Antibodies to N-terminal Peptides of Low MrSubunits of Wheat Glutenin. II. Detection of Subunits Encoded by Different Loci |
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| Institution: | 1. CRISCEB, Research Center of Computational and Biotechnological Sciences, Second University of Naples, via Costantinopoli 16, 80138 Naples, Italy;2. Department of Biochemistry and Biophysics, Second University of Naples, via Costantinopoli 16, 80138 Naples, Italy;3. Department of Agrobiology and Agrochemistry, University of Tuscia, via S. Camillo de Lellis, 01100 Viterbo, Italy;4. Department of Environmental Sciences, University of Tuscia, via S. Camillo de Lellis, 01100 Viterbo, Italy;1. Washington University School of Medicine, Department of Surgery, St. Louis, Missouri USA;1. Research Control Department, Nisshin Flour Milling Co., Ltd., Nihonbashi, Chuo-ku, Tokyo 103, Japan;2. Department of Food Science and Technology, Faculty of Agriculture, Kyoto University, Kyoto 606, Japan;1. Quality Wheat Cooperative Research Centre Ltd;2. CSIRO Plant Industry, GPO Box 1600, Canberra, ACT 2601, Australia |
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| Abstract: | A panel of anti-peptide antibodies specific for each of the different N-terminal sequence types of B- and C-low molecular mass glutenin subunits (L MrGS) were utilised in immunoblotting studies to identify the chromosomal location of genes encoding different sequences and to characterise the allelic variation of the encoding loci. The MET-type sequences were predominantly found among the B- subunits, while the α- and γ- sequences predominated in the C- subunits. The quantitatively major SHIPGLERPS sequence was found in both the B- and C- mobility regions. Using either biotypes in the cultivar, Aroona or genetic lines containing double rye chromosome 1 substitutions and thus expressing only single LMr GS alleles, the sequences were determined for most of the major polypeptides expressed by each LMr GS allele. The L MrGS from different genomes encoded different numbers of each sequence type. Furthermore, different polypeptides within a particular «block» of subunits encoded by a given allele often had differing N-terminal sequences. However, subunits of similar electrophoretic mobilities encoded by different alleles at each locus usually had identical N-terminal sequences, suggesting that they may instead differ in the number of repeats. In Chinese Spring, genes encoding the SHIPGLERPS and METSHIPGL sequence types were predominantly present on chromosomes 1B and 1D, while the related METSRVPGL sequence was only encoded on 1D. In contrast, the METSCIPGL, α- and γ-sequences were encoded on each of chromosomes 1A, 1B and 1D. Several different electrophoretic and immunoblotting approaches using null lines suggested that some of the α-type L MrGS may also be encoded by group 6 chromosomes, particularly 6D. The anti- SHIPGLERPS antibody also recognised chromosome 1B encoded β-, γ- and ω-gliadins, while the anti-METSRVPGL antibody recognised 1D encoded α- and β-gliadins. The absence of sequences within the major gliadin families that are highly homologous to the latter two N-terminal L MrGS sequences may suggest that some monomeric L MrGS could exist within the electrophoretically-resolved gliadins. These antibodies will provide valuable reagents for the study of the roles of particular L MrGS families in the structure and function of the glutenin macropolymer, the role of different LMr GS types in determining the influence of allelic variation of L MrGS composition on dough properties, and potentially in the development of diagnostics for these flour components. |
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