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1. Identification of differential gene expression in in vitro FSH treated pig granulosa cells using suppression subtractive hybridization

Author

Tosser-Klopp G, Dehais P, Frappart PO, Bonnet A, and Hatey F

Subjects
Gynecology and obstetrics, RG1-991, Reproduction, QH471-489
Abstract

Abstract FSH, which binds to specific receptors on granulosa cells in mammals, plays a key role in folliculogenesis. Its biological activity involves stimulation of intercellular communication and upregulation of steroidogenesis, but the entire spectrum of the genes regulated by FSH has yet to be fully characterized. In order to find new regulated transcripts, however rare, we have used a Suppression Subtractive Hybridization approach (SSH) on pig granulosa cells in primary culture treated or not with FSH. Two SSH libraries were generated and 76 clones were sequenced after selection by differential screening. Sixty four different sequences were identified, including 3 novel sequences. Experiments demonstrated the presence of 25 regulated transcripts. A gene ontology analysis of these 25 genes revealed (1) catalytic; (2) transport; (3) signal transducer; (4) binding; (5) anti-oxidant and (6) structural activities. These findings may deepen our understanding of FSH's effects. Particularly, they suggest that FSH is involved in the modulation of peroxidase activity and remodelling of chromatin.

Published
2006
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3. Y-chromosomal haplogroups from wild and domestic goats reveal ancient migrations and recent introgressions

Author

Lenstra, J.A., Consortium, VarGoats, Nijman, I.J., Rosen, B.D., Bardou, P., Faraut, T., Cumer, T., Daly, K.G., Zheng, Z., Cai, Y., Asadollahpour, H., Kul, Çınar B., Zhang, W.-Y., E, G., Ayin, A., Bakhtin, M., Balteanu, V.A., Barfield, D., Baird, H., Berger, B., Blichfeldt, T., Boink, G., Bugiwati, S.R.A., Cai, Z., Carolan, S., Clark, E., Cubric-Curik, V., Dagong, M.I.A., Dorji, T., Drew, L., Guo, J., Hallsson, J., Horvat, S., Kantanen, J., Kawaguchi, F., Kazymbet, P., Khayatzadeh, N., Kim, N., Kumar Shah, M., Liao, Y., Martínez, A., Masangkay, J.S., Masaoka, M., Mazza, R., McEwan, J., Milanesi, M., Omar, F.Md., Nomura, Y., Ouchene-Khelifi, N.-A., Pereira, F., Sahana, G., Sasazaki, S., Da Silva, A., Simčič, M., Sölkner, J., Sutherland, A., Tigchelaar, J., Zhang, H., Consortium, Econogene, Ajmone-Marsan, P., Bradley, D.G., Colli, L., Drögemüller, C., Lei, C., Mannen, H., Pompanon, F., Tosser-Klopp, G., Jiang, Y., Veerkamp, R. F., and de Haas, Y.

Subjects
630 Agriculture, 590 Animals (Zoology), 570 Life sciences, biology
Abstract

By its paternal transmission, Y-chromosomal haplotypes are sensitive markers of population history and male-mediated introgression. We used whole-genome sequences (WGSs) of 386 domestic goats from 75 modern breeds and 7 wild goat species generated by the VarGoats goat genome project. Phylogenetic analyses indicated five domestic haplogroups Y1AA, Y1AB, Y1B, Y2A and Y2B. Haplogroup distributions for 180 domestic breeds indicate ancient paternal population bottlenecks during the migration into northern Europe, southern Asia and Africa. Sharing of haplogroups reveals male-mediated introgressions: from Asia into Madagascar and, more recently, into the South-African Boer goat; then from this breed into other southeastern African goats; and from Europe into native Korean and Ugandan goats. This study illustrates the power of the Y-chromosomal variation for the reconstructing the history of domestic species with a wide geographic range.

Published
2023

5. Geographical contrasts of Y-chromosomal haplogroups from wild and domestic goats reveal ancient migrations and recent introgressions

Author

Nijman, I. J., Rosen, B. D., Bardou, P., Faraut, T., Cumer, T., Daly, K. G., Zheng, Z., Cai, Y., Asadollahpour, H., Kul, B. C., Zhang, W. -Y., Guangxin, E., Ayin, A., Baird, H., Bakhtin, M., Balteanu, V. A., Barfield, D., Berger, B., Blichfeldt, T., Boink, G., Bugiwati, S. R. A., Cai, Z., Carolan, S., Clark, E., Cubric-Curik, V., Dagong, M. I. A., Dorji, T., Drew, L., Guo, J., Hallsson, J., Horvat, S., Kantanen, J., Kawaguchi, F., Kazymbet, P., Khayatzadeh, N., Kim, N., Shah, M. K., Liao, Y., Martinez, A., Masangkay, J., Masaoka, M., Mazza, R., Mcewan, J., Milanesi, M., Omar, F. M., Nomura, Y., Ouchene-Khelifi, N. -A., Pereira, F., Sahana, G., Salavati, M., Sasazaki, S., Da Silva, A., Simcic, M., Solkner, J., Sutherland, A., Tigchelaar, J., Zhang, H., Ajmone-Marsan, P., Bradley, D. G., Colli, L., Drogemuller, C., Jiang, Y., Lei, C., Mannen, H., Pompanon, F., Tosser-Klopp, G., Lenstra, J. A., Kijas, J., Guldbrandtsen, B., Denoyelle, L., Sarry, J., le Talouarn, E., Alberti, A., Orvain, C., Engelen, S., Duby, D., Martin, P., Danchin, C., Duclos, D., Allain, D., Arquet, R., Mandonnet, N., Naves, M., Palhiere, I., Rupp, R., Rezaei, H. R., Foran, M., Stella, A., Del Corvo, M., Crisa, A., Marletta, D., Crepaldi, P., Ottino, M., Randi, E., Mujibi, D. F., Gondwe, T., Benjelloun, B., Taela, M. D. G., Nash, O., Moaeen-ud-Din, M., Visser, C., Goyache, F., Alvarez, I., Amills, M., Sanchez, A., Capote, J., Jordana, J., Pons, A., Balears, I., Molina, A., Mruttu, H. A., Masiga, C. W., Van Tassell, C. P., Reecy, J., Luikart, G., Sikosana, J., Anila, H., Petrit, D., Roswitha, B., Philippe, B., Aziz, F., Christos, P., El-Barody, M. A. A., Pierre, T., Phillip, E., Gordon, L., Albano, B. -P., Stephanie, Z., Michel, T., Georg, E., Horst, B., Eveline, I. -A., Luhken, G., Krugmann, D., Eva-Maria, P., Shirin, L., Katja, G., Christina, P., Jutta, R., Marco, B., Andreas, G., Al Tarrayrah, J., Georgios, K., Olga, K., Katerina, K., Christina, L., Anton, I., Lazlo, F., Gabriele, C., Elisabetta, M., Marco, P., Antonello, C., Tiziana, S., Mario, C., Francesca, F., Stefano, G., Marta, M., Bordonaro, S., Giuseppe, D. U., Fabio, P., Mariasilvia, D. A., Alessio, V., Irene, C., Lorraine, P., Mahamoud, A. -S., Van Cann, L. M., Roman, N., Popielarczyk, D., Ewa, S., Augustin, V., Susana, D., Javier, C., Oscar, C., David, G., Regis, C., Gabriela, O. -R., Glowatzki, M. -L., Okan, E., Inci, T., Evren, K., Mike, B., Trinidad, P., Gabriela, J., Godfrey, H., Stella, D., Louise, W., Martin, T., Sam, J., and Riccardo, S.

Subjects
haplogroup, introgresija, domestication, goat, introgression, migration, phylogeography, Y-chromosome, Evolution, MITOCHONDRIAL-DNA, FLOW, Haplotypes/genetics, divje koze, DNA, Mitochondrial, DNA, Mitochondrial/genetics, Behavior and Systematics, BREEDS, Y Chromosome, Goats/genetics, Genetics, Animals, domače koze, Ecology, Evolution, Behavior and Systematics, Phylogeny, udc:575:636.39, kozorogi, Ecology, 630 Agriculture, Goats, Genetic Variation, NETWORKS, DIFFERENTIATION, genetika, Haplotypes, ORIGINS, GENETIC DIVERSITY, 590 Animals (Zoology), 570 Life sciences, biology, Y Chromosome/genetics
Abstract

By their paternal transmission, Y-chromosomal haplotypes are sensitive markers of population history and male-mediated introgression. Previous studies identified biallelic single-nucleotide variants in the SRY, ZFY and DDX3Y genes, which in domestic goats identified four major Y-chromosomal haplotypes, Y1A, Y1B, Y2A and Y2B, with a marked geographical partitioning. Here, we extracted goat Y-chromosomal variants from whole-genome sequences of 386 domestic goats (75 breeds) and seven wild goat species, which were generated by the VarGoats goat genome project. Phylogenetic analyses indicated domestic haplogroups corresponding to Y1B, Y2A and Y2B, respectively, whereas Y1A is split into Y1AA and Y1AB. All five haplogroups were detected in 26 ancient DNA samples from southeast Europe or Asia. Haplotypes from present-day bezoars are not shared with domestic goats and are attached to deep nodes of the trees and networks. Haplogroup distributions for 186 domestic breeds indicate ancient paternal population bottlenecks and expansions during migrations into northern Europe, eastern and southern Asia, and Africa south of the Sahara. In addition, sharing of haplogroups indicates male-mediated introgressions, most notably an early gene flow from Asian goats into Madagascar and the crossbreeding that in the 19th century resulted in the popular Boer and Anglo-Nubian breeds. More recent introgressions are those from European goats into the native Korean goat population and from Boer goat into Uganda, Kenya, Tanzania, Malawi and Zimbabwe. This study illustrates the power of the Y-chromosomal variants for reconstructing the history of domestic species with a wide geographical range.

Published
2022

6. The SNP-Based Profiling of Montecristo Feral Goat Populations Reveals a History of Isolation, Bottlenecks, and the Effects of Management

Author

Somenzi, Elisa, Senczuk, G., Ciampolini, R., Cortellari, M., Vajana, Elia, Tosser-Klopp, G., Pilla, F., Ajmone Marsan, Paolo, Crepaldi, P., Colli, Licia, Somenzi E., Vajana E., Ajmone Marsan P. (ORCID:0000-0003-3165-4579), Colli L. (ORCID:0000-0002-7221-2905), Somenzi, Elisa, Senczuk, G., Ciampolini, R., Cortellari, M., Vajana, Elia, Tosser-Klopp, G., Pilla, F., Ajmone Marsan, Paolo, Crepaldi, P., Colli, Licia, Somenzi E., Vajana E., Ajmone Marsan P. (ORCID:0000-0003-3165-4579), and Colli L. (ORCID:0000-0002-7221-2905)

Abstract

The Montecristo wild goat is an endangered feral population that has been on the homony-mous island in the Tuscan Archipelago since ancient times. The origins of Montecristo goats are still debated, with authors dating their introduction either back to Neolithic times or between the 6th and 13th century of the Common Era. To investigate the evolutionary history and relationships of this population we assembled a 50K SNP dataset including 55 Mediterranean breeds and two nuclei of Montecristo goats sampled on the island and from an ex situ conservation project. Diversity levels, gene flow, population structure, and genetic relationships were assessed through multiple approaches. The insular population scored the lowest values of both observed and expected heterozygosity, high-lighting reduced genetic variation, while the ex situ nucleus highlighted a less severe reduction. Multivariate statistics, network, and population structure analyses clearly separated the insular nucleus from all other breeds, including the population of Montecristo goats from the mainland. Moreover, admixture and gene flow analyses pinpointed possible genetic inputs received by the two Montecristo goat nuclei from different sources, while Runs of Homozygosity (ROHs) indicated an ancient bottleneck/founder effect in the insular population and recent extensive inbreeding in the ex situ one. Overall, our results suggest that Montecristo goats experienced several demographic fluctuations combined with admixture events over time and highlighted a noticeable differentiation between the two nuclei.

Published
2022

7. Y-chromosomal haplogroups from wild and domestic goats reveal ancient migrations and recent introgressions

Author

Lenstra, J.A., VarGoats Consortium, Nijman, I.J., Rosen, B.D., Bardou, P., Faraut, T., Cumer, T., Daly, K.G., Zheng, Z., Cai, Y., Asadollahpour, H., Kul, B., Zhang, W.-Y., E, G., Ayin, A., Bakhtin, M., Bâlteanu, V.A., Barfield, D., Baird, H., Berger, B., Blichfeldt, T., Boink, G., Bugiwati, S.R.A., Cai, Z., Carolan, S., Clark, E., Cubric-Curik, Vlatka, Dagong, M.I.A., Dorji, T., Drew, L., Guo, J., Hallsson, J., Horvat, S., Kantanen, J., Kawaguchi, F., Kazymbet, P., Khayatzadeh, N., Kim, N., Kumar Shah, M., Liao, Y., Martínez, A., Masangkay, J. S., Masaoka, M., Mazza, R., McEwan, J., Milanesi, M., Omar, F. Md., Nomura, Y., Ouchene-Khelifi, N.-A., Pereira, F., Sahana, G., Sasazaki, S., Da Silva, A., Simčič, M., Sölkner, J., Sutherland, A., Tigchelaar, J., Zhang, H., Econogene Consortium, Ajmone- Marsan, P., Bradley, D. G., Colli, L., Drögemüller, C., Lei, C., Mannen, H., Pompanon, F., Tosser-Klopp, G., and Jiang, Y.

Subjects
wild and domestic goats, Y-chromosome, haplogroups, migrations, introgressions
Abstract

By its paternal transmission, Y-chromosomal haplotypes are sensitive markers of population history and male-mediated introgression. We used whole-genome sequences (WGSs) of 386 domestic goats from 75 modern breeds and 7 wild goat species generated by the VarGoats goat genome project. Phylogenetic analyses indicated five domestic haplogroups Y1AA, Y1AB, Y1B, Y2A and Y2B. Haplogroup distributions for 180 domestic breeds indicate ancient paternal population bottlenecks during the migration into northern Europe, southern Asia and Africa. Sharing of haplogroups reveals male-mediated introgressions: from Asia into Madagascar and, more recently, into the South-African Boer goat ; then from this breed into other southeastern African goats ; and from Europe into native Korean and Ugandan goats. This study illustrates the power of the Y-chromosomal variation for the reconstructing the history of domestic species with a wide geographic range.

Published
2022

8. VarGoats project : a dataset of 1159 whole-genome sequences to dissect Capra hircus global diversity

Author

Denoyelle, L., Talouarn, E., Bardou, P., Colli, L., Alberti, A., Danchin, C., Del Corvo, M., Engelen, S., Orvain, C., Palhiere, I., Rupp, R., Sarry, J., Salavati, M., Amills, M., Clark, E., Crepaldi, P., Faraut, T., Masiga, C. W., Pompanon, F., Rosen, B. D., Stella, A., Van Tassell, C. P., Tosser-Klopp, G., Kijas, J., Guldbrandtsen, B., Kantanen, J., Duby, D., Martin, P., Duclos, D., Allain, D., Arquet, R., Mandonnet, N., Naves, M., Carolan, S., Foran, M., Crisa, A., Marletta, D., Ottino, M., Randi, E., Benjelloun, B., Lenstra, H., Moaeen-ud-Din, M., Reecy, J., Goyache, F., Alvarez, I., Capote, J., Jordana, J., Pons, A., Martinez, A., Molina, A., Rosen, B., Drogemuller, C., Luikart, G., Mruttu, H. A., Gondwe, T., Sikosana, J., Taela, M. D. G., Nash, O., Agence Nationale de la Recherche (France), Région Occitanie / Pyrénées-Méditerranée, Ministère de l’Enseignement supérieur et de la Recherche (France), Biotechnology and Biological Sciences Research Council (UK), Bill & Melinda Gates Foundation, Department for International Development (UK), Center for Tropical Studies and Conservation (US), University of Edinburgh, Scottish Government's Rural and Environment Science and Analytical Services, Laboratoire d'Ecologie Alpine (LECA ), Université Savoie Mont Blanc (USMB [Université de Savoie] [Université de Chambéry])-Centre National de la Recherche Scientifique (CNRS)-Université Grenoble Alpes (UGA), Génétique Physiologie et Systèmes d'Elevage (GenPhySE ), Ecole Nationale Vétérinaire de Toulouse (ENVT), Institut National Polytechnique (Toulouse) (Toulouse INP), Université de Toulouse (UT)-Université de Toulouse (UT)-Institut National Polytechnique (Toulouse) (Toulouse INP), Université de Toulouse (UT)-Université de Toulouse (UT)-École nationale supérieure agronomique de Toulouse (ENSAT), Université de Toulouse (UT)-Université de Toulouse (UT)-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE), Système d'Information des GENomes des Animaux d'Elevage (SIGENAE), Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE), Università cattolica del Sacro Cuore [Piacenza e Cremona] (Unicatt), Génomique métabolique (UMR 8030), Genoscope - Centre national de séquençage [Evry] (GENOSCOPE), Université Paris-Saclay-Direction de Recherche Fondamentale (CEA) (DRF (CEA)), Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Université Paris-Saclay-Direction de Recherche Fondamentale (CEA) (DRF (CEA)), Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Université d'Évry-Val-d'Essonne (UEVE)-Centre National de la Recherche Scientifique (CNRS), Institut de l'élevage (IDELE), Università cattolica del Sacro Cuore [Milano] (Unicatt), The Roslin Institute, Biotechnology and Biological Sciences Research Council (BBSRC), Centre for Tropical Livestock Genetics and Health [Edimburgh] (CTLGH), Centre for Research in Agricultural Genomics (CRAG), Università degli Studi di Milano = University of Milan (UNIMI), Tropical Institute of Development Innovations (TRIDI), USDA Agricultural Research Service [Beltsville, Maryland], USDA-ARS : Agricultural Research Service, Consiglio Nazionale delle Ricerche [Milano] (CNR), CSIRO Agriculture and Food (CSIRO), Unité de Recherches Zootechniques (URZ), APIS-GENE, Occitanie region, Ministere de l'Enseignement superieur, de la Recherche et de l'Innovation, United States Agency for International Development (USAID), CGIAR:OPP1127286, ACTIVEGOAT & CAPRISNP projects, UK Research & Innovation (UKRI) : BBS/OS/GC/000012F, ANR-10-INBS-0009,France-Génomique,Organisation et montée en puissance d'une Infrastructure Nationale de Génomique(2010), ANR-11-INBS-0003,CRB-Anim,Réseau de Centres de Ressources Biologiques pour les animaux domestiques(2011), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-École nationale supérieure agronomique de Toulouse [ENSAT]-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE), Direction de Recherche Fondamentale (CEA) (DRF (CEA)), Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Université Paris-Saclay-Centre National de la Recherche Scientifique (CNRS)-Université d'Évry-Val-d'Essonne (UEVE), University of Milan, and Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Centre National de la Recherche Scientifique (CNRS)-Université d'Évry-Val-d'Essonne (UEVE)

Subjects
[SDV.BIO]Life Sciences [q-bio]/Biotechnology, [SDV]Life Sciences [q-bio], Short Communication, Single-nucleotide polymorphism, 610 Medicine & health, Biology, QH426-470, Genome, SF1-1100, Domestication, Animals, Domestication, Genetic Variation, Genomics, Goats, Genome, Genome-Wide Association Study, 03 medical and health sciences, Capra hircus, Genetics, Animals, Indel, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, Genetic association, 2. Zero hunger, 0303 health sciences, Genetic diversity, [SDV.BA.MVSA]Life Sciences [q-bio]/Animal biology/Veterinary medicine and animal Health, Settore AGR/17 - ZOOTECNICA GENERALE E MIGLIORAMENTO GENETICO, 630 Agriculture, Goats, 0402 animal and dairy science, Genetic Variation, 04 agricultural and veterinary sciences, General Medicine, Genomics, 15. Life on land, 040201 dairy & animal science, Animal culture, Evolutionary biology, 570 Life sciences, biology, 590 Animals (Zoology), Animal Science and Zoology, Reference genome, Genome-Wide Association Study
Abstract

[Background]: Since their domestication 10,500 years ago, goat populations with distinctive genetic backgrounds have adapted to a broad variety of environments and breeding conditions. The VarGoats project is an international 1000-genome resequencing program designed to understand the consequences of domestication and breeding on the genetic diversity of domestic goats and to elucidate how speciation and hybridization have modeled the genomes of a set of species representative of the genus Capra., [Findings]: A dataset comprising 652 sequenced goats and 507 public goat sequences, including 35 animals representing eight wild species, has been collected worldwide. We identified 74,274,427 single nucleotide polymorphisms (SNPs) and 13,607,850 insertion-deletions (InDels) by aligning these sequences to the latest version of the goat reference genome (ARS1). A Neighbor-joining tree based on Reynolds genetic distances showed that goats from Africa, Asia and Europe tend to group into independent clusters. Because goat breeds from Oceania and Caribbean (Creole) all derive from imported animals, they are distributed along the tree according to their ancestral geographic origin., [Conclusions]: We report on an unprecedented international effort to characterize the genome-wide diversity of domestic goats. This large range of sequenced individuals represents a unique opportunity to ascertain how the demographic and selection processes associated with post-domestication history have shaped the diversity of this species. Data generated for the project will also be extremely useful to identify deleterious mutations and polymorphisms with causal effects on complex traits, and thus will contribute to new knowledge that could be used in genomic prediction and genome-wide association studies., We are grateful to France Génomique “Call for high impact projects” (ANR‐10‐INBS‐09‐08) for selecting our project and providing us the resources to sequence 400 goats. We would like to mention that APIS-GENE funded some WGS sequences through ACTIVEGOAT & CAPRISNP projects. We thank the Occitanie region and the Animal Genetics Division of the French National Institute for Agriculture, Food and Environment (INRAE-GA) for financing the PhD of ET. We thank the Ministère de l'Enseignement supérieur, de la Recherche et de l'Innovation for financing LD. We thank André Eggen (Illumina) for providing chips to genotype 192 animals. We thank the Animal Genetics Division of the French National Institute for Agriculture, Food and Environment (INRAE-GA) for funding VarGoats2 grant, which allowed DNA extraction and genotyping of 384 animals and CRB-Anim, Grant Agreement ANR-11-INBS-0003, (https://crb-anim.fr/) for funding French local breeds sampling. We thank the Italian Goat and Sheep Breeders Association (AssoNaPa) for supporting in sampling. Whole-genome sequencing libraries for the African goats were prepared and sequenced by Edinburgh Genomics and funded via Biotechnology and Biological Sciences Research Council research grant (BBS/OS/GC/000012F) ‘Reference genome and population sequencing of African goats’ awarded to The Roslin Institute. USDA-ARS with funding from USAID funded the collection of samples from Uganda, Tanzania, Malawi, Mozambique and Zimbabwe. EC and MS were partially supported by the Bill & Melinda Gates Foundation and with UK aid from the UK Government’s Department for International Development (Grant Agreement OPP1127286) under the auspices of the Centre for Tropical Livestock Genetics and Health (CTLGH), established jointly by the University of Edinburgh, SRUC (Scotland’s Rural College), and the International Livestock Research Institute. The findings and conclusions contained within are those of the authors and do not necessarily reflect positions or policies of the Bill & Melinda Gates Foundation nor the UK Government.

Published
2021

9. Molecular characterization of the Montecristo feral goats in the Mediterranean context

Author

Somenzi, E., Senczuk, G., Ciampolini, R., Cortellari, M., Randi, E., Tosser-Klopp, G., Pilla, F., Ajmone-Marsan, P., Crepaldi, P., and Colli, L.

Subjects
Genomic Markers, Runs Of Homozygosity, Goat, Montecristo, SNPs, Genomic Markers, feral goats, Molecular characterization, Mediterranean context, Runs Of Homozygosity, ROHs, Goat, ROHs, feral goats, Montecristo, Mediterranean context, Molecular characterization, SNPs
Published
2021

10. Strongyle-resistant sheep express their potential across environments and leave limited scope for parasite plasticity

Author

Sallé, G., primary, Deiss, V., additional, Marquis, C., additional, Tosser-Klopp, G., additional, Cortet, J., additional, Serreau, D., additional, Koch, C., additional, Marcon, D., additional, Bouvier, F., additional, Jacquiet, P., additional, Holroyd, N., additional, Blanchard, A., additional, Cotton, J.A., additional, Mialon, M.M., additional, and Moreno-Romieux, C., additional

Published
2020
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11. Signatures of selection and environmental adaptation across the goat genome post-domestication 06 Biological Sciences 0604 Genetics

Author

Bertolini F., Servin B., Talenti A., Rochat E., Kim E.S., Oget C., Palhiere I., Crisa A., Catillo G., Steri R., Amills M., Colli L., Marras G., Milanesi M., Nicolazzi E., Rosen B.D., Van Tassell C.P., Guldbrandtsen B., Sonstegard T.S., Tosser-Klopp G., Stella A., Rothschild M.F., Joost S., Crepaldi P., Iowa State University, Technical University of Denmark (DTU), ENVT, Università Degli Studi di Milano, Ecole Polytechnique Fédérale de Lausanne (EPFL), Recombinetics Inc, Research Centre for Animal Production and Acquaculture, CSIC-IRTA-UAB-UB, Università Cattolica Del S. Cuore, Fondazione Parco Tecnologico Padano (PTP), Universidade Estadual Paulista (Unesp), ARS USDA, and Aarhus University

Subjects
goats, Ecology, Behavior and Systematics, Settore AGR/17 - ZOOTECNICA GENERALE E MIGLIORAMENTO GENETICO, Evolution, Genetics, Animal Science and Zoology, adaptation, Ecology, Evolution, Behavior and Systematics, selection signatures
Abstract

Made available in DSpace on 2019-10-06T15:24:30Z (GMT). No. of bitstreams: 0 Previous issue date: 2018-11-19 Background: Since goat was domesticated 10,000 years ago, many factors have contributed to the differentiation of goat breeds and these are classified mainly into two types: (i) adaptation to different breeding systems and/or purposes and (ii) adaptation to different environments. As a result, approximately 600 goat breeds have developed worldwide; they differ considerably from one another in terms of phenotypic characteristics and are adapted to a wide range of climatic conditions. In this work, we analyzed the AdaptMap goat dataset, which is composed of data from more than 3000 animals collected worldwide and genotyped with the CaprineSNP50 BeadChip. These animals were partitioned into groups based on geographical area, production uses, available records on solid coat color and environmental variables including the sampling geographical coordinates, to investigate the role of natural and/or artificial selection in shaping the genome of goat breeds. Results: Several signatures of selection on different chromosomal regions were detected across the different breeds, sub-geographical clusters, phenotypic and climatic groups. These regions contain genes that are involved in important biological processes, such as milk-, meat- or fiber-related production, coat color, glucose pathway, oxidative stress response, size, and circadian clock differences. Our results confirm previous findings in other species on adaptation to extreme environments and human purposes and provide new genes that could explain some of the differences between goat breeds according to their geographical distribution and adaptation to different environments. Conclusions: These analyses of signatures of selection provide a comprehensive first picture of the global domestication process and adaptation of goat breeds and highlight possible genes that may have contributed to the differentiation of this species worldwide. Department of Animal Science Iowa State University National Institute of Aquatic Resources Technical University of Denmark (DTU) GenPhySE INRA Université de Toulouse INPT ENVT Dipartimento di Medicina Veterinaria Università Degli Studi di Milano Laboratory of Geographic Information Systems (LASIG) School of Architecture Civil and Environmental Engineering (ENAC) Ecole Polytechnique Fédérale de Lausanne (EPFL) Recombinetics Inc Consiglio per la Ricerca in Agricoltura e l'Analisi dell'Economia Agraria (CREA) Research Centre for Animal Production and Acquaculture Centre for Research in Agricultural Genomics (CRAG) CSIC-IRTA-UAB-UB Campus Universitat Autonoma de Barcelona DIANA Dipartimento di Scienze Animali della Nutrizione e Degli Alimenti Università Cattolica Del S. Cuore BioDNA Centro di Ricerca sulla Biodiversità e sul DNA Antico Università Cattolica Del S. Cuore Fondazione Parco Tecnologico Padano (PTP) Department of Support Production and Animal Health School of Veterinary Medicine São Paulo State University (UNESP) Animal Genomics and Improvement Laboratory ARS USDA Center for Quantitative Genetics and Genomics Aarhus University Department of Support Production and Animal Health School of Veterinary Medicine São Paulo State University (UNESP)

Published
2018

15. Coordinated international action to accelerate genome-to-phenome with FAANG, the Functional Annotation of Animal Genomes project

Author

Tosser-Klopp, G., Zhou, H., Palti, Y., Nanduri, B., Tixier-Boichard, M., Silverstein, J., Plastow, G. S., Sarropoulou, E., Brauning, R., Zhao, S., Rohrer, G. A., Elsik, C. G., Cheng, H. H., Giuffra, E., Notredame, C., Khatib, H., Vilkki, J., Couldrey, C., Archibald, A. L., Tellam, R. L., Schmidt, C. J., Reecy, J. M., Clarke, L., Huang, L. S., Groenen, M. A., McEwan, J. C., Burt, D. W., Kim, H., Bottema, C. D., Kijas, J. W., Dalrymple, B. P., White, S. N., Burgess, S. C., Hayes, B. J., McCarthy, F. M., Moore, S., Foissac, S., Lunney, J. K., Andersson, L., Tuggle, C. K., and Casas, E.

Published
2015
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16. Coordinated international action to accelerate genome-to-phenome with FAANG, the Functional Annotation of Animal Genomes project : open letter

Author

Archibald, A.L., Bottema, C.D., Brauning, R., Burgess, S.C., Burt, D.W., Casas, E., Cheng, H.H., Clarke, L., Couldrey, C., Dalrymple, B.P., Elsik, C.G., Foissac, S., Giuffra, E., Groenen, M.A.M., Hayes, B.J., Huang, L.S., Khatib, H., Kijas, J.W., Kim, H., Lunney, J.K., McCarthy, F.M., McEwan, J., Moore, S., Nanduri, B., Notredame, C., Palti, Y., Plastow, G.S., Reecy, J.M., Rohrer, G., Sarropoulou, E., Schmidt, C.J., Silverstein, J., Tellam, R.L., Tixier-Boichard, M., Tosser-klopp, G., Tuggle, C.K., Vilkki, J., White, S.N., Zhao, S., and Zhou, H.

Subjects
WIAS, Life Science, Fokkerij en Genomica, Animal Breeding and Genomics
Abstract

We describe the organization of a nascent international effort, the Functional Annotation of Animal Genomes (FAANG) project, whose aim is to produce comprehensive maps of functional elements in the genomes of domesticated animal species.

Published
2015

17. Design and characterization of a 52K SNP chip for goats

Author

Tosser-Klopp G., Bardou P., Bouchez O., Cabau C., Crooijmans R., Dong Y., Donnadieu-Tonon C., Eggen A., Heuven H.C.M., Jamli S., Jiken A.J., Klopp C., Lawley C.T., McEwan J., Martin P., Moreno C.R., Mulsant P., Nabihoudine I., Pailhoux E., Palhiere I., Rupp R., Sarry J., Sayre B.L., Tircazes A., Wang J., Wang W., Zhang W., Ajmone P., Amills M., Boitard S., Faraut T., San Cristobal M., Servin B., Chen W., Cheng S., Liu X., Pan S., Song C., Xu X., Ye C., Zhang B., Lv J., Li X., Ren L., Shi P., Yu J., Faruque O., Lenstra H., Poli M.A., Zhao J., Rui S., Zhang Y., Stella A., Valentini A., Zhao S., Ecole Nationale Vétérinaire de Toulouse - ENVT (FRANCE), Institut National Polytechnique de Toulouse - INPT (FRANCE), Institut National de la Recherche Agronomique - INRA (FRANCE), Laboratoire de Génétique Cellulaire (LGC), Ecole Nationale Vétérinaire de Toulouse (ENVT), Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-Institut National de la Recherche Agronomique (INRA), Animal Breeding and Genomics Centre, Wageningen University and Research Centre [Wageningen] (WUR), Kunming Institute of Zoology, State Key Laboratory of Genetic Resources and Evolution, Chinese Academy of Sciences [Changchun Branch] (CAS), Faculty of Veterinary Medicine, Utrecht University [Utrecht], Strategic Livestock Research Centre, Malaysian Agricultural Research Development Institute, Unité de Biométrie et Intelligence Artificielle (UBIA), Institut National de la Recherche Agronomique (INRA), Invermay Agricultural Center, AgResearch, Génétique Animale et Biologie Intégrative (GABI), Institut National de la Recherche Agronomique (INRA)-AgroParisTech, Station d'Amélioration Génétique des Animaux (SAGA), Biologie du Développement et Reproduction (BDR), Department of Biology, Virginia State University, Inner Mongolia Key Laboratory of Animal Genetics, Breeding and Reproduction, Inner Mongolia Agricultural University, ANR-09-GENM-009-03 GENIDOV, ANR CHEST-454, CAPRISNIP programme: UNCEIA, CAPGENES and APIS-GENE French Breeding organizations, Institut National de la Recherche Agronomique (INRA)-Ecole Nationale Vétérinaire de Toulouse (ENVT), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées, Wageningen University and Research [Wageningen] (WUR), Biologie du développement et reproduction (BDR), Centre National de la Recherche Scientifique (CNRS)-École nationale vétérinaire d'Alfort (ENVA)-Institut National de la Recherche Agronomique (INRA), Institut National Polytechnique de Toulouse - Toulouse INP (FRANCE), and Amills i Eras, Marcel

Subjects
[SDV.SA]Life Sciences [q-bio]/Agricultural sciences, Gene Identification and Analysis, lcsh:Medicine, Sequence assembly, polledness, Molecular Inversion Probe, Genome, Sequence alignment, generation, single-nucleotide polymorphisms, lcsh:Science, Génétique, Animal Management, Genetics, 0303 health sciences, Multidisciplinary, Goats, Illumina 52K SNP Chip, goat, Agriculture, Genomics, 04 agricultural and veterinary sciences, Tag SNP, SNP genotyping, Grasslands, Research Article, dbSNP, Animal Breeding and Genomics, Biology, Molecular Genetics, 03 medical and health sciences, Genetic Mutation, Biologie animale, Genome-Wide Association Studies, Fokkerij en Genomica, BioNanoTechnology, genome, prp gene, Alleles, 030304 developmental biology, classical scrapie, capra-hircus, lcsh:R, Sequence assembly tools, 0402 animal and dairy science, association, snp, Genome analysis, 040201 dairy & animal science, Sustainable Agriculture, genotyping assay, Genetic Polymorphism, WIAS, lcsh:Q, Veterinary Science, Cattle, Animal Genetics, Population Genetics, Genomic databases, discovery, Reference genome
Abstract

The success of Genome Wide Association Studies in the discovery of sequence variation linked to complex traits in humans has increased interest in high throughput SNP genotyping assays in livestock species. Primary goals are QTL detection and genomic selection. The purpose here was design of a 50-60,000 SNP chip for goats. The success of a moderate density SNP assay depends on reliable bioinformatic SNP detection procedures, the technological success rate of the SNP design, even spacing of SNPs on the genome and selection of Minor Allele Frequencies (MAF) suitable to use in diverse breeds. Through the federation of three SNP discovery projects consolidated as the International Goat Genome Consortium, we have identified approximately twelve million high quality SNP variants in the goat genome stored in a database together with their biological and technical characteristics. These SNPs were identified within and between six breeds (meat, milk and mixed): Alpine, Boer, Creole, Katjang, Saanen and Savanna, comprising a total of 97 animals. Whole genome and Reduced Representation Library sequences were aligned on >10 kb scaffolds of the de novo goat genome assembly. The 60,000 selected SNPs, evenly spaced on the goat genome, were submitted for oligo manufacturing (Illumina, Inc) and published in dbSNP along with flanking sequences and map position on goat assemblies (i.e. scaffolds and pseudo-chromosomes), sheep genome V2 and cattle UMD3.1 assembly. Ten breeds were then used to validate the SNP content and 52,295 loci could be successfully genotyped and used to generate a final cluster file. The combined strategy of using mainly whole genome Next Generation Sequencing and mapping on a contig genome assembly, complemented with Illumina design tools proved to be efficient in producing this GoatSNP50 chip. Advances in use of molecular markers are expected to accelerate goat genomic studies in coming years. Copyright: © 2014 Tosser-Klopp et al.

Published
2014

18. Combining GWAS and RNA-Seq approaches for detection of the causal mutation for hereditary junctional epidermolysis bullosa in sheep

Author

Ministerio de Educación, Cultura y Deporte (España), Ministerio de Economía y Competitividad (España), Suárez-Vega, Aroa, Gutiérrez Gil, Beatriz, Benavides, Julio, Pérez Pérez, Valentín, Tosser Klopp, G., Klopp, Christophe, Keennel, Stephen J., Arranz, Juan José, Ministerio de Educación, Cultura y Deporte (España), Ministerio de Economía y Competitividad (España), Suárez-Vega, Aroa, Gutiérrez Gil, Beatriz, Benavides, Julio, Pérez Pérez, Valentín, Tosser Klopp, G., Klopp, Christophe, Keennel, Stephen J., and Arranz, Juan José

Abstract

In this study, we demonstrate the use of a genome-wide association mapping together with RNA-seq in a reduced number of samples, as an efficient approach to detect the causal mutation for a Mendelian disease. Junctional epidermolysis bullosa is a recessive genodermatosis that manifests with neonatal mechanical fragility of the skin, blistering confined to the lamina lucida of the basement membrane and severe alteration of the hemidesmosomal junctions. In Spanish Churra sheep, junctional epidermolysis bullosa (JEB) has been detected in two commercial flocks. The JEB locus was mapped to Ovis aries chromosome 11 by GWAS and subsequently fine-mapped to an 868-kb homozygous segment using the identical-by-descent method. The ITGB4, which is located within this region, was identified as the best positional and functional candidate gene. The RNA-seq variant analysis enabled us to discover a 4-bp deletion within exon 33 of the ITGB4 gene (c.4412_4415del). The c.4412_4415del mutation causes a frameshift resulting in a premature stop codon at position 1472 of the integrin beta 4 protein. A functional analysis of this deletion revealed decreased levels of mRNA in JEB skin samples and the absence of integrin beta 4 labeling in immunohistochemical assays. Genotyping of c.4412_4415del showed perfect concordance with the recessive mode of the disease phenotype. Selection against this causal mutation will now be used to solve the problem of JEB in flocks of Churra sheep. Furthermore, the identification of the ITGB4 mutation means that affected sheep can be used as a large mammal animal model for the human form of epidermolysis bullosa with aplasia cutis. Our approach evidences that RNA-seq offers cost-effective alternative to identify variants in the species in which high resolution exome-sequencing is not straightforward.

Published
2015

19. Design and Characterization of a 52K SNP Chip for Goats

Author

Tosser-klopp, G., Bardou, P., Bouchez, O., Cabau, C., Crooijmans, R.P.M.A., Dong, Y., Donnadieu-Tonon, C., Eggen, A., Heuven, H.C.M., Jamli, S., Jiken, A.J., Klopp, C., Lawley, C.T., McEwen, J., Martin, P., Moreno, C.R., Mulsant, P., Nabihoudine, I., Pailhoux, E., Palhiere, I., Rupp, R., Sarry, J., Sayre, B.L., Tircazes, A., Wang, J., Wang, W., Zhang, W.G., Tosser-klopp, G., Bardou, P., Bouchez, O., Cabau, C., Crooijmans, R.P.M.A., Dong, Y., Donnadieu-Tonon, C., Eggen, A., Heuven, H.C.M., Jamli, S., Jiken, A.J., Klopp, C., Lawley, C.T., McEwen, J., Martin, P., Moreno, C.R., Mulsant, P., Nabihoudine, I., Pailhoux, E., Palhiere, I., Rupp, R., Sarry, J., Sayre, B.L., Tircazes, A., Wang, J., Wang, W., and Zhang, W.G.

Abstract

The success of Genome Wide Association Studies in the discovery of sequence variation linked to complex traits in humans has increased interest in high throughput SNP genotyping assays in livestock species. Primary goals are QTL detection and genomic selection. The purpose here was design of a 50–60,000 SNP chip for goats. The success of a moderate density SNP assay depends on reliable bioinformatic SNP detection procedures, the technological success rate of the SNP design, even spacing of SNPs on the genome and selection of Minor Allele Frequencies (MAF) suitable to use in diverse breeds. Through the federation of three SNP discovery projects consolidated as the International Goat Genome Consortium, we have identified approximately twelve million high quality SNP variants in the goat genome stored in a database together with their biological and technical characteristics. These SNPs were identified within and between six breeds (meat, milk and mixed): Alpine, Boer, Creole, Katjang, Saanen and Savanna, comprising a total of 97 animals. Whole genome and Reduced Representation Library sequences were aligned on >10 kb scaffolds of the de novo goat genome assembly. The 60,000 selected SNPs, evenly spaced on the goat genome, were submitted for oligo manufacturing (Illumina, Inc) and published in dbSNP along with flanking sequences and map position on goat assemblies (i.e. scaffolds and pseudo-chromosomes), sheep genome V2 and cattle UMD3.1 assembly. Ten breeds were then used to validate the SNP content and 52,295 loci could be successfully genotyped and used to generate a final cluster file. The combined strategy of using mainly whole genome Next Generation Sequencing and mapping on a contig genome assembly, complemented with Illumina design tools proved to be efficient in producing this GoatSNP50 chip. Advances in use of molecular markers are expected to accelerate goat genomic studies in coming years.

Published
2014

20. Methods for interpreting lists of affected genes obstained in a DNA microarray experiment

Author

Hedegaard, J., Arce, A.M.G., Bicciato, S., Bonnet, A., Buitenhuis, B., Collado, M.C., Conley, L.N., San Cristobal, M., Ferrari, F., Garrido, J.J., Groenen, M.A.M., Hornshoj, H., Hulsegge, B., Jiang, L., Jimenez-Marin, A., Kommadath, A., Lagarrigue, S., Leunissen, J.A.M., Liaubet, L., Neerincx, P., Nie, H., van der Poel, W.H.M., Prickett, D., Ramirez-Boo, M., Rebel, J.M.J., Robert-Granie, C., Skarman, A., Smits, M.A., Sorensen, P., Tosser-klopp, G., and Watson, M.

Subjects
CVI - Divisie Virologie, Rural Development Sociology, Bioinformatics, EPS-4, Bioinformatica, WIAS, CVI - Divisie Bacteriologie en TSE's, Life Science, Fokkerij en Genomica, Animal Breeding and Genomics, Leerstoelgroep Rurale ontwikkelingssociologie, Wageningen Livestock Research, CVI - Division Virology
Abstract

Background - The aim of this paper was to describe and compare the methods used and the results obtained by the participants in a joint EADGENE (European Animal Disease Genomic Network of Excellence) and SABRE (Cutting Edge Genomics for Sustainable Animal Breeding) workshop focusing on post analysis of microarray data. The participating groups were provided with identical lists of microarray probes, including test statistics for three different contrasts, and the normalised log-ratios for each array, to be used as the starting point for interpreting the affected probes. The data originated from a microarray experiment conducted to study the host reactions in broilers occurring shortly after a secondary challenge with either a homologous or heterologous species of Eimeria. Results - Several conceptually different analytical approaches, using both commercial and public available software, were applied by the participating groups. The following tools were used: Ingenuity Pathway Analysis, MAPPFinder, LIMMA, GOstats, GOEAST, GOTM, Globaltest, TopGO, ArrayUnlock, Pathway Studio, GIST and AnnotationDbi. The main focus of the approaches was to utilise the relation between probes/genes and their gene ontology and pathways to interpret the affected probes/genes. The lack of a well-annotated chicken genome did though limit the possibilities to fully explore the tools. The main results from these analyses showed that the biological interpretation is highly dependent on the statistical method used but that some common biological conclusions could be reached. Conclusion - It is highly recommended to test different analytical methods on the same data set and compare the results to obtain a reliable biological interpretation of the affected genes in a DNA microarray experiment

Published
2009

21. Analysis of the real EADGENE data set: Comparison of methods and guidelines for data normalisation and selection of differentially expressed genes

Author

Jafrezic, F., de Koning, D.J., Boettcher, P., Bonnet, A., Buitenhuis, B., Closset, R., Dejean, S., Delmas, C., Detilleux, J.C., Dovc, P., Duval, M., Foulley, J.L., Hedegaard, J., Hoprnshoj, H., Hulsegge, B., Janss, L., Jensen, K., Jiang, L., Lavric, M., Cao Le, K.A., Lund, M.S., Malinverni, R., Marot, G., Nie, H., Petzl, W., Pool, M.H., Robert-Granie, C., Cristobal, M., van Schothorst, E.M., Schuberth, H.J., Sorensen, P., Stella, A., Tosser-klopp, G., Waddington, D., Watson, M., Yang, M., Zerbe, H., Seyfert, H.M., Station de Génétique Quantitative et Appliquée (SGQA), Institut National de la Recherche Agronomique (INRA), BBSRC Roslin Institute, Partenaires INRAE, Parco Tecnologico Padano, Laboratoire de Génétique Cellulaire (LGC), Institut National de la Recherche Agronomique (INRA)-Ecole Nationale Vétérinaire de Toulouse (ENVT), Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées, Faculty of Agricultural Sciences, Department of Genetics and Biotechnology, Aarhus University [Aarhus], Faculty of Veterinary Medicine, Université de Liège, Université Toulouse III - Paul Sabatier (UT3), Université Fédérale Toulouse Midi-Pyrénées, Station d'Amélioration Génétique des Animaux (SAGA), University of Ljubljana, Animal Sciences Group, Wageningen University and Research [Wageningen] (WUR), Wageningen University and Research Centre (WUR), Clinic for Ruminants, Ludwig-Maximilians-Universität München (LMU), Immunology Unit, University of Veterinary Medicine, Institute for Animal Health, and Leibniz Institute for Farm Animal Biology (FBN)

Subjects
[SDV.GEN]Life Sciences [q-bio]/Genetics, differentially expressed genes, mixed-model, RIKILT - Business Unit Veiligheid & Gezondheid, education, NORMALISATION, cdna microarray data, Animal Breeding and Genomics, microarray data, QUALITY CONTROL, DIFFERENTIALLY EXPRESSED GENES, MASTITIS RESISTANCE, MICROARRAY DATA, normalisation, quality control, mastitis resistance, WIAS, RIKILT - Business Unit Safety & Health, Fokkerij en Genomica, Wageningen Livestock Research
Abstract

A large variety of methods has been proposed in the literature for microarray data analysis. The aim of this paper was to present techniques used by the EADGENE (European Animal Disease Genomics Network of Excellence) WP1.4 participants for data quality control, normalisation and statistical methods for the detection of differentially expressed genes in order to provide some more general data analysis guidelines. All the workshop participants were given a real data set obtained in an EADGENE funded microarray study looking at the gene expression changes following artificial infection with two different mastitis causing bacteria: Escherichia coli and Staphylococcus aureus. It was reassuring to see that most of the teams found the same main biological results. In fact, most of the differentially expressed genes were found for infection by E. coli between uninfected and 24 h challenged udder quarters. Very little transcriptional variation was observed for the bacteria S. aureus. Lists of differentially expressed genes found by the different research teams were, however, quite dependent on the method used, especially concerning the data quality control step. These analyses also emphasised a biological problem of cross-talk between infected and uninfected quarters which will have to be dealt with for further microarray studies

Published
2007

22. Analysis of the real EADGENE data set: Multivariate approaches and post analyis

Author

Sorensen, P., Bonnet, A., Buitenhuis, B., Closset, R., Dejean, S., Delmas, C., Duval, M., Glass, L., Hedegaard, J., Hornshoj, H., Hulsegge, B., Jaffrezic, F., Jensen, K., Jiang, L., de Koning, D.J., Lê Cao, K.A., Nie, H., Petzl, W., Pool, M.H., Robert-Granie, C., San Cristobal, M., Lund, M.S., van Schothorst, E.M., Schuberth, H.J., Seyfert, H.M., Tosser-klopp, G., Waddington, D., Watson, D., Yang, W., and Zerbe, H.

Subjects
biology, RIKILT - Business Unit Veiligheid & Gezondheid, WIAS, RIKILT - Business Unit Safety & Health, association, escherichia-coli, gene-expression data, Fokkerij en Genomica, Animal Breeding and Genomics, bioconductor, Wageningen Livestock Research
Abstract

The aim of this paper was to describe, and when possible compare, the multivariate methods used by the participants in the EADGENE WP1.4 workshop. The first approach was for class discovery and class prediction using evidence from the data at hand. Several teams used hierarchical clustering (HC) or principal component analysis (PCA) to identify groups of differentially expressed genes with a similar expression pattern over time points and infective agent (E. coli or S. aureus). The main result from these analyses was that HC and PCA were able to separate tissue samples taken at 24 h following E. coli infection from the other samples. The second approach identified groups of differentially co-expressed genes, by identifying clusters of genes highly correlated when animals were infected with E. coli but not correlated more than expected by chance when the infective pathogen was S. aureus. The third approach looked at differential expression of predefined gene sets. Gene sets were defined based on information retrieved from biological databases such as Gene Ontology. Based on these annotation sources the teams used either the GlobalTest or the Fisher exact test to identify differentially expressed gene sets. The main result from these analyses was that gene sets involved in immune defence responses were differentially expressed.

Published
2007

26. Genetic diversity and investigation of polledness in divergent goat populations using 52 088 SNPs

Author

Kijas, James, Ortiz, Judith S., McCulloch, R., James, Andrew, Brice, B., Swain, B., Tosser-Klopp, G., Kijas, James, Ortiz, Judith S., McCulloch, R., James, Andrew, Brice, B., Swain, B., and Tosser-Klopp, G.

Abstract

The recent availability of a genome-wide SNP array for the goat genome dramatically increases the power to investigate aspects of genetic diversity and to conduct genome-wide association studies in this important domestic species. We collected and analysed genotypes from 52 088 SNPs in Boer, Cashmere and Rangeland goats that had both polled and horned individuals. Principal components analysis revealed a clear genetic division between animals for each population, and model-based clustering successfully detected evidence of admixture that matched aspects of their recorded history. For example, shared co-ancestry was detected, suggesting Boer goats have been introgressed into the Rangeland population. Further, allele frequency data successfully tracked the altered genetic profile that has taken place after 40 years of breeding Australian Cashmere goats using the Rangeland animals as the founding population. Genome-wide association mapping of the POLL locus revealed a strong signal on goat chromosome 1. The 769-kb critical interval contained the polled intersex syndrome locus, confirming the genetic basis in non-European animals is the same as identified previously in Saanen goats. Interestingly, analysis of the haplotypes carried by a small set of sex-reversed animals, known to be associated with polledness, revealed some animals carried the wild-type chromosome associated with the presence of horns. This suggests a more complex basis for the relationship between polledness and the intersex condition than initially thought while validating the application of the goat SNP50 BeadChip for fine-mapping traits in goat. © The Author(s) and Commonwealth of Australia. Animal Genetics © 2012 Stichting International Foundation for Animal Genetics.

Published
2013

27. Introgression from Domestic Goat Generated Variation at the Major Histocompatibility Complex of Alpine Ibex

Author

Grossen C., Keller L., Biebach I., Zhang W., Tosser-Klopp G., Ajmone P., Amills M., Boitard S., Chen W., Cheng S., Dong Y., Faraut T., Faruque O., Heuven H., Jinshan Z., Jun L., Lenstra H., Li X., Liu X., Moreno C., Mulsant P., Pan S., Poli M.A., Ren L., Rui S., Rupp R., Cristobal M.S., Sayre B.L., Servin B., Shi P., Song C., Stella A., Valentini A., Xianglong L., XU X., Yanjun Z., Ye C., Yu J., Zhang B., Zhao S., Croll D., Department of Zoology, Auburn University (AU), Institute of Evolutionary Biology and Environmental Studies, Universität Zürich [Zürich] = University of Zurich (UZH), Kunming Institute of Zoology, State Key Laboratory of Genetic Resources and Evolution, Chinese Academy of Sciences [Changchun Branch] (CAS), University of British Columbia (UBC), Laboratoire de Génétique Cellulaire (LGC), Institut National de la Recherche Agronomique (INRA)-Ecole Nationale Vétérinaire de Toulouse (ENVT), Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées, Chinese Academy of Sciences (CAS), Swiss National Science Foundation [PBLAP3-14584, PA00P3_145360], Swiss Federal Office for the Environment, University of Zurich, and Grossen, Christine

Subjects
Evolutionary Genetics, 0106 biological sciences, haplotype, Cancer Research, Introgression, [SDV]Life Sciences [q-bio], HLA-DR beta-Chains, Balancing selection, 01 natural sciences, Linkage Disequilibrium, Major Histocompatibility Complex, Natural Selection, 1306 Cancer Research, chromosome, Genome Evolution, Phylogeny, Genetics (clinical), Genetics, Evolutionary Theory, 0303 health sciences, biology, Goats, loci, Chromosomal region, 590 Animals (Zoology), Research Article, Gene Flow, 2716 Genetics (clinical), Evolutionary Processes, Capra ibex, intron, lcsh:QH426-470, chèvre, Immunology, complexe majeur d'histocompatibilité, Locus (genetics), 010603 evolutionary biology, 10127 Institute of Evolutionary Biology and Environmental Studies, 03 medical and health sciences, 1311 Genetics, Genetic variation, 1312 Molecular Biology, Animals, Allele, Molecular Biology, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, Evolutionary Biology, Polymorphism, Genetic, Base Sequence, Genetic Drift, Haplotype, Biology and Life Sciences, Computational Biology, allèle, Sequence Analysis, DNA, DNA sequence, genetic association, biology.organism_classification, lcsh:Genetics, 1105 Ecology, Evolution, Behavior and Systematics, Haplotypes, Genetic Polymorphism, 570 Life sciences, Clinical Immunology, Population Genetics, Microsatellite Repeats
Abstract

The major histocompatibility complex (MHC) is a crucial component of the vertebrate immune system and shows extremely high levels of genetic polymorphism. The extraordinary genetic variation is thought to be ancient polymorphisms maintained by balancing selection. However, introgression from related species was recently proposed as an additional mechanism. Here we provide evidence for introgression at the MHC in Alpine ibex (Capra ibex ibex). At a usually very polymorphic MHC exon involved in pathogen recognition (DRB exon 2), Alpine ibex carried only two alleles. We found that one of these DRB alleles is identical to a DRB allele of domestic goats (Capra aegagrus hircus). We sequenced 2489 bp of the coding and non-coding regions of the DRB gene and found that Alpine ibex homozygous for the goat-type DRB exon 2 allele showed nearly identical sequences (99.8%) to a breed of domestic goats. Using Sanger and RAD sequencing, microsatellite and SNP chip data, we show that the chromosomal region containing the goat-type DRB allele has a signature of recent introgression in Alpine ibex. A region of approximately 750 kb including the DRB locus showed high rates of heterozygosity in individuals carrying one copy of the goat-type DRB allele. These individuals shared SNP alleles both with domestic goats and other Alpine ibex. In a survey of four Alpine ibex populations, we found that the region surrounding the DRB allele shows strong linkage disequilibria, strong sequence clustering and low diversity among haplotypes carrying the goat-type allele. Introgression at the MHC is likely adaptive and introgression critically increased MHC DRB diversity in the genetically impoverished Alpine ibex. Our finding contradicts the long-standing view that genetic variability at the MHC is solely a consequence of ancient trans-species polymorphism. Introgression is likely an underappreciated source of genetic diversity at the MHC and other loci under balancing selection., PLoS Genetics, 10 (6), ISSN:1553-7390, ISSN:1553-7404

Published
2014

29. Function of genes: Principal stages in the use of genetic information

Author

Christine Leroux, Tosser-Klopp, G., Unité de recherche Génétique Biochimique et Cytogénétique (LGBC), Institut National de la Recherche Agronomique (INRA), Laboratoire de Génétique Cellulaire (LGC), Institut National de la Recherche Agronomique (INRA)-Ecole Nationale Vétérinaire de Toulouse (ENVT), Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées, and ProdInra, Migration

Subjects
[SDV.SA]Life Sciences [q-bio]/Agricultural sciences, traduction, GENE EXPRESSION, GENES, maturation, [SDV]Life Sciences [q-bio], adn, ARNM, séquence nucléotidique, GENETIQUE, Agricultural sciences, [SDV] Life Sciences [q-bio], ARNT, arn t, information génétique, protéine, régulation, arn r, transcription, Sciences agricoles, ComputingMilieux_MISCELLANEOUS, expression des gènes
Abstract

National audience; L’utilisation de l’information portée par l’ADN nécessite une étape de transcription des gènes en ARN et, dans certains cas, une phase de traduction en protéine. La transcription est un phénomène complexe, régulé (un gène eucaryote contient des séquences régulatrices permettant l’initiation et la régulation de la transcription) qui produit trois types d’ARN : les ARN messagers (ARNm), les ARN de transfert (ARNt) et les ARN ribosomiques (ARNr). Les ARNt et les ARNr sont des constituants de la machinerie de traduction des ARNm. En effet, après la transcription, l’ARNm va être maturé (épissage, polyadénylation ...) puis va sortir du noyau pour aller dans le cytoplasme où sa séquence nucléotidique sera traduite en séquence d’acides aminés. Les protéines acquièrent ensuite leur structure définitive après des modifications posttraductionnelles diverses. La régulation de l’expression des gènes peut intervenir à chacune des étapes (transcription, maturation et/ou traduction).

Published
2000

30. Analysis of the real EADGENE data set: Multivariate approaches and post analysis (Open Access publication)

Author

Sorensen, P, Bonnet, A, Buitenhuis, B, Closset, R, Dejean, S, Delmas, C, Duval, M, Glass, L, Hedegaard, J, Hornshoj, H, Hulsegge, I, Jaffrezic, F, Jensen, K, Jiang, L, De Koning, D-J, Le Cao, K-A, Nie, H, Petzl, W, Pool, MH, Robert-Granie, C, Cristobal, MS, Lund, MS, Van Schothorst, EM, Schuberth, H-J, Seyfert, H-M, Tosser-Klopp, G, Waddington, D, Watson, M, Yang, W, Zerbe, H, Sorensen, P, Bonnet, A, Buitenhuis, B, Closset, R, Dejean, S, Delmas, C, Duval, M, Glass, L, Hedegaard, J, Hornshoj, H, Hulsegge, I, Jaffrezic, F, Jensen, K, Jiang, L, De Koning, D-J, Le Cao, K-A, Nie, H, Petzl, W, Pool, MH, Robert-Granie, C, Cristobal, MS, Lund, MS, Van Schothorst, EM, Schuberth, H-J, Seyfert, H-M, Tosser-Klopp, G, Waddington, D, Watson, M, Yang, W, and Zerbe, H

Abstract

The aim of this paper was to describe, and when possible compare, the multivariate methods used by the participants in the EADGENE WP1.4 workshop. The first approach was for class discovery and class prediction using evidence from the data at hand. Several teams used hierarchical clustering (HC) or principal component analysis (PCA) to identify groups of differentially expressed genes with a similar expression pattern over time points and infective agent (E. coli or S. aureus). The main result from these analyses was that HC and PCA were able to separate tissue samples taken at 24 h following E. coli infection from the other samples. The second approach identified groups of differentially co-expressed genes, by identifying clusters of genes highly correlated when animals were infected with E. coli but not correlated more than expected by chance when the infective pathogen was S. aureus. The third approach looked at differential expression of predefined gene sets. Gene sets were defined based on information retrieved from biological databases such as Gene Ontology. Based on these annotation sources the teams used either the GlobalTest or the Fisher exact test to identify differentially expressed gene sets. The main result from these analyses was that gene sets involved in immune defence responses were differentially expressed.

Published
2007

31. Analysis of the real EADGENE data set: Comparison of methods and guidelines for data normalisation and selection of diffrentially expressed genes (Open Access publication)

Author

Jaffrezic, F, De Koning, D-J, Boettcher, PJ, Bonnet, A, Buitenhuis, B, Closset, R, Dejean, S, Delmas, C, Detilleux, JC, Dovc, P, Duval, M, Foulley, J-L, Hedegaard, J, Hornshoj, H, Hulsegge, I, Janss, L, Jensen, K, Jiang, L, Lavric, M, Le Cao, K-A, Lund, MS, Malinverni, R, Marot, G, Nie, H, Petzl, W, Pool, MH, Granie, CR, Cristobal, MS, Van Schothorst, EM, Schuberth, H-J, Sorensen, P, Stella, A, Tosser-Klopp, G, Waddington, D, Watson, M, Yang, W, Zerbe, H, Seyfert, H-M, Jaffrezic, F, De Koning, D-J, Boettcher, PJ, Bonnet, A, Buitenhuis, B, Closset, R, Dejean, S, Delmas, C, Detilleux, JC, Dovc, P, Duval, M, Foulley, J-L, Hedegaard, J, Hornshoj, H, Hulsegge, I, Janss, L, Jensen, K, Jiang, L, Lavric, M, Le Cao, K-A, Lund, MS, Malinverni, R, Marot, G, Nie, H, Petzl, W, Pool, MH, Granie, CR, Cristobal, MS, Van Schothorst, EM, Schuberth, H-J, Sorensen, P, Stella, A, Tosser-Klopp, G, Waddington, D, Watson, M, Yang, W, Zerbe, H, and Seyfert, H-M

Abstract

A large variety of methods has been proposed in the literature for microarray data analysis. The aim of this paper was to present techniques used by the EADGENE (European Animal Disease Genomics Network of Excellence) WP1.4 participants for data quality control, normalisation and statistical methods for the detection of differentially expressed genes in order to provide some more general data analysis guidelines. All the workshop participants were given a real data set obtained in an EADGENE funded microarray study looking at the gene expression changes following artificial infection with two different mastitis causing bacteria: Escherichia coli and Staphylococcus aureus. It was reassuring to see that most of the teams found the same main biological results. In fact, most of the differentially expressed genes were found for infection by E. coli between uninfected and 24 h challenged udder quarters. Very little transcriptional variation was observed for the bacteria S. aureus. Lists of differentially expressed genes found by the different research teams were, however, quite dependent on the method used, especially concerning the data quality control step. These analyses also emphasised a biological problem of cross-talk between infected and uninfected quarters which will have to be dealt with for further microarray studies.

Published
2007

32. The GENETPIG database:a tool for comparative mapping in pig (Sus scrofa)

Author

Karsenty, E., Barillot, E., Tosser-Klopp, G.., Lahbib-Mansais, Y., Milan, D., Hatey, F., Cirera, Susanna, Sawera, Milena, Jørgensen, Claus Bøttcher, Chowdhary, B., Fredholm, F., Wimmers, K., Ponsuksili, S., Davoli, R., Fontanesi, L., Braglia, S., Zambonelli, P., Bigi, D., Neuenschwander, S., Gellin, J., Karsenty, E., Barillot, E., Tosser-Klopp, G.., Lahbib-Mansais, Y., Milan, D., Hatey, F., Cirera, Susanna, Sawera, Milena, Jørgensen, Claus Bøttcher, Chowdhary, B., Fredholm, F., Wimmers, K., Ponsuksili, S., Davoli, R., Fontanesi, L., Braglia, S., Zambonelli, P., Bigi, D., Neuenschwander, S., and Gellin, J.

Published
2003

40. Conserved synteny and gene order difference between human chromosome 12 and pig chromosome 5.

Author

Goureau, A., Garrigues, A., Tosser-Klopp, G., Lahbib-Mansais, Y., Chardon, P., and Yerle, M.

Subjects
HUMAN chromosomes, GENOMES, MICROSATELLITE repeats, SMALL intestine, CYTOGENETICS, ARTIFICIAL chromosomes
Abstract

A comparative map of human chromosome 12 (HSA 12) and pig chromosome 5 (SSC 5) was constructed using ten pig expressed sequence tags (ESTs). These ESTs were isolated from primary granulosa cell cultures by differential display (EST b10b), or from a granulosa cDNA library (VIIIE1, DRIM, N*9, RIIID2 and RVIC1) or from a small intestine cDNA library (ATPSB, ITGB7, MYH9, and STAT2). Also used were two Traced Orthologous Amplified Sequence Tags (TOASTs) (LALBA, TRA1), one microsatellite-associated gene (IGF1) and finally five human YACs selected for their cytogenetic position, with a view to increasing the number of informative markers for the comparison. Large-insert clones were obtained by screening a pig bacterial artificial chromosome (BAC) library with specific primers for each EST and TOAST and for IGF1. These BACs were used as probes for fluorescent in situ hybridisation (FISH) both on porcine and human metaphases. In addition, the human YACs were FISH mapped on pig chromosomes. This allowed us to refine and, in some cases, to correct the previous mapping obtained with a somatic cell hybrid panel. While these data confirm chromosome painting results showing that the distal part of SSC 5p arm is conserved on HSA 22, while the rest of the chromosome corresponds to HSA 12, they also demonstrate gene-order differences between human and pig. In addition, it was also possible to determine the position of the synteny breakpoint. Copyright © 2001 S. Karger AG, Basel [ABSTRACT FROM AUTHOR]

Published
2001
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41. Analysis of the real EADGENE data set: Multivariate approaches and post analysis (Open Access publication)

Author

Schuberth Hans-Joachim, van Schothorst Evert M, Lund Mogens, San Cristobal Magali, Robert-Granié Christèle, Pool Marco H, Petzl Wolfram, Nie Haisheng, Cao Kim-Anh, de Koning Dirk-Jan, Jiang Li, Jensen Kirsty, Hulsegge Ina, Jaffrézic Florence, Hornshøj Henrik, Hedegaard Jakob, Glass Liz, Duval Mylène, Delmas Céline, Déjean Sébastien, Closset Rodrigue, Buitenhuis Bart, Bonnet Agnès, Sørensen Peter, Seyfert Hans-Martin, Tosser-Klopp Gwenola, Waddington David, Watson Michael, Yang Wei, and Zerbe Holm

Subjects
bovine annotation, bovine microarray, gene set analysis, mastitis, multivariate approaches, Animal culture, SF1-1100, Genetics, QH426-470
Abstract

Abstract The aim of this paper was to describe, and when possible compare, the multivariate methods used by the participants in the EADGENE WP1.4 workshop. The first approach was for class discovery and class prediction using evidence from the data at hand. Several teams used hierarchical clustering (HC) or principal component analysis (PCA) to identify groups of differentially expressed genes with a similar expression pattern over time points and infective agent (E. coli or S. aureus). The main result from these analyses was that HC and PCA were able to separate tissue samples taken at 24 h following E. coli infection from the other samples. The second approach identified groups of differentially co-expressed genes, by identifying clusters of genes highly correlated when animals were infected with E. coli but not correlated more than expected by chance when the infective pathogen was S. aureus. The third approach looked at differential expression of predefined gene sets. Gene sets were defined based on information retrieved from biological databases such as Gene Ontology. Based on these annotation sources the teams used either the GlobalTest or the Fisher exact test to identify differentially expressed gene sets. The main result from these analyses was that gene sets involved in immune defence responses were differentially expressed.

Published
2007
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42. Analysis of a simulated microarray dataset: Comparison of methods for data normalisation and detection of differential expression (Open Access publication)

Author

Mouzaki Daphné, Marot Guillemette, Lê Cao Kim-Anh, Lavrič Miha, Jiménez-Marín Ángeles, Jaffrézic Florence, Hulsegge Ina, Garrido-Pavón Juan, Foulley Jean-Louis, Duval Mylène, Dovč Peter, Delmas Céline, Baron Michael, Pérez-Alegre Mónica, Watson Michael, Pool Marco H, Robert-Granié Christèle, San Cristobal Magali, Tosser-Klopp Gwenola, Waddington David, and de Koning Dirk-Jan

Subjects
gene expression, two colour microarray, simulation, statistical analysis, Animal culture, SF1-1100, Genetics, QH426-470
Abstract

Abstract Microarrays allow researchers to measure the expression of thousands of genes in a single experiment. Before statistical comparisons can be made, the data must be assessed for quality and normalisation procedures must be applied, of which many have been proposed. Methods of comparing the normalised data are also abundant, and no clear consensus has yet been reached. The purpose of this paper was to compare those methods used by the EADGENE network on a very noisy simulated data set. With the a priori knowledge of which genes are differentially expressed, it is possible to compare the success of each approach quantitatively. Use of an intensity-dependent normalisation procedure was common, as was correction for multiple testing. Most variety in performance resulted from differing approaches to data quality and the use of different statistical tests. Very few of the methods used any kind of background correction. A number of approaches achieved a success rate of 95% or above, with relatively small numbers of false positives and negatives. Applying stringent spot selection criteria and elimination of data did not improve the false positive rate and greatly increased the false negative rate. However, most approaches performed well, and it is encouraging that widely available techniques can achieve such good results on a very noisy data set.

Published
2007
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43. Analysis of the real EADGENE data set: Comparison of methods and guidelines for data normalisation and selection of differentially expressed genes (Open Access publication)

Author

Sørensen Peter, Schuberth Hans-Joachim, van Schothorst Evert M, San Cristobal Magali, Robert-Granié Christèle, Pool Marco H, Petzl Wolfram, Nie Haisheng, Marot Guillemette, Malinverni Roberto, Lund Mogens, Cao Kim-Anh, Lavrič Miha, Jiang Li, Jensen Kirsty, Janss Luc, Hulsegge Ina, Hornshøj Henrik, Hedegaard Jakob, Foulley Jean-Louis, Duval Mylène, Dovč Peter, Detilleux Johanne C, Delmas Céline, Déjean Sébastien, Closset Rodrigue, Buitenhuis Bart, Bonnet Agnès, Boettcher Paul J, de Koning Dirk-Jan, Jaffrézic Florence, Stella Alessandra, Tosser-Klopp Gwenola, Waddington David, Watson Michael, Yang Wei, Zerbe Holm, and Seyfert Hans-Martin

Subjects
quality control, differentially expressed genes, mastitis resistance, microarray data, normalisation, Animal culture, SF1-1100, Genetics, QH426-470
Abstract

Abstract A large variety of methods has been proposed in the literature for microarray data analysis. The aim of this paper was to present techniques used by the EADGENE (European Animal Disease Genomics Network of Excellence) WP1.4 participants for data quality control, normalisation and statistical methods for the detection of differentially expressed genes in order to provide some more general data analysis guidelines. All the workshop participants were given a real data set obtained in an EADGENE funded microarray study looking at the gene expression changes following artificial infection with two different mastitis causing bacteria: Escherichia coli and Staphylococcus aureus. It was reassuring to see that most of the teams found the same main biological results. In fact, most of the differentially expressed genes were found for infection by E. coli between uninfected and 24 h challenged udder quarters. Very little transcriptional variation was observed for the bacteria S. aureus. Lists of differentially expressed genes found by the different research teams were, however, quite dependent on the method used, especially concerning the data quality control step. These analyses also emphasised a biological problem of cross-talk between infected and uninfected quarters which will have to be dealt with for further microarray studies.

Published
2007
Full Text
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44. The GENETPIG database

Author

Karsenty, E., Barillot, E., Tosser-Klopp, G., Lahbib-Mansais, Y., Milan, D., Hatey, F., Susanna Cirera, Milena Sawera, Claus Bottcher Jorgensen, Chowdhary, B., Fredholm, F., Wimmers, K., Ponsuksili, S., Davoli, R., Fontanesi, L., Braglia, S., Zambonelli, P., Bigi, D., Neuenschwander, S., and Gellin, J.

45. Functional study and regional mapping of 44 hormono-regulated genes isolated from a porcine granulosa cell library

Author

Hatey François, Yerle Martine, Bonnet Agnès, and Tosser-Klopp Gwenola

Subjects
pig, ovarian follicle, cDNA mapping, comparative RT-PCR, comparative map, Animal culture, SF1-1100, Genetics, QH426-470
Abstract

Abstract cDNA clones from a pig granulosa cell cDNA library were isolated by differential hybridisation for follicle stimulating hormone (FSH) regulation in granulosa cells in a previous study. The clones that did not match any known sequence were studied for their expression in granulosa cells (treated or not by FSH) and in fresh isolated ovarian follicles mainly by comparative RT-PCR analysis. These results give functional data on genes that may be implicated in follicular growing. These ESTs have been localised on the porcine genome, using a somatic cell hybrid panel, providing new type I markers on the porcine map and information on the comparative map between humans and pigs.

Published
2001
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47. Transcriptome profiling of sheep granulosa cells and oocytes during early follicular development obtained by Laser Capture Microdissection

Author

Bonnet Agnes, Bevilacqua Claudia, Benne Francis, Bodin Loys, Cotinot Corinne, Liaubet Laurence, Sancristobal Magali, Sarry Julien, Terenina Elena, Martin Patrice, Tosser-Klopp Gwenola, and Mandon-Pepin Beatrice

Subjects
Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background Successful achievement of early folliculogenesis is crucial for female reproductive function. The process is finely regulated by cell-cell interactions and by the coordinated expression of genes in both the oocyte and in granulosa cells. Despite many studies, little is known about the cell-specific gene expression driving early folliculogenesis. The very small size of these follicles and the mixture of types of follicles within the developing ovary make the experimental study of isolated follicular components very difficult. The recently developed laser capture microdissection (LCM) technique coupled with microarray experiments is a promising way to address the molecular profile of pure cell populations. However, one main challenge was to preserve the RNA quality during the isolation of single cells or groups of cells and also to obtain sufficient amounts of RNA. Using a new LCM method, we describe here the separate expression profiles of oocytes and follicular cells during the first stages of sheep folliculogenesis. Results We developed a new tissue fixation protocol ensuring efficient single cell capture and RNA integrity during the microdissection procedure. Enrichment in specific cell types was controlled by qRT-PCR analysis of known genes: six oocyte-specific genes (SOHLH2, MAEL, MATER, VASA, GDF9, BMP15) and three granulosa cell-specific genes (KL, GATA4, AMH). A global gene expression profile for each follicular compartment during early developmental stages was identified here for the first time, using a bovine Affymetrix chip. Most notably, the granulosa cell dataset is unique to date. The comparison of oocyte vs. follicular cell transcriptomes revealed 1050 transcripts specific to the granulosa cell and 759 specific to the oocyte. Functional analyses allowed the characterization of the three main cellular events involved in early folliculogenesis and confirmed the relevance and potential of LCM-derived RNA. Conclusions The ovary is a complex mixture of different cell types. Distinct cell populations need therefore to be analyzed for a better understanding of their potential interactions. LCM and microarray analysis allowed us to identify novel gene expression patterns in follicular cells at different stages and in oocyte populations.

Published
2011
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48. A pig multi-tissue normalised cDNA library: large-scale sequencing, cluster analysis and 9K micro-array resource generation

Author

Soares Marcelo B, Bonaldo Maria F, Benne Francis, Hugot Karine, Iannuccelli Eddie, Bonnet Agnès, Hatey François, and Tosser-Klopp Gwenola

Subjects
Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background Domestic animal breeding and product quality improvement require the control of reproduction, nutrition, health and welfare in these animals. It is thus necessary to improve our knowledge of the major physiological functions and their interactions. This would be greatly enhanced by the availability of expressed gene sequences in the databases and by cDNA arrays allowing the transcriptome analysis of any function. The objective within the AGENAE French program was to initiate a high-throughput cDNA sequencing program of a 38-tissue normalised library and generate a diverse microarray for transcriptome analysis in pig species. Results We constructed a multi-tissue cDNA library, which was normalised and subtracted to reduce the redundancy of the clones. Expressed Sequence Tags were produced and 24449 high-quality sequences were released in EMBL database. The assembly of all the public ESTs (available through SIGENAE website) resulted in 40786 contigs and 54653 singletons. At least one Agenae sequence is present in 11969 contigs (12.5%) and in 9291 of the deeper-than-one-contigs (22.8%). Sequence analysis showed that both normalisation and subtraction processes were successful and that the initial tissue complexity was maintained in the final libraries. A 9K nylon cDNA microarray was produced and is available through CRB-GADIE. It will allow high sensitivity transcriptome analyses in pigs. Conclusion In the present work, a pig multi-tissue cDNA library was constructed and a 9K cDNA microarray designed. It contributes to the Expressed Sequence Tags pig data, and offers a valuable tool for transcriptome analysis.

Published
2008
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49. Local adaptations of Mediterranean sheep and goats through an integrative approach

Author

Marco Cavalazzi, Gwenola Tosser-Klopp, Dominique Taurisson-Mouret, Bruno Serranito, Stephen J. G. Hall, Anne Da Silva, Eric Rouvellac, Marie Bal, Elena Ciani, Johannes A. Lenstra, Badr Benjelloun, François Pompanon, Carole Moreno-Romieux, Bertrand Servin, Pablo Vidal, Génomique AniMale, Amélioration, Adaptation (GAMAA), PEIRENE (PEIRENE), Institut Génomique, Environnement, Immunité, Santé, Thérapeutique (GEIST), Université de Limoges (UNILIM)-Université de Limoges (UNILIM)-Institut Génomique, Environnement, Immunité, Santé, Thérapeutique (GEIST), Université de Limoges (UNILIM)-Université de Limoges (UNILIM)-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE), Muséum national d'Histoire naturelle (MNHN), Laboratoire de Géographie Physique et Environnementale (GEOLAB), Université Blaise Pascal - Clermont-Ferrand 2 (UBP)-Université Clermont Auvergne [2017-2020] (UCA [2017-2020])-Université Clermont Auvergne (UCA)-Institut Sciences de l'Homme et de la Société (IR SHS UNILIM), Université de Limoges (UNILIM)-Université de Limoges (UNILIM)-Centre National de la Recherche Scientifique (CNRS), Universidad Catolica de Valencia (UCV), Dynamiques du droit (DD), Université de Montpellier (UM)-Centre National de la Recherche Scientifique (CNRS)-Université Montpellier 1 (UM1), Università degli studi di Bari Aldo Moro (UNIBA), Génétique Physiologie et Systèmes d'Elevage (GenPhySE ), Ecole Nationale Vétérinaire de Toulouse (ENVT), Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-École nationale supérieure agronomique de Toulouse [ENSAT]-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE), Estonian University of Life Sciences (EMU), Universiteit Utrecht, Laboratoire d'Ecologie Alpine (LECA ), Université Savoie Mont Blanc (USMB [Université de Savoie] [Université de Chambéry])-Centre National de la Recherche Scientifique (CNRS)-Université Grenoble Alpes (UGA), Institut national de la recherche agronomique [Maroc] (INRA Maroc), One Health Toxicologie, Université Blaise Pascal - Clermont-Ferrand 2 (UBP)-Institut Sciences de l'Homme et de la Société (IR SHS UNILIM), Université de Limoges (UNILIM)-Université de Limoges (UNILIM)-Université Clermont Auvergne [2017-2020] (UCA [2017-2020])-Centre National de la Recherche Scientifique (CNRS)-Université Clermont Auvergne (UCA), Université de Montpellier (UM)-Centre National de la Recherche Scientifique (CNRS), Università degli studi di Bari Aldo Moro = University of Bari Aldo Moro (UNIBA), Université de Toulouse (UT)-Université de Toulouse (UT)-Institut National Polytechnique (Toulouse) (Toulouse INP), Université de Toulouse (UT)-Université de Toulouse (UT)-École nationale supérieure agronomique de Toulouse (ENSAT), Université de Toulouse (UT)-Université de Toulouse (UT)-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE), Serranito B., Cavalazzi M., Vidal P., Taurisson-Mouret D., Ciani E., Bal M., Rouvellac E., Servin B., Moreno-Romieux C., Tosser-Klopp G., Hall S.J.G., Lenstra J.A., Pompanon F., Benjelloun B., and Da Silva A.

Subjects
0106 biological sciences, Mediterranean climate, Ecological selection, Population genetics, Molecular biology, Acclimatization, Breeding, 01 natural sciences, Intergenic region, Lung function, 2. Zero hunger, 0303 health sciences, Multidisciplinary, Mediterranean Region, Goats, Altitude, [SDV.BID.EVO]Life Sciences [q-bio]/Biodiversity/Populations and Evolution [q-bio.PE], Ecological genetics, Ruminants, Adaptation, Physiological, Breed, Heat stress, Habitat, Italy, Goat, Medicine, France, Science, Climate change, Context (language use), [SDV.SA.ZOO]Life Sciences [q-bio]/Agricultural sciences/Zootechny, Biology, 010603 evolutionary biology, Mediterranean area, Article, historical archives, 03 medical and health sciences, Animals, General, Selection (genetic algorithm), Ecosystem, 030304 developmental biology, Animal breeding, Sheep, Animal, [SDV.GEN.GA]Life Sciences [q-bio]/Genetics/Animal genetics, Evolutionary biology, Spain, Adaptation, Function (biology)
Abstract

In a context of climate change, identifying the genes underlying adaptations to extreme environments is essential. Small ruminants are adapted to a wide variety of habitats and thus, are promising study models. Here, we considered 17 goat and 25 sheep local Mediterranean breeds, in Italy, France and Spain. We proposed, and empirically tested a new methodology to highlight selection signatures in relation to the environments. Based on historical archives, we selected the breeds potentially most linked to a territory and defined their original geographical cradle, including transhumant pastoral areas. For both species, the cradles were arranged along latitudinal gradient of aridity and altitude. Then we used the programs PCAdapt and LFMM. Considering cradles, instead of current GPS coordinates, markedly improved the sensitivity of the LFMM analyses. All the results combined with a systematic literature review, revealed a set of genes with potentially key adaptive roles. Some of these genes, have been found implicated in lipid metabolism (SUCLG2, BMP2), hypoxia/heat stress (UBE2R2/UBAP2), lung function (BMPR2), seasonal patterns (SOX2, DPH6) or neuronal function (TRPC4, TRPC6). For the intergenic region between PCDH9 and KLH1, as well as NBEA, identified in both species, the adaptive role could be strong. We found for RXFP2, associated with sheep horn development, and MSRB3 and SLC26A4, both associated with hearing of sheep, a strong association with the environment gradient. We conclude that our new methodology, which considers breeds in their historical, environmental and anthropological context, provides novel and essential information on local breeds and their unique adaptations.

Published
2021

50. Signatures of selection and environmental adaptation across the goat genome post-domestication

Author

Roberto Steri, Curtis P. Van Tassell, Andrea Talenti, Gabriele Marras, Marcel Amills, Francesca Bertolini, Bernt Guldbrandtsen, Licia Colli, Alessandra Crisà, Benjamin D. Rosen, Max F. Rothschild, Gennaro Catillo, Ezequiel L. Nicolazzi, Stéphane Joost, Bertrand Servin, Claire Oget, Gwenola Tosser-Klopp, Tad S. Sonstegard, Eui-Soo Kim, Isabelle Palhiere, Alessandra Stella, Paola Crepaldi, Marco Milanesi, Estelle Rochat, Génétique Physiologie et Systèmes d'Elevage (GenPhySE ), École nationale supérieure agronomique de Toulouse [ENSAT]-Institut National de la Recherche Agronomique (INRA)-Ecole Nationale Vétérinaire de Toulouse (ENVT), Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-Institut National Polytechnique (Toulouse) (Toulouse INP), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées, Università degli Studi di Milano, Iowa State University, Bertolini F., Servin B., Talenti A., Rochat E., Kim E.S., Oget C., Palhiere I., Crisa A., Catillo G., Steri R., Amills M., Colli L., Marras G., Milanesi M., Nicolazzi E., Rosen B.D., Van Tassell C.P., Guldbrandtsen B., Sonstegard T.S., Tosser-Klopp G., Stella A., Rothschild M.F., Joost S., and Crepaldi P.

Subjects
0301 basic medicine, smith-magenis syndrome, Range (biology), Acclimatization, [SDV]Life Sciences [q-bio], MathematicsofComputing_GENERAL, Breeding, Genome, adamts metalloproteases, Domestication, genomic, receptor mc1r, lcsh:SF1-1100, 630 Agriculture, genetic, goat, phenotypic, production, Goats, TheoryofComputation_GENERAL, General Medicine, genetic diversity, important traits, Phenotype, 590 Animals (Zoology), Research Article, Autre (Sciences du Vivant), Coat, Genotype, lcsh:QH426-470, dna-sequence, sexual-behavior, Biology, Polymorphism, Single Nucleotide, 03 medical and health sciences, positive selection, Genetic variation, Genetics, Animals, Selection, Genetic, Ecology, Evolution, Behavior and Systematics, Selection (genetic algorithm), coat color, Genetic diversity, Animal, missense mutation, Genetic Variation, Sequence Analysis, DNA, lcsh:Genetics, 030104 developmental biology, Evolutionary biology, Animal Science and Zoology, lcsh:Animal culture, Adaptation
Abstract

AdaptMap consortium., [Background]: Since goat was domesticated 10,000 years ago, many factors have contributed to the differentiation of goat breeds and these are classified mainly into two types: (i) adaptation to different breeding systems and/or purposes and (ii) adaptation to different environments. As a result, approximately 600 goat breeds have developed worldwide; they differ considerably from one another in terms of phenotypic characteristics and are adapted to a wide range of climatic conditions. In this work, we analyzed the AdaptMap goat dataset, which is composed of data from more than 3000 animals collected worldwide and genotyped with the CaprineSNP50 BeadChip. These animals were partitioned into groups based on geographical area, production uses, available records on solid coat color and environmental variables including the sampling geographical coordinates, to investigate the role of natural and/or artificial selection in shaping the genome of goat breeds., [Results]: Several signatures of selection on different chromosomal regions were detected across the different breeds, sub-geographical clusters, phenotypic and climatic groups. These regions contain genes that are involved in important biological processes, such as milk-, meat- or fiber-related production, coat color, glucose pathway, oxidative stress response, size, and circadian clock differences. Our results confirm previous findings in other species on adaptation to extreme environments and human purposes and provide new genes that could explain some of the differences between goat breeds according to their geographical distribution and adaptation to different environments., [Conclusions]: These analyses of signatures of selection provide a comprehensive first picture of the global domestication process and adaptation of goat breeds and highlight possible genes that may have contributed to the differentiation of this species worldwide., Authors are grateful to all breeders and AdaptMap members who provided data to the initiative (http://www.goatadaptmap.org/) that are described in Stella et al.. The authors from the University of Milan are grateful to Stefano Frattini who was supported by the GenHome project, for supporting coordinating meetings. Support for Francesca Bertolini was provided by State of Iowa, hatch and Ensminger funds. Financial support provided in part by the Illumina Greater Good grant is appreciated.

Published
2018

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