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ISHS Acta Horticulturae 556: V International Congress on Hazelnut

RAPD MARKERS FOR SELF-INCOMPATIBILITY IN CORYLUS AVELLANA L.

Authors:   N.V. Bassil, A.N. Azarenko
Keywords:   hazelnut, filbert, sporophytic self-incompatibility, bulked segregant analysis, SCAR, PCR
Abstract:
We used a bulked segregant analysis approach in a population of 84 hazelnut (Corylus avellana L.) seedlings of the cross OSU 316.139 (S1S6) x OSU 265.096 (S3S4) in an attempt to identify random amplified polymorphic DNA (RAPD) markers linked to incompatibility alleles. DNA samples from five trees each were pooled to form bulks for the four S-allele combinations. Superbulks of 10 trees, each devoid of a single allele, were then created. Initial screening of the DNA from parents and superbulks with 460 random primers identified five possible S-allele markers. When the entire population was screened, only one marker, OPN201300, was linked to an S-allele. OPN201300 was present in all 52 S3 progeny, and absent in 28 of the 31 non-S3 individuals, giving a recombination rate of 3.75% in this population. However, OPN201300 was not linked to the S3 allele outside the original population. Work with previously identified RAPD marker OPI07750 showed that it is an excellent marker for the S2 allele. This marker was cloned and two pairs of sequence characterized amplified region (SCAR) primers were made. Each pair identified one monomorphic 700 bp band in all individuals and another 750 bp DNA fragment that co-segregated with the S2 allele. Attempts to sequence both bands consistently resulted in identical nucleotide sequences. Searches in the Databank revealed 28% identity at the amino acid level to a putative reverse transcriptase from Oryza sativa and to a reverse transcriptase domain from Arabidopsis thaliana. Efforts are underway to characterize the S2 marker and determine its usefulness in cloning the self-incompatibility locus.

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