R. Gangaraj, Aditi Kundu, G. Prakash, Amrita Das, A. Nagaraja, Deeba Kamil
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In this investigation, we assessed eleven <i>A. niger</i> strains (AN-1 to AN-11) against four guava wilt pathogens (<i>Fusarium oxysporum</i> f. sp. <i>psidii</i>, <i>F. falciforme</i>, <i>F. chlamydosporum</i>, and <i>F. verticillioides</i>) using a dual culture assay. All strains demonstrated effective by restricting the mycelial growth of pathogens, among them AN-11 displayed maximum inhibition of 86.33%, followed by the AN-3 (84.27%). The UPLC-QToF-ESIMS analysis was undertaken to explore the secondary metabolites of AN-11 responsible for inhibiting <i>F. oxysporum</i> f. sp. <i>psidii.</i> The crude extracts were obtained from <i>F. oxysporum</i> f. sp. <i>psidii</i>, AN-11 and their interaction using ethyl acetate as a solvent. After evaporating, the crude fractions were analysed using UPLC-QToF-ESIMS with an Acquity UPLC and a SCIEX SelexION Triple QuadTM 5500 System. From the ethyl acetate extract of <i>F. oxysporum</i> f. sp. <i>psidii</i>, approximately 14 metabolites involved in pathogenicity were identified. Similarly, analysis of AN-11 crude extract revealed 25 metabolites, and notably, 41 metabolites were identified during the interaction between AN-11 and <i>F. oxysporum</i> f. sp. <i>psidii</i>, including kotanin, isokotanin A, aurofusarin, kojic acid, pyranonigrin, aurasperone F, hexylitaconic acid, asperazine, bicoumanigrin, chloramphenicol, cephalosporin C, fusarin C, zearalonone, fonsecin B, malformin A, and others. Among these, 21 metabolites were produced only during the interaction and have antimicrobial properties. This study highlights the significant potential of the AN-11 strain in generating a diverse array of non-volatile secondary metabolites with antimicrobial properties. 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引用次数: 0
摘要
番石榴枯萎病是一种毁灭性的土传病害,会给番石榴果园造成重大损失。这种病害一旦在田间发生,管理起来就非常具有挑战性。因此,有必要探索一种有效、经济、可持续的管理策略。黑曲霉是一种生物防治真菌,已被证明对包括番石榴枯萎病病原体在内的各种土传病原体有效。它能产生多种水解酶和次级代谢产物。然而,目前还没有对黑僵菌的次级代谢产物进行广泛研究。在这项研究中,我们使用双重培养试验评估了 11 株黑僵菌菌株(AN-1 至 AN-11)对四种番石榴枯萎病病原体(Fusarium oxysporum f. sp. psidii、F. falciforme、F. chlamydosporum 和 F. verticillioides)的抗性。所有菌株都能有效限制病原体的菌丝生长,其中 AN-11 的抑制率最高,达 86.33%,其次是 AN-3(84.27%)。通过 UPLC-QToF-ESIMS 分析,研究了 AN-11 抑制 F. oxysporum f. sp. psidii 的次生代谢物。以乙酸乙酯为溶剂,从 F. oxysporum f. sp. psidii、AN-11 及其交互作用中提取粗提物。蒸发后,使用 Acquity UPLC 和 SCIEX SelexION Triple QuadTM 5500 系统进行 UPLC-QToF-ESIMS 分析。从 F. oxysporum f. sp. psidii 的乙酸乙酯提取物中鉴定出了约 14 种与致病性有关的代谢物。同样,对 AN-11 粗提取物的分析也发现了 25 种代谢物,值得注意的是,在 AN-11 与 F. oxysporum f. sp.在 AN-11 与 F oxysporum f. sp. psidii 的相互作用过程中,共鉴定出 41 种代谢物,包括柯坦宁、异柯坦宁 A、乌洛托品、麴酸、吡喃尼格林、欧拉司酮 F、己基硝酸、天冬酰胺、双库马尼格林、氯霉素、头孢菌素 C、扶桑素 C、玉米赤霉烯酮、丰塞菌素 B、恶霉菌素 A 等。其中,21 种代谢物仅在相互作用过程中产生,并具有抗菌特性。这项研究表明,AN-11 菌株在产生一系列具有抗菌特性的非挥发性次生代谢物方面潜力巨大。可以进一步提取和研究这些代谢物对其他土传病原体的功效,并有可能将其开发成控制植物病害的配方。
Profiling of bioactive secondary metabolites from Aspergillus niger against a guava wilt pathogen, Fusarium oxysporum f. sp. psidii
Guava wilt is a devastating soil-borne disease that causes significant losses in guava orchards. Management of the disease is very challenging once established in the field. Therefore, there is a need to explore for an effective, economical, and sustainable management strategies. Aspergillus niger, a bio-control fungus, has been demonstrated effectiveness against various soil-borne pathogens including guava wilt pathogens. It produces a diverse hydrolysing enzymes and secondary metabolites. However, no extensive study has been undertaken to profile the secondary metabolites of A. niger. In this investigation, we assessed eleven A. niger strains (AN-1 to AN-11) against four guava wilt pathogens (Fusarium oxysporum f. sp. psidii, F. falciforme, F. chlamydosporum, and F. verticillioides) using a dual culture assay. All strains demonstrated effective by restricting the mycelial growth of pathogens, among them AN-11 displayed maximum inhibition of 86.33%, followed by the AN-3 (84.27%). The UPLC-QToF-ESIMS analysis was undertaken to explore the secondary metabolites of AN-11 responsible for inhibiting F. oxysporum f. sp. psidii. The crude extracts were obtained from F. oxysporum f. sp. psidii, AN-11 and their interaction using ethyl acetate as a solvent. After evaporating, the crude fractions were analysed using UPLC-QToF-ESIMS with an Acquity UPLC and a SCIEX SelexION Triple QuadTM 5500 System. From the ethyl acetate extract of F. oxysporum f. sp. psidii, approximately 14 metabolites involved in pathogenicity were identified. Similarly, analysis of AN-11 crude extract revealed 25 metabolites, and notably, 41 metabolites were identified during the interaction between AN-11 and F. oxysporum f. sp. psidii, including kotanin, isokotanin A, aurofusarin, kojic acid, pyranonigrin, aurasperone F, hexylitaconic acid, asperazine, bicoumanigrin, chloramphenicol, cephalosporin C, fusarin C, zearalonone, fonsecin B, malformin A, and others. Among these, 21 metabolites were produced only during the interaction and have antimicrobial properties. This study highlights the significant potential of the AN-11 strain in generating a diverse array of non-volatile secondary metabolites with antimicrobial properties. These metabolites could be further extracted and investigated for their efficacy against other soil borne pathogens and potentially developed into formulations for controlling plant diseases.
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