Identification of Nostoc punctiforme akinete-expressed genes using differential display.
TL;DR: To identify genes associated with akinete development, differential display was used to amplify and compare cDNA from a wild‐type and zwf mutant strain of N. punctiforme following a switch to dark heterotrophic conditions and three novel akinete‐expressed genes were identified.
Abstract: Akinetes are spore-like resting cells formed by certain filamentous cyanobacteria that have increased resistance to environmental stress. They can be found at low frequencies in dense cultures experiencing low light or phosphate limitation, but also form at high frequencies in a zwf mutant strain of Nostoc punctiforme following dark incubation in the presence of fructose. The wild-type strain is capable of facultative heterotrophic growth under these conditions and does not form akinetes. To identify genes associated with akinete development, differential display was used to amplify and compare cDNA from a wild-type and zwf mutant strain of N. punctiforme following a switch to dark heterotrophic conditions. Screening of candidate genes by reverse transcriptase real-time quantitative PCR and subsequent testing for akinete-specific expression using GFP transcriptional reporter plasmids lead to the identification of three novel akinete-expressed genes. The genes identified from the screening encoded for proteins homologous to an aminopeptidase (aapN), a zinc protease (hap) and an ATP-binding cassette (ABC)-type transporter (aet). Expression of hap was also increased in developing hormogonia, a transient type of differentiated filament capable of gliding motility. Transcriptional start sites for akinete-expressed genes were determined using random amplification of cDNA ends (RACE), and promoter regions were compared with orthologues in other filamentous cyanobacteria to identify putative regulatory sequences.
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Dissertation•
12 Dec 2017
TL;DR: Les akinetes sont des cellules de resistance produites par les cyanobacteries de l'ordre des Nostocales as discussed by the authors, i.e., cells capable of persisting in surface des sediments pendant la periode hivernale puis de germer au printemps.
Abstract: Les akinetes sont des cellules de resistance produites par les cyanobacteries de l’ordre des Nostocales. Issues de la differenciation de cellules vegetatives, les akinetes sont capables de persister en surface des sediments pendant la periode hivernale puis de germer au printemps pour recoloniser la colonne d’eau. Le suivi des populations pelagiques et benthiques effectue pendant deux annees sur le lac d’Aydat a montre que les akinetes presents a la surface des sediments sont representatifs de la diversite et de l’abondance, des proliferations nostocaleennes passees. Leur capacite a persister dans les sediments sur de longues echelles de temps a permis de mettre en evidence la presence de cyanobacteries il y a plusieurs milliers d’annees. La presence recurrente d’akinetes dans les sediments jusqu’a la periode actuelle indique la persistance d’un niveau trophique eleve sur l’ensemble de l’histoire de ce lac. Parallelement, le potentiel toxique des akinetes, etudie via la detection des genes anaC et mcyA, a montre la co-occurrence de ces deux cyanotoxines des les premiers blooms cyanobacteriens, il y a plus de 6700 ans ainsi que la recurrence d’anaC, associe a Dolichospermum macrosporum, au moins sur les 30 dernieres annees. Par ailleurs, d’importantes differences de pourcentage d’integrite des akinetes ont ete observees en fonction des especes, variant en moyenne de 5 a 60% pour les deux especes dominantes, D. macrosporum et D. flos-aquae respectivement. Cette variabilite serait le reflet des interactions ecologiques survenues dans la colonne d’eau et traduirait des strategies ecologiques differentes. De meme, la capacite et le temps de germination semblent etre espece dependante, ce qui permettrait un etalement de la periode de recrutement en fonction des conditions environnementales. Malgre une perte globale de viabilite avec le temps, des akinetes enfouis depuis 1800 ans dans les sediments ont revele leur capacite a germer, confirmant l'importance de ces cellules de resistance dans la perennisation a long terme des proliferations nostocaleennes.
4 citations
05 Aug 2014
TL;DR: The cyanobacteria strains from marine environment of the São Paulo state are a promising source of protease inhibitors, cyanotoxins and bioactive compounds with antibacterial, antifungal and antitumor activities.
Abstract: Cyanobacteria from coastal environment: phylogeny, gene and chemical prospecting of bioactive molecules The phylum Cyanobacteria is a phylogenetically coherent group, although presenting great diversity, and its systematic have been constantly reviewed. These microorganisms are also targets of biotechnological studies due to the production of toxins and the search for novel substances of pharmacological interest. Among the strains analyzed in this study, sequences of the 16S rRNA gene were generated for seven and, than, analyzed with sequences previously obtained. At least two groups may represent new cyanobacterial genera, while a group of Cyanobium proves to be endemic of Brazilian mangroves. Genes of the proteases inhibitors, aeuruginosin, cyanopeptolin and microviridin, were detected and the production of aeruginosin was confirmed by LC-MS for Nostoc and Cyanobium. The amino acid sequences of microviridin precursor indicated the production of three new variants in fifteen cyanobacterial strains of the genera Cyanobium, Synechococcus, Cyanobacterium, Nostoc and Nodosilinea. The genetic potential for production of cylindrospermopsin (cyrJ) was confirmed in twenty-six strains. In five strains of the genera Nostoc and Cyanobium the mcyD, mcyE and mcyG genes, which are involved in the microcystin biosynthesis, were found. The McyG sequence of Nostoc sp. CENA175 was phylogenetically grouped with sequences of microcystin-producing strains. The sxtA and sxtI genes, from saxitoxin biosynthesis, were found in nine strains of the genera Cyanobium, Oxynema, Leptolyngbya, Nodosilinea and Nostoc. The SxtI sequence of Leptolyngbya sp. CENA134 showed similarity ≥70 % with hypothetical proteins, while the sequences of Nostoc sp. CENA159 and Nostoc sp. CENA160 showed similarity ≥82% with O-carbamoyltransferase. In the phylogenetic analysis, the SxtI sequence of Nostoc sp. CENA160 grouped with sequences of strains that produce saxitoxin. In chemical analysis, the fraction 3 of the Oxynema sp. CENA135 extract revealed a substance with poly-unsaturated fatty acids characteristics and the fraction 2 of Nostoc sp. CENA175 extract indicated an aromatic structure, attached to an aliphatic chain. Other three extracts obtained from Cyanobium sp. CENA157, Nodosilinea sp. CENA183 and Nostoc sp. CENA184 were promising for the presence of nitrogenous substances. Bioactivity assays revealed that 48 % of the methanolic extracts inhibited the growth of at least one isolate of bacteria and/or yeast. The extracts of Cyanobium sp. CENA142 and Cyanobacterium sp. CENA169 were efficient against six pathogenic bacteria. In the inhibition assays of tumor cells, the DCM extract of Cyanobium sp. CENA154 (100 mg·mL) moderately inhibited the growth of 3LL cells. Ethanol extracts of Oxynema sp. CENA135 (20 mg·mL) and Cyanobium sp. CENA154 (100 mg·mL) were able to inhibit cultures of CT26 cells. In tests conducted with glioma cell lines (U251), breast cancer (MCF-7) and lung cancer (NCI-H460), the DCM extract of Cyanobium sp. CENA136 caused 50 % of growth inhibition, respectively, when used at concentrations of 7.8, 27.1 and 14.0 mg·mL. Thus, besides their phylogenetically diversity, the cyanobacteria strains from marine environment of the São Paulo state are a promising source of protease inhibitors, cyanotoxins and bioactive compounds with antibacterial, antifungal and antitumor activities.
3 citations
Cites background from "Identification of Nostoc punctiform..."
...26 Os acinetos são células similares a esporos, frequentemente mais largas que as células vegetativas, apresentando-se com granulação conspícua (MEEKS et al., 2002; ARGUETA et al., 2006)....
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01 Jan 2019
TL;DR: It is proposed that polyphasic approach of classification and reassessment of old taxonomic status may be necessary before patenting/commercialization of biotechnological processes/products.
Abstract: Cyanobacteria possess a host of proteases which unlike heterotrophs do not take part in protein nutrition. Instead, they maintain homeostasis of several vital functions, namely photosynthesis, nitrogen fixation, cellular assembly and disintegration, stress acclimation, and defense against predators. Herein, we review the Clp, FtsH, Deg/HtrA, Ctp, and SppA proteases, which under regular and photooxidative stress conditions maintain the integrity of photosynthetic and cytoplasmic membranes, periplasmic proteins, and photosystem particles, including the core complex protein, D1. The HetR protease by coordinating with the Alr3815 protease enables heterocyte differentiation and protection of nitrogenase from oxygen stress. The cell aggregation PteB proteases and caspases regulate the biomass density of cyanobacterial assemblages, and cyanophycinase mobilizes the reserve N, cyanophycin. Macrocyclization proteases mature up the ribosomally synthesized cyclic peptides of cyanobactin class with varied bioactivities. Numerous cyano-proteases listed in the UniProt database are homologues of eubacteria and higher plants with mostly unknown functions but with immense evolutionary significance in understanding the gene flow across bacteria and chloroplasts. Proteases are exclusive and therefore can be tailor-made to customize peptide drug synthesis and to formulate food additives and antimalarial, antivirulence, and antithrombotic agents. Notwithstanding these opportunities, taxonomic inadequacy and lack of proper nomenclature have adversely affected different biotechnological application processes. As a remedy, we propose that polyphasic approach of classification and reassessment of old taxonomic status may be necessary before patenting/commercialization of biotechnological processes/products.
2 citations
15 May 2009
TL;DR: This work shows that three of the sigma factor genes present in the Anabaena sp.
Abstract: Identification of Novel Regulatory Mechanisms Controlling Heterocyst Development in Anabaena Sp. Strain PCC 7120. (August 2008) Maria Ramona Aldea, B.S., Babes-Bolyai University; M.S., Babes-Bolyai University Chair of Advisory Committee: Dr. James W. Golden The regulatory mechanisms that govern heterocyst development in Anabaena sp. strain PCC 7120 have been continuously refined over the last two decades. In this work, we show that three of the sigma factor genes present in the Anabaena sp. strain PCC 7120 genome are developmentally regulated. Time-lapse microscopy of gfp reporter strains indicated that expression of sigC, sigG, and sigE is upregulated specifically in differentiating cells at 4 h, 9 h and 16 h, respectively, after induction of heterocyst development. We proposed that the sigma factors encoded by these genes are involved in regulation of heterocyst-specific genes whose expression is relatively coincident with that of sigC, sigG, or sigE. Indeed, inactivation of the sigC gene caused delayed and reduced expression of genes required for the early stages of heterocyst development, and caused delayed development. Inactivation of the sigE gene caused a considerable drop in expression of nifH, a late gene required for nitrogen fixation. We also provide evidence that c-di-GMP, a novel bacterial second messenger, is involved in regulating heterocyst development. The all2874 gene encodes a bona fide diguanylate cyclase, which synthesizes c-di-GMP, and the gene's inactivation resulted in
1 citations
Cites background from "Identification of Nostoc punctiform..."
...punctiforme following dark incubation in the presence of fructose (9)....
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01 Jan 2018
TL;DR: This document summarizes current capabilities, research and operational priorities, and plans for further studies that were established at the 2015 USGS workshop on quantitative hazard assessments of earthquake-triggered landsliding and liquefaction in the Central American region.
Abstract: .................................................................................................................... xi
1 citations
References
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TL;DR: A group of programs that will interact with each other has been developed for the Digital Equipment Corporation VAX computer using the VMS operating system.
Abstract: The University of Wisconsin Genetics Computer Group (UWGCG) has been organized to develop computational tools for the analysis and publication of biological sequence data. A group of programs that will interact with each other has been developed for the Digital Equipment Corporation VAX computer using the VMS operating system. The programs available and the conditions for transfer are described.
14,575 citations
"Identification of Nostoc punctiform..." refers methods in this paper
...Sequence features were identified using Wisconsin Genetics Computer Group (GCG) package of programs (Devereux et al., 1984), and BLAST tools available through the National Center for Biotechnology Information (http://www....
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...Sequence features were identified using Wisconsin Genetics Computer Group (GCG) package of programs (Devereux et al., 1984), and BLAST tools available through the National Center for Biotechnology Information (http://www.ncbi.nlm.nih.gov/)....
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TL;DR: Results are consistent with a function for P-glycoprotein as an energy-dependent efflux pump responsible for decreased drug accumulation in multidrug-resistant cells.
1,914 citations
"Identification of Nostoc punctiform..." refers background in this paper
...NpF0062 protein is also 26% similar and 47% identical over 589 amino acids (E-value 1e-43) to the human multidrug ABC transporter MDR1 (Chen et al., 1986)....
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TL;DR: The Conserved Domain Search service (CD-Search), a web-based tool for the detection of structural and functional domains in protein sequences, uses BLAST(R) heuristics to provide a fast, interactive service, and searches a comprehensive collection of domain models.
Abstract: We describe the Conserved Domain Search service (CD-Search), a web-based tool for the detection of structural and functional domains in protein sequences. CD-Search uses BLAST® heuristics to provide a fast, interactive service, and searches a comprehensive collection of domain models. Search results are displayed as domain architecture cartoons and pairwise alignments between the query and domain-model consensus sequences. Search results may be visualized in further detail by embedding the query sequence into multiple alignment displays and by mapping onto three-dimensional molecular graphic displays of known structures within the domain family. CD-Search can be accessed at http://www.ncbi.nlm.nih.gov/Structure/cdd/wrpsb.cgi.
1,882 citations
"Identification of Nostoc punctiform..." refers background in this paper
...The inferred Aet amino acid sequence is most closely homologous to the COG 1132 group of proteins (Marchler-Bauer and Bryant, 2004) containing multidrug transporters for export of hydrophobic compounds and components of lipopolysaccharides....
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...The second identified gene (NpR4070) was homologous to the beta subunit of a group of heterodimeric proteins comprising the M16 family of zinc-dependent proteases (Marchler-Bauer and Bryant, 2004)....
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Book•
28 Feb 1995
TL;DR: This work focuses on the study of the structure and function of the Photosystem II Reaction Center in Cyanobacteria, which consists of Chloroplast Origins and Evolution, and its role in the Evolution of the Universal Enzyme.
Abstract: Preface. Color Plates. 1. Molecular Evolution and Taxonomy of the Cyanobacteria A. Wilmotte. 2. The Oceanic Cyanobacterial Picoplankton N.G. Carr, N.H. Mann. 3. Prochlorophytes: the 'Other' Cyanobacteria? H.C.P. Matthijs, et al. 4. Molecular Biology of Cyanelles W. Loffelhardt, H.J. Bohnert. 5. Chloroplast Origins and Evolution S.E. Douglas. 6. Supramolecular Membrane Organization E. Gantt. 7. Phycobilisome and Phycobiliprotein Structures W.A. Sidler. 8. The Use of Cyanobacteria in the Study of the Structure and Function of Photosystem II B.A. Barry, et al. 9. The Cytochrome b6f Complex T. Kallas. 10. Photosystem I in Cyanobacteria J.H. Golbeck. 11. The F-type ATPase in Cyanobacteria: Pivotal Point in the Evolution of the Universal Enzyme W.D. Frasch. 12. Soluble Electron Transfer Catalysts of Cyanobacteria L.Z. Morand, et al. 13. Cyanobacterial Respiration G. Schmetterer. 14. The Biochemistry and Molecular Regulation of Carbon Dioxide Metabolism in Cyanobacteria F.R. Tabita. 15. Physiological and Molecular Studies on the Response of Cyanobacteria to Changes in the Ambient Inorganic Carbon Concentration A. Kaplan, et al. 16. Assimilatory Nitrogen Metabolism and its Regulation E. Flores, A. Herrero. 17. Biosynthesis of Cyanobacterial Tetrapyrrole Pigments: Hemes, Chlorophylls, and Phycobilins S.I. Beale. 18. Carotenoids in Cyanobacteria J. Hirschberg, D. Chamovitz. 18. Genetic Analysis of Cyanobacteria T. Thiel. 20. The Transcription Apparatus and the Regulation of Transcription Initiation S.E. Curtis, J.A. Martin. 21. The Responses of Cyanobacteria to Environmental Conditions: Light and Nutrients A.R. Grossman, et al. 22. Short-Term and Long-Term Adaptation of the Photosynthetic Apparatus: Homeostatic Properties of Thylakoids Y. Fujita, et al. 23. Light-Responsive Gene Expression and the Biochemistry of the Photosystem II Reaction Center S.S. Golden. 24. Thioredoxins in Cyanobacteria: Structure and Redox Regulation of Enzyme Activity F.K. Gleason. 25. Iron Deprivation: Physiology and Gene Regulation N.A. Straus. 26. The Cyanobacterial Heat-Shock Response and the Molecular Chaperones R. Webb, L.A. Sherman. 27. Heterocyst Metabolism and Development C.P. Wolk, et al. 28. Differentiation of Hormogonia and Relationships with Other Biological Processes N. Tandeau de Marsac. Organism Index. Gene and Gene Product Index. Subject Index.
1,289 citations
TL;DR: DNA Strider is a new integrated DNA and Protein sequence analysis program written with the C language for the Macintosh Plus, SE and II computers, designed as an easy to learn and use program as well as a fast and efficient tool for the day-to-day sequence analysis work.
Abstract: DNA Strider is a new integrated DNA and Protein sequence analysis program written with the C language for the Macintosh Plus, SE and II computers. It has been designed as an easy to learn and use program as well as a fast and efficient tool for the day-to-day sequence analysis work. The program consists of a multi-window sequence editor and of various DNA and Protein analysis functions. The editor may use 4 different types of sequences (DNA, degenerate DNA, RNA and one-letter coded protein) and can handle simultaneously 6 sequences of any type up to 32.5 kB each. Negative numbering of the bases is allowed for DNA sequences. All classical restriction and translation analysis functions are present and can be performed in any order on any open sequence or part of a sequence. The main feature of the program is that the same analysis function can be repeated several times on different sequences, thus generating multiple windows on the screen. Many graphic capabilities have been incorporated such as graphic restriction map, hydrophobicity profile and the CAI plot- codon adaptation index according to Sharp and Li. The restriction sites search uses a newly designed fast hexamer look-ahead algorithm. Typical runtime for the search of all sites with a library of 130 restriction endonucleases is 1 second per 10,000 bases. The circular graphic restriction map of the pBR322 plasmid can be therefore computed from its sequence and displayed on the Macintosh Plus screen within 2 seconds and its multiline restriction map obtained in a scrolling window within 5 seconds.
984 citations
"Identification of Nostoc punctiform..." refers methods in this paper
...Sequences were manipulated using DNA Strider (Marck, 1988) and BioBike (Massar et al., 2005)....
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...Sequences were manipulated using DNA Strider (Marck, 1988) and BioBike (Massar et al....
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