TY - JOUR A1 - Hackenberg, Claudia A1 - Hakanpaeae, Johanna A1 - Cai, Fei A1 - Antonyuk, Svetlana A1 - Eigner, Caroline A1 - Meissner, Sven A1 - Laitaoja, Mikko A1 - Janis, Janne A1 - Kerfeld, Cheryl A. A1 - Dittmann, Elke A1 - Lamzin, Victor S. T1 - Structural and functional insights into the unique CBS-CP12 fusion protein family in cyanobacteria JF - Proceedings of the National Academy of Sciences of the United States of America N2 - Cyanobacteria are important photosynthetic organisms inhabiting a range of dynamic environments. This phylum is distinctive among photosynthetic organisms in containing genes encoding uncharacterized cystathionine beta-synthase (CBS)-chloroplast protein (CP12) fusion proteins. These consist of two domains, each recognized as stand-alone photosynthetic regulators with different functions described in cyanobacteria (CP12) and plants (CP12 and CBSX). Here we show that CBS-CP12 fusion proteins are encoded in distinct gene neighborhoods, several unrelated to photosynthesis. Most frequently, CBS-CP12 genes are in a gene cluster with thioredoxin A (TrxA), which is prevalent in bloom-forming, marine symbiotic, and benthic mat cyanobacteria. Focusing on a CBS-CP12 from Microcystis aeruginosa PCC 7806 encoded in a gene cluster with TrxA, we reveal that the domain fusion led to the formation of a hexameric protein. We show that the CP12 domain is essential for hexamerization and contains an ordered, previously structurally uncharacterized N-terminal region. We provide evidence that CBS-CP12, while combining properties of both regulatory domains, behaves different from CP12 and plant CBSX. It does not form a ternary complex with phosphoribulokinase (PRK) and glyceraldehyde-3-phosphate dehydrogenase. Instead, CBS-CP12 decreases the activity of PRK in an AMP-dependent manner. We propose that the novel domain architecture and oligomeric state of CBS-CP12 expand its regulatory function beyond those of CP12 in cyanobacteria. KW - crystal structure KW - hexamer KW - redox KW - Microcystis aeruginosa Y1 - 2018 U6 - https://doi.org/10.1073/pnas.1806668115 SN - 0027-8424 VL - 115 IS - 27 SP - 7141 EP - 7146 PB - National Acad. of Sciences CY - Washington ER - TY - THES A1 - Meissner, Sven T1 - Implications of Microcystin Production in Microcystis aeruginosa PCC 7806 T1 - Effekte der Produktion von Microcystin in Microcystis aeruginosa PCC 7806 N2 - Cyanobacteria produce about 40 percent of the world’s primary biomass, but also a variety of often toxic peptides such as microcystin. Mass developments, so called blooms, can pose a real threat to the drinking water supply in many parts of the world. This study aimed at characterizing the biological function of microcystin production in one of the most common bloom-forming cyanobacterium Microcystis aeruginosa. In a first attempt, the effect of elevated light intensity on microcystin production and its binding to cellular proteins was studied. Therefore, conventional microcystin quantification techniques were combined with protein-biochemical methods. RubisCO, the key enzyme for primary carbon fixation was a major microcystin interaction partner. High light exposition strongly stimulated microcystin-protein interactions. Up to 60 percent of the total cellular microcystin was detected bound to proteins, i.e. inaccessible for standard quantification procedures. Underestimation of total microcystin contents when neglecting the protein fraction was also demonstrated in field samples. Finally, an immuno-fluorescence based method was developed to identify microcystin producing cyanobacteria in mixed populations. The high light induced microcystin interaction with proteins suggested an impact of the secondary metabolite on the primary metabolism of Microcystis by e.g. modulating the activity of enzymes. For addressing that question, a comprehensive GC/MS-based approach was conducted to compare the accumulation of metabolites in the wild-type of Microcystis aeruginosa PCC 7806 and the microcystin deficient ΔmcyB mutant. From all 501 detected non-redundant metabolites 85 (17 percent) accumulated significantly different in either of both genotypes upon high light exposition. Accumulation of compatible solutes in the ΔmcyB mutant suggests a role of microcystin in fine-tuning the metabolic flow to prevent stress related to excess light, high oxygen concentration and carbon limitation. Co-analysis of the widely used model cyanobacterium Synechocystis PCC 6803 revealed profound metabolic differences between species of cyanobacteria. Whereas Microcystis channeled more resources towards carbohydrate synthesis, Synechocystis invested more in amino acids. These findings were supported by electron microscopy of high light treated cells and the quantification of storage compounds. While Microcystis accumulated mainly glycogen to about 8.5 percent of its fresh weight within three hours, Synechocystis produced higher amounts of cyanophycin. The results showed that the characterization of species-specific metabolic features should gain more attention with regard to the biotechnological use of cyanobacteria. N2 - Cyanobakterien produzieren etwa 40 Prozent der primären Biomasse auf der Welt aber auch giftige Peptide wie das leberschädigende Microcystin. Massenvorkommen, so genannte Blaualgenblüten, gefährden vielerorts regelmäßig die Trinkwasserversorgung. Diese Arbeit hatte zum Ziel, den Einfluss der Microcystinproduktion auf physiologische Abläufe in dem weit verbreiteten blütenbildenden Cyanobakterium Microcystis aeruginosa zu charakterisieren. Zum einen, wurde hierfür der Einfluss der Beleuchtungsintensität auf die Produktion von Microcystin und dessen Bindung an zelluläre Proteine ermittelt. Hierzu wurden etablierte Quantifizierungstechniken mit biochemischen Methoden kombiniert. RubisCO, das Schlüsselenzym zur primären Kohlenstofffixierung, war ein Hauptinteraktionspartner von Microcystin. Hohe Beleuchtungsintensität erhöhte die Menge von an Proteine gebundenem Microcystin. Bis zu 60 Prozent des gesamten zellulären Microcystins lag an Proteine gebunden vor, d.h. es wurde durch Standardquantifizierungsmethoden nicht erfasst. Die Notwendigkeit, zur Quantifizierung des gesamten Microcystins die Proteinfraktion mit einzubeziehen, wurde auch in Freilandproben demonstriert. Die Entwicklung einer immunofluoreszenzbasierten Methode erlaubte die Unterscheidung von toxischen und nichttoxischen Microcystis-Kolonien in Freilandproben. Die starklichtinduzierte Interaktion von Microcystin mit Proteinen deutete auf einen möglichen Einfluss des Sekundärmetabolits auf den Primärstoffwechsel von Microcystis hin. Um dieser Frage nachzugehen, wurde ein umfassender GC/MS-basierter Versuch durchgeführt, um die Akkumulation von Metaboliten im Microcystin produzierenden Stamm Microcystis aeruginosa PCC 7806 und dessen microcystinfreier ΔmcyB-mutierten Variante vergleichen zu können. Es zeigte sich, dass Microcystin einen Einfluss auf die Akkumulation von 85 (17 Prozent) aller 501 detektierten Metaboliten unter erhöhter Beleuchtungsstärke hatte. Besonders die vermehrte Synthese osmotisch aktiver Substanzen in der ΔmcyB Mutante, verstanden als generelle Reaktion auf allgemeinen Stress, deutete auf eine Beteiligung von Microcystin in der metabolischen Justierung von Microcystis hin. Die Parallelanalyse des Modellstamms Synechocystis PCC 6803 offenbarte grundsätzliche metabolische Unterschiede zwischen verschiedenen Cyanobakterienspezies. Demnach produzierte Microcystis vor allem Kohlehydrate und Synechocystis eher Aminosäuren. Die GC/MS-basierten Ergebnisse wurden durch elektronmikroskopische Aufnahmen und die Quantifizierung von Speichermetaboliten gestützt. Innerhalb drei Stunden bewirkte Starklicht die Akkumulation von Glykogen in Microcystis auf ca. 8.5 Prozent des Frischgewichts, wohingegen Synechocystis mehr Cyanophycin produzierte. Die Ergebnisse zeigten, dass im Hinblick auf die biotechnologische Nutzung von Cyanobakterien, die Charakterisierung speziesspezifischer metabolischer Eigenschaften mehr Beachtung finden sollte. KW - microcystin KW - Microcystin KW - cyanobacteria KW - Cyanobakterien Y1 - 2014 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-75199 ER - TY - JOUR A1 - Barchewitz, Tino A1 - Guljamow, Arthur A1 - Meißner, Sven A1 - Timm, Stefan A1 - Henneberg, Manja A1 - Baumann, Otto A1 - Hagemann, Martin A1 - Dittmann, Elke T1 - Non-canonical localization of RubisCO under high-light conditions in the toxic cyanobacterium Microcystis aeruginosa PCC7806 JF - Environmental microbiology N2 - The frequent production of the hepatotoxin microcystin (MC) and its impact on the lifestyle of bloom-forming cyanobacteria are poorly understood. Here, we report that MC interferes with the assembly and the subcellular localization of RubisCO, in Microcystis aeruginosa PCC7806. Immunofluorescence, electron microscopic and cellular fractionation studies revealed a pronounced heterogeneity in the subcellular localization of RubisCO. At high cell density, RubisCO particles are largely separate from carboxysomes in M. aeruginosa and relocate to the cytoplasmic membrane under high-light conditions. We hypothesize that the binding of MC to RubisCO promotes its membrane association and enables an extreme versatility of the enzyme. Steady-state levels of the RubisCO CO2 fixation product 3-phosphoglycerate are significantly higher in the MC-producing wild type. We also detected noticeable amounts of the RubisCO oxygenase reaction product secreted into the medium that may support the mutual interaction of M. aeruginosa with its heterotrophic microbial community. Y1 - 2019 U6 - https://doi.org/10.1111/1462-2920.14837 SN - 1462-2912 SN - 1462-2920 VL - 21 IS - 12 SP - 4836 EP - 4851 PB - Wiley CY - Hoboken ER - TY - JOUR A1 - Meissner, Sven A1 - Fastner, Jutta A1 - Dittmann-Thünemann, Elke T1 - Microcystin production revisited conjugate formation makes a major contribution JF - Environmental microbiology N2 - The impact of environmental stimuli on the production of the widespread cyanobacterial hepatotoxin microcystin (MC) is under debate. Whereas transcriptional studies of the biosynthetic genes suggest a clear influence of light conditions on toxin production the data for the metabolite itself are inconsistent and highly strain-specific. Here, we have reassessed the MC content by using two immunological detection techniques that allow a parallel quantification of MC in the methanolic extracts and the residual pellet fraction that contains high molecular weight proteins. Our results show a significant proportion of MC in the protein bound fraction in strains of Microcystis and Planktothrix and of the related toxin nodularin (NOD) in Nodularia. Moreover, we could show a very strong increase of MC after high light illumination in the protein fraction contributing to a significant overall increase in MC production under these conditions that is not seen in extracts analysed by LC-MS and ELISA. The fact that a considerable portion of MC is neglected with current analysis techniques was also confirmed for selected field samples. Immunofluorescence studies suggest strain-specific differences in the amount of MC conjugate formation. Y1 - 2013 U6 - https://doi.org/10.1111/1462-2920.12072 SN - 1462-2912 VL - 15 IS - 6 SP - 1810 EP - 1820 PB - Wiley-Blackwell CY - Hoboken ER - TY - JOUR A1 - Meissner, Sven A1 - Steinhauser, Dirk A1 - Dittmann-Thünemann, Elke T1 - Metabolomic analysis indicates a pivotal role of the hepatotoxin microcystin in high light adaptation of Microcystis JF - Environmental microbiology N2 - Microcystis is a freshwater cyanobacterium frequently forming nuisance blooms in the summer months. The genus belongs to the predominant producers of the potent hepatotoxin microcystin. The success of Microcystis and its remarkable resistance to high light conditions are not well understood. Here, we have compared the metabolic response of Microcystis aeruginosaPCC7806, its microcystin-deficient mcyB mutant (Mut) and the cyanobacterial model organism SynechocystisPCC6803 to high light exposure of 250molphotonsm(-2)s(-1) using GC/MS-based metabolomics. Microcystis wild type and Mut show pronounced differences in their metabolic reprogramming upon high light. Seventeen percent of the detected metabolites showed significant differences between the two genotypes after high light exposure. Whereas the microcystin-producing wild type shows a faster accumulation of glycolate upon high light illumination, loss of microcystin leads to an accumulation of general stress markers such as trehalose and sucrose. The study further uncovers differences in the high light adaptation of the bloom-forming cyanobacterium Microcystis and the model cyanobacterium Synechocystis. Most notably, Microcystis invests more into carbon reserves such as glycogen after high light exposure. Our data shed new light on the lifestyle of bloom-forming cyanobacteria, the role of the widespread toxin microcystin and the metabolic diversity of cyanobacteria. Y1 - 2015 U6 - https://doi.org/10.1111/1462-2920.12565 SN - 1462-2912 SN - 1462-2920 VL - 17 IS - 5 SP - 1497 EP - 1509 PB - Wiley-Blackwell CY - Hoboken ER - TY - JOUR A1 - Zilliges, Yvonne A1 - Kehr, Jan-Christoph A1 - Meissner, Sven A1 - Ishida, Keishi A1 - Mikkat, Stefan A1 - Hagemann, Martin A1 - Kaplan, Aaron A1 - Börner, Thomas A1 - Dittmann-Thünemann, Elke T1 - The cyanobacterial hepatotoxin microcystin binds to proteins and increases the fitness of microcystis under oxidative stress conditions JF - PLoS one N2 - Microcystins are cyanobacterial toxins that represent a serious threat to drinking water and recreational lakes worldwide. Here, we show that microcystin fulfils an important function within cells of its natural producer Microcystis. The microcystin deficient mutant Delta mcyB showed significant changes in the accumulation of proteins, including several enzymes of the Calvin cycle, phycobiliproteins and two NADPH-dependent reductases. We have discovered that microcystin binds to a number of these proteins in vivo and that the binding is strongly enhanced under high light and oxidative stress conditions. The nature of this binding was studied using extracts of a microcystin-deficient mutant in vitro. The data obtained provided clear evidence for a covalent interaction of the toxin with cysteine residues of proteins. A detailed investigation of one of the binding partners, the large subunit of RubisCO showed a lower susceptibility to proteases in the presence of microcystin in the wild type. Finally, the mutant defective in microcystin production exhibited a clearly increased sensitivity under high light conditions and after hydrogen peroxide treatment. Taken together, our data suggest a protein-modulating role for microcystin within the producing cell, which represents a new addition to the catalogue of functions that have been discussed for microbial secondary metabolites. Y1 - 2011 U6 - https://doi.org/10.1371/journal.pone.0017615 SN - 1932-6203 VL - 6 IS - 3 PB - PLoS CY - San Fransisco ER -