Panax notoginseng transcription factor WRKY15 modulates resistance to Fusarium solani by up-regulating osmotin-like protein expression and inducing JA/SA signaling pathways

Linlin Su; Lilei Zheng; Hanlin Wang; Yuan Qu; Feng Ge; Diqiu Liu

doi:10.1186/s12870-023-04373-x

Panax notoginseng transcription factor WRKY15 modulates resistance to Fusarium solani by up-regulating osmotin-like protein expression and inducing JA/SA signaling pathways

BMC Plant Biol. 2023 Jul 17;23(1):362. doi: 10.1186/s12870-023-04373-x.

Authors

Linlin Su^#^{1

2}, Lilei Zheng^#^{1

2}, Hanlin Wang^{1

2}, Yuan Qu^{1

2}, Feng Ge^{1

2}, Diqiu Liu^{3

4}

Affiliations

¹ Faculty of Life Science and Technology, Kunming University of Science and Technology, Kunming, 650500, Yunnan, China.
² Yunnan Provincial Key Laboratory of Panax notoginseng, Kunming, 650500, Yunnan, China.
³ Faculty of Life Science and Technology, Kunming University of Science and Technology, Kunming, 650500, Yunnan, China. Diqiuliu@126.com.
⁴ Yunnan Provincial Key Laboratory of Panax notoginseng, Kunming, 650500, Yunnan, China. Diqiuliu@126.com.

^# Contributed equally.

Abstract

Background: Panax notoginseng (Burk) F. H. Chen is a valuable traditional Chinese medicinal plant, but its commercial production is seriously affected by root rot caused by some pathogenic fungi, including Fusarium solani. Nevertheless, the genetic breeding for disease resistance of P. notoginseng remains limited. The WRKY transcription factors have been revealed to play important roles in plant defense responses, which might provide an inspiration for resistance improvement in P. notoginseng.

Results: In this study, the regulatory mechanism of transcription factor PnWRKY15 on P. notoginseng resistance to F. solani infection was revealed. The suppressed expression of PnWRKY15 via RNA interference increased the sensitivity of P. notoginseng to F. solani and decreased the expression levels of some defense-related genes, including PnOLP1, which encodes an osmotin-like protein that confers resistance to F. solani. Ectopic expression of PnWRKY15 in the model plant tobacco significantly enhanced the resistance to F. solani. Moreover, the transcriptome sequencing analysis discovered that some pathogenesis-related genes were expressed at higher levels in the PnWRKY15-overexpressing tobacco than that in the wild-type tobacco. In addition, the jasmonic acid (JA) and salicylic acid (SA) signaling pathways were evidently induced by PnWRKY15-overexpression, that was evidenced by that the JA and SA contents were significantly higher in the PnWRKY15-overexpressing tobacco than that in the wild-type. Furthermore, PnWRKY15, which was localized in the nucleus, can trans-activate and up-regulate PnOLP1 expression according to the EMSA, yeast one-hybrid and co-expression assays.

Conclusions: PnWRKY15 contributes to P. notoginseng resistance to F. solani by up-regulating the expression of resistance-related gene PnOLP1 and activating JA/SA signaling pathways. These findings will help to further elucidate the transcriptional regulatory mechanism associated with the P. notoginseng defense response to F. solani.

Keywords: Fusarium solani; Jasmonic acid; Osmotin; Panax notoginseng; Salicylic acid; WRKY transcription factor.

MeSH terms

Fusarium* / metabolism
Gene Expression Regulation, Plant
Panax notoginseng* / genetics
Plant Breeding
Plant Diseases / genetics
Plant Diseases / microbiology
Salicylic Acid / metabolism
Signal Transduction
Transcription Factors / genetics
Transcription Factors / metabolism

Panax notoginseng transcription factor WRKY15 modulates resistance to Fusarium solani by up-regulating osmotin-like protein expression and inducing JA/SA signaling pathways

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