@article{StangeDesirKakaretal.2015,
  author    = {Stange, Katja and D{\´e}sir, Julie and Kakar, Naseebullah and Mueller, Thomas D. and Budde, Birgit S. and Gordon, Christopher T. and Horn, Denise and Seemann, Petra and Borck, Guntram},
  title     = {A hypomorphic BMPR1B mutation causes du Pan acromesomelic dysplasia},
  series = {Orphanet Journal of Rare Diseases},
  volume    = {10},
  journal   = {Orphanet Journal of Rare Diseases},
  number    = {84},
  doi       = {10.1186/s13023-015-0299-5},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-151650},
  year      = {2015},
  abstract  = {Background: Grebe dysplasia, Hunter-Thompson dysplasia, and du Pan dysplasia constitute a spectrum of skeletal dysplasias inherited as an autosomal recessive trait characterized by short stature, severe acromesomelic shortening of the limbs, and normal axial skeleton. The majority of patients with these disorders have biallelic loss-of-function mutations of GDF5. In single instances, Grebe dysplasia and a Grebe dysplasia-like phenotype with genital anomalies have been shown to be caused by mutations in BMPR1B, encoding a GDF5 receptor. Methods: We clinically and radiologically characterised an acromesomelic chondrodysplasia in an adult woman born to consanguineous parents. We sequenced GDF5 and BMPR1B on DNA of the proposita. We performed 3D structural analysis and luciferase reporter assays to functionally investigate the identified BMPR1B mutation. Results: We extend the genotype-phenotype correlation in the acromesomelic chondrodysplasias by showing that the milder du Pan dysplasia can be caused by a hypomorphic BMPR1B mutation. We show that the homozygous c.91C>T, p.(Arg31Cys) mutation causing du Pan dysplasia leads to a significant loss of BMPR1B function, but to a lesser extent than the previously reported p.Cys53Arg mutation that results in the more severe Grebe dysplasia. Conclusions: The phenotypic severity gradient of the clinically and radiologically related acromesomelic chondrodysplasia spectrum of skeletal disorders may be due to the extent of functional impairment of the ligand-receptor pair GDF5-BMPR1B.},
  language  = {en}
}
@article{PlanesNinolesRubioetal.2015,
  author    = {Planes, Maria D. and Ni{\~n}oles, Regina and Rubio, Lourdes and Bissoli, Gaetano and Bueso, Eduardo and Garc{\´i}a-S{\´a}nchez, Mar{\´i}a J. and Alejandro, Santiago and Gonzalez-Guzm{\´a}n, Miguel and Hedrich, Rainer and Rodriguez, Pedro L. and Fern{\´a}ndez, Jos{\´e} A. and Serrano, Ram{\´o}n},
  title     = {A mechanism of growth inhibition by abscisic acid in germinating seeds of Arabidopsis thaliana based on inhibition of plasma membrane \(H^+\)-ATPase and decreased cytosolic pH, \(K^+\), and anions},
  series = {Journal of Experimental Botany},
  volume    = {66},
  journal   = {Journal of Experimental Botany},
  number    = {3},
  doi       = {10.1093/jxb/eru442},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-121221},
  pages     = {813-25},
  year      = {2015},
  abstract  = {The stress hormone abscisic acid (ABA) induces expression of defence genes in many organs, modulates ion homeostasis and metabolism in guard cells, and inhibits germination and seedling growth. Concerning the latter effect, several mutants of Arabidopsis thaliana with improved capability for \(H^+\) efflux (wat1-1D, overexpression of AKT1 and ost2-1D) are less sensitive to inhibition by ABA than the wild type. This suggested that ABA could inhibit \(H^+\) efflux (\(H^+\)-ATPase) and induce cytosolic acidification as a mechanism of growth inhibition. Measurements to test this hypothesis could not be done in germinating seeds and we used roots as the most convenient system. ABA inhibited the root plasma-membrane H+-ATPase measured in vitro (ATP hydrolysis by isolated vesicles) and in vivo (\(H^+\) efflux from seedling roots). This inhibition involved the core ABA signalling elements: PYR/PYL/RCAR ABA receptors, ABA-inhibited protein phosphatases (HAB1), and ABA-activated protein kinases (SnRK2.2 and SnRK2.3). Electrophysiological measurements in root epidermal cells indicated that ABA, acting through the PYR/PYL/RCAR receptors, induced membrane hyperpolarization (due to \(K^+\) efflux through the GORK channel) and cytosolic acidification. This acidification was not observed in the wat1-1D mutant. The mechanism of inhibition of the \(H^+\)-ATPase by ABA and its effects on cytosolic pH and membrane potential in roots were different from those in guard cells. ABA did not affect the in vivo phosphorylation level of the known activating site (penultimate threonine) of (\(H^+\)-ATPase in roots, and SnRK2.2 phosphorylated in vitro the C-terminal regulatory domain of (\(H^+\)-ATPase while the guard-cell kinase SnRK2.6/OST1 did not.},
  language  = {en}
}
@article{SexauerBhasinSchoenetal.2023,
  author    = {Sexauer, Moritz and Bhasin, Hemal and Sch{\"o}n, Maria and Roitsch, Elena and Wall, Caroline and Herzog, Ulrike and Markmann, Katharina},
  title     = {A micro RNA mediates shoot control of root branching},
  series = {Nature Communications},
  volume    = {14},
  journal   = {Nature Communications},
  doi       = {10.1038/s41467-023-43738-6},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-357472},
  year      = {2023},
  abstract  = {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.},
  language  = {en}
}
@article{PalamidesJodeleitFoehlingeretal.2016,
  author    = {Palamides, Pia and Jodeleit, Henrika and F{\"o}hlinger, Michael and Beigel, Florian and Herbach, Nadja and Mueller, Thomas and Wolf, Eckhard and Siebeck, Matthias and Gropp, Roswitha},
  title     = {A mouse model for ulcerative colitis based on NOD-scid IL2R gamma(null) mice reconstituted with peripheral blood mononuclear cells from affected individuals},
  series = {Disease Models \& Mechanisms},
  volume    = {9},
  journal   = {Disease Models \& Mechanisms},
  doi       = {10.1242/dmm.025452},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-164946},
  pages     = {985-997},
  year      = {2016},
  abstract  = {Animal models reflective of ulcerative colitis (UC) remain a major challenge, and yet are crucial to understand mechanisms underlying the onset of disease and inflammatory characteristics of relapses and remission. Mouse models in which colitis-like symptoms are induced through challenge with toxins such as oxazolone, dextran sodium sulfate (DSS) or 2,4,6-trinitrobenzenesulfonic acid (TNBS) have been instrumental in understanding the inflammatory processes of UC. However, these neither reflect the heterogeneous symptoms observed in the UC-affected population nor can they be used to test the efficacy of inhibitors developed against human targets where high sequence and structural similarity of the respective ligands is lacking. In an attempt to overcome these problems, we have developed a mouse model that relies on NOD-scid IL2R γnull mice reconstituted with peripheral blood mononuclear cells derived from UC-affected individuals. Upon challenge with ethanol, mice developed colitis-like symptoms and changes in the colon architecture, characterized by influx of inflammatory cells, edema, crypt loss, crypt abscesses and epithelial hyperplasia, as previously observed in immune-competent mice. TARC, TGFβ1 and HGF expression increased in distal parts of the colon. Analysis of human leucocytes isolated from mouse spleen revealed an increase in frequencies of CD1a+, CD64+, CD163+ and TSLPR+ CD14+ monocytes, and antigen-experienced CD44+ CD4+ and CD8+ T-cells in response to ethanol. Analysis of human leucocytes from the colon of challenged mice identified CD14+ monocytes and CD11b+ monocytes as the predominant populations. Quantitative real-time PCR (RT-PCR) analysis from distal parts of the colon indicated that IFNγ might be one of the cytokines driving inflammation. Treatment with infliximab ameliorated symptoms and pathological manifestations, whereas pitrakinra had no therapeutic benefit. Thus, this model is partially reflective of the human disease and might help to increase the translation of animal and clinical studies.},
  language  = {en}
}
@article{JahnSchmidtMock2014,
  author    = {Jahn, Martin T. and Schmidt, Katrin and Mock, Thomas},
  title     = {A novel cost effective and high-throughput isolation and identification method for marine microalgae},
  series = {Plant Methods},
  volume    = {10},
  journal   = {Plant Methods},
  number    = {26},
  doi       = {10.1186/1746-4811-10-26},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-121255},
  year      = {2014},
  abstract  = {BACKROUND: Marine microalgae are of major ecologic and emerging economic importance. Biotechnological screening schemes of microalgae for specific traits and laboratory experiments to advance our knowledge on algal biology and evolution strongly benefit from culture collections reflecting a maximum of the natural inter- and intraspecific diversity. However, standard procedures for strain isolation and identification, namely DNA extraction, purification, amplification, sequencing and taxonomic identification still include considerable constraints increasing the time required to establish new cultures. RESULTS: In this study, we report a cost effective and high-throughput isolation and identification method for marine microalgae. The throughput was increased by applying strain isolation on plates and taxonomic identification by direct PCR (dPCR) of phylogenetic marker genes in combination with a novel sequencing electropherogram based screening method to assess the taxonomic diversity and identity of the isolated cultures. For validation of the effectiveness of this approach, we isolated and identified a range of unialgal cultures from natural phytoplankton communities sampled in the Arctic Ocean. These cultures include the isolate of a novel marine Chlorophyceae strain among several different diatoms. CONCLUSIONS: We provide an efficient and effective approach leading from natural phytoplankton communities to isolated and taxonomically identified algal strains in only a few weeks. Validated with sensitive Arctic phytoplankton, this approach overcomes the constraints of standard molecular characterisation and establishment of unialgal cultures."},
  language  = {en}
}
@article{ShepardChevalPeterlinetal.2016,
  author    = {Shepard, Blythe D. and Cheval, Lydie and Peterlin, Zita and Firestein, Stuart and Koepsell, Hermann and Doucet, Alain and Pluznick, Jennifer L.},
  title     = {A Renal Olfactory Receptor Aids in Kidney Glucose Handling},
  series = {Scientific Reports},
  volume    = {6},
  journal   = {Scientific Reports},
  number    = {35215},
  doi       = {10.1038/srep35215},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-167605},
  year      = {2016},
  abstract  = {Olfactory receptors (ORs) are G protein-coupled receptors which serve important sensory functions beyond their role as odorant detectors in the olfactory epithelium. Here we describe a novel role for one of these ORs, Olfr1393, as a regulator of renal glucose handling. Olfr1393 is specifically expressed in the kidney proximal tubule, which is the site of renal glucose reabsorption. Olfr1393 knockout mice exhibit urinary glucose wasting and improved glucose tolerance, despite euglycemia and normal insulin levels. Consistent with this phenotype, Olfr1393 knockout mice have a significant decrease in luminal expression of Sglt1, a key renal glucose transporter, uncovering a novel regulatory pathway involving Olfr1393 and Sglt1. In addition, by utilizing a large scale screen of over 1400 chemicals we reveal the ligand profile of Olfr1393 for the first time, offering new insight into potential pathways of physiological regulation for this novel signaling pathway.},
  language  = {en}
}
@article{HarthKotzschHuetal.2010,
  author    = {Harth, Stefan and Kotzsch, Alexander and Hu, Junli and Sebald, Walter and Mueller, Thomas D.},
  title     = {A Selection Fit Mechanism in BMP Receptor IA as a Possible Source for BMP Ligand-Receptor Promiscuity},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-68497},
  year      = {2010},
  abstract  = {Background: Members of the TGF-b superfamily are characterized by a highly promiscuous ligand-receptor interaction as is readily apparent from the numeral discrepancy of only seven type I and five type II receptors available for more than 40 ligands. Structural and functional studies have been used to address the question of how specific signals can be deduced from a limited number of receptor combinations and to unravel the molecular mechanisms underlying the protein-protein recognition that allow such limited specificity. Principal Findings: In this study we have investigated how an antigen binding antibody fragment (Fab) raised against the extracellular domain of the BMP receptor type IA (BMPR-IA) recognizes the receptor's BMP-2 binding epitope and thereby neutralizes BMP-2 receptor activation. The crystal structure of the complex of the BMPR-IA ectodomain bound to the Fab AbD1556 revealed that the contact surface of BMPR-IA overlaps extensively with the contact surface for BMP-2 interaction. Although the structural epitopes of BMPR-IA to both binding partners coincides, the structures of BMPR-IA in the two complexes differ significantly. In contrast to the structural differences, alanine-scanning mutagenesis of BMPR-IA showed that the functional determinants for binding to the antibody and BMP-2 are almost identical. Conclusions: Comparing the structures of BMPR-IA bound to BMP-2 or bound to the Fab AbD1556 with the structure of unbound BMPR-IA shows that binding of BMPR-IA to its interaction partners follows a selection fit mechanism, possibly indicating that the ligand promiscuity of BMPR-IA is inherently encoded by structural adaptability. The functional and structural analysis of the BMPR-IA binding antibody AbD1556 mimicking the BMP-2 binding epitope may thus pave the way for the design of low-molecular weight synthetic receptor binders/inhibitors.},
  subject      = {Physiologische Chemie},
  language  = {en}
}
@article{DindasDreyerHuangetal.2021,
  author    = {Dindas, Julian and Dreyer, Ingo and Huang, Shouguang and Hedrich, Rainer and Roelfsema, M. Rob G.},
  title     = {A voltage-dependent Ca\(^{2+}\) homeostat operates in the plant vacuolar membrane},
  series = {New Phytologist},
  volume    = {230},
  journal   = {New Phytologist},
  number    = {4},
  doi       = {10.1111/nph.17272},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-259627},
  pages     = {1449-1460},
  year      = {2021},
  abstract  = {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.},
  language  = {en}
}
@phdthesis{Nhan2007,
  author    = {Nhan, Pham Phuoc},
  title     = {Accumulation and biological activity of oxidized lipids in Anabaena PCC 7120},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-24347},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2007},
  abstract  = {Oxylipine sind wichtige biologisch aktive Verbindungen, die entscheidende Rollen in der Abwehr, dem Wachstum, der Entwicklung und der Reproduktion von Pflanzen und Tieren spielen. Oxylipine k{\"o}nnen entweder {\"u}ber enzymatische Wege oder eine Radikal-katalysierte Reaktion gebildet werden. Enzymatische und nicht-enzymatische Oxidationsprodukte der Arachidons{\"a}ure (C20:4) in Tieren sind Prostaglandine und Isoprostane. In Pflanzen werden ausgehend von der \&\#61537;-Linolens{\"a}ure (C18:3) {\"u}ber einen enzymatischen Weg OPDA und Jasmons{\"a}ure und durch Radikal-katalysierte Reaktion Phytoprostane gebildet. Die Membranen von Cyanobakterien enthalten, {\"a}hnlich denen von Pflanzen, einen großen Anteil an mehrfach unges{\"a}ttigten Fetts{\"a}uren, ca. 25\% der gesamten Fetts{\"a}uren. Biosynthese und Funktionen der Oxylipine wurden an zwei Modell-Cyanobakterien, Anabaena PCC 7120 und Synechocystis PCC 6803 untersucht: 1. Das fadenf{\"o}rmige Cyanobakterium Anabaena PCC 7120 kann Phytoprostane Typ I und II sowie Hydroxyfetts{\"a}uren {\"a}hnlich wie Pflanzen produzieren aber die enzymatische Ausstattung zur Bildung von Jasmonaten (12-oxo-Phytodiens{\"a}ure und Jasmons{\"a}ure) und Prostaglandinen ist nicht vorhanden. Die erhaltenen Daten stellen den ersten Nachweis f{\"u}r das Vorkommen von Phytoprostanen in Cyanobakterien bzw. bei Prokaryonten dar. 2. Durch GC-MS Analyse wurden E1- and F1-Phytoprostane in Anabaena PCC 7120 in freier und veresterter Form detektiert. Die Spiegel sind vergleichbar mit denen in Pflanzen und lagen im Bereich von ng/g TG. PPF1 ließen sich nicht in einw{\"o}chigen Kulturen nachweisen, die Spiegel in sechsw{\"o}chigen Kulturen lagen bei 142 ng/l. Die Spiegel von PPE1 waren hingegen in ein- und sechsw{\"o}chigen Kulturen {\"a}hnlich und lagen bei ca. 20 ng/g TG. Die Mengen an freien PPE1 in den Zellen waren mit 80.5 \&\#61617; 23.6 etwa viermal h{\"o}her als die von PPF1 mit 24.1 \&\#61617; 10.9 ng/g TG. Allerdings gab es keine signifikanten Unterschiede in den Spiegeln an gesamten PPF1 und PPE1 in den Zellen, sie lagen im Bereich von 150 bis zu ca. 200 ng/g TG. 3. Die Akkumulation von Phytoprostanen in Anabaena ist induzierbar. Nach der Kombination von oxidativem Stress (200 µM H2O2 oder 10 µM CuSO4) und hoher Lichtintensit{\"a}t (330 µE.m-2.s-1) f{\"u}r 8 h stiegen die Spiegel an gesamten PPE1 und PPF1 um den Faktor 2 bis 4 an. Interessanterweise f{\"u}hrte im Gegensatz zu h{\"o}heren Pflanzen die Applikation von oxidativem Stress oder hoher Lichtintensit{\"a}t alleine nicht zur Induktion der Phytoprostanakkumulation in diesen Cyanobakterien. 4. Eine Vorbehandlung von Anabaena Zellen mit exogenen Phytoprostanen f{\"u}hrte zu einer erh{\"o}hten Toleranz gegen{\"u}ber oxidativem Stress. Alle Phytoprostane außer PPE1 zeigten einen Schutzeffekt. Eine Mischung von PPA1 Typ I und II ergab den h{\"o}chsten Schutzeffekt. Eine Vorinkubation von Anabena Zellen mit 100 µM PPA1-type I/II f{\"u}r 16 h sch{\"u}tzte 84.2\% beziehungsweise 77.5\% der Zellen vor einer anschießenden lethalen Applikation von 1 mM H2O2 beziehungsweise 50 µM CuSO4 f{\"u}r 5 h. Ohne eine Oxylipin-Vorinkubation starben etwa 98\% der Zellen. {\"U}berraschenderweise ergab auch die Vorbehandlung mit anderen, enzymatisch gebildeten Oxylipinen aus Tieren und Pflanzen einen Schutzeffekt, der allerdings nur 10 bis 30\% betrug. Dagegen sch{\"u}tzte eine Phytoprostan-Vorbehandlung nicht Pseudomonas syringae und Escherichia coli gegen toxische Mengen von Wasserstoffperoxid. Allerdings fehlen in den Membranen dieser Bakterien mehrfach unges{\"a}ttigte Fetts{\"a}uren und deshalb endogen oxydierte Lipide. 5. Eine exogene Applikation von 100 µM PPF1 oder 1,5 mM H2O2 f{\"u}hrte in Anabaena nicht zu einer Induktion der Expression des isiA Gens. Oxylipin-Behandlungen zeigten auch keine Wirkung auf Shinorin- und Tocopherol-Spiegel in Anabaena. Die Applikation von 100 µM PPF1 f{\"u}r 6 h f{\"u}hrte aber zu {\"A}nderungen im Proteinmuster in Anabaena. Der gr{\"o}ßte Teil der differentiellen Proteine wurde durch PPF1 herunterreguliert. Bei vielen dieser Proteine handelt es sich um photosynthetische Proteine. Da ein oxidativer Stress nur in der Kombination mit hoher Lichtintensit{\"a}t die Lipidperoxidation erh{\"o}ht, k{\"o}nnte die negative Regulation der Photosynthese nach Erkennung von oxydierten Lipiden (Phytoprostanen) eine {\"U}berlebens-Strategie sein um Sch{\"a}den durch peroxidierte Lipide zu vermeiden. 6. Tote Pflanzen k{\"o}nnten eine haupts{\"a}chliche Quelle der exogenen Phytoprostane in der nat{\"u}rlichen Umgebung von Anabaena sein. Trockenes Heu gibt PPE1 und PPF1 (11 µg/g TG) an die w{\"a}sserige Umgebung ab. Anabaena ist ein typisches Cyanobakterium in Reisfeldern. Nach der Ernte bleiben meist die nicht genutzten Teile der Reispflanzen auf dem Feld. Diese k{\"o}nnten Phytoprostane abgeben, die wiederum einen Einfluß auf die Cyanobakterien im Reis-{\"O}kosystem haben k{\"o}nnten. 7. Eine neue Kategorie von Oxylipinen, die Phytoprostane Typ III und IV, wurden in vitro identifiziert und quantifiziert. Die beiden Haupt-Phytoprostane, PPE1 und PPF1 (Typ III und IV), k{\"o}nnen durch die Autoxidation der \&\#61543;-Linolens{\"a}ure oder des Borretschsamen{\"o}ls (enth{\"a}lt 25\% der \&\#61543;-Linolens{\"a}ure) gewonnen werden. Nach 12 Tagen Autoxidation und anschließender Hydrolyse wurden aus 1 g Borretschsamen{\"o}l 112,71 ± 1,93 µg PPF1 und 3,80 ± 0,14 mg PPE1 isoliert. PPB1 und PPA1 (Typ III und IV) wurden durch Isomerisierung und Dehydratisierung von PPE1 hergestellt. Die Ausbeute von PPB1 lag bei 1,71 ± 0,04 mg/g {\"O}l (Typ III) und 2,09 ± 0,12 mg/g {\"O}l (Typ IV), die von PPA1 lag bei 8,38 ± 0,35 µg/g und 10,18 ± 0,30 µg/g {\"O}l. 8. Es wurde eine schnelle HPLC-MS/MS Methode f{\"u}r die Analytik der Phytoprostane und Phytohormone entwickelt. Diese Methode wurde f{\"u}r die Quantifizierung von freien und veresterten E1- and F1-Phytoprostane Typ III und IV in Synechocystis PCC 6803 angewendet. Die Phytoprostane Typ III und IV sind in vivo in freier und veresterter Form vorhanden. Die Spiegel der gesamten PPE1 Typ III und IV in Synechocystis sind mindestens doppelt so hoch wie die von PPF1. Im Gegensatz zu Anabaena, waren PPE1 und PPF1 in ein- und sechsw{\"o}chigen Kulturen von Synechocystis detektierbar. Die Spiegel an freien PPF1 im Medium (231,8 ± 36,2 ng/l) und in den Zellen (164,9 ± 15,2 ng/g TG) waren niedriger als die von PPE1 (1003,3 ± 365,2 ng/l und 2331,0 ± 87,7 ng/g TG).},
  subject      = {Oxidativer Stress},
  language  = {en}
}
@article{AbdelmohsenYangHornetal.2014,
  author    = {Abdelmohsen, Usama Ramadan and Yang, Chen and Horn, Hannes and Hajjar, Dina and Ravasi, Timothy and Hentschel, Ute},
  title     = {Actinomycetes from Red Sea Sponges: Sources for Chemical and Phylogenetic Diversity},
  doi       = {10.3390/md12052771},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-112882},
  year      = {2014},
  abstract  = {The diversity of actinomycetes associated with marine sponges collected off Fsar Reef (Saudi Arabia) was investigated in the present study. Forty-seven actinomycetes were cultivated and phylogenetically identified based on 16S rRNA gene sequencing and were assigned to 10 different actinomycete genera. Eight putatively novel species belonging to genera Kocuria, Mycobacterium, Nocardia, and Rhodococcus were identified based on sequence similarity values below 98.2\% to other 16S rRNA gene sequences available in the NCBI database. PCR-based screening for biosynthetic genes including type I and type II polyketide synthases (PKS-I, PKS-II) as well as nonribosomal peptide synthetases (NRPS) showed that 20 actinomycete isolates encoded each at least one type of biosynthetic gene. The organic extracts of nine isolates displayed bioactivity against at least one of the test pathogens, which were Gram-positive and Gram-negative bacteria, fungi, human parasites, as well as in a West Nile Virus protease enzymatic assay. These results emphasize that marine sponges are a prolific resource for novel bioactive actinomycetes with potential for drug discovery.},
  subject      = {Meeresschw{\"a}mme},
  language  = {en}
}