The PKS–NRPS Gene <i>BBA_09856</i> Deletion Mutant of <i>Beauveria bassiana</i> Enhanced Its Virulence Against <i>Ostrinia furnacalis</i> Larvae and Strengthened the Host Plant’s Resistance to <i>Botrytis cinerea</i> as an Endotype

The PKS–NRPS Gene <i>BBA_09856</i> Deletion Mutant of <i>Beauveria bassiana</i> Enhanced Its Virulence Against <i>Ostrinia furnacalis</i> Larvae and Strengthened the Host Plant’s Resistance to <i>Botrytis cinerea</i> as an Endotype

Nonribosomal peptide synthetase (NRPS) and polyketide synthase (PKS) play crucial roles in the development and pathogenicity of the entomopathogenic fungus <i>Beauveria bassiana</i>. However, they are among the few biosynthetic gene clusters with unknown functions in <i>B. bassiana...

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Main Authors: Yanan Wang, Xiaowei Zou, Xiaomin Zhu, Ji Qi, Jianfeng Liu, Zhengkun Zhang
Format: Article
Language:English
Published: MDPI AG 2025-03-01
Series:Journal of Fungi
Subjects:
<i>Beauveria bassiana</i>
entomopathogenic fungi
nonribosomal peptide synthetase
polyketide synthase
mycoinsecticides
Online Access:https://www.mdpi.com/2309-608X/11/3/197
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author Yanan Wang
Xiaowei Zou
Xiaomin Zhu
Ji Qi
Jianfeng Liu
Zhengkun Zhang
author_facet Yanan Wang
Xiaowei Zou
Xiaomin Zhu
Ji Qi
Jianfeng Liu
Zhengkun Zhang
author_sort Yanan Wang
collection DOAJ
description Nonribosomal peptide synthetase (NRPS) and polyketide synthase (PKS) play crucial roles in the development and pathogenicity of the entomopathogenic fungus <i>Beauveria bassiana</i>. However, they are among the few biosynthetic gene clusters with unknown functions in <i>B. bassiana</i>. To investigate the role of the hybrid PKS–NRPS synthetase gene <i>BBA_09856</i> in <i>B. bassiana</i>, we constructed a mutant strain, ∆<i>BBA09856</i>-WT, by deleting the <i>BBA_09856</i> gene through Agrobacterium-mediated transformation. We then analyzed the biological characteristics of the mutant strain and the virulence of the mutant strain toward <i>Ostrinia furnacalis</i> larvae, as well as its antagonistic effects against the phytopathogen <i>Botrytis cinerea</i>. We found that the average growth rate of the three mutant strains, ∆<i>BBA09856</i>-WT, was significantly higher compared to the wild-type (WT) strain on the 15th day of culture on potato dextrose agar (PDA) plates (7.01 cm vs. 6.30 cm, <i>p</i> < 0.01). Additionally, the average spore production(3.16 × 10<sup>7</sup>/cm<sup>2</sup> vs. 9.95 × 10<sup>6</sup>/cm<sup>2</sup>, <i>p</i> < 0.001) and germination rate (82.50% vs. 54.72%, 12 h, <i>p</i> < 0.001) were significantly different between the three mutant strains, ∆<i>BBA09856</i>-WT, and the WT strain. The average survival rates of <i>O. furnacalis</i> infected with the WT strain and the three mutant strains, ∆<i>BBA09856</i>-WT, after 8 days were 61.66%, and 30.00%, respectively, indicating that the pathogenicity of the tested mutant strains was significantly greater than that of the WT strain. The results of the dual culture test indicated that the inhibitory rates of the WT and ∆<i>BBA09856</i>-WT strains against <i>B. cinerea</i> were 40.25% and 47.65%, respectively (<i>p</i> < 0.001). Similarly, in the dual culture test, the WT strain reduced the growth of <i>B. cinerea</i> by 9.90%, while the ∆<i>BBA09856</i>-WT exhibited a significantly greater inhibition rate of 28.29% (<i>p</i> < 0.05). The diameters of disease spots, measured 6 d after inoculation with <i>B. cinerea</i> in the tomato treatment groups, revealed significant differences in endophytic colonization between the WT and ∆<i>BBA09856</i>-WT strains in the WT+Bc and ∆<i>BBA09856</i>-WT+Bc treatment groups (15.26 mm vs. 12.16 mm, <i>p</i> < 0.01). Notably, ∆<i>BBA09856</i>-WT exhibited enhanced virulence toward <i>O. furnacalis</i> larvae and increased antagonistic activity against <i>B. cinerea</i>. Our results indicate that the gene <i>BBA_09856</i> may have a negative correlation with the development and virulence of <i>B. bassiana</i> toward the insect pest <i>O. furnacalis</i> larvae, as well as its antagonism against <i>B. cinerea</i>. These findings suggest that molecular techniques, such as gene editing, could be employed to develop superior strains of <i>B. bassiana</i> for the biological control of plant diseases and insect pests.
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spelling doaj-art-c1811109c8cf4f09ad8fe508316b21ea2025-08-20T01:48:46ZengMDPI AGJournal of Fungi2309-608X2025-03-0111319710.3390/jof11030197The PKS–NRPS Gene <i>BBA_09856</i> Deletion Mutant of <i>Beauveria bassiana</i> Enhanced Its Virulence Against <i>Ostrinia furnacalis</i> Larvae and Strengthened the Host Plant’s Resistance to <i>Botrytis cinerea</i> as an EndotypeYanan Wang0Xiaowei Zou1Xiaomin Zhu2Ji Qi3Jianfeng Liu4Zhengkun Zhang5College of Life Sciences, Jilin Normal University, Siping 136000, ChinaKey Laboratory of Integrated Pest Management on Crops in Northeast China, Ministry of Agriculture and Rural Affairs, Institute of Plant Protection, Jilin Academy of Agricultural Sciences, Changchun 130033, ChinaKey Laboratory of Integrated Pest Management on Crops in Northeast China, Ministry of Agriculture and Rural Affairs, Institute of Plant Protection, Jilin Academy of Agricultural Sciences, Changchun 130033, ChinaCollege of Life Sciences, Jilin Normal University, Siping 136000, ChinaCollege of Life Sciences, Jilin Normal University, Siping 136000, ChinaKey Laboratory of Integrated Pest Management on Crops in Northeast China, Ministry of Agriculture and Rural Affairs, Institute of Plant Protection, Jilin Academy of Agricultural Sciences, Changchun 130033, ChinaNonribosomal peptide synthetase (NRPS) and polyketide synthase (PKS) play crucial roles in the development and pathogenicity of the entomopathogenic fungus <i>Beauveria bassiana</i>. However, they are among the few biosynthetic gene clusters with unknown functions in <i>B. bassiana</i>. To investigate the role of the hybrid PKS–NRPS synthetase gene <i>BBA_09856</i> in <i>B. bassiana</i>, we constructed a mutant strain, ∆<i>BBA09856</i>-WT, by deleting the <i>BBA_09856</i> gene through Agrobacterium-mediated transformation. We then analyzed the biological characteristics of the mutant strain and the virulence of the mutant strain toward <i>Ostrinia furnacalis</i> larvae, as well as its antagonistic effects against the phytopathogen <i>Botrytis cinerea</i>. We found that the average growth rate of the three mutant strains, ∆<i>BBA09856</i>-WT, was significantly higher compared to the wild-type (WT) strain on the 15th day of culture on potato dextrose agar (PDA) plates (7.01 cm vs. 6.30 cm, <i>p</i> < 0.01). Additionally, the average spore production(3.16 × 10<sup>7</sup>/cm<sup>2</sup> vs. 9.95 × 10<sup>6</sup>/cm<sup>2</sup>, <i>p</i> < 0.001) and germination rate (82.50% vs. 54.72%, 12 h, <i>p</i> < 0.001) were significantly different between the three mutant strains, ∆<i>BBA09856</i>-WT, and the WT strain. The average survival rates of <i>O. furnacalis</i> infected with the WT strain and the three mutant strains, ∆<i>BBA09856</i>-WT, after 8 days were 61.66%, and 30.00%, respectively, indicating that the pathogenicity of the tested mutant strains was significantly greater than that of the WT strain. The results of the dual culture test indicated that the inhibitory rates of the WT and ∆<i>BBA09856</i>-WT strains against <i>B. cinerea</i> were 40.25% and 47.65%, respectively (<i>p</i> < 0.001). Similarly, in the dual culture test, the WT strain reduced the growth of <i>B. cinerea</i> by 9.90%, while the ∆<i>BBA09856</i>-WT exhibited a significantly greater inhibition rate of 28.29% (<i>p</i> < 0.05). The diameters of disease spots, measured 6 d after inoculation with <i>B. cinerea</i> in the tomato treatment groups, revealed significant differences in endophytic colonization between the WT and ∆<i>BBA09856</i>-WT strains in the WT+Bc and ∆<i>BBA09856</i>-WT+Bc treatment groups (15.26 mm vs. 12.16 mm, <i>p</i> < 0.01). Notably, ∆<i>BBA09856</i>-WT exhibited enhanced virulence toward <i>O. furnacalis</i> larvae and increased antagonistic activity against <i>B. cinerea</i>. Our results indicate that the gene <i>BBA_09856</i> may have a negative correlation with the development and virulence of <i>B. bassiana</i> toward the insect pest <i>O. furnacalis</i> larvae, as well as its antagonism against <i>B. cinerea</i>. These findings suggest that molecular techniques, such as gene editing, could be employed to develop superior strains of <i>B. bassiana</i> for the biological control of plant diseases and insect pests.https://www.mdpi.com/2309-608X/11/3/197<i>Beauveria bassiana</i>entomopathogenic funginonribosomal peptide synthetasepolyketide synthasemycoinsecticides
spellingShingle Yanan Wang
Xiaowei Zou
Xiaomin Zhu
Ji Qi
Jianfeng Liu
Zhengkun Zhang
The PKS–NRPS Gene <i>BBA_09856</i> Deletion Mutant of <i>Beauveria bassiana</i> Enhanced Its Virulence Against <i>Ostrinia furnacalis</i> Larvae and Strengthened the Host Plant’s Resistance to <i>Botrytis cinerea</i> as an Endotype
Journal of Fungi
<i>Beauveria bassiana</i>
entomopathogenic fungi
nonribosomal peptide synthetase
polyketide synthase
mycoinsecticides
title The PKS–NRPS Gene <i>BBA_09856</i> Deletion Mutant of <i>Beauveria bassiana</i> Enhanced Its Virulence Against <i>Ostrinia furnacalis</i> Larvae and Strengthened the Host Plant’s Resistance to <i>Botrytis cinerea</i> as an Endotype
title_full The PKS–NRPS Gene <i>BBA_09856</i> Deletion Mutant of <i>Beauveria bassiana</i> Enhanced Its Virulence Against <i>Ostrinia furnacalis</i> Larvae and Strengthened the Host Plant’s Resistance to <i>Botrytis cinerea</i> as an Endotype
title_fullStr The PKS–NRPS Gene <i>BBA_09856</i> Deletion Mutant of <i>Beauveria bassiana</i> Enhanced Its Virulence Against <i>Ostrinia furnacalis</i> Larvae and Strengthened the Host Plant’s Resistance to <i>Botrytis cinerea</i> as an Endotype
title_full_unstemmed The PKS–NRPS Gene <i>BBA_09856</i> Deletion Mutant of <i>Beauveria bassiana</i> Enhanced Its Virulence Against <i>Ostrinia furnacalis</i> Larvae and Strengthened the Host Plant’s Resistance to <i>Botrytis cinerea</i> as an Endotype
title_short The PKS–NRPS Gene <i>BBA_09856</i> Deletion Mutant of <i>Beauveria bassiana</i> Enhanced Its Virulence Against <i>Ostrinia furnacalis</i> Larvae and Strengthened the Host Plant’s Resistance to <i>Botrytis cinerea</i> as an Endotype
title_sort pks nrps gene i bba 09856 i deletion mutant of i beauveria bassiana i enhanced its virulence against i ostrinia furnacalis i larvae and strengthened the host plant s resistance to i botrytis cinerea i as an endotype
topic <i>Beauveria bassiana</i>
entomopathogenic fungi
nonribosomal peptide synthetase
polyketide synthase
mycoinsecticides
url https://www.mdpi.com/2309-608X/11/3/197
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