12 research outputs found
Breeding oat for resistance to the crown rust pathogen Puccinia coronata f. sp. avenae: achievements and prospects
Crown rust, caused by Puccinia coronata f. sp. avenae (Pca), is a significant impediment to global oat production. Some 98 alleles at 92 loci conferring resistance to Pca in Avena have been designated; however, allelic relationships and chromosomal locations of many of these are unknown. Long-term monitoring of Pca in Australia, North America and elsewhere has shown that it is highly variable even in the absence of sexual recombination, likely due to large pathogen populations that cycle between wild oat communities and oat crops. Efforts to develop cultivars with genetic resistance to Pca began in the 1950s. Based almost solely on all all-stage resistance, this has had temporary benefits but very limited success. The inability to eradicate wild oats, and their common occurrence in many oat growing regions, means that future strategies to control Pca must be based on the assumption of a large and variable prevailing pathogen population with high evolutionary potential, even if cultivars with durable resistance are deployed and grown widely. The presence of minor gene, additive APR to Pca in hexaploid oat germplasm opens the possibility of pyramiding several such genes to give high levels of resistance. The recent availability of reference genomes for diploid and hexaploid oat will undoubtedly accelerate efforts to discover, characterise and develop high throughput diagnostic markers to introgress and pyramid resistance to Pca in high yielding adapted oat germplasm.Financial support from Judith and David Coffey and family, the Grains Research and Development Corporation (GRDC: DAS00133, UOS1707-003RTX, UOS2104-001RTX) and the University of Sydney is gratefully acknowledged. Some of the unpublished research reported on was undertaken as part of a long running program on national cereal rust surveillance, conducted at the University of Sydney since 1921. EP is funded by Spanish Ministry of Science and Innovation [PID2019-104518RB-100], (AEI/FEDER, UE) and regional government through the AGR-253 group, the European Regional and Social Development Funds.Peer reviewe
Zr贸偶nicowanie genetyczne dzikich i uprawnych form rumianku przy wykorzystaniu marker贸w ISSR
Chamomilla recutita (L.) Rausch. is a wide known herbal plant which has many medical attributes and find applications in pharmacy, nutritional and sanitary industries. Estimating genetic diversity in population is very important to protect variety of chamomile species. The objective of this study was characterization of chamomile germplasm using ISSR markers. Among 20 screened ISSR primers, only 5 produced polymorphic and repeatable fragments. In total primers produced 48 fragments out of which 41 (85.4%) were polymorphic. The average PIC value for the amplification products was 0.340. Based on ISSR markers the genetic similarity matrices were produced. The mean genetic similarity was calculated at 0.653. Present study demonstrated that ISSR markers provided a practical and effective method to evaluate the genetic similarity and relationships of chamomile genotypes. Analyzed chamomile genotypes were characterized by quite high genetic similarity; it suggested that there is necessity to find new sources of genetic diversity in chamomile in wild populations.Celem przeprowadzonych bada艅 by艂a charakterystyka genotyp贸w rumianku wykorzystuj膮c markery ISSR. Spo艣r贸d 20 testowanych starter贸w ISSR jedynie 5 inicjowa艂o amplifikacj臋 polimorficznych i powtarzalnych produkt贸w. 艁膮cznie uzyskano 48 fragment贸w, z kt贸rych 41 (85,4%) by艂o polimorficznych. 艣rednia warto艣膰 PIC dla uzyskanych produkt贸w amplifikacji wynosi艂a 0,340. Wykorzystuj膮c markery ISSR, utworzono matryce podobie艅stwa genetycznego. 艣rednia warto艣膰 podobie艅stwa analizowanych genotyp贸w wynosi艂a 0,653. Przeprowadzone badania potwierdzaj膮 przydatno艣膰 metody ISSR do oceny podobie艅stwa genetycznego rumianku. Analizowane genotypy charakteryzowa艂y si臋 wysokim podobie艅stwem genetycznym, co wskazuje na konieczno艣膰 poszukiwania nowych 藕r贸de艂 polimorfizmu w艣r贸d dzikich gatunk贸w, w celu poszerzenia zmienno艣ci genetycznej uprawnych form rumianku
Analiza zr贸偶nicowania genetycznego w艣r贸d genotyp贸w Arnica montana L. za pomoc膮 marker贸w RAPD
Arnica montana L. is one of the most important herbal plants used in medicine, pharmaceutical and cosmetic industry. The number of studies performed with molecular markers on arnica genotypes is very limited. Because of this fact the aims of presented examination were optimization of protocols DNA isolation from fresh leaves of A. montana and identification of genetic diversity among this plant genotypes. In presented study to obtain pure DNA Plant & Fungi DNA Purification Kit (EURx) were used. To clean obtained DNA long and slow electrophoresis and isolation DNA from gels were used. A. montana genotypes were analyzed using 40 RAPD primers (Operon Technologies), out of which 12 produced high number of polymorphic and repeatable fragments. In total, selected primers produced 120 fragments, among them 111 (92.5%) were polymorphic. The genetic similarity matrices were produced based on RAPD using the Dice鈥檚 coefficient. RAPD based genetic similarity was estimated between 0.535 and 0.945. The highest genetic similarity was estimated among GA17 and GA18 genotypes, which are closely located on the obtained dendrogramme.Arnica montana L. jest jedn膮 z najcenniejszych ro艣lin zielarskich wykorzystywanych w medycynie, farmacji i przemy艣le kosmetycznym. W dost臋pnej literaturze liczba doniesie艅 zwi膮zanych z analiz膮 molekularn膮 arniki jest znikoma, dlatego te偶 celem prezentowanych bada艅 by艂a optymalizacja procesu izolacji DNA ze 艣wie偶ych li艣ci oraz identyfikacja zr贸偶nicowania genetycznego oparta na markerach RAPD. W prezentowanej pracy w celu uzyskania czystego DNA do izolacji wykorzystano zestaw DNA Plant & Fungi DNA Purification Kit (Euro) oraz oczyszczanie za pomoc膮 d艂ugiej elektroforezy w 偶elu agarozowym. Spo艣r贸d testowanych 40 starter贸w RPAD do analiz wybrano 12 generuj膮cych stabilne i polimorficzne wzory pr膮偶k贸w. Wyselekcjonowane startery amplifikowa艂y 120 fragment贸w, spo艣r贸d kt贸rych 111 (92,5%) by艂o polimorficznych. Wykorzystujac markery RAPD utworzono matryce podobie艅stwa genetycznego. 艣rednia warto艣膰 podobie艅stwa analizowanych genotyp贸w wynosi艂a 0.886. Najwy偶szy wsp贸艂czynnik podobie艅stwa genetycznego oszacowano pomi臋dzy genotypami GA17 i GA18, kt贸re ulokowa艂y si臋 blisko siebie na uzyskanym dendrogramie