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Patricia E. Klein
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doi:10.1534/genetics.104.026765
A more recent version of this article appeared on February 1, 2005.
REGULAR RESEARCH PAPERS |
Molecular Cytogenetic Maps of Sorghum Linkage Groups 2 and 8
Jeong-Soon Kim 1, Patricia E. Klein 1, Robert R. Klein 2, H. James A. Price 1, John E. Mullet 1 and David M. Stelly 1*
1 Texas A&M University
2 USDA-ARS
* To whom correspondence should be addressed. E-mail: stelly{at}tamu.edu.
Submitted on January 24, 2004
Revised on May 18, 2004
Accepted on 4 October 2004
To integrate genetic, physical and cytological perspectives of the Sorghum bicolor genome, we selected 40 landed bacterial artificial chromosome (BAC) clones that contain different linkage map markers, 21 from linkage group 2 (LG-02) and 19 from LG-08. Multi-BAC probe cocktails were constructed for each chromosome from the landed BACs, which were also pre-evaluated for FISH signal quality, relative position and collective chromosome coverage. Comparison to the corresponding linkage map revealed full concordance of locus order between cytological and prior segregation analyses. The pericentromeric heterochromatin constituted a large quasi-uniform block in each bivalent, and was especially large in the bivalent corresponding to LG-08. Centromere positions in LG-02 and LG-08 were progressively delimited using FISH to identify landed BACs for which the FISH signals visibly flanked the centromere. Alignment of linkage and cytological maps revealed that pericentromeric heterochromatin of these sorghum chromosomes is largely devoid of recombination, which is mostly relegated to the more distal regions, which are largely euchromatic. This suggests that the sorghum genome is thus even more amenable to physical mapping of genes and positional cloning than C-value alone might suggest. As a prelude to positional cloning of the fertility restorer, Rf1, FISH of BAC clones flanking the Rf1 locus were used to delimit the chromosomal position of the gene. FISH of BACs that contain the most proximal linkage markers enabled localization of Rf1 to a ~0.4 Mbp euchromatic region of LG-08. Cytogenetic analyses of Rf1 and other trait loci will aid in assessing the feasibility of positional cloning and help formulate strategies required for cloning this and other agriculturally ritical genes.
Key Words: BAC, FISH, fertility restorer gene, genome map, sorghum
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