Genetical control and linkage relationships of isozyme markers in sugar beet (B. vulgaris L.) |
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Authors: | E. Smed J. P. C. Van Geyt M. Oleo |
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Affiliation: | (1) Breeding Station Maribo, DK-4960 Holeby, Denmark;(2) Instituut voor Moleculaire Biologie, Vrije Universiteit Brussel, Dienst Plantengenetika, B-1640 St Genesius Rode, Belgium;(3) Present address: Phytotec, Dep. Recherche, Pl. L. Pasteur 1, B-1348 Louvain-la-Neuve, Belgium |
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Abstract: | Summary Five isozyme systems were genetically investigated. The different separation techniques, the developmental expression and the use as marker system in sugar beet genetics and breeding is discussed. Isocitrate dehydrogenase was controlled by two genes. The gene products form inter- as well as intralocus dimers, even with the gene products of the Icd gene in B. procumbens and B. patellaris. Adenylate kinase was controlled by one gene. Three different allelic forms were detected, which were active as monomeric proteins. Glucose phosphate isomerase showed two zones of activity. One zone was polymorphic. Three allelic variants, active as dimers, were found. Phosphoglucomutase also showed two major zones of activity. One zone was polymorphic and coded for monomeric enzymes. Two allelic forms were found in the accessions studied. The cathodal peroxidase system was controlled by two independent genes, of which only one was polymorphic. The gene products are active as monomers. Linkage was found between red hypocotyl color (R) and Icd2. Pgm1, Gpi2, Ak1 and the Icd2-R linkage group segregated independently. |
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Keywords: | Beta vulgaris Sugar beet Isozymes Genetics Linkage |
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