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Featured researches published by Anne Oustry-Vaiman.


Mammalian Genome | 2002

Cytogenetic localization of 136 genes in the horse: comparative mapping with the human genome

Dragan Milenkovic; Anne Oustry-Vaiman; Teri L. Lear; Alain Billault; Denis Mariat; François Piumi; Laurent Schibler; Edmond Cribiu; Gérard Guérin

The aim of this study was to increase the number of type I markers on the horse cytogenetic map and to improve comparison with maps of other species, thus facilitating positional candidate cloning studies. BAC clones from two different sources were FISH mapped: homologous horse BAC clones selected from our newly extended BAC library using consensus primer sequences and heterologous goat BAC clones. We report the localization of 136 genes on the horse cytogenetic map, almost doubling the number of cytogenetically mapped genes with 48 localizations from horse BAC clones and 88 from goat BAC clones. For the first time, genes were mapped to ECA13p, ECA29, and probably ECA30. A total of 284 genes are now FISH mapped on the horse chromosomes. Comparison with the human map defines 113 conserved segments that include new homologous segments not identified by Zoo-FISH on ECA7 and ECA13p.


Mammalian Genome | 1999

Construction and characterization of a sheep BAC library of three genome equivalents

D. Vaiman; Alain Billault; Kamila Tabet-Aoul; Laurent Schibler; Didier Vilette; Anne Oustry-Vaiman; Catherine Soravito; Edmond Cribiu

A sheep BAC library of over three genome equivalents was constructed and arrayed in superpools and row, column, and plate pools. The library contains 90,000 clones distributed in 39 superpools. The average insert size was estimated at 123 kb. The library was screened by PCR with 77 primer pairs corresponding to ovine microsatellites distributed throughout the genome. The probability of finding a random sequence in the library could be estimated at 0.96.


Biology of Reproduction | 2003

Expression Profiles and Chromosomal Localization of Genes Controlling Meiosis and Follicular Development in the Sheep Ovary

Beatrice Mandon-Pepin; Anne Oustry-Vaiman; Bernard Vigier; François Piumi; Edmond Cribiu; Corinne Cotinot

Abstract In female sheep fetuses, two of the most crucial stages of ovarian development are prophase of meiosis I and follicle formation. In the present study, sheep ovaries collected on Days 25, 38, 49, 56, 67, 75, 94, and 120 of gestation, at birth, and in adulthood were tested by reverse transcription-polymerase chain reaction (RT-PCR) for the expression of 14 genes known to be involved in the ovarian differentiation in diverse organisms. The aim of this study was to determine 1) the expression pattern of six genes involved in germ cell development or meiosis (DMC1, SPO11, MSH4, MSH5, DAZL, and Boule) and five ovary-derived factors (OVOL1, SIAH2, DIAPH2, FOXL2, and FGF9), 2) the onset of gene expression for several members of the bone morphogenetic protein (BMP) pathway involved in follicular development (GDF9, BMP15, BMPR-IB), and 3) the chromosomal localization of seven of these genes in the sheep genome. The RT-PCR analysis revealed that the two germline-specific genes, DAZL and Boule, were expressed between 49 and 94 days postcoitum (dpc) with a similar pattern to typical meiosis genes (DMC1, MSH4, and MSH5), suggesting their possible participation in prophase of meiosis I. GDF9 and OVOL1 gene transcription started at 56 dpc and extended until birth, while BMP15 presented a more restricted window of expression between 94 dpc and birth, corresponding to the formation of first growing follicles. The homologous ovine genes for SPO11, DMC1, MSH5, DAZL, FGF9, DIAPH2, and SIAH2 were located on OAR 13q21–22, 3q35, 20q22, 19q13, 10q15, Xq44, and 1q41–42, respectively. In sheep, quantitative trait loci affecting female reproductive capacities are currently being detected. The ontology and precise mapping of ovarian genes will be useful to identify potential candidate genes that might underlie these effects.


Chromosome Research | 2002

Sheep/human comparative map in a chromosome region involved in scrapie incubation time shows multiple breakpoints between human chromosomes 14 and 15 and sheep chromosomes 7 and 18

Gian Mario Cosseddu; Anne Oustry-Vaiman; Benoı̂t Jego; Carole Moreno; Sead Taourit; Edmond Cribiu; Jean-Michel Elsen; D. Vaiman

A chromosome region involved in scrapie incubation time was identified on sheep chromosome 18 (OAR18). Since OAR18 (and OAR7) share conserved chromosome segments with human chromosomes HSA14 and HSA15, a dense map of type I markers was constructed by FISH mapping of bacterial artificial chromosomes containing genes located on these human chromosomes. In this study, we used the complete human sequence information (gene positions in megabases, Mb) to locate approximately one gene every 2 Mb on HSA15 (19 genes mapped between 19.51 and 66.02 Mb) and on HSA14 (11 genes between 73.24 and 102.62 Mb). Combined with previous work carried out in cattle and goats, our results made it possible to refine the comparative map between ruminants and humans for these two highly rearranged chromosomes (10 segments on HSA15 and 7 on HSA14). Furthermore, we identified relatively short intervals containing evolutionary breakpoints, which is a prerequisite to position them precisely. This work is also the first step in the cloning of the region involved in scrapie incubation period in sheep.


Genetics Selection Evolution | 2000

Cytogenetical anchoring of sheep linkage map and syntenic groups using a sheep BAC library

Kamila Tabet-Aoul; Anne Oustry-Vaiman; D. Vaiman; Nadhira Saidi-Mehtar; E. P. Cribiu; Frédéric Lantier

In order to simultaneously integrate linkage and syntenic groups to the ovine chromosomal map, a sheep bacterial artificial chromosome (BAC) library was screened with previously assigned microsatellites using a sheep-hamster hybrid panel and genetic linkage. Thirty-three BACs were obtained, fluorescently labelled and hybridised on sheep-goat hybrid metaphases (2n = 57). This study allowed us, (i), to anchor all linkage groups on sheep chromosomes, (ii), to give information on the probable position of the centromere on the linkage map for the centromeric chromosomes, (iii), to contradict the previous orientation of the ovine × linkage group by the mapping of BMS1008 on OARXq38. Concerning our somatic cell hybrid panel, this study resulted in the assignment of all the previously unassigned groups to ovine chromosomes and a complete characterisation of the hybrid panel. In addition, since hybridisations were performed on a sheep-goat hybrid, new marker/anchoring points were added to the caprine cytogenetic map.


Mammalian Genome | 2000

Regional characterization of a hamster–sheep somatic cell hybrid panel

Kamila Tabet-Aoul; Laurent Schibler; D. Vaiman; Anne Oustry-Vaiman; Isabelle Lantier; Nadhira Saidi-Mehtar; E. P. Cribiu; Frédéric Lantier

Abstract. The regional characterization of a previously obtained hamster–sheep hybrid panel is reported. Using data available from ruminant maps (sheep, cattle, and goat), we have selected a set of 300 markers and have analyzed them by PCR in this hybrid panel. Results obtained for 204 markers show the presence of all sheep chromosomes (including gonosomes) in entire or fragmented form. Analysis of syntenies has given 130 types of answer defining segments of variable sizes. This study has led to the regional characterization of this panel and provides comparative data on a set of bovine and caprine markers. With the level of characterization now achieved for this hybrid panel, the regional assignment of new genes or markers to sheep chromosomes can be rapidly obtained. Finally, this panel will help to collect new data for comparative mapping of domestic animals and to highlight the conservation of syntenic groups between closely related species, that is, sheep, cattle, and goat.


Genetics Selection Evolution | 2000

Cytogenetic mapping of 25 goat mammary gland Expressed Sequence Tags (ESTs)

Fabienne Le Provost; Laurent Schibler; Anne Oustry-Vaiman; Patrice Martin; Edmond Cribiu

Today, there is a shift towards a positional candidate approach in the molecular identification of genes. This study reports on an Expressed Sequence Tags (ESTs) mapping initiative in goats, based on sequence information gathered from a previous mammary gland cDNA systematic sequencing project. A total of 25 novel genes was localised cytogenetically on 16 goat chromosomes. Six of these ESTs were found to map to cattle milk QTL regions. These results made it possible to assess the use of ESTs as a shortcut to the molecular identification of some QTLs and as a valuable tool for comparative mapping.


Genome Research | 2000

Fine Mapping Suggests that the Goat Polled Intersex Syndrome and the Human Blepharophimosis Ptosis Epicanthus Syndrome Map to a 100-kb Homologous Region

Laurent Schibler; Edmond Cribiu; Anne Oustry-Vaiman; Jean-Pierre Furet; Daniel Vaiman


Genomics | 1999

High-resolution human/goat comparative map of the goat polled/intersex syndrome (PIS): the human homologue is contained in a human YAC from HSA3q23.

D. Vaiman; Laurent Schibler; Anne Oustry-Vaiman; Eric Pailhoux; Tom Goldammer; Milena Stevanovic; Jean-Pierre Furet; Manfred Schwerin; Corinne Cotinot; Marc Fellous; Edmond Cribiu


Animal Genetics | 1999

FISH mapping assignment of two horse BAC clones containing HMS41 and HTG3 microsatellites

Sophie Godard; Anne Oustry-Vaiman; E. P. Cribiu; Gérard Guérin

Collaboration


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Edmond Cribiu

Institut national de la recherche agronomique

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Laurent Schibler

Institut national de la recherche agronomique

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D. Vaiman

Institut national de la recherche agronomique

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E. P. Cribiu

Institut national de la recherche agronomique

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Kamila Tabet-Aoul

Institut national de la recherche agronomique

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Frédéric Lantier

Institut national de la recherche agronomique

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Corinne Cotinot

Institut national de la recherche agronomique

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Gérard Guérin

Institut national de la recherche agronomique

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Isabelle Lantier

Institut national de la recherche agronomique

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Jean-Pierre Furet

Institut national de la recherche agronomique

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