stomatal conductance or photosynthesis. In contrast, pulses of 5000 ppb O\(_{3}\) induced cell death, systemic Ca\(^{2+}\) signals and an irreversible drop in stomatal conductance and photosynthetic capacity.
We conclude that mesophyll cells respond to ozone in a few seconds by distinct pattern of plasma membrane depolarizations accompanied by an increase in the cytosolic calcium ion (Ca\(^{2+}\)) level. These responses became systemic only at very high ozone concentrations. Thus, plants have rapid mechanism to sense and discriminate the strength of ozone signals.
Cytosolic calcium signals are evoked by a large variety of biotic and abiotic stimuli and play an important role in cellular and long distance signalling in plants. While the function of the plasma membrane in cytosolic Ca\(^{2+}\) signalling has been intensively studied, the role of the vacuolar membrane remains elusive.
A newly developed vacuolar voltage clamp technique was used in combination with live-cell imaging, to study the role of the vacuolar membrane in Ca\(^{2+}\) and pH homeostasis of bulging root hair cells of Arabidopsis.
Depolarisation of the vacuolar membrane caused a rapid increase in the Ca\(^{2+}\) concentration and alkalised the cytosol, while hyperpolarisation led to the opposite responses.
The relationship between the vacuolar membrane potential, the cytosolic pH and Ca2+ concentration suggests that a vacuolar H\(^{+}\)/Ca\(^{2+}\) exchange mechanism plays a central role in cytosolic Ca2+ homeostasis. Mathematical modelling further suggests that the voltage-dependent vacuolar Ca\(^{2+}\) homeostat could contribute to calcium signalling when coupled to a recently discovered K\(^{+}\) channel-dependent module for electrical excitability of the vacuolar membrane.
Background
While leaves are far more accessible for analysing plant defences, roots are hidden in the soil, leading to difficulties in studying soil-borne interactions. Inoculation strategies for infecting model plants with model root pathogens are described in the literature, but it remains demanding to obtain a methodological overview. To address this challenge, this study uses the model root pathogen Verticillium longisporum on Arabidopsis thaliana host plants and provides recommendations for selecting appropriate infection systems to investigate how plants cope with root pathogens.
Results
A novel root infection system is introduced, while two existing ones are precisely described and optimized. Step-by-step protocols are presented and accompanied by pathogenicity tests, transcriptional analyses of indole-glucosinolate marker genes and independent confirmations using reporter constructs. Advantages and disadvantages of each infection system are assessed. Overall, the results validate the importance of indole-glucosinolates as secondary metabolites that limit the Verticillium propagation in its host plant.
Conclusion
Detailed assistances on studying host defence strategies and responses against V. longisporum is provided. Furthermore, other soil-borne microorganisms (e.g., V. dahliae) or model plants, such as economically important oilseed rape and tomato, can be introduced in the infection systems described. Hence, these proven manuals can support finding a root infection system for your specific research questions to further decipher root-microbe interactions.
Epidermal fragments enriched in guard cells (GCs) were isolated from the halophyte quinoa (Chenopodium quinoa Wild.) species, and the response at the proteome level was studied after salinity treatment of 300 mM NaCl for 3 weeks. In total, 2147 proteins were identified, of which 36% were differentially expressed in response to salinity stress in GCs. Up and downregulated proteins included signaling molecules, enzyme modulators, transcription factors and oxidoreductases. The most abundant proteins induced by salt treatment were desiccation-responsive protein 29B (50-fold), osmotin-like protein OSML13 (13-fold), polycystin-1, lipoxygenase, alpha-toxin, and triacylglycerol lipase (PLAT) domain-containing protein 3-like (eight-fold), and dehydrin early responsive to dehydration (ERD14) (eight-fold). Ten proteins related to the gene ontology term “response to ABA” were upregulated in quinoa GC; this included aspartic protease, phospholipase D and plastid-lipid-associated protein. Additionally, seven proteins in the sucrose–starch pathway were upregulated in the GC in response to salinity stress, and accumulation of tryptophan synthase and L-methionine synthase (enzymes involved in the amino acid biosynthesis) was observed. Exogenous application of sucrose and tryptophan, L-methionine resulted in reduction in stomatal aperture and conductance, which could be advantageous for plants under salt stress. Eight aspartic proteinase proteins were highly upregulated in GCs of quinoa, and exogenous application of pepstatin A (an inhibitor of aspartic proteinase) was accompanied by higher oxidative stress and extremely low stomatal aperture and conductance, suggesting a possible role of aspartic proteinase in mitigating oxidative stress induced by saline conditions.
Guard cells control the aperture of plant stomata, which are crucial for global fluxes of CO\(_2\) and water. In turn, guard cell anion channels are seen as key players for stomatal closure, but is activation of these channels sufficient to limit plant water loss? To answer this open question, we used an optogenetic approach based on the light-gated anion channelrhodopsin 1 (GtACR1). In tobacco guard cells that express GtACR1, blue- and green-light pulses elicit Cl\(^-\) and NO\(_3\)\(^-\) currents of -1 to -2 nA. The anion currents depolarize the plasma membrane by 60 to 80 mV, which causes opening of voltage-gated K+ channels and the extrusion of K+. As a result, continuous stimulation with green light leads to loss of guard cell turgor and closure of stomata at conditions that provoke stomatal opening in wild type. GtACR1 optogenetics thus provides unequivocal evidence that opening of anion channels is sufficient to close stomata.
Simple Summary
Abiotic and biotic stress conditions result in profound changes in plant lipid metabolism. Vegetable oil consists of triacylglycerols, which are important energy and carbon storage compounds in seeds of various plant species. These compounds are also present in vegetative tissue, and levels have been reported to increase with different abiotic stresses in leaves. This work shows that triacylglycerols accumulate in roots and in distal, non-treated leaves upon treatment with a fungal pathogen or lipopolysaccharide (a common bacterial-derived elicitor in animals and plants). Treatment of leaves with a bacterial pathogen or a bacterial effector molecule results in triacylglycerol accumulation in leaves, but not systemically in roots. These results suggest that elicitor molecules are sufficient to induce an increase in triacylglycerol levels, and that unidirectional long-distance signaling from roots to leaves is involved in pathogen and elicitor-induced triacylglycerol accumulation.
Abstract
Interaction of plants with the environment affects lipid metabolism. Changes in the pattern of phospholipids have been reported in response to abiotic stress, particularly accumulation of triacylglycerols, but less is known about the alteration of lipid metabolism in response to biotic stress and leaves have been more intensively studied than roots. This work investigates the levels of lipids in roots as well as leaves of Arabidopsis thaliana in response to pathogens and elicitor molecules by UPLC-TOF-MS. Triacylglycerol levels increased in roots and systemically in leaves upon treatment of roots with the fungus Verticillium longisporum. Upon spray infection of leaves with the bacterial pathogen Pseudomonas syringae, triacylglycerols accumulated locally in leaves but not in roots. Treatment of roots with a bacterial lipopolysaccharide elicitor induced a strong triacylglycerol accumulation in roots and leaves. Induction of the expression of the bacterial effector AVRRPM1 resulted in a dramatic increase of triacylglycerol levels in leaves, indicating that elicitor molecules are sufficient to induce accumulation of triacylglycerols. These results give insight into local and systemic changes to lipid metabolism in roots and leaves in response to biotic stresses.
Climate change is increasing the frequency and intensity of warming and drought periods around the globe, currently representing a threat to many plant species. Understanding the resistance and resilience of plants to climate change is, therefore, urgently needed. As date palm (Phoenix dactylifera) evolved adaptation mechanisms to a xeric environment and can tolerate large diurnal and seasonal temperature fluctuations, we studied the protein expression changes in leaves, volatile organic compound emissions, and photosynthesis in response to variable growth temperatures and soil water deprivation. Plants were grown under controlled environmental conditions of simulated Saudi Arabian summer and winter climates challenged with drought stress. We show that date palm is able to counteract the harsh conditions of the Arabian Peninsula by adjusting the abundances of proteins related to the photosynthetic machinery, abiotic stress and secondary metabolism. Under summer climate and water deprivation, these adjustments included efficient protein expression response mediated by heat shock proteins and the antioxidant system to counteract reactive oxygen species formation. Proteins related to secondary metabolism were downregulated, except for the P. dactylifera isoprene synthase (PdIspS), which was strongly upregulated in response to summer climate and drought. This study reports, for the first time, the identification and functional characterization of the gene encoding for PdIspS, allowing future analysis of isoprene functions in date palm under extreme environments. Overall, the current study shows that reprogramming of the leaf protein profiles confers the date palm heat- and drought tolerance. We conclude that the protein plasticity of date palm is an important mechanism of molecular adaptation to environmental fluctuations.
Key message
Mobile laser scanning and geometrical analysis revealed relationships between tree geometry and seed dispersal mechanism, latitude of origin, as well as growth.
Abstract
The structure and dynamics of a forest are defined by the architecture and growth patterns of its individual trees. In turn, tree architecture and growth result from the interplay between the genetic building plans and environmental factors. We set out to investigate whether (1) latitudinal adaptations of the crown shape occur due to characteristic solar elevation angles at a species’ origin, (2) architectural differences in trees are related to seed dispersal strategies, and (3) tree architecture relates to tree growth performance. We used mobile laser scanning (MLS) to scan 473 trees and generated three-dimensional data of each tree. Tree architectural complexity was then characterized by fractal analysis using the box-dimension approach along with a topological measure of the top heaviness of a tree. The tree species studied originated from various latitudinal ranges, but were grown in the same environmental settings in the arboretum. We found that trees originating from higher latitudes had significantly less top-heavy geometries than those from lower latitudes. Therefore, to a certain degree, the crown shape of tree species seems to be determined by their original habitat. We also found that tree species with wind-dispersed seeds had a higher structural complexity than those with animal-dispersed seeds (p < 0.001). Furthermore, tree architectural complexity was positively related to the growth performance of the trees (p < 0.001). We conclude that the use of 3D data from MLS in combination with geometrical analysis, including fractal analysis, is a promising tool to investigate tree architecture.
Das Adapterprotein TRAF2 und seine Bedeutung für die Todesrezeptor-vermittelte Signaltransduktion
(2020)
Während die Rolle des tumor necrosis factor (TNF) receptor associated factor (TRAF)2 in der Signaltransduktion der TRAF-interagierenden Rezeptoren der TNF Receptor (TNFR)- Superfamily (TNFRSF) bereits in der Vergangenheit umfassend erforscht wurde, ist die Rolle und Funktion dieses Adapterproteins für die Signalgebung der Todesrezeptoren nicht vollständig aufgeklärt. Die unklare Funktion der Really Interesting New Gene (RING) E3 Ligase Domäne in TRAF2 und die Abhängigkeit von Caspasen für die Aktivierung des klassischen nuclear factor κB (NFκB)-Signalweges führten in dieser Arbeit zur Herstellung von CRISPR/Cas9 knockout (KO) Zellen, bei denen TRAF2 in der Kolorektalkarzinomzelllinie HCT116 als auch in den Fibrosarkomzellen HT1080 ausgeschaltet wurde. Diese Zellen wurden zuvor so modifiziert, dass die Apoptose „downstream“ der Caspase-8-Aktivierung nicht weiter induzierbar war. HCT116-Zellen exprimierten hierzu ein mutiertes Allel der Phosphoinositide 3-kinase (PI3K) und HT1080-Bcl2-TNFR2 Zellen das anti-apoptotische Protein B-cell lymphoma 2 (Bcl2).
Im Fokus dieser Arbeit waren die Todesrezeptoren TNFR1, TNF-Related Apoptosis Inducing Receptor (TRAILR)1/2 und Cluster of Differentiation(CD)95. In den TRAF2-KO Zelllinien war der alternative NFκB Signalweg konstitutiv aktiv und der TNFR1-induzierte klassische NFκB-Signalweg inhibiert. Die proinflammatorische Signalgebung in Form der Interleukin (IL)8 Produktion war in den CD95-artigen Todesrezeptoren signifikant, aber nicht vollständig, reduziert und erfolgte Caspase-8-Aktivität unabhängig. Der Effekt der TRAF2-Deletion konnte durch eine Rekonstitution von TRAF2, jedoch nicht durch eine Überexpression von TRAF1 wiederhergestellt werden.
Des Weiteren führte die TRAF2-Defizienz zu einer verstärkten Procaspase-8- Prozessierung nach Aktivierung von Todesrezeptoren, die überraschenderweise mit einer Reduktion der Caspase-8-Aktivität einherging. Die Prozessierung der Procaspase-8, jedoch nicht die Aktivierung des klassischen NFκB-Signalweges wurde vermutlich durch eine verringerte Rekrutierung von cellular inhibitor of apoptosis protein (cIAP)1 an den TNFR1 erreicht. Die Expression der anti-apoptotischen Proteine FADD-like ICE (FLICE) Inhibitory Protein (FLIP)Long(L), FLIPShort(S) und cIAP1 wurde nicht von der TRAF2-Depletion beeinflusst.
Somit konnte in dieser Arbeit ein nicht-obligatorischer Effekt von TRAF2 auf die Regulation der proinflammatorischen Todesrezeptor-vermittelten Signaltransduktion nachgewiesen werden, die durch TRAF1 nicht ersetzt werden kann. Des Weiteren wurde eine bisher nicht beschriebene, stabilisierende Wirkung von TRAF2 auf die Capsase-8-Aktivität gezeigt.