The technique of simultaneous G banding and in situ hybridization has been developed in plants for the first time. Using this technique, RFLP marker umc58 closely linked with the hm1 gene dictating Helminthosporiu...The technique of simultaneous G banding and in situ hybridization has been developed in plants for the first time. Using this technique, RFLP marker umc58 closely linked with the hm1 gene dictating Helminthosporium carbonum susceptibility1 was localized onto 1L3 (chromosome 1, long arm, the third band from the centromere to the end of the arm), 5L5 and 9L5. The results demonstrated that umc58 was a triplicated sequence. It was deduced that umc58 probably was in a duplicated region that includes a part of Helminthosporium carbonum susceptibility genes (hm1 and hm2), as the hybridization sites of umc58 in chromosomes 1 and 9 were those at which the genes localize. The techniques of simultaneous G banding and ISH in plants are discussed.展开更多
In order to precisely recognize and karyotype Brassica napus L. chromosomes, C0t-1 DNA was extracted from its genomic DNA, labeled with biotin-1 1-dUTP and in situ hybridized. The hybridized locations were detected by...In order to precisely recognize and karyotype Brassica napus L. chromosomes, C0t-1 DNA was extracted from its genomic DNA, labeled with biotin-1 1-dUTP and in situ hybridized. The hybridized locations were detected by Cy3-conjugated streptavidin. Specific fluorescence in situ hybridization (FISH) signal bands were detected on all individual chromosome pairs. Each chromosome pair showed specific banding patterns. The B. napus karyotype has been constructed, for the first time, on the basis of both Cot-1 DNA FISH banding patterns and chromosome morphology.展开更多
文摘The technique of simultaneous G banding and in situ hybridization has been developed in plants for the first time. Using this technique, RFLP marker umc58 closely linked with the hm1 gene dictating Helminthosporium carbonum susceptibility1 was localized onto 1L3 (chromosome 1, long arm, the third band from the centromere to the end of the arm), 5L5 and 9L5. The results demonstrated that umc58 was a triplicated sequence. It was deduced that umc58 probably was in a duplicated region that includes a part of Helminthosporium carbonum susceptibility genes (hm1 and hm2), as the hybridization sites of umc58 in chromosomes 1 and 9 were those at which the genes localize. The techniques of simultaneous G banding and ISH in plants are discussed.
文摘In order to precisely recognize and karyotype Brassica napus L. chromosomes, C0t-1 DNA was extracted from its genomic DNA, labeled with biotin-1 1-dUTP and in situ hybridized. The hybridized locations were detected by Cy3-conjugated streptavidin. Specific fluorescence in situ hybridization (FISH) signal bands were detected on all individual chromosome pairs. Each chromosome pair showed specific banding patterns. The B. napus karyotype has been constructed, for the first time, on the basis of both Cot-1 DNA FISH banding patterns and chromosome morphology.
