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Developing transgenic wheat to encounter rusts and powdery mildew by overexpressing barley chi26 gene for fungal resistance

Plant Methods. 2018; 
Hala F. Eissa, Sameh E. Hassanien, Ahmed M. Ramadan, Moustafa M. El‑Shamy, Osama M. Saleh, Ahmed M. Shokry, Mohamed Abdelsattar, Yasser B. Morsy, Maher A. El‑Maghraby, Hussien F. Alameldin, Sabah M. Hassan, Gamal H. Osman, Hesham T. Mahfouz, Gharib A. Gad El‑Karim, Magdy A. Madkour and Ahmed Bahieldin
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Gene Synthesis The expression of chi26 gene was also tested for transgenic lines for T3–T9 generations. For each sample, 2 µg of total RNA was used to synthesize first strand cDNA with oligo(dT) using Revert Aid Premium Reverse Transcriptase (Thermo Scientific™ cat. no. EP0451), and chi2 gene-specific primers (designed by GenScript Real-time PCR Primer Design, www.genscript.com/ssl-bin/app/ primer) (Additional file 2: Table S2). Get A Quote

摘要

Background: The main aim of this study was to improve fungal resistance in bread wheat via transgenesis. Trans‑ genic wheat plants harboring barley chitinase (chi26) gene, driven by maize ubi promoter, were obtained using biolistic bombardment, whereas the herbicide resistance gene, bar, driven by the CaMV 35S promoter was used as a selectable marker. Results: Molecular analysis confirmed the integration, copy number, and the level of expression of the chi26 gene in four independent transgenic events. Chitinase enzyme activity was detected using a standard enzymatic assay. The expression levels of chi26 gene in the different transgenic lines, compared to their respective controls, were deter‑ mined using qR... More

关键词

Transgenesis, Southern, qPCR, Chitinase activity, qRT‑PCR, Substantial equivalence