Genetic transformation of Persian melon (Cucumis melo L.) via Agrobacterium
عنوان مقاله: Genetic transformation of Persian melon (Cucumis melo L.) via Agrobacterium
شناسه ملی مقاله: JR_IJGPB-12-1_002
منتشر شده در در سال 1402
شناسه ملی مقاله: JR_IJGPB-12-1_002
منتشر شده در در سال 1402
مشخصات نویسندگان مقاله:
داود نادری - Department of Horticulture, Isfahan (Khorasgan) Branch, Islamic Azad University, Isfahan, Iran.
امیر موسوی - Department of Plant Molecular Biotechnology, National Institute of Genetic Engineering and Biotechnology, Tehran, Iran.
محمود لطفی - Department of Horticulture, College of Aburaihan, University of Tehran, Pakdasht, Tehran, Iran.
خلاصه مقاله:
داود نادری - Department of Horticulture, Isfahan (Khorasgan) Branch, Islamic Azad University, Isfahan, Iran.
امیر موسوی - Department of Plant Molecular Biotechnology, National Institute of Genetic Engineering and Biotechnology, Tehran, Iran.
محمود لطفی - Department of Horticulture, College of Aburaihan, University of Tehran, Pakdasht, Tehran, Iran.
A reliable Agrobacterium-mediated transformation and regeneration protocol was developed for commercially important endemic Persian melon cultigens (Cucumis melo L.) comprising ‘Eyvanaki’, ‘Samsoori’, and ‘Khatooni’. The effect of selective Murashige and Skoog (MS) medium containing various concentrations of ۶-benzyl adenine (BA) (۰, ۰.۵, ۱, and ۱.۵ mg l-۱) and ۱ mg l-۱ Gibberellic acid (GA۳) on regeneration of cotyledon, hypocotyl, and cotyledonary petioles derived from ۶-day-old in vitro grown seedlings of the three Persian melons were investigated. For transformation, the sensitivity to kanamycin (Km) concentrations (۰, ۵۰, ۷۵, ۱۰۰, ۱۲۵ mg l-۱ ), the effect of three A. tumefaciens strains (GV۳۱۰۳, LBA۴۴۰۴, and AGL۰), inoculation time (۰.۵, ۱, ۵, and ۳۰ min), and co-cultivation time (۲۴, ۴۸, and ۷۲ h) on direct shoot regeneration of cotyledonary petiole of ‘Samsoori’ were investigated. Shoot regeneration from cotyledonary petiole explants received the highest attention. Cotyledonary petiole segments of ‘Samsoori’ and ‘Khatooni’ treated respectively with ۱.۰ mg l-۱ and ۱.۵ mg l-۱ BA exhibited the highest potential for shoot multiplication; while the regeneration rate of ‘Eyvanaki’ was drastically lower. Putative transgenic ‘Samsoori’ plantlets selected in ۱۰۰ mg l-۱ Km were subcultured on elongation MS medium composed of ۱۰۰ mg l-۱ Km, ۰.۱ mg l-۱ BA, ۱ mg l-۱ GA۳ plus ۴۰۰ mg l-۱ CTX, and then successfully rooted on growth regulator-free MS medium for two weeks. Using histochemical GUS assay along with genomic PCR screening for GusA and VirG genes, the efficiency of transformation was estimated to be ۱۰% for AGL۰ and ۶% in LBA۴۴۰۴.
کلمات کلیدی: AGL۰, Cucumis melo, Multiple buds, organogenesis, Reporter genes, Transgenic plant
صفحه اختصاصی مقاله و دریافت فایل کامل: https://civilica.com/doc/1950189/