ABSTRACT
Apple scab, caused by Venturia inaequalis, is a major fungal disease worldwide. Cultivation of scab-resistant cultivars would reduce the chemical footprint of apple production. However, new apple cultivars carrying durable resistances should be developed to prevent or at least slow the breakdown of resistance against races of V. inaequalis. One way to achieve durable resistance is to pyramid multiple scab resistance genes in a cultivar. The choice of the resistance genes to be combined in the pyramids should take into account the frequency of resistance breakdown and the geographical distribution of apple scab isolates able to cause such breakdowns. In order to acquire this information and to make it available to apple breeders, the VINQUEST project (www.vinquest.ch) was initiated in 2009. Ten years after launching this project, 24 partners from 14 countries regularly contribute data. From 2009 to 2018, nearly 9,000 data points have been collected. This information has been used to identify the most promising apple scab resistance genes for developing cultivars with durable resistance, which to date are: Rvi5, Rvi11, Rvi12, Rvi14, and Rvi15. As expected, Rvi1, together with Rvi3 and Rvi8, were often overcome, and have little value for scab resistance breeding. Rvi10 may also belong to this group. On the other hand, Rvi2, Rvi4, Rvi6, Rvi7, Rvi9, and Rvi13 are still useful for breeding, but their use is recommended only in extended pyramids of ≥3 resistance genes.
Subject(s)
Ascomycota , Malus/genetics , Breeding , Genes, Plant , Plant DiseasesABSTRACT
Blumeria graminis f. sp. tritici (B.g. tritici) is the causal agent of the wheat powdery mildew disease. The highly fragmented B.g. tritici genome available so far has prevented a systematic analysis of effector genes that are known to be involved in host adaptation. To study the diversity and evolution of effector genes we produced a chromosome-scale assembly of the B.g. tritici genome. The genome assembly and annotation was achieved by combining long-read sequencing with high-density genetic mapping, bacterial artificial chromosome fingerprinting and transcriptomics. We found that the 166.6 Mb B.g. tritici genome encodes 844 candidate effector genes, over 40% more than previously reported. Candidate effector genes have characteristic local genomic organization such as gene clustering and enrichment for recombination-active regions and certain transposable element families. A large group of 412 candidate effector genes shows high plasticity in terms of copy number variation in a global set of 36 isolates and of transcription levels. Our data suggest that copy number variation and transcriptional flexibility are the main drivers for adaptation in B.g. tritici. The high repeat content may play a role in providing a genomic environment that allows rapid evolution of effector genes with selection as the driving force.
Subject(s)
Ascomycota/genetics , Chromosomes, Fungal/genetics , Genome, Fungal , Triticum/microbiology , Chromosome Mapping , DNA Copy Number Variations/genetics , DNA Transposable Elements/genetics , Gene Expression Regulation, Fungal , Genes, Fungal , Multigene Family , Polymorphism, Genetic , Recombination, Genetic/genetics , Transcription, GeneticABSTRACT
The commonly applied method for the examination of self-adhesive stamps mainly focuses on DNA-profiling while neglecting potential fingerprint evidence. In our preliminary study it was shown that in an uncontrolled environment, fingerprints are transferred from the adhesive side of stamps onto the envelope within the first two days after application. Fingerprints can therefore be examined independently after the separation of the stamp from the envelope. The aim of this study was to develop a novel approach, which enables the combination of fingerprint development and the analysis of DNA traces originating from the same evidence, and to implement this into routine processes. Furthermore, this approach was compared with the edge fragment approach, the commonly applied standard method in our laboratory. The results showed that the novel approach is very beneficial for forensic examination of self-adhesive postage stamps on letters. Moreover, it enables parallel evaluation of dactyloscopic and DNA evidence without having an increased risk of contamination, PCR interference or altering of the fingerprint. The chance of obtaining useful forensic evidence for downstream database searching was increased from 50.0% to 83.3%. This novel method was shown to be valuable for the parallel evaluation of dactyloscopic and DNA trace material originating from the same evidence.
Subject(s)
Dermatoglyphics , Resin Cements , Adhesives , DNA , DNA FingerprintingABSTRACT
Cross-kingdom RNA interference (RNAi) is a biological process allowing plants to transfer small regulatory RNAs to invading pathogens to trigger the silencing of target virulence genes. Transient assays in cereal powdery mildews suggest that silencing of one or two effectors could lead to near loss of virulence, but evidence from stable RNAi lines is lacking. We established transient host-induced gene silencing (HIGS) in wheat, and demonstrate that targeting an essential housekeeping gene in the wheat powdery mildew pathogen (Blumeria graminis f. sp. tritici) results in significant reduction of virulence at an early stage of infection. We generated stable transgenic RNAi wheat lines encoding a HIGS construct simultaneously silencing three B.g. tritici effectors including SvrPm3 a1/f1 , a virulence factor involved in the suppression of the Pm3 powdery mildew resistance gene. We show that all targeted effectors are effectively downregulated by HIGS, resulting in reduced fungal virulence on adult wheat plants. Our findings demonstrate that stable HIGS of effector genes can lead to quantitative gain of resistance without major pleiotropic effects in wheat.