Genomic analysis of sorghum by fluorescence in situ hybridization

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dc.contributor.advisor Stelly, David M. en_US
dc.contributor.advisor Price, H. James en_US
dc.creator Kim, Jeong-Soon en_US
dc.date.accessioned 2004-11-15T19:49:05Z
dc.date.available 2004-11-15T19:49:05Z
dc.date.created 2003-08 en_US
dc.date.issued 2004-11-15T19:49:05Z
dc.identifier.uri http://handle.tamu.edu/1969.1/1184
dc.description.abstract The reliability of genome analysis and proficiency of genetic manipulation in vivo and in vitro are increased by assignment of linkage groups to specific chromosomes, placement of centromeres, orientation with respect to telomeres, and linear alignment with respect to chromosomal features and dimensions. I undertook five studies aimed at integrating sorghum genomics and cytogenetics at several levels. The results help establish an entirely new "cyto-genomics" resource, impacts of which are likely to be broad. In the first study, I developed a FISH-based karyotyping system for Sorghum bicolor Moench. I used integrated structural genomic resources, including linkage maps and large-insert clonal libraries of sorghum genomic DNA to develop a 17-locus probe cocktail for simultaneous fluorescent in situ hybridization (FISH). This probe enabled facile identification of all chromosome pairs in mitotic chromosome spreads. Perhaps just as important, I established time-efficient means to select sorghum BAC clones for multi-probe FISH. Thus, an integrated cyto-genomics system for sorghum can be constructed without need of chromosome flow sorting or microdissection, both of which are difficult and costly. In the second study, hybridization of DNA clones from 37 different genomic regions enabled the assignment of linkage groups and orientation of linkage maps to chromosomes. Comparisons between genetic and physical distances throughout the genome enabled a new nomenclature for linkage group designation in sorghum. The results provide an integrated nomenclature system of Sorghum bicolor chromosomes and linkage groups. In the third study, I created high-resolution maps by FISH to pachytene bivalents for two linkage groups (B and H), and defined relationships between pericentromeric heterochromatin, centromeres, mapped markers and recombination rates. These relationships will help guide the development and use of sorghum genomics. In the fifth study, I used FISH in two ongoing gene-targeted efforts. For the maturity gene ma5 and fertility restoration gene rfl, I estimated physical lengths between currently available flanking molecular markers. This enables estimation of recombination densities in these regions and assessment of the applicability of map-based and -assisted cloning. en_US
dc.description.provenance Made available in DSpace on 2004-11-15T19:49:05Z (GMT). No. of bitstreams: 2 etd-tamu-2003B-2003070623-KIM-1.pdf: 10453593 bytes, checksum: 9513b4dd09b79fce87f7770539a73325 (MD5) etd-tamu-2003B-2003070623-KIM-1.pdf.txt: 174793 bytes, checksum: 75d2cd695747aebd770639c97df4603b (MD5) en
dc.format.extent 10453593 bytes
dc.format.extent 174793 bytes
dc.format.medium electronic en_US
dc.format.mimetype application/pdf
dc.format.mimetype text/plain
dc.language.iso en_US en_US
dc.publisher Texas A&M University en_US
dc.subject FISH en_US
dc.subject sorghum en_US
dc.subject chromosome en_US
dc.subject DNA en_US
dc.subject gene en_US
dc.subject cytogenetic map en_US
dc.subject physical map en_US
dc.title Genomic analysis of sorghum by fluorescence in situ hybridization en_US
thesis.degree.department Soil and Crop Sciences en_US
thesis.degree.discipline Plant Breeding en_US
thesis.degree.grantor Texas A&M University en_US
thesis.degree.name Ph. D. en_US
thesis.degree.level Doctoral en_US
dc.contributor.committeeMember Zhang, Hong Bin en_US
dc.contributor.committeeMember Mullet, John E. en_US
dc.contributor.committeeMember Rooney, William L. en_US
dc.type.genre Electronic Dissertation en_US
dc.type.material text en_US
dc.format.digitalOrigin born digital en_US

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