Gene cloning in repeat-rich polyploid genomes remains challenging. Here, we describe a strategy for overcoming major bottlenecks in cloning of the powdery mildew resistance gene (R-gene) Pm69 derived from tetraploid wild emmer wheat. A conventional positional cloning approach was not effective owing to suppressed recombination. Chromosome sorting was compromised by insufficient purity. A Pm69 physical map, constructed by assembling Oxford Nanopore Technology (ONT) long-read genome sequences, revealed a rapidly evolving nucleotide-binding leucine-rich repeat (NLR) R-gene cluster with structural variations. A single candidate NLR was identified by anchoring RNA sequencing reads from susceptible mutants to ONT contigs and was validated by virus-induced gene silencing. Pm69 is likely a newly evolved NLR and was discovered in only one location across the wild emmer wheat distribution range in Israel. Pm69 was successfully introgressed into cultivated wheat, and a diagnostic molecular marker was used to accelerate its deployment and pyramiding with other R-genes.
Dissection of a rapidly evolving wheat resistance gene cluster by long-read genome sequencing accelerated the cloning of Pm69.
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作者:Li Yinghui, Wei Zhen-Zhen, Sela Hanan, Govta Liubov, Klymiuk Valentyna, Roychowdhury Rajib, Chawla Harmeet Singh, Ens Jennifer, Wiebe Krystalee, Bocharova Valeria, Ben-David Roi, Pawar Prerna B, Zhang Yuqi, Jaiwar Samidha, Molnár István, Doležel Jaroslav, Coaker Gitta, Pozniak Curtis J, Fahima Tzion
| 期刊: | Plant Communications | 影响因子: | 11.600 |
| 时间: | 2024 | 起止号: | 2024 Jan 8; 5(1):100646 |
| doi: | 10.1016/j.xplc.2023.100646 | ||
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