BackgroundCommon bean was one of the first crops that benefited from the development and utilization of molecular marker-assisted selection (MAS) for major disease resistance genes. Efficiency of MAS for breeding common bean is still hampered, however, due to the dominance, linkage phase, and loose linkage of previously developed markers. Here we applied in silico bulked segregant analysis (BSA) to the BeanCAP diversity panel, composed of over 500 lines and genotyped with the BARCBEAN_3 6K SNP BeadChip, to develop codominant and tightly linked markers to the I gene controlling resistance to Bean common mosaic virus (BCMV).ResultsWe physically mapped the genomic region underlying the I gene. This locus, in the distal arm of chromosome Pv02, contains seven putative NBS-LRR-type disease resistance genes. Two contrasting bulks, containing BCMV host differentials and ten BeanCAP lines with known disease reaction to BCMV, were subjected to in silico BSA for targeting the I gene and flanking sequences. Two distinct haplotypes, containing a cluster of six single nucleotide polymorphisms (SNP), were associated with resistance or susceptibility to BCMV. One-hundred and twenty-two lines, including 115 of the BeanCAP panel, were screened for BCMV resistance in the greenhouse, and all of the resistant or susceptible plants displayed distinct SNP haplotypes as those found in the two bulks. The resistant/susceptible haplotypes were validated in 98 recombinant inbred lines segregating for BCMV resistance. The closest SNP (~25-32 kb) to the distal NBS-LRR gene model for the I gene locus was targeted for conversion to codominant KASP (Kompetitive Allele Specific PCR) and CAPS (Cleaved Amplified Polymorphic Sequence) markers. Both marker systems accurately predicted the disease reaction to BCMV conferred by the I gene in all screened lines of this study.ConclusionsWe demonstrated the utility of the in silico BSA approach using genetically diverse germplasm, genotyped with a high-density SNP chip array, to discover SNP variation at a specific targeted genomic region. In common bean, many disease resistance genes are mapped and their physical genomic position can now be determined, thus the application of this approach will facilitate further development of codominant and tightly linked markers for use in MAS.Electronic supplementary materialThe online version of this article (doi:10.1186/1471-2164-15-903) contains supplementary material, which is available to authorized users.
An ideotype breeding strategy to improve an economically important trait is achievable if subcomponent phenotypes most associated with the trait are targeted for selection. The success of this strategy in modern breeding history can be highlighted in dry bean (Phaseolus vulgaris L.), where an enhancement in dry bean production was facilitated in the last 25 yr by replacing Type III prostrate growth habit with Type II upright growth habit. This growth habit leads to disease avoidance and enables cost‐effective management practices. To better understand the ideotype breeding trajectory in dry bean, and guarantee further improvements, we characterized 16 traits at three locations using a panel consisting of 122 genotypes with different growth habits. Among the growth habit types, significant differences were detected for seven architectural traits, three seed yield (SY) traits, and one phenological trait. Genetic variance was greater in the Type II genotypes than the Type III genotypes for five of the significant traits, including canopy height (CNH) and SY. Furthermore, in Type II genotypes, moderate narrow‐sense heritability was detected for CNH, lodging (LDG), plant length (PL), and stem diameter (STD), suggesting positive gain can be made for growth habit from crosses between Type II genotypes. A network analysis of Type II genotypes revealed these four traits are highly correlated, and suggests possible genetic relatedness among the traits. Breeders often use CNH as a selection criterion, and the positive correlation between this trait and STD suggests a possible anatomical mechanism responsible for the more upright plant types.
Ergothioneine, a histidine derivative, is concentrated in conidia of ascomycetous fungi. To investigate the function of ergothioneine, we crossed the wild type Neurospora crassa (Egt(+)) and an ergothioneine non-producer (Egt(-), Δegt-1, a knockout in NCU04343.5) and used the Egt(+) and Egt(-) progeny strains for phenotypic analyses. Compared to the Egt(+) strains, Egt(-) strains had a 59% reduction in the number of conidia produced on Vogel's agar. After storage of Egt(+) and Egt(-) conidia at 97% and 52% relative humidity (RH) for a time course to either 17 or 98 days, respectively, Egt(-) strains had a 23% and a 18% reduction in life expectancy at 97% and 52% RH, respectively, compared to the Egt(+) strains. Based on a Cu(II) reduction assay with the chelator bathocuproinedisulfonic acid disodium salt, ergothioneine accounts for 38% and 33% of water-soluble antioxidant capacity in N. crassa conidia from seven and 20 day-old cultures, respectively. In contrast, ergothioneine did not account for significant (α=0.05) anti-oxidant capacity in mycelia, which have lower concentrations of ergothioneine than conidia. The data are consistent with the hypothesis that ergothioneine has an antioxidant function in vivo. In contrast, experiments on the spontaneous mutation rate in Egt(+) and Egt(-) strains and on the effects of 254 nm UV light on mutation rate and conidial viability do not support the hypothesis that ergothioneine protects DNA in vivo.
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