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15 results on '"Gustafson-Seabury A"'

1. A high resolution RH map of the bovine major histocompatibility complex

Author

Womack James E, Raudsepp Terje, Cothran Marian, Gustafson-Seabury Ashley L, Fritz Krista L, Childers Christopher P, Brinkmeyer-Langford Candice L, and Skow Loren C

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

Abstract Background The cattle MHC is termed the bovine leukocyte antigen (BoLA) and, along with the MHCs of other ruminants, is unique in its genomic organization. Consequently, correct and reliable gene maps and sequence information are critical to the study of the BoLA region. The bovine genome sequencing project has produced two assemblies (Btau_3.1 and 4.0) that differ substantially from each other and from conventional gene maps in the BoLA region. To independently compare the accuracies of the different sequence assemblies, we have generated a high resolution map of BoLA using a 12,000rad radiation hybrid panel. Seventy-seven unique sequence tagged site (STS) markers chosen at approximately 50 kb intervals from the Btau 2.0 assembly and spanning the IIa-III-I and IIb regions of the bovine MHC were mapped on a 12,000rad bovine radiation hybrid (RH) panel to evaluate the different assemblies of the bovine genome sequence. Results Analysis of the data generated a high resolution RH map of BoLA that was significantly different from the Btau_3.1 assembly of the bovine genome but in good agreement with the Btau_4.0 assembly. Of the few discordancies between the RH map and Btau_4.0, most could be attributed to closely spaced markers that could not be precisely ordered in the RH panel. One probable incorrectly-assembled sequence and three missing sequences were noted in the Btau_4.0 assembly. The RH map of BoLA is also highly concordant with the sequence-based map of HLA (NCBI build 36) when reordered to account for the ancestral inversion in the ruminant MHC. Conclusion These results strongly suggest that studies using Btau_3.1 for analyses of the BoLA region should be reevaluated in light of the Btau_4.0 assembly and indicate that additional research is needed to produce a complete assembly of the BoLA genomic sequences.

Published
2009
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2. A BAC contig map over the proximal ∼3.3 Mb region of horse chromosome 21

Author

Ashley Gustafson-Seabury, Candice Brinkmeyer-Langford, Bhanu P. Chowdhary, and Terje Raudsepp

Subjects
Genetics, Contig, Horse, Biology, Chromosome 21, Molecular Biology, Genetics (clinical)
Abstract

A total of 207 BAC clones containing 155 loci were isolated and arranged into a map of linearly ordered overlapping clones over the proximal part of horse chromosome 21 (ECA21), which corresponds to the proximal half of the short arm of human chromosome 19 (HSA19p) and part of HSA5. The clones form two contigs – each corresponding to the respective human chromosomes – that are estimated to be separated by a gap of ∼200 kb. Of the 155 markers present in the two contigs, 141 (33 genes and 108 STS) were generated and mapped in this study. The BACs provide a 4–5× coverage of the region and span an estimated length of ∼3.3 Mb. The region presently contains one mapped marker per 22 kb on average, which represents a major improvement over the previous resolution of one marker per 380 kb obtained through the generation of a dense RH map for this segment. Dual color fluorescence in situ hybridization on metaphase and interphase chromosomes verified the relative order of some of the BACs and helped to orient them accurately in the contigs. Despite having similar gene order and content, the equine region covered by the contigs appears to be distinctly smaller than the corresponding region in human (3.3 Mb vs. 5.5–6 Mb) because the latter harbors a host of repetitive elements and gene families unique to humans/primates. Considering limited representation of the region in the latest version of the horse whole genome sequence EquCab2, the dense map developed in this study will prove useful for the assembly and annotation of the sequence data on ECA21 and will be instrumental in rapid search and isolation of candidate genes for traits mapped to this region.

Published
2008

3. Viability of equine embryos after puncture of the capsule and biopsy for preimplantation genetic diagnosis

Author

David L. Hartman, Katrin Hinrichs, Young Ho Choi, Ashley Gustafson-Seabury, Fernando L. Riera, S.B. Bliss, Bhanu P. Chowdhary, Jaime E. Roldán, and I. C. Velez

Subjects
Embryology, medicine.medical_specialty, Pregnancy Rate, Cell Survival, Biopsy, Embryonic Development, Gestational Age, Biology, Preimplantation genetic diagnosis, Andrology, Endocrinology, Embryo cryopreservation, Pregnancy, medicine, Animals, Blastocyst, Horses, Preimplantation Diagnosis, Peptidylprolyl isomerase, Gynecology, medicine.diagnostic_test, Parturition, Obstetrics and Gynecology, Trophoblast, Embryo, Cell Biology, Pregnancy rate, medicine.anatomical_structure, Reproductive Medicine, embryonic structures, Pregnancy, Animal, Female
Abstract

The equine embryo possesses a capsule that is considered essential for its survival. We assessed viability after breaching the capsule of early (Day 6) and expanded (Day 7 and 8) equine blastocysts by micromanipulation. The capsule was penetrated using a Piezo drill, and trophoblast biopsy samples were obtained for genetic analysis. Pregnancy rates for Day-6 embryos, which had intact zonae pellucidae at the time of recovery, were 3/3 for those biopsied immediately after recovery and 2/3 for those biopsied after being shipped overnight under warm (∼28 °C) conditions. The pregnancy rates for encapsulated Day-7 expanded blastocysts were 5/6 for those biopsied immediately and 5/6 for those biopsied after being shipped overnight warm. Two of four encapsulated Day-8 blastocysts, 790 and 1350 μm in diameter, established normal pregnancies after biopsy. Nine mares were allowed to maintain pregnancy, and they gave birth to nine normal foals. Biopsied cells from eight embryos that produced foals were subjected to whole-genome amplification. Sex was successfully determined from amplified DNA in 8/8 embryos. Identification of disease-causing mutations matched in the analyses of 6/6 samples for the sodium channel, voltage-gated, type IV, alpha subunit (SCN4A) gene and in 6/7 samples for the peptidylprolyl isomerase B (PPIB) gene, in embryo-foal pairs. Thus, the capsule of the equine embryo can be breached without impairing viability. Further work is needed to determine whether this breach is transient or permanent. These findings are relevant to the understanding of equine embryo development and to the establishment of methods for micromanipulation and embryo cryopreservation in this species.

Published
2010

4. Total RNA isolation from stallion sperm and testis biopsies

Author

Terje Raudsepp, Charles C. Love, P. J. Das, Ashley Gustafson-Seabury, Bhanu P. Chowdhary, Monika Vishnoi, Nandina Paria, Dickson D. Varner, and Sankar P. Chaki

Subjects
Male, Quality Control, Biopsy, Semen analysis, Biology, Andrology, Food Animals, Testis, medicine, Animals, Horses, Small Animals, Cryopreservation, Messenger RNA, medicine.diagnostic_test, urogenital system, Equine, Reverse Transcriptase Polymerase Chain Reaction, RNA, Sperm, Molecular biology, Spermatozoa, Reverse transcriptase, Semen Analysis, genomic DNA, Genetic Techniques, Trizol, Animal Science and Zoology, RNA extraction, Semen Preservation
Abstract

Sperm mRNA transcriptional profiles can be used to evaluate male fertility, yet differences between species in sperm attributes and packaging require adjustments in sperm RNA isolation protocols. The objective was to optimize RNA isolation methodology for fresh, frozen, and extended ejaculates, and epididymal sperm of stallions. Additionally, a protocol for RNA isolation from testis biopsies was established. Separation of sperm from somatic cells was critical for assuring the isolation of sperm-specific RNA. The highest purity was obtained by centrifuging ejaculates and epididymal sperm at 200 x g for 30 min through a 40% Equipure silanized silica particle solution. Sperm RNA isolation was more efficient with TRIzol reagent than with a spin-column based method; it resulted in 2 microg of total RNA per 100 x 10(6) sperm. To evaluate RNA quantity and quality, we used a NanoDrop spectrophotometer and Agilent Bioanalyzer. A protocol for reverse transcriptase PCR with equine primers for PRM2 and PTPRC genes was developed to determine sperm RNA contamination with genomic DNA or RNA from somatic cells. By these methods, hybridization- and sequencing-quality RNA was isolated from 11 samples of stallion sperm. Stallion testis biopsy with a 14 gauge 22 mm deep biopsy needle yielded approximately 12 microg of good quality total RNA, and could serve as an alternative to excision surgery for sample procurement. Compared to RNA isolation from testis, the sperm required advanced processing and RNA quality control. The described methodologies provided a foundation to establish functional genomic studies of stallion fertility.

Published
2009

5. A high resolution RH map of the bovine major histocompatibility complex

Author

Ashley Gustafson-Seabury, Krista L. Fritz, Christopher P. Childers, Terje Raudsepp, James E. Womack, Loren C. Skow, Marian Cothran, and Candice Brinkmeyer-Langford

Subjects
Genetic Markers, lcsh:QH426-470, lcsh:Biotechnology, Biology, Synteny, Genome, Major Histocompatibility Complex, Sequence-tagged site, lcsh:TP248.13-248.65, Genetics, Animals, Humans, Radiation hybrid mapping, Sequence Tagged Sites, Genomic organization, Radiation Hybrid Mapping, Gene map, Genome, Human, Reproducibility of Results, Genomics, Chromosomes, Mammalian, lcsh:Genetics, Bovine genome, Cattle, Human genome, Databases, Nucleic Acid, Research Article, Biotechnology
Abstract

Background The cattle MHC is termed the bovine leukocyte antigen (BoLA) and, along with the MHCs of other ruminants, is unique in its genomic organization. Consequently, correct and reliable gene maps and sequence information are critical to the study of the BoLA region. The bovine genome sequencing project has produced two assemblies (Btau_3.1 and 4.0) that differ substantially from each other and from conventional gene maps in the BoLA region. To independently compare the accuracies of the different sequence assemblies, we have generated a high resolution map of BoLA using a 12,000rad radiation hybrid panel. Seventy-seven unique sequence tagged site (STS) markers chosen at approximately 50 kb intervals from the Btau 2.0 assembly and spanning the IIa-III-I and IIb regions of the bovine MHC were mapped on a 12,000rad bovine radiation hybrid (RH) panel to evaluate the different assemblies of the bovine genome sequence. Results Analysis of the data generated a high resolution RH map of BoLA that was significantly different from the Btau_3.1 assembly of the bovine genome but in good agreement with the Btau_4.0 assembly. Of the few discordancies between the RH map and Btau_4.0, most could be attributed to closely spaced markers that could not be precisely ordered in the RH panel. One probable incorrectly-assembled sequence and three missing sequences were noted in the Btau_4.0 assembly. The RH map of BoLA is also highly concordant with the sequence-based map of HLA (NCBI build 36) when reordered to account for the ancestral inversion in the ruminant MHC. Conclusion These results strongly suggest that studies using Btau_3.1 for analyses of the BoLA region should be reevaluated in light of the Btau_4.0 assembly and indicate that additional research is needed to produce a complete assembly of the BoLA genomic sequences.

Published
2009

6. A 4103 marker integrated physical and comparative map of the horse genome

Author

Glenda Goh, Loren C. Skow, Leslie A. Lyons, Tosso Leeb, Christopher M. Seabury, E. Stallknecht-Rice, Keith Durkin, Candice Brinkmeyer-Langford, Ottmar Distl, Bhanu P. Chowdhary, Maria Cecilia T. Penedo, Gérard Guérin, H. Yasue, Terje Raudsepp, Ashley Gustafson-Seabury, Alejandro A. Schäffer, M. L. Wagner, Matthew M. Binns, James R. Mickelson, Kamal Khazanehdari, James N. MacLeod, Teruaki Tozaki, Eun Joon Lee, Richa Agarwala, Unité de recherche Génétique Biochimique et Cytogénétique (LGBC), Institut National de la Recherche Agronomique (INRA), and ProdInra, Migration

Subjects
Genetic Markers, Chromosomes, Artificial, Bacterial, [SDV]Life Sciences [q-bio], Computational biology, Biology, Genome, Article, 03 medical and health sciences, Cytogenetics, Species Specificity, Genetics, medicine, Animals, Horses, Molecular Biology, Gene, Genetics (clinical), X chromosome, ComputingMilieux_MISCELLANEOUS, In Situ Hybridization, Fluorescence, 030304 developmental biology, Whole genome sequencing, PHYSICAL MAPS, 0303 health sciences, Radiation Hybrid Mapping, Autosome, medicine.diagnostic_test, 630 Agriculture, 030302 biochemistry & molecular biology, Breakpoint, Chromosome Mapping, Physical Chromosome Mapping, [SDV] Life Sciences [q-bio], Horse genome, GENETIC MAPS, 570 Life sciences, biology, 590 Animals (Zoology), Lod Score, Fluorescence in situ hybridization
Abstract

A comprehensive second-generation whole genome radiation hybrid (RH II), cytogenetic and comparative map of the horse genome (2n = 64) has been developed using the 5000rad horse × hamster radiation hybrid panel and fluorescence in situ hybridization (FISH). The map contains 4,103 markers (3,816 RH; 1,144 FISH) assigned to all 31 pairs of autosomes and the X chromosome. The RH maps of individual chromosomes are anchored and oriented using 857 cytogenetic markers. The overall resolution of the map is one marker per 775 kilobase pairs (kb), which represents a more than five-fold improvement over the first-generation map. The RH II incorporates 920 markers shared jointly with the two recently reported meiotic maps. Consequently the two maps were aligned with the RH II maps of individual autosomes and the X chromosome. Additionally, a comparative map of the horse genome was generated by connecting 1,904 loci on the horse map with genome sequences available for eight diverse vertebrates to highlight regions of evolutionarily conserved syntenies, linkages, and chromosomal breakpoints. The integrated map thus obtained presents the most comprehensive information on the physical and comparative organization of the equine genome and will assist future assemblies of whole genome BAC fingerprint maps and the genome sequence. It will also serve as a tool to identify genes governing health, disease and performance traits in horses and assist us in understanding the evolution of the equine genome in relation to other species.

Published
2008

7. A BAC contig map over the proximal approximately 3.3 Mb region of horse chromosome 21

Author

C, Brinkmeyer-Langford, T, Raudsepp, A, Gustafson-Seabury, and B P, Chowdhary

Subjects
Evolution, Molecular, Chromosome Walking, Chromosomes, Artificial, Bacterial, Contig Mapping, Base Sequence, Species Specificity, Animals, Humans, Horses, Polymerase Chain Reaction, In Situ Hybridization, Fluorescence, DNA Primers, Sequence Tagged Sites
Abstract

A total of 207 BAC clones containing 155 loci were isolated and arranged into a map of linearly ordered overlapping clones over the proximal part of horse chromosome 21 (ECA21), which corresponds to the proximal half of the short arm of human chromosome 19 (HSA19p) and part of HSA5. The clones form two contigs - each corresponding to the respective human chromosomes - that are estimated to be separated by a gap of approximately 200 kb. Of the 155 markers present in the two contigs, 141 (33 genes and 108 STS) were generated and mapped in this study. The BACs provide a 4-5x coverage of the region and span an estimated length of approximately 3.3 Mb. The region presently contains one mapped marker per 22 kb on average, which represents a major improvement over the previous resolution of one marker per 380 kb obtained through the generation of a dense RH map for this segment. Dual color fluorescence in situ hybridization on metaphase and interphase chromosomes verified the relative order of some of the BACs and helped to orient them accurately in the contigs. Despite having similar gene order and content, the equine region covered by the contigs appears to be distinctly smaller than the corresponding region in human (3.3 Mb vs. 5.5-6 Mb) because the latter harbors a host of repetitive elements and gene families unique to humans/primates. Considering limited representation of the region in the latest version of the horse whole genome sequence EquCab2, the dense map developed in this study will prove useful for the assembly and annotation of the sequence data on ECA21 and will be instrumental in rapid search and isolation of candidate genes for traits mapped to this region.

Published
2007

8. High-resolution RH map of horse chromosome 22 reveals a putative ancestral vertebrate chromosome

Author

Loren C. Skow, James R. Mickelson, Ashley Gustafson-Seabury, M. L. Wagner, Glenda Goh, Srinivas R. Kata, Bhanu P. Chowdhary, Teruaki Tozaki, Terje Raudsepp, and James E. Womack

Subjects
Genetics, Chromosomes, Artificial, Bacterial, Radiation Hybrid Mapping, Autosome, Gene map, Biology, Biological Evolution, Polymerase Chain Reaction, Chromosomes, Rats, Chromosome 17 (human), Mice, Chromosome 16, Chromosome 19, Gene Order, Vertebrates, Animals, Humans, Horses, Chromosome 21, Chromosome 22, In Situ Hybridization, Fluorescence, Synteny, Sequence Tagged Sites
Abstract

High-resolution gene maps of individual equine chromosomes are essential to identify genes governing traits of economic importance in the horse. In pursuit of this goal we herein report the generation of a dense map of horse chromosome 22 (ECA22) comprising 83 markers, of which 52 represent specific genes and 31 are microsatellites. The map spans 831 cR over an estimated 64 Mb of physical length of the chromosome, thus providing markers at approximately 770 kb or 10 cR intervals. Overall, the resolution of the map is to date the densest in the horse and is the highest for any of the domesticated animal species for which annotated sequence data are not yet available. Comparative analysis showed that ECA22 shares remarkable conservation of gene order along the entire length of dog chromosome 24, something not yet found for an autosome in evolutionarily diverged species. Comparison with human, mouse, and rat homologues shows that ECA22 can be traced as two conserved linkage blocks, each related to individual arms of the human homologue-HSA20. Extending the comparison to the chicken genome showed that one of the ECA22 blocks that corresponds to HSA20q shares synteny conservation with chicken chromosome 20, suggesting the segment to be ancestral in mammals and birds.

Published
2004

13. A 4,103 marker integrated physical and comparative map of the horse genome

Author

Raudsepp, T., primary, Gustafson-Seabury, A., additional, Durkin, K., additional, Wagner, M.L., additional, Goh, G., additional, Seabury, C.M., additional, Brinkmeyer-Langford, C., additional, Lee, E-J., additional, Agarwala, R., additional, Stallknecht-Rice, E., additional, Schäffer, A.A., additional, Skow, L.C., additional, Tozaki, T., additional, Yasue, H., additional, Penedo, M.C.T., additional, Lyons, L.A., additional, Khazanehdari, K.A., additional, Binns, M.M., additional, MacLeod, J.N., additional, Distl, O., additional, Guérin, G., additional, Leeb, T., additional, Mickelson, J.R., additional, and Chowdhary, B.P., additional

Published
2008
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15. A BAC contig map over the proximal approximately 3.3 Mb region of horse chromosome 21.

Author

Brinkmeyer-Langford C, Raudsepp T, Gustafson-Seabury A, and Chowdhary BP

Subjects
Animals, Base Sequence, Chromosome Walking, Chromosomes, Artificial, Bacterial genetics, DNA Primers genetics, Evolution, Molecular, Humans, In Situ Hybridization, Fluorescence veterinary, Polymerase Chain Reaction veterinary, Sequence Tagged Sites, Species Specificity, Contig Mapping veterinary, Horses genetics
Abstract

A total of 207 BAC clones containing 155 loci were isolated and arranged into a map of linearly ordered overlapping clones over the proximal part of horse chromosome 21 (ECA21), which corresponds to the proximal half of the short arm of human chromosome 19 (HSA19p) and part of HSA5. The clones form two contigs - each corresponding to the respective human chromosomes - that are estimated to be separated by a gap of approximately 200 kb. Of the 155 markers present in the two contigs, 141 (33 genes and 108 STS) were generated and mapped in this study. The BACs provide a 4-5x coverage of the region and span an estimated length of approximately 3.3 Mb. The region presently contains one mapped marker per 22 kb on average, which represents a major improvement over the previous resolution of one marker per 380 kb obtained through the generation of a dense RH map for this segment. Dual color fluorescence in situ hybridization on metaphase and interphase chromosomes verified the relative order of some of the BACs and helped to orient them accurately in the contigs. Despite having similar gene order and content, the equine region covered by the contigs appears to be distinctly smaller than the corresponding region in human (3.3 Mb vs. 5.5-6 Mb) because the latter harbors a host of repetitive elements and gene families unique to humans/primates. Considering limited representation of the region in the latest version of the horse whole genome sequence EquCab2, the dense map developed in this study will prove useful for the assembly and annotation of the sequence data on ECA21 and will be instrumental in rapid search and isolation of candidate genes for traits mapped to this region., (Copyright 2008 S. Karger AG, Basel.)

Published
2008
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