Biotechnology Bulletin ›› 2026, Vol. 42 ›› Issue (2): 338-350.doi: 10.13560/j.cnki.biotech.bull.1985.2025-0603
SUN Yan-sen1(
), WEI Li-xiang1, LI Ruo-bing1, ZHANG Cheng-zhi1, NIE Yu-hang1, LI Jie1, CAI Xue-peng2, QIAO Jun1, MENG Qing-ling1(
)
Received:2025-06-12
Online:2026-02-26
Published:2026-03-17
Contact:
MENG Qing-ling
E-mail:763203488@qq.com;xjmqlqj@163.com
SUN Yan-sen, WEI Li-xiang, LI Ruo-bing, ZHANG Cheng-zhi, NIE Yu-hang, LI Jie, CAI Xue-peng, QIAO Jun, MENG Qing-ling. Regulatory Roles of Transcription Factor AOL-113 in Mycelial Growth, Stress Response, and Predatory Ability of Arthrobotrys oligospora[J]. Biotechnology Bulletin, 2026, 42(2): 338-350.
引物名称 Primer name | 引物序列 Primer sequence (5′-3′) | 长度 Length (bp) | 基因目的 Gene description |
|---|---|---|---|
| AOL-113-F/AOL-113-R | ATGTCGTTGAAACGGTCG/GTCATTCCAGCTTGATAGAACCG | 3 213 | AOL-113基因全长 |
| AOL-113-5F-pUC19 | 1 861 | AOL-113基因5′端基因序列 | |
| AOL-113-5R-HygR | |||
| HygR-F-113-5R | 1 441 | 潮霉素抗性基因 | |
| HygR-R-113-3F | |||
| AOL-113-3F-HygR | 1 865 | AOL-113基因3′端基因序列 | |
| AOL-113-3R-pUC19 | |||
| CΔ AOL-113-5F-pUC19 | 3 482 | CΔ AOL-113基因回补全长及5′端侧翼序列 | |
| CΔ AOL-113-5R-NeoR | |||
| NeoR-F-113-5R | 919 | G-418抗性基因 | |
| NeoR-R-113-3F | |||
| CΔ AOL-113-3F-pUC19 | 1 382 | CΔ AOL-113 3′端基因序列 | |
| CΔ AOL-113-3R-pUC19 | |||
| Δ AOL-113YZ-F/Δ AOL-113YZ-R | GTATACTTACCAACCTGCTCC/ GCTACTTCCTGATGATATCCTTC | 3 827/2 209 | 野生型和缺失转化子菌株的验证 |
| CΔ AOL-113YZ-F/CΔ AOL-113YZ-R | CTTCCTCTTCAATTCCTCTTACAAGG/ GGTCATGGTGAAGGATATACTTGT | 3 445/2 301 | 回补株转化子菌株的验证 |
Table 1 Specific primers used in the study
引物名称 Primer name | 引物序列 Primer sequence (5′-3′) | 长度 Length (bp) | 基因目的 Gene description |
|---|---|---|---|
| AOL-113-F/AOL-113-R | ATGTCGTTGAAACGGTCG/GTCATTCCAGCTTGATAGAACCG | 3 213 | AOL-113基因全长 |
| AOL-113-5F-pUC19 | 1 861 | AOL-113基因5′端基因序列 | |
| AOL-113-5R-HygR | |||
| HygR-F-113-5R | 1 441 | 潮霉素抗性基因 | |
| HygR-R-113-3F | |||
| AOL-113-3F-HygR | 1 865 | AOL-113基因3′端基因序列 | |
| AOL-113-3R-pUC19 | |||
| CΔ AOL-113-5F-pUC19 | 3 482 | CΔ AOL-113基因回补全长及5′端侧翼序列 | |
| CΔ AOL-113-5R-NeoR | |||
| NeoR-F-113-5R | 919 | G-418抗性基因 | |
| NeoR-R-113-3F | |||
| CΔ AOL-113-3F-pUC19 | 1 382 | CΔ AOL-113 3′端基因序列 | |
| CΔ AOL-113-3R-pUC19 | |||
| Δ AOL-113YZ-F/Δ AOL-113YZ-R | GTATACTTACCAACCTGCTCC/ GCTACTTCCTGATGATATCCTTC | 3 827/2 209 | 野生型和缺失转化子菌株的验证 |
| CΔ AOL-113YZ-F/CΔ AOL-113YZ-R | CTTCCTCTTCAATTCCTCTTACAAGG/ GGTCATGGTGAAGGATATACTTGT | 3 445/2 301 | 回补株转化子菌株的验证 |
Fig. 1 Molecular characteristics and phylogenetic analysis of the Zn2(II)Cys6-type transcription factor AOL-113 of A. oligosporaA: Domain characteristic of transcription factor AOL-113. B: Phylogenetic analysis of different fungi based on transcription factor AOL-113orthologs
Fig. 2 Construction and screening of deletion strains and complementary strainsA: Electrophoresis detection results of deletion strains. M: DL-5000 DNA marker; 1: negative control; 2-3: positive clones of deletion strains. B: Electrophoresis detection results of complementary strains. M: DL-5000 DNA marker; 1: positive clones of complementary strains; 2-4: negative control
Fig. 3 Comparison of growth rate and mycelial cell lengthA: TG, YPSSA, TYGA, PDA and CMY media were incubated at 28 ℃ for 5 d for colony morphology observation and growth rate measurement. B: CFW staining of mycelia. Scale = 20 μm, the hyphal septa are denoted by white arrows. *P<0.05, **P<0.01. The same below
Fig. 6 Comparison of sporulation rate, spore germination rate and fluorescence observation of conidiaA: Side view of the phloem peduncle. B: Determination of sporulation rate. C: Spore germination rate. D: Observation of conidial germination. E: Fluorescence observation of conidia and spore length determination
Fig. 7 Comparison of the trap formation and predatory abilityA: Trap formation and traps counts at different time points. B: Observations of nematode predation and determination of predation rate
Fig. 8 Analysis of DEGs between WT and Δ AOL-113 of Arthrobotrys oligospora exposed to sodium acetate (SA)A: Volcano plot of DEGs. Up-regulated DEGs in red; down-regulated DEGs in blue. B: GO enrichment analysis of downregulated DEGs. C: KEGG enrichment analysis of downregulated DEGs. D: Validation of transcriptomic sequencing using RT-qPCR
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