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Background: Xanthophyllomyces dendrorhous is a basal agaricomycete with uncertain taxonomic placement, known for its unique ability to produce astaxanthin, a carotenoid with antioxidant properties. It was the aim of this study to elucidate the organization of its CoA-derived pathways and to use the genomic information of X. dendrorhous for a phylogenomic investigation of the Basidiomycota.
Results: The genome assembly of a haploid strain of Xanthophyllomyces dendrorhous revealed a genome of 19.50 Megabases with 6385 protein coding genes. Phylogenetic analyses were conducted including 48 fungal genomes. These revealed Ustilaginomycotina and Agaricomycotina as sister groups. In the latter a well-supported sister-group relationship of two major orders, Polyporales and Russulales, was inferred. Wallemia occupies a basal position within the Agaricomycotina and X. dendrorhous represents the basal lineage of the Tremellomycetes, highlighting that the typical tremelloid parenthesomes have either convergently evolved in Wallemia and the Tremellomycetes, or were lost in the Cystofilobasidiales lineage. A detailed characterization of the CoA-related pathways was done and all genes for fatty acid, sterol and carotenoid synthesis have been assigned.
Conclusions: The current study ascertains that Wallemia with tremelloid parenthesomes is the most basal agaricomycotinous lineage and that Cystofilobasidiales without tremelloid parenthesomes are deeply rooted within Tremellomycetes, suggesting that parenthesomes at septal pores might be the core synapomorphy for the Agaricomycotina. Apart from evolutionary insights the genome sequence of X. dendrorhous will facilitate genetic pathway engineering for optimized astaxanthin or oxidative alcohol production.
Epigenetic dysregulation contributes to the high cardiovascular disease burden in chronic kidney disease (CKD) patients. Although microRNAs (miRNAs) are central epigenetic regulators, which substantially affect the development and progression of cardiovascular disease (CVD), no data on miRNA dysregulation in CKD-associated CVD are available until now. We now performed high-throughput miRNA sequencing of peripheral blood mononuclear cells from ten clinically stable hemodialysis (HD) patients and ten healthy controls, which allowed us to identify 182 differentially expressed miRNAs (e.g., miR-21, miR-26b, miR-146b, miR-155). To test biological relevance, we aimed to connect miRNA dysregulation to differential gene expression. Genome-wide gene expression profiling by MACE (Massive Analysis of cDNA Ends) identified 80 genes to be differentially expressed between HD patients and controls, which could be linked to cardiovascular disease (e.g., KLF6, DUSP6, KLF4), to infection / immune disease (e.g., ZFP36, SOCS3, JUND), and to distinct proatherogenic pathways such as the Toll-like receptor signaling pathway (e.g., IL1B, MYD88, TICAM2), the MAPK signaling pathway (e.g., DUSP1, FOS, HSPA1A), and the chemokine signaling pathway (e.g., RHOA, PAK1, CXCL5). Formal interaction network analysis proved biological relevance of miRNA dysregulation, as 68 differentially expressed miRNAs could be connected to 47 reciprocally expressed target genes. Our study is the first comprehensive miRNA analysis in CKD that links dysregulated miRNA expression with differential expression of genes connected to inflammation and CVD. After recent animal data suggested that targeting miRNAs is beneficial in experimental CVD, our data may now spur further research in the field of CKD-associated human CVD.
Bacteria communicate via small diffusible molecules to mediate group-coordinated behavior, a process designated as quorum sensing. The basic molecular quorum sensing system of Gram-negative bacteria consists of a LuxI-type autoinducer synthase producing acyl-homoserine lactones (AHLs) as signaling molecules, and a LuxR-type receptor detecting the AHLs to control expression of specific genes. However, many proteobacteria possess one or more unpaired LuxR-type receptors that lack a cognate LuxI-like synthase, referred to as LuxR solos. The enteric and insect pathogenic bacteria of the genus Photorhabdus harbor an extraordinarily high number of LuxR solos, more than any other known bacteria, and all lack a LuxI-like synthase. Here, we focus on the presence and the different types of LuxR solos in the three known Photorhabdus species using bioinformatics analyses. Generally, the N-terminal signal-binding domain (SBD) of LuxR-type receptors sensing AHLs have a motif of six conserved amino acids that is important for binding and specificity of the signaling molecule. However, this motif is altered in the majority of the Photorhabdus-specific LuxR solos, suggesting the use of other signaling molecules than AHLs. Furthermore, all Photorhabdus species contain at least one LuxR solo with an intact AHL-binding motif, which might allow the ability to sense AHLs of other bacteria. Moreover, all three species have high AHL-degrading activity caused by the presence of different AHL-lactonases and AHL-acylases, revealing a high quorum quenching activity against other bacteria. However, the majority of the other LuxR solos in Photorhabdus have a N-terminal so-called PAS4-domain instead of an AHL-binding domain, containing different amino acid motifs than the AHL-sensors, which potentially allows the recognition of a highly variable range of signaling molecules that can be sensed apart from AHLs. These PAS4-LuxR solos are proposed to be involved in host sensing, and therefore in inter-kingdom signaling. Overall, Photorhabdus species are perfect model organisms to study bacterial communication via LuxR solos and their role for a symbiotic and pathogenic life style.
Die rheumatoide Arthritis (RA) ist eine idiopathische chronisch-entzündliche Systemerkrankung, mit primärer Gelenkmanifestation. Die fortschreitende Gelenkentzündung ist die Folge einer immunologischen Fehlerkennung von Gelenkstrukturen durch dysregulierte B- und T-Lymphozyten. So lassen sich in bis zu 70% der entzündeten Gelenke von RA-Patienten IgG-Autoantikörper gegen das knorpelspezifische Kollagen Typ II (CII) nachweisen.
In dieser Arbeit wurde die CII-Epitop-spezifische humorale Autoimmunantwort in der Pathogenese der RA auf molekularer Ebene analysiert. Im Mittelpunkt stehen hierbei bereits gut charakterisierte B-Zell-Epitope auf dem CII, die über die Speziesbarrieren hinweg evolutionär konserviert sind und sowohl in der humanen RA als auch in der murinen Experimentalerkrankung des CIA-Modell (Collagen-Induced-Arthritis) immundominante Strukturen der humoralen arthritogenen Autoimmunität darstellen.
Ein Teilaspekt der Arbeit war die Aufklärung des molekularen Mechanismus, der den katabolen Effekten des murinen arthritogenen CII-Autoantikörper (UL-1) auf den chondrozytären Matrixmetabolismus zugrunde liegt, gewidmet. Der gegen ein immundominantes Epitop (U1-Epitop) auf dem CII gerichtete monoklonale Antikörper kann unabhängig von seinen Fc-vermittelten inflammatorischen Effektorfunktionen, eine direkte Schädigung der Knorpelmatrix über eine Modulation des Chondrozytenmetabolismus im CIA-Modell bewirken. Basierend auf der Analyse von Sequenzhomologien des U1-Epitopes konnte eine immunologische Kreuzreaktivität mit dem LIF (Leukemia-Inhibitory-Factor)-Rezeptor auf Chondrozyten nachgewiesen werden. Weitergehende funktionelle Studien haben jedoch gezeigt, dass die Rezeptorbindung durch den Antikörper keine intrazellulären Signalwege aktiviert, die an der aus der Literatur bekannten Proteoglykan-depletierenden Wirkung des Zytokins LIF beteiligt sind. Während somit eine UL-1 abhängige Aktivierung des LIF-Rezeptors als Erklärungsmodell der katabolen Antikörperwirkung ausscheidet, konnten die funktionellen in vitro Studien eine spezifische UL-1 Antikörper abhängige Src-Kinaseaktivierung in den humanen Chondrozyten als Ansatzpunkt für zukünftige Studien nachweisen.
In der RA-Pathogenese wird die Bedeutung posttranslationaler Modifikationen, insbesondere der Deiminierung von Argininresten unter Bildung von Citrullin für die Neoepitopgenerierung diskutiert. Autoantikörper gegen citrullinierte Peptide (ACPA, anti-citrullinated-peptides-antibody) gelten als diagnostische und verlaufsprädiktive Marker der RA. Zielstrukturen für ACPAs sind nicht nur einige ubiquitär exprimierte Proteine, sondern auch das knorpelspezifische CII. In dieser Arbeit konnte erstmals die in vitro Bindung CII-spezifischer ACPAs an Knorpelgewebe von RA-Patienten, das als asserviertes Biomaterial aus Synovektomie- bzw. Gelenkersatzoperationen zur Verfügung stand, nachgewiesen werden. Darüber hinaus gelang der erstmalige Nachweis einer chondrozytären Expression der für die posttranslationale Modifikation verantwortlichen Peptidylarginin-Deiminasen (PAD) PAD2 und PAD4 im Knorpelgewebe und ihre Hochregulation in den Chondrozyten unter oxidativem und genotoxischem Stress. Diese Stressoren sind an degenerativen Knorpel-veränderungen in der Pathogenese der Osteoarthrose (OA) beteiligt, sodass die Ergebnisse dieser Arbeit die Hypothese stützen, dass Degenerationsprozesse des alternden Knorpels zur Expression kollagenmodifiziernder PAD-Enzyme führen und damit die immunologische Selbsttoleranz des Knorpelgewebes durch Neoepitop-Generation in der Knorpelmatrix schwächen können.
Ein zentraler Aspekt der Arbeit galt der Analyse der CII-spezifischen humoralen Immunantwort im Blut und in der entzündlich veränderten Synovialmembran von RA-Patienten über die vergleichenden Analyse der rearrangierten Immunglobulingene in epitopspezifisch über biotinylierte CII-Peptide markierten B- und Plasmazellen. Die Isolation der markierten Zellen erfolgte mittels Laser-Mikrodissektion aus dem Gewebe und durchflusszytometrisch aus dem peripheren Blut. Die anschließende Sequenzanalyse der mittels semi-nested Einzelzell-PCR amplifizierten, für die variable Region der leichten und schweren Antikörperkette kodierenden V-Gene, ergab für die Erkennung des immundominanten CIIC1-Epitopes eine präferentielle V-Genverwendung. Darüber hinaus spricht der Nachweis höherer Mutationsraten in synovialen Plasmazellen im Vergleich zu CII-spezifischen B-Zellen im Blut für eine lokale synoviale Affinitätsreifung der Antikörperantwort. Die Klonierung der amplifizierten V-Gene in einen eukaryotischen Expressionsvektor ermöglicht die Expression rekombinanter Antikörper und deren Validierung im ELISA. Zukünftige Affinitätsbestimmungen und Kristallstrukturanalysen dienen dem verbesserten molekularen Verständnis der CII-Antikörpererkennung und murine Antikörper-transferexperimente der Evaluation der Arthritogenität der humanen CII-Antikörperantwort. Fernziel ist die Entwicklung einer auf der CII-Antigenspezifität beruhenden immunmodularischen Therapie der RA.
Die Interaktion zwischen der Kannenpflanze Nepenthes bicalcarata und der mit ihr assoziierten Camponotus schmitzi stand im Zentrum der Arbeit. Dabei wurden vier Themenbereiche zur genaueren Bearbeitung ausgewählt. Drei davon (Kapitel 3, 5 und 6) sind in vier Artikeln bereits in Fachzeitschriften publiziert worden (siehe Kapitel 14.1.2). Die Untersuchungen aus Kapitel 4 sind noch unveröffentlicht. Entsprechend den sich entwickenden Ergebnissen wurden zudem auch vergleichende Untersuchungen zu anderen mehr oder minder im gleichen Habitat vorkommenden Nepenthes Arten, N. gracilis, N. ampullaria, N. mirabilis var echinostoma, N. rafflesiana und N. albomarginata durchgeführt.
The aim of this study was to assess whether endosperm-specific carotenoid biosynthesis influenced core metabolic processes in maize embryo and endosperm and how global seed metabolism adapted to this expanded biosynthetic capacity. Although enhancement of carotenoid biosynthesis was targeted to the endosperm of maize kernels, a concurrent up-regulation of sterol and fatty acid biosynthesis in the embryo was measured. Targeted terpenoid analysis, and non-targeted metabolomic, proteomic, and transcriptomic profiling revealed changes especially in carbohydrate metabolism in the transgenic line. In-depth analysis of the data, including changes of metabolite pools and increased enzyme and transcript concentrations, gave a first insight into the metabolic variation precipitated by the higher up-stream metabolite demand by the extended biosynthesis capacities for terpenoids and fatty acids. An integrative model is put forward to explain the metabolic regulation for the increased provision of terpenoid and fatty acid precursors, particularly glyceraldehyde 3-phosphate and pyruvate or acetyl-CoA from imported fructose and glucose. The model was supported by higher activities of fructokinase, glucose 6-phosphate isomerase, and fructose 1,6-bisphosphate aldolase indicating a higher flux through the glycolytic pathway. Although pyruvate and acetyl-CoA utilization was higher in the engineered line, pyruvate kinase activity was lower. A sufficient provision of both metabolites may be supported by a by-pass in a reaction sequence involving phosphoenolpyruvate carboxylase, malate dehydrogenase, and malic enzyme.
The forest, savanna, and grassland biomes, and the transitions between them, are expected to undergo major changes in the future due to global climate change. Dynamic global vegetation models (DGVMs) are very useful for understanding vegetation dynamics under the present climate, and for predicting its changes under future conditions. However, several DGVMs display high uncertainty in predicting vegetation in tropical areas. Here we perform a comparative analysis of three different DGVMs (JSBACH, LPJ-GUESS-SPITFIRE and aDGVM) with regard to their representation of the ecological mechanisms and feedbacks that determine the forest, savanna, and grassland biomes, in an attempt to bridge the knowledge gap between ecology and global modeling. The outcomes of the models, which include different mechanisms, are compared to observed tree cover along a mean annual precipitation gradient in Africa. By drawing on the large number of recent studies that have delivered new insights into the ecology of tropical ecosystems in general, and of savannas in particular, we identify two main mechanisms that need improved representation in the examined DGVMs. The first mechanism includes water limitation to tree growth, and tree–grass competition for water, which are key factors in determining savanna presence in arid and semi-arid areas. The second is a grass–fire feedback, which maintains both forest and savanna presence in mesic areas. Grasses constitute the majority of the fuel load, and at the same time benefit from the openness of the landscape after fires, since they recover faster than trees. Additionally, these two mechanisms are better represented when the models also include tree life stages (adults and seedlings), and distinguish between fire-prone and shade-tolerant forest trees, and fire-resistant and shade-intolerant savanna trees. Including these basic elements could improve the predictive ability of the DGVMs, not only under current climate conditions but also and especially under future scenarios.
Die im Mittelhirn lokalisierten dopaminergen (DA) Neurone sind in einer Vielzahl von Hirnfunktionen involviert und werden aufgrund von anatomischen, molekularen sowie funktionellen Unterschieden in mehrere Subpopulationen aufgeteilt. DA Neurone, die in der Substantia nigra (SN) pars compacta lokalisiert sind, spielen durch ihre Projektion in das dorsale Striatum eine Rolle in der Steuerung der Willkürmotorik. Die Area tegmentalis ventralis (VTA) enthält DA Neurone, die in den präfrontalen Cortex, die basolateralen Amygdala sowie den Nucleus accumbens projizieren und in höheren kognitiven Funktionen, wie dem Arbeitsgedächtnis, der Motivation sowie belohnungsassoziierten Lernvorgängen involviert sind.
In dieser Arbeit wurden die differentiellen Eigenschaften des transienten A-Typ Kaliumstroms sowie dessen Funktion für die intrinsische elektrische Aktivität und die Integration von synaptischen Eingängen in Subpopulationen von DA Neuronen untersucht. Dieser spannungsgesteuerte Strom ist an der Kontrolle der Schrittmacheraktivität beteiligt, beeinflusst die Form und Dauer von Aktionspotentialen und moduliert die Erregbarkeit des somatodendritischen Kompartiments. Der A-Typ Kaliumkanal besteht in DA Neuronen aus einem Tetramer von porenbildenden KV4.3 α-Untereinheiten. Die Koexpression von akzessorischen β-Untereinheiten moduliert maßgeblich die biophysikalischen Parameter des A-Stroms, wie z. B. die Kinetik der Inaktivierung sowie die Spannungsabhängigkeit der Aktivierung und Inaktivierung. Zu diesen β-Untereinheiten gehören die cytoplasmatischen Kaliumkanal-interagierenden Proteine (KChIPs) sowie die transmembranären Dipeptidylpeptidase-ähnlichen Proteine (DPPLs). Während in DA SN Neuronen vor allem KChIP3 exprimiert wird und einen schnell inaktivierenden A-Strom gewährleistet, sind DA VTA Neurone durch die zusätzliche Expression der KChIP4a Splice-Variante charakterisiert, welche durch Inhibition der schnellen Inaktivierung in einem langsam inaktivierenden A-Strom resultiert. Die Bedeutung der differentiellen KChIP4a-Expression für DA Mittelhirnneurone wurde mit Hilfe von KChIP4-Knock-Out (KO)-Mäusen untersucht. Alle Versuche wurden in vitro an akuten Hirnschnitten adulter Wildtyp (WT)- und KChIP4-KO-Tiere durchgeführt und die DA neurochemische Identität sowie die Lage der gemessenen Zellen im Anschluss immunhistochemisch bestätigt. Die biophysikalischen Eigenschaften des A-Stroms wurden mit der Patch-Clamp Technik in der nucleated outside-out Konfiguration untersucht, welche optimale Bedingungen für Voltage-Clamp Experimente gewährleistet. Der A-Strom in DA VTA Neuronen aus KChIP4-KO-Tieren wies dabei eine siebenfach schnellere Inaktivierungskinetik als in vergleichbaren Neuronen aus WT-Tieren auf, während die Inaktivierungskinetik in DA SN Neuronen aus KChIP4-KO-Tieren lediglich um den Faktor zwei schneller war. Außerdem wurde festgestellt, dass selektiv in DA VTA Neuronen das halbmaximale Aktivierungspotential ebenfalls von der KChIP4-Expression abhängig war. Somit konnte gezeigt werden, dass die Expression von KChIP4 für die charakteristischen A-Strom-Eigenschaften von DA VTA Neuronen verantwortlich ist.
Die funktionelle Rolle des KChIP4-vermittelten langsamen A-Stroms wurde mit Hilfe von Current-Clamp Messungen in Ganzzellableitungen untersucht. Dabei wurde deutlich, dass die Expression von KChIP4 die Spontanaktivität von DA SN und VTA Neuronen nicht beeinflusst. Das für DA VTA Neuronen charakteristische verzögerte Wiedereintreten der Spontanaktivität nach einer Inhibition zeigte allerdings eine Abhängigkeit von der KChIP4-Expression, da der sog. rebound delay in DA VTA Neuronen aus KChIP4-KO-Tieren signifikant kürzer war, als in Zellen aus WT-Tieren. Dies konnte sowohl durch Strominjektionen, die in ihrer Kinetik GABAergen synaptischen Eingängen ähnelten, als auch nach direkter Aktivierung von GABA-Rezeptoren durch iontophoretische GABA-Applikation bestätigt werden. KChIP4 könnte somit einen internen Verzögerungsmechanismus nach einer transienten Inhibition von DA Neuronen gewährleisten, die z.B. bei Präsentation von aversiven Stimuli sowie beim Ausbleiben von erwarteten Belohnungen auftritt. Somit könnte die physiologische Relevanz des KChIP4-gesteuerten A-Stroms in der Integration von inhibitorischen synaptischen Eingängen im Kontext von belohnungsgesteuerten Lernprozessen liegen.
Ongoing and predicted global change makes understanding and predicting species’ range shifts an urgent scientific priority. Here, we provide a synthetic perspective on the so far poorly understood effects of interspecific interactions on range expansion rates. We present theoretical foundations for how interspecific interactions may modulate range expansion rates, consider examples from empirical studies of biological invasions and natural range expansions as well as process-based simulations, and discuss how interspecific interactions can be more broadly represented in process-based, spatiotemporally explicit range forecasts. Theory tells us that interspecific interactions affect expansion rates via alteration of local population growth rates and spatial displacement rates, but also via effects on other demographic parameters. The best empirical evidence for interspecific effects on expansion rates comes from studies of biological invasions. Notably, invasion studies indicate that competitive dominance and release from specialized enemies can enhance expansion rates. Studies of natural range expansions especially point to the potential for competition from resident species to reduce expansion rates. Overall, it is clear that interspecific interactions may have important consequences for range dynamics, but also that their effects have received too little attention to robustly generalize on their importance. We then discuss how interspecific interactions effects can be more widely incorporated in dynamic modeling of range expansions. Importantly, models must describe spatiotemporal variation in both local population dynamics and dispersal. Finally, we derive the following guidelines for when it is particularly important to explicitly represent interspecific interactions in dynamic range expansion forecasts: if most interacting species show correlated spatial or temporal trends in their effects on the target species, if the number of interacting species is low, and if the abundance of one or more strongly interacting species is not closely linked to the abundance of the target species.
Translation fidelity and efficiency require multiple ribosomal (r)RNA modifications that are mostly mediated by small nucleolar (sno)RNPs during ribosome production. Overlapping basepairing of snoRNAs with pre-rRNAs often necessitates sequential and efficient association and dissociation of the snoRNPs, however, how such hierarchy is established has remained unknown so far. Here, we identify several late-acting snoRNAs that bind pre-40S particles in human cells and show that their association and function in pre-40S complexes is regulated by the RNA helicase DDX21. We map DDX21 crosslinking sites on pre-rRNAs and show their overlap with the basepairing sites of the affected snoRNAs. While DDX21 activity is required for recruitment of the late-acting snoRNAs SNORD56 and SNORD68, earlier snoRNAs are not affected by DDX21 depletion. Together, these observations provide an understanding of the timing and ordered hierarchy of snoRNP action in pre-40S maturation and reveal a novel mode of regulation of snoRNP function by an RNA helicase in human cells.
The ancestors to the Australian marsupials entered Australia around 60 (54-72) million years ago from Antarctica, and radiated into the four living orders Peramelemorphia, Dasyuromorphia, Diprotodontia and Notoryctemorphia. The relationship between the four Australian marsupial orders has been a long-standing question, because different phylogenetic studies were not able to consistently reconstruct the same topology. Initial in silico analysis of the Tasmanian devil genome and experimental screening in the seven marsupial orders revealed 20 informative transposable element insertions for resolving the inter- and intraordinal relationships of Australian and South American orders. However, the retrotransposon insertions support three conflicting topologies regarding Peramelemorphia, Dasyuromorphia and Notoryctemorphia, indicating that the split between the three orders may be best understood as a network. This finding is supported by a phylogenetic re-analysis of nuclear gene sequences, using a consensus network approach that allows depicting hidden phylogenetic conflict, otherwise lost when forcing the data into a bifurcating tree. The consensus network analysis agrees with the transposable element analysis in that all possible topologies regarding Peramelemorphia, Dasyuromorphia, and Notoryctemorphia in a rooted four-taxon topology are equally well supported. In addition, retrotransposon insertion data supports the South American order Didelphimorphia being the sistergroup to all other living marsupial orders. The four Australian orders originated within three million years at the Cretaceous-Paleogene boundary. The rapid divergences left conflicting phylogenetic information in the genome possibly generated by incomplete lineage sorting or introgressive hybridisation, leaving the relationship among Australian marsupial orders unresolvable as a bifurcating process million years later.
One of the most challenging aspects of RT-qPCR data analysis is the identification of reliable reference genes. Ideally, they should be neither induced nor repressed under different experimental conditions. To date, few reference genes have been adequately studied for sugarcane (Saccharum spp.) using statistical approaches. In this work, six candidate genes (αTUB, GAPDH, H1, SAMDC, UBQ, and 25S rRNA) were tested for gene expression normalization of sugarcane root tissues from drought-tolerant and -sensitive accessions after continuous dehydration (24 h). By undergoing different approaches (GeNorm, NormFinder, and BestKeeper), it was shown that most of them could be used in combinations for normalization purposes, with the exception of SAMDC. Nevertheless three of them (H1, αTUB, and GAPDH) were considered the most reliable reference genes. Their suitability as reference genes validated the expression profiles of two targets (AS and PFPα1), related to SuperSAGE unitags, in agreement with results revealed by previous in silico analysis. The other two sugarcane unitags (ACC oxidase and PIP1-1), after salt stress (100 mM NaCl), presented their expressions validated in the same way. In conclusion, these reference genes will be useful for dissecting gene expression in sugarcane roots under abiotic stress, especially in transcriptomic studies using SuperSAGE or RNAseq approaches.
Ursine bears are a mammalian subfamily that comprises six morphologically and ecologically distinct extant species. Previous phylogenetic analyses of concatenated nuclear genes could not resolve all relationships among bears, and appeared to conflict with the mitochondrial phylogeny. Evolutionary processes such as incomplete lineage sorting and introgression can cause gene tree discordance and complicate phylogenetic inferences, but are not accounted for in phylogenetic analyses of concatenated data. We generated a high-resolution data set of autosomal introns from several individuals per species and of Y-chromosomal markers. Incorporating intraspecific variability in coalescence-based phylogenetic and gene flow estimation approaches, we traced the genealogical history of individual alleles. Considerable heterogeneity among nuclear loci and discordance between nuclear and mitochondrial phylogenies were found. A species tree with divergence time estimates indicated that ursine bears diversified within less than 2 My. Consistent with a complex branching order within a clade of Asian bear species, we identified unidirectional gene flow from Asian black into sloth bears. Moreover, gene flow detected from brown into American black bears can explain the conflicting placement of the American black bear in mitochondrial and nuclear phylogenies. These results highlight that both incomplete lineage sorting and introgression are prominent evolutionary forces even on time scales up to several million years. Complex evolutionary patterns are not adequately captured by strictly bifurcating models, and can only be fully understood when analyzing multiple independently inherited loci in a coalescence framework. Phylogenetic incongruence among gene trees hence needs to be recognized as a biologically meaningful signal.
The degradation of natural forests to modified forests threatens subtropical and tropical biodiversity worldwide. Yet, species responses to forest modification vary considerably. Furthermore, effects of forest modification can differ, whether with respect to diversity components (taxonomic or phylogenetic) or to local (α-diversity) and regional (β-diversity) spatial scales. This real-world complexity has so far hampered our understanding of subtropical and tropical biodiversity patterns in human-modified forest landscapes. In a subtropical South African forest landscape, we studied the responses of three successive plant life stages (adult trees, saplings, seedlings) and of birds to five different types of forest modification distinguished by the degree of within-forest disturbance and forest loss. Responses of the two taxa differed markedly. Thus, the taxonomic α-diversity of birds was negatively correlated with the diversity of all plant life stages and, contrary to plant diversity, increased with forest disturbance. Conversely, forest disturbance reduced the phylogenetic α-diversity of all plant life stages but not that of birds. Forest loss neither affected taxonomic nor phylogenetic diversity of any taxon. On the regional scale, taxonomic but not phylogenetic β-diversity of both taxa was well predicted by variation in forest disturbance and forest loss. In contrast to adult trees, the phylogenetic diversity of saplings and seedlings showed signs of contemporary environmental filtering. In conclusion, forest modification in this subtropical landscape strongly shaped both local and regional biodiversity but with contrasting outcomes. Phylogenetic diversity of plants may be more threatened than that of mobile species such as birds. The reduced phylogenetic diversity of saplings and seedlings suggests losses in biodiversity that are not visible in adult trees, potentially indicating time-lags and contemporary shifts in forest regeneration. The different responses of taxonomic and phylogenetic diversity to forest modifications imply that biodiversity conservation in this subtropical landscape requires the preservation of natural and modified forests.
By far not all genetic information is expressed by mRNA coding regions of the DNA. 98% of the human genome is not encoding for proteins. Therefore, these non-coding regions have been considered as “junk DNA” for a long time [1, 2]. The last years, new high throughput sequencing techniques have allowed the elucidation of the heterogeneous population of non-coding RNAs (ncRNAs, Table 1). RNAs longer than 200 nucleotides (nt) belong to the family of long non-coding RNAs (lncRNAs). They can exhibit numerous functions: The biggest family of RNAs is represented by the ribosomal RNAs (rRNAs). Together with the transfer RNAs (tRNAs) they are essential for the translation of mRNA into an amino acid sequence.
Mit dem Namen Gerhard Quinkert verbindet man in Frankfurt vor allem die Öffnung der Chemie für die Biologie. Das war damals ein außergewöhnlicher Schritt, der dank einer gezielten Berufungspolitik realisiert wurde. Der Organische Chemiker hat das "Frankfurter Modell" Ende der 1970er Jahre entwickelt.
Jetzt, nach Beendigung vieler Jahre der Lehre und Forschung an der Goethe-Universität, kann ich diese Zeit mit einem Abstand überdenken. Der Freiraum für solch nicht zweckgerichtetes Verhalten ist während der praktischen Tätigkeit an der Universität äußerst gering und muss hart erkämpft werden, wie jedes Stück Freiheit. Rückblickend sehe ich, dass der Wunsch, über das Detailwissen hinaus ganzheitliche Zusammenhänge zu betrachten und über die eigene Fachgrenze hinauszugehen, meinen Weg geprägt hat.
DNA damage in oocytes induces a switch of the quality control factor TAp63α from dimer to tetramer
(2011)
TAp63a, a homolog of the p53 tumor suppressor, is a quality control factor in the female germline. Remarkably, already undamaged oocytes express high levels of the protein, suggesting that TAp63a’s activity is under tight control of an inhibitory mechanism. Biochemical studies have proposed that inhibition requires the C-terminal transactivation inhibitory domain. However, the structural mechanism of TAp63a inhibition remains unknown. Here, we show that TAp63a is kept in an inactive dimeric state. We reveal that relief of inhibition leads to tetramer formation with ~20-fold higher DNA affinity. In vivo, phosphorylation-triggered tetramerization of TAp63a is not reversible by dephosphorylation. Furthermore, we show that a helix in the oligomerization domain of p63 is crucial for tetramer stabilization and competes with the transactivation domain for the same binding site. Our results demonstrate how TAp63a is inhibited by complex domain-domain interactions that provide the basis for regulating quality control in oocytes.
Here we present a formal description of Biremis panamae Barka, Witkowski et Weisenborn sp. nov., which was isolated from the marine littoral environment of the Pacific Ocean coast of Panama. The description is based on morphology (light and electron microscopy) and the rbcL, psbC and SSU sequences of one clone of this species. The new species is included in Biremis due to its morphological features; i.e. two marginal rows of foramina, chambered striae, and girdle composed of numerous punctate copulae. The new species also possesses a striated valve face which is not seen in most known representatives of marine littoral Biremis species. In this study we also present the relationship of Biremis to other taxa using morphology, DNA sequence data and observations of auxosporulation. Our results based on these three sources point to an evolutionary relationship between Biremis, Neidium and Scoliopleura. The unusual silicified incunabular caps present in them are known otherwise only in Muelleria, which is probably related to the Neidiaceae and Scoliotropidaceae. We also discuss the relationship between Biremis and the recently described Labellicula and Olifantiella.