Cyanophycin (multi-L-arginyl-poly-L-aspartate), a water-insoluble reserve polymer of cyanobacteria, is a product of nonribosomal peptide synthesis. The purification of cyanophycin synthetase of the cyanobacterium Anabaena variabilis is described. In sodium dodecylsulfate/polyacrylamide gel electrophoresis, the enzyme preparation shows one band with an apparent molecular mass of 100 kDa. The native enzyme has an apparent molecular mass of approximately 230 kDa, as determined by size-exclusion chromatography, suggesting that the active form is a homodimer. During catalysis, ATP is converted to ADP. The gene coding for cyanophycin synthetase has been identified in the sequenced genome of Synechocystis sp. PCC 6803. The C-terminal 60% of the deduced amino acid sequence of cyanophycin synthetase show sequence similarity to enzymes of the superfamily of ligases involved in the biosynthesis of murein and of folyl-poly(γ-glutamate). Cells of Escherichia coli harbouring the gene on a plasmid express active synthetase and accumulate cyanophycin-like material. The results prove that a single enzyme catalyzes the de novo synthesis of cyanophycin.Keywords : non-ribosomal peptide synthesis; cyanobacteria ; cyanophycin synthetase; purification; heterologous expression.Most cyanobacteria contain the nitrogen-rich reserve mateFrom the cyanobacterium Anabaena cylindrica, Simon [9] has enriched an enzyme that synthesizes cyanophycin in vitro rial multi-L-arginyl-poly (L-aspartic acid) (trivial name, cyanoand has studied the basic properties of the biosynthetic reaction. phycin), which is deposited in the cytoplasm in the form of gran-The substrates of the reaction are the constituent amino acids Lules [1Ϫ4]. In this polymer, nearly all β-carboxy groups of a arginine and L-aspartic acid, Mg-ATP, and cyanophycin as poly(aspartate) backbone are linked to A-amino groups of argiprimer [9]. In a strict sense, the assay measures an elongation nine residues by iso-peptide bonds, resulting in an approximate reaction. A thiol reagent such as 2-mercaptoethanol and K ϩ were 1:1 stoichiometry of aspartate/arginine [1,5,6]. The polymer is found to be required for full activity [9]. The latter properties the product of nonribosomal peptide synthesis [7]. Its molecular are, in addition to the formation of iso-peptide bonds, reminismass, as estimated by SDS/PAGE, in a given cyanobacterial specent of the requirements of the biosynthesis of glutathione [10] cies is not uniform, but ranges over about 25Ϫ100 kDa [1]. Cyaand of poly(γ-D-glutamate) [11]. nophycin is also present in filamentous cyanobacteria such asIn this communication, we describe the purification of cyaAnabaena which differentiate, in a semiregular pattern, so-called nophycin synthetase from the cyanobacterium Anabaena varheterocysts, cells specialized for fixation of N 2 under aerobic iabilis American Type Culture Collection (ATCC) 29413. It is conditions. In these species, cyanophycin may not only serve as demonstrated that a homodimer of a 100-kDa protein incorpoa reserve material,...
Cyanobacteria are versatile unicellular phototrophic microorganisms that are highly abundant in many environments. Owing to their capability to utilize solar energy and atmospheric carbon dioxide for growth, cyanobacteria are increasingly recognized as a prolific resource for the synthesis of valuable chemicals and various biofuels. To fully harness the metabolic capabilities of cyanobacteria necessitates an in-depth understanding of the metabolic interconversions taking place during phototrophic growth, as provided by genome-scale reconstructions of microbial organisms. Here we present an extended reconstruction and analysis of the metabolic network of the unicellular cyanobacterium Synechocystis sp. PCC 6803. Building upon several recent reconstructions of cyanobacterial metabolism, unclear reaction steps are experimentally validated and the functional consequences of unknown or dissenting pathway topologies are discussed. The updated model integrates novel results with respect to the cyanobacterial TCA cycle, an alleged glyoxylate shunt, and the role of photorespiration in cellular growth. Going beyond conventional flux-balance analysis, we extend the computational analysis to diurnal light/dark cycles of cyanobacterial metabolism.
The biosynthesis of glycogen or starch is one of the main strategies developed by living organisms for the intracellular storage of carbon and energy. In phototrophic organisms, such polyglucans accumulate due to carbon fixation during photosynthesis and are used to provide maintenance energy for cell integrity, function and viability in dark periods. Moreover, it is assumed that glycogen enables cyanobacteria to cope with transient starvation conditions, as observed in most micro-organisms. Here, glycogen accumulates when an appropriate carbon source is available in sufficient amounts but growth is inhibited by lack of other nutrients. In this study, the role of glycogen in energy and carbon metabolism of phototrophic cyanobacteria was first analysed via a comparative physiological and metabolic characterization of knockout mutants defective in glycogen synthesis. We first proved the role of glycogen as a respiratory substrate in periods of darkness, the role of glycogen as a reserve to survive starvation periods such as nitrogen depletion and the role of glycogen synthesis as an ameliorator of carbon excess conditions in the model organism Synechocystis sp. PCC 6803. We provide striking new insights into the complex carbon and nitrogen metabolism of non-diazotrophic cyanobacteria: a phenotype of sensitivity to photomixotrophic conditions and of reduced glucose uptake, a non-bleaching phenotype based on an impaired acclimation response to nitrogen depletion and furthermore a phenotype of energy spilling. This study shows that the analysis of deficiencies in glycogen metabolism is a valuable tool for the identification of metabolic regulatory principles and signals.
and Manchester Interdisciplinary Biocentre, University of Manchester, M1 7DN Manchester, United Kingdom (R.S.) Unicellular cyanobacteria have attracted growing attention as potential host organisms for the production of valuable organic products and provide an ideal model to understand oxygenic photosynthesis and phototrophic metabolism. To obtain insight into the functional properties of phototrophic growth, we present a detailed reconstruction of the primary metabolic network of the autotrophic prokaryote Synechocystis sp. PCC 6803. The reconstruction is based on multiple data sources and extensive manual curation and significantly extends currently available repositories of cyanobacterial metabolism. A systematic functional analysis, utilizing the framework of flux-balance analysis, allows the prediction of essential metabolic pathways and reactions and allows the identification of inconsistencies in the current annotation. As a counterintuitive result, our computational model indicates that photorespiration is beneficial to achieve optimal growth rates. The reconstruction process highlights several obstacles currently encountered in the context of large-scale reconstructions of metabolic networks.Cyanobacteria are among the evolutionarily oldest organisms and are the only known prokaryotes capable of plant-like oxygenic photosynthesis. As primary producers in aquatic environments, they play an important role in global CO 2 assimilation and oxygen recycling. Recently, cyanobacteria have also attracted growing attention for economic purposes, including drug discovery and as prolific producers of natural products (Sielaff et al., 2006;Tan, 2007). In particular their ability to directly convert atmospheric CO 2 into biomass and organic compounds, driven by sunlight, offers considerable potential as a novel and renewable resource for bioenergy (Deng and Coleman, 1999;Atsumi et al., 2009;Mascarelli, 2009;Lindberg et al., 2010).Among the diverse cyanobacterial strains, Synechocystis sp. PCC 6803 is one of the most extensively studied model organisms for the analysis of photosynthetic processes. With a rich compendium of genomic, biochemical, and physiological data available, Synechocystis sp. PCC 6803, therefore, offers an ideal starting point to obtain insights into the systemic properties of phototrophic metabolism. The prerequisite for such a systemic description is a detailed reconstruction of the metabolic network of the organism: that is, a reconstruction of the comprehensive set of enzyme-catalyzed reactions required to support cellular growth and maintenance. Once a metabolic reconstruction is available, the vast array of methods developed by computational systems biology over the past decades allows us to dissect the functioning and interplay of possible metabolic routes and biochemical interconversions. In this respect, constraint-based modeling, most notably flux-balance analysis (FBA), has become a quasi-standard in the field. FBA is increasingly utilized to elucidate and characterize largescale network...
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