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Determination of cAMP and protein content in dormant chlamydospore and non-dormant chlamydospore of Duddingtonia flagrans
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  • Fenghui Wang,
  • Bo-Bo Wang,
  • Xiaojun Yang,
  • Yi-bo Jia,
  • Shu-Yue Tian,
  • Xin Li,
  • Xi-chen Zhang,
  • yanming wei,
  • Jing Zhang,
  • Kui-Zheng Cai
Fenghui Wang
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Bo-Bo Wang
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Xiaojun Yang
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Shu-Yue Tian
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Xi-chen Zhang
Jilin University
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yanming wei
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Jing Zhang
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Kui-Zheng Cai
Northwest University for Nationalities

Corresponding Author:ckz000@126.com

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Abstract

Duddingtonia flagrans, a nematode-eating fungus, is an effective component of animal parasitic nematode biocontrol agents. In the dried formulation, the majority of spores are in an endogenous dormant state. This study focuses on dormant chlamydospore and non-dormant chlamydospore of D. flagrans to investigate the differences in cAMP and protein content between the two types of spores. In this study, cAMP and soluble proteins were extracted from the non-dormant chlamydospore and dormant chlamydospore of D. flagrans isolates SDH035 and DH055, respectively. The cAMP Direct Immunoassay Kit and Bradford protein concentration assay kit (Coomassie brilliant blue method) were used to detect the cAMP and protein content in two types of spores. Results showed that the content of cAMP in dormant spores of both isolates was significantly higher than that in non-dormant spores (p<0.05). The protein content of dormant spores in DH055 bacteria was significantly higher than that of non-dormant spores (p<0.05). In addition, the protein content of dormant spores of the SDH035 strain was slightly higher than that of non-dormant spores, but the difference was not significant (p>0.05). The results obtained in this study provide evidence for the biochemical mechanism of chlamydospore dormancy or the germination of the nematophagous fungus D. flagrans.
Submitted to Journal of Basic Microbiology
11 Feb 2024Editorial Decision: Revise Minor
24 Feb 20241st Revision Received
25 Feb 2024Submission Checks Completed
25 Feb 2024Assigned to Editor
25 Feb 2024Review(s) Completed, Editorial Evaluation Pending
25 Feb 2024Reviewer(s) Assigned
02 Mar 2024Editorial Decision: Accept