131 results on '"Vitulo, Nicola"'
Search Results
102. Grapevine Rootstocks Differentially Affect the Rate of Ripening and Modulate Auxin-Related Genes in Cabernet Sauvignon Berries
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Corso, Massimiliano, primary, Vannozzi, Alessandro, additional, Ziliotto, Fiorenza, additional, Zouine, Mohamed, additional, Maza, Elie, additional, Nicolato, Tommaso, additional, Vitulo, Nicola, additional, Meggio, Franco, additional, Valle, Giorgio, additional, Bouzayen, Mondher, additional, Müller, Maren, additional, Munné-Bosch, Sergi, additional, Lucchin, Margherita, additional, and Bonghi, Claudio, additional
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- 2016
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103. Profiling of skeletal muscle Ankrd2 protein in human cardiac tissue and neonatal rat cardiomyocytes
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Jasnić, Jovana, Nestorović, Aleksandra, Savić, Slobodan, Karasek, Sinisa, Vitulo, Nicola, Valle, Giorgio, Faulkner, Georgine, Radojković, Dragica, Kojić, Snežana, Jasnić, Jovana, Nestorović, Aleksandra, Savić, Slobodan, Karasek, Sinisa, Vitulo, Nicola, Valle, Giorgio, Faulkner, Georgine, Radojković, Dragica, and Kojić, Snežana
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Muscle-specific mechanosensors Ankrd2/Arpp (ankyrin repeat protein 2) and Ankrd1/CARP (cardiac ankyrin repeat protein) have an important role in transcriptional regulation, myofibrillar assembly, cardiogenesis and myogenesis. In skeletal muscle myofibrils, Ankrd2 has a structural role as a component of a titin associated stretch-sensing complex, while in the nucleus it exerts regulatory function as transcriptional co-factor. It is also involved in myogenic differentiation and coordination of myoblast proliferation. Although expressed in the heart, the role of Ankrd2 in the cardiac muscle is completely unknown. Recently, we have shown that hypertrophic and dilated cardiomyopathy pathways are altered upon Ankrd2 silencing suggesting the importance of this protein in cardiac tissue. Here we provide the underlying basis for the functional investigation of Ankrd2 in the heart. We confirmed reduced Ankrd2 expression levels in human heart in comparison with Ankrd1 using RNAseq and Western blot. For the first time we demonstrated that, apart from the sarcomere and nucleus, both proteins are localized to the intercalated disks of human cardiomyocytes. We further tested the expression and localization of endogenous Ankrd2 in rat neonatal cardiomyocytes, a well-established model for studying cardiac-specific proteins. Ankrd2 was found to be expressed in both the cytoplasm and nucleus, independently from maturation status of cardiomyocytes. In contrast to Ankrd1, it is not responsive to the cardiotoxic drug Doxorubicin, suggesting that different mechanisms govern their expression in cardiac cells.
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- 2015
104. ScaMPI: a program for genome Scaffolding using Mate Paired Information
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Telatin, A., Corteggiani Carpinelli, E., Campagna, Davide, Forcato, Claudio, Vitulo, Nicola, and Valle, Giorgio
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- 2013
105. A web-based platform to retrieve user-ranked data from human exome/genome sequencing projects
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Forcato, Claudio, Albiero, A., Vitulo, Nicola, Vezzi, Alessandro, and Valle, Giorgio
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- 2012
106. Physical Mapping of Bread Wheat Chromosome 5A: An Integrated Approach
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Barabaschi, Delfina, primary, Magni, Federica, additional, Volante, Andrea, additional, Gadaleta, Agata, additional, Šimková, Hana, additional, Scalabrin, Simone, additional, Prazzoli, Maria Lucia, additional, Bagnaresi, Paolo, additional, Lacrima, Katia, additional, Michelotti, Vania, additional, Desiderio, Francesca, additional, Orrù, Luigi, additional, Mazzamurro, Valentina, additional, Fricano, Agostino, additional, Mastrangelo, AnnaMaria, additional, Tononi, Paola, additional, Vitulo, Nicola, additional, Jurman, Irena, additional, Frenkel, Zeev, additional, Cattonaro, Federica, additional, Morgante, Michele, additional, Blanco, Antonio, additional, Doležel, Jaroslav, additional, Delledonne, Massimo, additional, Stanca, Antonio M., additional, Cattivelli, Luigi, additional, and Valè, Giampiero, additional
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- 2015
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107. SATRAP: SOLiD Assembler TRAnslation Program
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Campagna, Davide, primary, Gasparini, Fabio, additional, Franchi, Nicola, additional, Manni, Lucia, additional, Telatin, Andrea, additional, Vitulo, Nicola, additional, Ballarin, Loriano, additional, and Valle, Giorgio, additional
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- 2015
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108. Transcription of LINE-derived sequences in exercise-induced stress in horses
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Capomaccio, S, VERINI SUPPLIZI, A, Galla, Giulio, Vitulo, Nicola, Barcaccia, Gianni, Felicetti, M, Silvestrelli, M, and Cappelli, K.
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stress ,Long Interspersed Nucleotide Elements ,exercise ,Physical Conditioning, Animal ,Leukocytes, Mononuclear ,Animals ,Horses ,transposable elements ,exonization ,horse - Abstract
A large proportion of mammalian genomes is represented by transposable elements (TE), most of them being long interspersed nuclear elements 1 (LINE-1 or L1). An increased expression of LINE-1 elements may play an important role in cellular stress-related conditions exerting drastic effects on the mammalian transcriptome. To understand the impact of TE on the known horse transcriptome, we masked the horse EST database, pointing out that the amount is consistent with other major vertebrates. A previously developed transcript-derived fragments (TDFs) dataset, deriving from exercise-stimulated horse peripheral blood mononuclear cells (PBMCs), was found to be enriched with L1 (26.8% in terms of bp). We investigated the involvement of TDFs in exercise-induced stress through bioinformatics and gene expression analysis. Results indicate that LINE-derived sequences are not only highly but also differentially expressed during physical effort, hinting at interesting scenarios in the regulation of gene expression in relation to exercise.
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- 2010
109. ZASP Interacts with the Mechanosensing Protein Ankrd2 and p53 in the Signalling Network of Striated Muscle
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Martinelli, Valentina C., Kyle, W. Buck, Kojić, Snežana, Vitulo, Nicola, Li, Zhaohui, Belgrano, Anna, Maiuri, Paolo, Banks, Lawrence, Vatta, Matteo, Valle, Giorgio, Faulkner, Georgine, Martinelli, Valentina C., Kyle, W. Buck, Kojić, Snežana, Vitulo, Nicola, Li, Zhaohui, Belgrano, Anna, Maiuri, Paolo, Banks, Lawrence, Vatta, Matteo, Valle, Giorgio, and Faulkner, Georgine
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ZASP is a cytoskeletal PDZ-LIM protein predominantly expressed in striated muscle. It forms multiprotein complexes and plays a pivotal role in the structural integrity of sarcomeres. Mutations in the ZASP protein are associated with myofibrillar myopathy, left ventricular non-compaction and dilated cardiomyopathy. The ablation of its murine homologue Cypher results in neonatal lethality. ZASP has several alternatively spliced isoforms, in this paper we clarify the nomenclature of its human isoforms as well as their dynamics and expression pattern in striated muscle. Interaction is demonstrated between ZASP and two new binding partners both of which have roles in signalling, regulation of gene expression and muscle differentiation; the mechanosensing protein Ankrd2 and the tumour suppressor protein p53. These proteins and ZASP form a triple complex that appears to facilitate poly-SUMOylation of p53. We also show the importance of two of its functional domains, the ZM-motif and the PDZ domain. The PDZ domain can bind directly to both Ankrd2 and p53 indicating that there is no competition between it and p53 for the same binding site on Ankrd2. However there is competition for this binding site between p53 and a region of the ZASP protein lacking the PDZ domain, but containing the ZM-motif. ZASP is negative regulator of p53 in transactivation experiments with the p53-responsive promoters, MDM2 and BAX. Mutations in the ZASP ZM-motif induce modification in protein turnover. In fact, two mutants, A165V and A171T, were not able to bind Ankrd2 and bound only poorly to alpha-actinin2. This is important since the A165V mutation is responsible for zaspopathy, a well characterized autosomal dominant distal myopathy. Although the mechanism by which this mutant causes disease is still unknown, this is the first indication of how a ZASP disease associated mutant protein differs from that of the wild type ZASP protein.
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- 2014
110. Transcriptome analysis in grapevine rootstock genotypes with contrasting tolerance to drought
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Italian Society of Agricoltural Genetics - Annual congress, Vannozzi, Alessandro, Corso, Massimiliano, Meggio, Franco, Vitulo, Nicola, Valle, Giorgio, Bonghi, Claudio, Lucchin, Margherita, Italian Society of Agricoltural Genetics - Annual congress, Vannozzi, Alessandro, Corso, Massimiliano, Meggio, Franco, Vitulo, Nicola, Valle, Giorgio, Bonghi, Claudio, and Lucchin, Margherita
- Abstract
info:eu-repo/semantics/nonPublished
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- 2014
111. A deep survey of alternative splicing in grape reveals changes in the splicing machinery related to tissue, stress condition and genotype.
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Vitulo, Nicola, Forcato, Claudio, Carpinelli, Elisa Corteggiani, Telatin, Andrea, Campagna, Davide, D'Angelo, Michela, Zimbello, Rosanna, Corso, Massimiliano, Vannozzi, Alessandro, Bonghi, Claudio, Lucchin, Margherita, Valle, Giorgio, Vitulo, Nicola, Forcato, Claudio, Carpinelli, Elisa Corteggiani, Telatin, Andrea, Campagna, Davide, D'Angelo, Michela, Zimbello, Rosanna, Corso, Massimiliano, Vannozzi, Alessandro, Bonghi, Claudio, Lucchin, Margherita, and Valle, Giorgio
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Alternative splicing (AS) significantly enhances transcriptome complexity. It is differentially regulated in a wide variety of cell types and plays a role in several cellular processes. Here we describe a detailed survey of alternative splicing in grape based on 124 SOLiD RNAseq analyses from different tissues, stress conditions and genotypes., info:eu-repo/semantics/published
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- 2014
112. Ecotype Diversity and Conversion in Photobacterium profundum Strains
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Lauro, Federico M., primary, Eloe-Fadrosh, Emiley A., additional, Richter, Taylor K. S., additional, Vitulo, Nicola, additional, Ferriera, Steven, additional, Johnson, Justin H., additional, and Bartlett, Douglas H., additional
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- 2014
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113. A deep survey of alternative splicing in grape reveals changes in the splicing machinery related to tissue, stress condition and genotype
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Vitulo, Nicola, primary, Forcato, Claudio, additional, Carpinelli, Elisa Corteggiani, additional, Telatin, Andrea, additional, Campagna, Davide, additional, D'Angelo, Michela, additional, Zimbello, Rosanna, additional, Corso, Massimiliano, additional, Vannozzi, Alessandro, additional, Bonghi, Claudio, additional, Lucchin, Margherita, additional, and Valle, Giorgio, additional
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- 2014
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114. ZASP Interacts with the Mechanosensing Protein Ankrd2 and p53 in the Signalling Network of Striated Muscle
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Martinelli, Valentina C., primary, Kyle, W. Buck, additional, Kojic, Snezana, additional, Vitulo, Nicola, additional, Li, Zhaohui, additional, Belgrano, Anna, additional, Maiuri, Paolo, additional, Banks, Lawrence, additional, Vatta, Matteo, additional, Valle, Giorgio, additional, and Faulkner, Georgine, additional
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- 2014
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115. RNA Sequencing of the Exercise Transcriptome in Equine Athletes
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Capomaccio, Stefano, primary, Vitulo, Nicola, additional, Verini-Supplizi, Andrea, additional, Barcaccia, Gianni, additional, Albiero, Alessandro, additional, D'Angelo, Michela, additional, Campagna, Davide, additional, Valle, Giorgio, additional, Felicetti, Michela, additional, Silvestrelli, Maurizio, additional, and Cappelli, Katia, additional
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- 2013
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116. PASS-bis: a bisulfite aligner suitable for whole methylome analysis of Illumina and SOLiD reads
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Campagna, Davide, primary, Telatin, Andrea, additional, Forcato, Claudio, additional, Vitulo, Nicola, additional, and Valle, Giorgio, additional
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- 2012
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117. First Survey of the Wheat Chromosome 5A Composition through a Next Generation Sequencing Approach
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Vitulo, Nicola, primary, Albiero, Alessandro, additional, Forcato, Claudio, additional, Campagna, Davide, additional, Dal Pero, Francesca, additional, Bagnaresi, Paolo, additional, Colaiacovo, Moreno, additional, Faccioli, Primetta, additional, Lamontanara, Antonella, additional, Šimková, Hana, additional, Kubaláková, Marie, additional, Perrotta, Gaetano, additional, Facella, Paolo, additional, Lopez, Loredana, additional, Pietrella, Marco, additional, Gianese, Giulio, additional, Doležel, Jaroslav, additional, Giuliano, Giovanni, additional, Cattivelli, Luigi, additional, Valle, Giorgio, additional, and Stanca, A. Michele, additional
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- 2011
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118. Development of an oligo DNA microarray for the European sea bass and its application to expression profiling of jaw deformity
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Ferraresso, Serena, primary, Milan, Massimo, additional, Pellizzari, Caterina, additional, Vitulo, Nicola, additional, Reinhardt, Richard, additional, Canario, Adelino VM, additional, Patarnello, Tomaso, additional, and Bargelloni, Luca, additional
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- 2010
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119. Development and validation of a gene expression oligo microarray for the gilthead sea bream (Sparus aurata)
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Ferraresso, Serena, primary, Vitulo, Nicola, additional, Mininni, Alba N, additional, Romualdi, Chiara, additional, Cardazzo, Barbara, additional, Negrisolo, Enrico, additional, Reinhardt, Richard, additional, Canario, Adelino VM, additional, Patarnello, Tomaso, additional, and Bargelloni, Luca, additional
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- 2008
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120. Characterization and Evolution of the Cell Cycle-Associated Mob Domain-Containing Proteins in Eukaryotes
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Vitulo, Nicola, primary, Vezzi, Alessandro, additional, Galla, Giulio, additional, Citterio, Sandra, additional, Marino, Giada, additional, Ruperti, Benedetto, additional, Zermiani, Monica, additional, Albertini, Emidio, additional, Valle, Giorgio, additional, and Barcaccia, Gianni, additional
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- 2007
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121. Laterally transferred elements and high pressure adaptation in Photobacterium profundum strains
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Campanaro, Stefano, primary, Vezzi, Alessandro, additional, Vitulo, Nicola, additional, Lauro, Federico M, additional, D'Angelo, Michela, additional, Simonato, Francesca, additional, Cestaro, Alessandro, additional, Malacrida, Giorgio, additional, Bertoloni, Giulio, additional, Valle, Giorgio, additional, and Bartlett, Douglas H, additional
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- 2005
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122. RAP: a new computer program for de novo identification of repeated sequences in whole genomes
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Campagna, Davide, primary, Romualdi, Chiara, additional, Vitulo, Nicola, additional, Del Favero, Micky, additional, Lexa, Matej, additional, Cannata, Nicola, additional, and Valle, Giorgio, additional
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- 2004
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123. Ecotype Diversity and Conversion in Photobacterium profundum Strains.
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Lauro, Federico M., Eloe-Fadrosh, Emiley A., Richter, Taylor K. S., Vitulo, Nicola, Ferriera, Steven, Johnson, Justin H., and Bartlett, Douglas H.
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PHOTOBACTERIUM ,BACTERIAL diversity ,BACTERIAL ecology ,MARINE bacteria ,BACTERIAL growth ,HYDROSTATIC pressure - Abstract
Photobacterium profundum is a cosmopolitan marine bacterium capable of growth at low temperature and high hydrostatic pressure. Multiple strains of P. profundum have been isolated from different depths of the ocean and display remarkable differences in their physiological responses to pressure. The genome sequence of the deep-sea piezopsychrophilic strain Photobacterium profundum SS9 has provided some clues regarding the genetic features required for growth in the deep sea. The sequenced genome of Photobacterium profundum strain 3TCK, a non-piezophilic strain isolated from a shallow-water environment, is now available and its analysis expands the identification of unique genomic features that correlate to environmental differences and define the Hutchinsonian niche of each strain. These differences range from variations in gene content to specific gene sequences under positive selection. Genome plasticity between Photobacterium bathytypes was investigated when strain 3TCK-specific genes involved in photorepair were introduced to SS9, demonstrating that horizontal gene transfer can provide a mechanism for rapid colonisation of new environments. [ABSTRACT FROM AUTHOR]
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- 2014
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124. Intestinal dysbiosis promotes immune dysregulation in an animal model of Alzheimer's disease.
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Santos‐Lima, Bruno, Zenaro, Elena, Slanzi, Anna, Pietronigro, Enrica Caterina, Lopez, Nicola, Terrabuio, Eleonora, Vitulo, Nicola, Bianca, Vittorina Della, and Constantin, Gabriela
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Background: Current evidence suggests that systemic inflammation promotes Alzheimer's Disease (AD) and recent reports demonstrated that circulating neutrophils migrate into the AD brain inducing neuroinflammation and cognitive deficits in animal models of AD. However, how peripheral immune dysregulation occurs and promotes neuroinflammation and memory decline in AD is still unknown. Even though descriptive reports suggest the involvement of the microbiome in AD, the mechanisms behind AD pathology are not explored. In this context, we aim to better understand the dysregulation of leukocyte subpopulations in AD by addressing the gut‐blood‐brain axis. Method: By taking advantage of the 3xTg‐AD mouse model we addressed peripheral inflammation during early disease stages. To this aim, we performed: 1) an intestinal microbiota analysis; 2) characterization of circulating inflammatory mediators; and 3) immunophenotypization of peripheral blood. Result: In our study we show a clear intestinal dysbiosis in the 3xTg‐AD mice, characterized by higher abundance of taxa known to cause proinflammatory conditions. In agreement, we also found increased intestinal permeability and accumulation of immature precursors and aged neutrophils in circulating blood, suggesting a strong peripheral dysregulation in the early phases of the disease. Conclusion: Altogether, our data suggest microbiota as a modulator of leukocyte activation and migration into the brain. Therefore, targeting the gut‐blood‐brain axis in AD could lead to new immunomodulatory strategies for AD treatment. [ABSTRACT FROM AUTHOR]
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- 2021
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125. A single polyploidization event at the origin of the tetraploid genome of Coffea arabica is responsible for the extremely low genetic variation in wild and cultivated germplasm
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Sara Pinosio, Gloria Pellegrino, Lucile Toniutti, Gabriele Magris, Timothy Schilling, Gabriele Di Gaspero, Benoît Bertrand, Seth C. Murray, Simone Scalabrin, Davide Scaglione, Amin Al Hakimi, Irena Jurman, Giorgio Graziosi, Nicola Vitulo, Giorgio Valle, Frederica Cattonaro, Michele Morgante, Manuela Rosanna Ruosi, Patricia E. Klein, Mario Cerutti, Luciano Navarini, Alberto Pallavicini, Lorenzo Del Terra, Furio Suggi Liverani, Nolan Bentley, Michele Vidotto, Christophe Montagnon, Federica Magni, William Solano, Scalabrin, Simone, Toniutti, Lucile, Di Gaspero, Gabriele, Scaglione, Davide, Magris, Gabriele, Vidotto, Michele, Pinosio, Sara, Cattonaro, Federica, Magni, Federica, Jurman, Irena, Cerutti, Mario, Suggi Liverani, Furio, Navarini, Luciano, Del Terra, Lorenzo, Pellegrino, Gloria, Ruosi, Manuela Rosanna, Vitulo, Nicola, Valle, Giorgio, Pallavicini, Alberto, Graziosi, Giorgio, Klein, Patricia E, Bentley, Nolan, Murray, Seth, Solano, William, Al Hakimi, Amin, Schilling, Timothy, Montagnon, Christophe, Morgante, Michele, and Bertrand, Benoit
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0106 biological sciences ,0301 basic medicine ,Germplasm ,Yemen ,Computational biology and bioinformatics ,Evolution ,Genetics ,Plant sciences ,Genomics ,Coffea arabica ,lcsh:Medicine ,Coffea ,01 natural sciences ,F30 - Génétique et amélioration des plantes ,Genome Size ,Dynamique des populations ,lcsh:Science ,Computational biology and bioinformatic ,2. Zero hunger ,Multidisciplinary ,Coffea arabica , genome sequencing, plants ,biology ,U10 - Informatique, mathématiques et statistiques ,plants ,Polyploïdie ,Center of origin ,genome sequencing ,Plant science ,Genome, Plant ,Costa Rica ,Crops, Agricultural ,xxxx ,Canephora ,Introgression ,Polymorphism, Single Nucleotide ,Article ,03 medical and health sciences ,Bioinformatique ,Genetic ,Genetic variation ,Genome size ,Genetic diversity ,Whole Genome Sequencing ,lcsh:R ,biology.organism_classification ,Tetraploidy ,030104 developmental biology ,Evolutionary biology ,Genomic ,lcsh:Q ,010606 plant biology & botany - Abstract
The genome of the allotetraploid species Coffea arabica L. was sequenced to assemble independently the two component subgenomes (putatively deriving from C. canephora and C. eugenioides) and to perform a genome-wide analysis of the genetic diversity in cultivated coffee germplasm and in wild populations growing in the center of origin of the species. We assembled a total length of 1.536 Gbp, 444 Mb and 527 Mb of which were assigned to the canephora and eugenioides subgenomes, respectively, and predicted 46,562 gene models, 21,254 and 22,888 of which were assigned to the canephora and to the eugeniodes subgenome, respectively. Through a genome-wide SNP genotyping of 736 C. arabica accessions, we analyzed the genetic diversity in the species and its relationship with geographic distribution and historical records. We observed a weak population structure due to low-frequency derived alleles and highly negative values of Taijma’s D, suggesting a recent and severe bottleneck, most likely resulting from a single event of polyploidization, not only for the cultivated germplasm but also for the entire species. This conclusion is strongly supported by forward simulations of mutation accumulation. However, PCA revealed a cline of genetic diversity reflecting a west-to-east geographical distribution from the center of origin in East Africa to the Arabian Peninsula. The extremely low levels of variation observed in the species, as a consequence of the polyploidization event, make the exploitation of diversity within the species for breeding purposes less interesting than in most crop species and stress the need for introgression of new variability from the diploid progenitors.
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- 2020
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126. Engineering a 3D in vitro model of human skeletal muscle at the single fiber scale
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Nicola Vitulo, Nicolò Mattei, Monica Giomo, Camilla Luni, Libero Vitiello, Giulia Selmin, Anna Urciuolo, Giorgio Valle, Nicola Elvassore, Massimo Vetralla, Rusha Ghua, Susi Zatti, Elena Serena, Urciuolo, Anna, Serena, Elena, Ghua, Rusha, Zatti, Susi, Giomo, Monica, Mattei, Nicolò, Vetralla, Massimo, Selmin, Giulia, Luni, Camilla, Vitulo, Nicola, Valle, Giorgio, Vitiello, Libero, and Elvassore, Nicola
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0301 basic medicine ,Muscle Fibers, Skeletal ,Cell Culture Techniques ,Molecular Conformation ,Skeletal muscle ,Gene Expression ,02 engineering and technology ,3D topology ,scaffold ,myogenic differentiation ,Muscle Development ,Sarcomere ,Biochemistry ,Myoblasts ,Dystrophin ,Mice ,Contractile Proteins ,Animal Cells ,ES-derived myoblasts ,Myosin ,Materials Testing ,Medicine and Health Sciences ,Morphogenesis ,Myocyte ,Musculoskeletal System ,Materials ,Cells, Cultured ,3D topological cues ,3D cell culture ,hydrogel scaffold ,Multidisciplinary ,Tissue Scaffolds ,Myogenesis ,Chemistry ,Muscles ,Stem Cells ,Skeletal muscle tissue engineering ,3D myogenic cell culture ,myobundles ,human myoblasts ,2D vs 3D in vitro culture comparison ,Cell Differentiation ,Hydrogels ,myobundle ,021001 nanoscience & nanotechnology ,Muscle Differentiation ,Cell biology ,Myotube differentiation ,medicine.anatomical_structure ,3D in vitro culture ,Physical Sciences ,Medicine ,Single-Cell Analysis ,Anatomy ,Cellular Types ,0210 nano-technology ,Extracellular matrix organization ,Research Article ,hydrogel laminin transcriptome ,Science ,Amorphous Solids ,Materials Science ,Motor Proteins ,Actin Motors ,Myosins ,Models, Biological ,03 medical and health sciences ,Molecular Motors ,medicine ,Genetics ,Animals ,Humans ,Dimethylpolysiloxanes ,Muscle, Skeletal ,Sarcolemma ,Tissue Engineering ,Biology and Life Sciences ,Proteins ,Cell Biology ,embryonic stem cell ,Cytoskeletal Proteins ,030104 developmental biology ,Skeletal Muscles ,Mixtures ,myotube ,myoblast ,hydrogel ,transcriptome ,Gels ,Developmental Biology - Abstract
The reproduction of reliable in vitro models of human skeletal muscle is made harder by the intrinsic 3D structural complexity of this tissue. Here we coupled engineered hydrogel with 3D structural cues and specific mechanical properties to derive human 3D muscle constructs ("myobundles") at the scale of single fibers, by using primary myoblasts or myoblasts derived from embryonic stem cells. To this aim, cell culture was performed in confined, laminin-coated micrometric channels obtained inside a 3D hydrogel characterized by the optimal stiffness for skeletal muscle myogenesis. Primary myoblasts cultured in our 3D culture system were able to undergo myotube differentiation and maturation, as demonstrated by the proper expression and localization of key components of the sarcomere and sarcolemma. Such approach allowed the generation of human myobundles of ~10 mm in length and ~120 μm in diameter, showing spontaneous contraction 7 days after cell seeding. Transcriptome analyses showed higher similarity between 3D myobundles and skeletal signature, compared to that found between 2D myotubes and skeletal muscle, mainly resulting from expression in 3D myobundles of categories of genes involved in skeletal muscle maturation, including extracellular matrix organization. Moreover, imaging analyses confirmed that structured 3D culture system was conducive to differentiation/maturation also when using myoblasts derived from embryonic stem cells. In conclusion, our structured 3D model is a promising tool for modelling human skeletal muscle in healthy and diseases conditions.
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- 2019
127. Multilevel comparative bioinformatics to investigate evolutionary relationships and specificities in gene annotations: An example for tomato and grapevine
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Maria Luisa Chiusano, Hamed Bostan, Marco Miralto, Nicola Vitulo, Giorgio Valle, Mario Pezzotti, Mohamed Zouine, Amalia Barone, Mondher Bouzayen, Luca Ambrosino, Luigi Frusciante, Valentino Ruggieri, Ambrosino, Luca, Ruggieri, Valentino, Bostan, Hamed, Miralto, Marco, Vitulo, Nicola, Zouine, Mohamed, Barone, Amalia, Bouzayen, Mondher, Frusciante, Luigi, Pezzotti, Mario, Valle, Giorgio, Chiusano, Maria Luisa, Department of Agriculture, Università degli studi di Napoli Federico II, Stazione Zoologica Anton Dohrn (SZN), Centre de Recerca en Agrigenòmica - Center for Research in Agricultural Genomics, Partenaires INRAE, North Carolina State University, Center for High Performance Simulation and Department of Chemical and Biomolecular Engineering, University of Verona (UNIVR), Génomique et Biotechnologie des Fruits (GBF), Institut National de la Recherche Agronomique (INRA)-École nationale supérieure agronomique de Toulouse [ENSAT]-Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées, Universita di Padova, Genopom Pro (PON02_00395_3082360) and HORT (PON02_00395_3215002) Projects (Ministero dell’Istruzione, dell’Università e della Ricerca (MIUR), Italy), The Cost Action FA1106, European Project: 289220,EC:FP7:PEOPLE,FP7-PEOPLE-2011-ITN,SPOT-ITN(2012), Producció Vegetal, Genòmica i Biotecnologia, Ministero dell'Istruzione, dell'Università e della Ricerca, and European Commission
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0106 biological sciences ,0301 basic medicine ,Transcription Factor ,[SDV]Life Sciences [q-bio] ,Messenger ,Gene regulatory network ,Bioinformatics ,01 natural sciences ,Genome ,Biochemistry ,Comparative genomics ,Orthologs ,Paralogs ,Tomato ,Grapevine ,Species specific gene loci ,Solanum lycopersicum ,Gene Expression Regulation, Plant ,Structural Biology ,Gene Regulatory Networks ,Vitis ,lcsh:QH301-705.5 ,Phylogeny ,Ortholog ,Gene Regulatory Network ,Applied Mathematics ,Computer Science Applications1707 Computer Vision and Pattern Recognition ,Biological Evolution ,Multilevel Analysi ,Computer Science Applications ,Multilevel Analysis ,lcsh:R858-859.7 ,DNA microarray ,Genome, Plant ,Protein domain ,Biology ,lcsh:Computer applications to medicine. Medical informatics ,03 medical and health sciences ,Comparative genomic ,[SDV.BV]Life Sciences [q-bio]/Vegetal Biology ,RNA, Messenger ,Lycopersicon esculentum ,Gene ,Molecular Biology ,Computational Biology ,Transcription Factors ,Molecular Sequence Annotation ,Research ,Paralog ,fungi ,Gene Annotation ,Plant ,Viti ,030104 developmental biology ,lcsh:Biology (General) ,Gene Expression Regulation ,RNA ,Function (biology) ,010606 plant biology & botany - Abstract
[Background]: “Omics” approaches may provide useful information for a deeper understanding of speciation events, diversification and function innovation. This can be achieved by investigating the molecular similarities at sequence level between species, allowing the definition of ortholog and paralog genes. However, the spreading of sequenced genome, often endowed with still preliminary annotations, requires suitable bioinformatics to be appropriately exploited in this framework., [Results]: We presented here a multilevel comparative approach to investigate on genome evolutionary relationships and peculiarities of two fleshy fruit species of relevant agronomic interest, Solanum lycopersicum (tomato) and Vitis vinifera (grapevine). We defined 17,823 orthology relationships between tomato and grapevine reference gene annotations. The resulting orthologs are associated with the detected paralogs in each species, permitting the definition of gene networks, useful to investigate the different relationships. The reconciliation of the compared collections in terms of an updating of the functional descriptions was also exploited. All the results were made accessible in ComParaLogs, a dedicated bioinformatics platform available at http://biosrv.cab.unina.it/comparalogs/gene/search., [Conclusions]: The aim of the work was to suggest a reliable approach to detect all similarities of gene loci between two species based on the integration of results from different levels of information, such as the gene, the transcript and the protein sequences, overcoming possible limits due to exclusive protein versus protein comparisons. This to define reliable ortholog and paralog genes, as well as species specific gene loci in the two species, overcoming limits due to the possible draft nature of preliminary gene annotations. Moreover, reconciled functional descriptions, as well as common or peculiar enzymatic classes and protein domains from tomato and grapevine, together with the definition of species-specific gene sets after the pairwise comparisons, contributed a comprehensive set of information useful to comparatively exploit the two species gene annotations and investigate on differences between species with climacteric and non-climacteric fruits. In addition, the definition of networks of ortholog genes and of associated paralogs, and the organization of web-based interfaces for the exploration of the results, defined a friendly computational bench-work in support of comparative analyses between two species., Publication costs for this manuscript were sponsored by the Genopom Pro (PON02_00395_3082360) and HORT (PON02_00395_3215002) Projects (Ministero dell’Istruzione, dell’Università e della Ricerca (MIUR), Italy) and from the Solanaceae Pollen Thermotolerance - Marie Curie Initial Training Network project (Grant Agreement No. 289220). This work is the frame of the Cost Action FA1106.
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- 2018
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128. High-throughput sequencing of microRNAs in glucocorticoid sensitive paediatric inflammatory bowel disease patients
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Gabriele Stocco, Marianna Lucafò, Nicola Vitulo, Claudio Forcato, Stefano Martelossi, Alessia Di Silvestre, Giorgio Valle, Giuliana Decorti, Rosanna Zimbello, Sara De Iudicibus, Marco Gerdol, Matteo Bramuzzo, Fabio De Pascale, Alessandro Ventura, Samuele Naviglio, De Iudicibus, Sara, Lucafò, Marianna, Vitulo, Nicola, Martelossi, Stefano, Zimbello, Rosanna, De Pascale, Fabio, Forcato, Claudio, Naviglio, Samuele, Di Silvestre, Alessia, Gerdol, Marco, Stocco, Gabriele, Valle, Giorgio, Ventura, Alessandro, Bramuzzo, Matteo, and Decorti, Giuliana
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0301 basic medicine ,glucocorticoids ,mRNA ,inflammatory bowel disease ,pediatric patients ,Male ,Pediatric patients ,Inflammatory bowel disease ,Transcriptome ,lcsh:Chemistry ,Pediatric patient ,Glucocorticoid ,Receptors ,Child ,lcsh:QH301-705.5 ,Spectroscopy ,Regulation of gene expression ,High-Throughput Nucleotide Sequencing ,General Medicine ,Computer Science Applications ,Adolescent ,Female ,Gene Expression Regulation ,Glucocorticoids ,Humans ,Inflammatory Bowel Diseases ,MicroRNAs ,Receptors, Glucocorticoid ,Biomarkers ,medicine.drug ,Biology ,Catalysis ,DNA sequencing ,Article ,Inorganic Chemistry ,03 medical and health sciences ,microRNA ,medicine ,Physical and Theoretical Chemistry ,Molecular Biology ,Gene ,Organic Chemistry ,Promoter ,030104 developmental biology ,lcsh:Biology (General) ,lcsh:QD1-999 ,Pharmacogenomics ,Cancer research - Abstract
The aim of this research was the identification of novel pharmacogenomic biomarkers for better understanding the complex gene regulation mechanisms underpinning glucocorticoid (GC) action in paediatric inflammatory bowel disease (IBD). This goal was achieved by evaluating high-throughput microRNA (miRNA) profiles during GC treatment, integrated with the assessment of expression changes in GC receptor (GR) heterocomplex genes. Furthermore, we tested the hypothesis that differentially expressed miRNAs could be directly regulated by GCs through investigating the presence of GC responsive elements (GREs) in their gene promoters. Ten IBD paediatric patients responding to GCs were enrolled. Peripheral blood was obtained at diagnosis (T0) and after four weeks of steroid treatment (T4). MicroRNA profiles were analyzed using next generation sequencing, and selected significantly differentially expressed miRNAs were validated by quantitative reverse transcription-polymerase chain reaction. In detail, 18 miRNAs were differentially expressed from T0 to T4, 16 of which were upregulated and 2 of which were downregulated. Out of these, three miRNAs (miR-144, miR-142, and miR-96) could putatively recognize the 3’UTR of the GR gene and three miRNAs (miR-363, miR-96, miR-142) contained GREs sequences, thereby potentially enabling direct regulation by the GR. In conclusion, we identified miRNAs differently expressed during GC treatment and miRNAs which could be directly regulated by GCs in blood cells of young IBD patients. These results could represent a first step towards their translation as pharmacogenomic biomarkers.
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- 2018
129. An improved reference of the grapevine genome reasserts the origin of the PN40024 highly homozygous genotype.
- Author
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Velt A, Frommer B, Blanc S, Holtgräwe D, Duchêne É, Dumas V, Grimplet J, Hugueney P, Kim C, Lahaye M, Matus JT, Navarro-Payá D, Orduña L, Tello-Ruiz MK, Vitulo N, Ware D, and Rustenholz C
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- Genotype, Chromosome Mapping, Base Sequence, Molecular Sequence Annotation, Genome, Plant, Vitis genetics
- Abstract
The genome sequence of the diploid and highly homozygous Vitis vinifera genotype PN40024 serves as the reference for many grapevine studies. Despite several improvements to the PN40024 genome assembly, its current version PN12X.v2 is quite fragmented and only represents the haploid state of the genome with mixed haplotypes. In fact, being nearly homozygous, this genome contains several heterozygous regions that are yet to be resolved. Taking the opportunity of improvements that long-read sequencing technologies offer to fully discriminate haplotype sequences, an improved version of the reference, called PN40024.v4, was generated. Through incorporating long genomic sequencing reads to the assembly, the continuity of the 12X.v2 scaffolds was highly increased with a total number decreasing from 2,059 to 640 and a reduction in N bases of 88%. Additionally, the full alternative haplotype sequence was built for the first time, the chromosome anchoring was improved and the number of unplaced scaffolds was reduced by half. To obtain a high-quality gene annotation that outperforms previous versions, a liftover approach was complemented with an optimized annotation workflow for Vitis. Integration of the gene reference catalogue and its manual curation have also assisted in improving the annotation, while defining the most reliable estimation of 35,230 genes to date. Finally, we demonstrated that PN40024 resulted from 9 selfings of cv. "Helfensteiner" (cross of cv. "Pinot noir" and "Schiava grossa") instead of a single "Pinot noir". These advances will help maintain the PN40024 genome as a gold-standard reference, also contributing toward the eventual elaboration of the grapevine pangenome., Competing Interests: Conflicts of interest The author(s) declare no conflict of interest., (© The Author(s) 2023. Published by Oxford University Press on behalf of the Genetics Society of America.)
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- 2023
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130. benchdamic: benchmarking of differential abundance methods for microbiome data.
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Calgaro M, Romualdi C, Risso D, and Vitulo N
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- Reproducibility of Results, Metagenomics, Software, Benchmarking
- Abstract
Summary: Recently, an increasing number of methodological approaches have been proposed to tackle the complexity of metagenomics and microbiome data. In this scenario, reproducibility and replicability have become two critical issues, and the development of computational frameworks for the comparative evaluations of such methods is of utmost importance. Here, we present benchdamic, a Bioconductor package to benchmark methods for the identification of differentially abundant taxa., Availability and Implementation: benchdamic is available as an open-source R package through the Bioconductor project at https://bioconductor.org/packages/benchdamic/., Supplementary Information: Supplementary data are available at Bioinformatics online., (© The Author(s) 2022. Published by Oxford University Press.)
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- 2023
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131. A leukemia-enriched cDNA microarray platform identifies new transcripts with relevance to the biology of pediatric acute lymphoblastic leukemia.
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De Pittà C, Tombolan L, Campo Dell'Orto M, Accordi B, te Kronnie G, Romualdi C, Vitulo N, Basso G, and Lanfranchi G
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- Adolescent, Bone Marrow metabolism, Child, Child, Preschool, Cluster Analysis, DNA, Complementary metabolism, Gene Library, Humans, Infant, Sequence Analysis, DNA, Gene Expression Regulation, Neoplastic, Oligonucleotide Array Sequence Analysis instrumentation, Oligonucleotide Array Sequence Analysis methods, Precursor Cell Lymphoblastic Leukemia-Lymphoma genetics
- Abstract
Background and Objectives: Microarray gene expression profiling has been widely applied to characterize hematologic malignancies, has attributed a molecular signature to leukemia subclasses and has allowed new subclasses to be distinguished. We set out to use microarray technology to identify novel genes relevant for leukemogenesis. To this end we used a unique leukemia-enriched cDNA microarray platform., Design and Methods: The systematic sequencing of cDNA libraries of normal and leukemic bone marrow allowed us to increase the number of genes to yield a new release of a previously generated cDNA microarray. Using this platform we analyzed the expression profiles of 4,670 genes in bone marrow samples from 18 pediatric patients with acute lymphoblastic leukemia (ALL)., Results: Expression profiling consistently distinguished the leukemia patients into three groups, those with T-ALL, B-ALL and B-ALL with MLL/AF4 rearrangement, in agreement with the clinical classification. Our platform identified 30 genes that best discriminate these three subtypes. Using mini-array technology these 30 genes were validated in another cohort of 17 patients. In particular we identified two novel genes not previously reported: endomucin (EMCN) and ubiquitin specific protease 33 (USP33) that appear to be over-expressed in B-ALL relative to their expression in T-ALL., Interpretation and Conclusions: Microarray technology not only allows the distinction between disease subclasses but also offers a chance to identify new genes involved in leukemogenesis. Our approach of using a unique platform has proven to be fruitful in identifying new genes and we suggest exploration of other malignancies using this approach.
- Published
- 2005
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