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Measuring chitinase and protease activity in cultures of fungal entomopathogens

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posted on 2023-05-03, 10:09 authored by Peter Cheong, Travis Glare, Michael Rostas, Stephen HainesStephen Haines
Entomopathogenic fungi produce a variety of destructive enzymes and metabolites to overcome the unique defense mechanisms of insects. In a first step, fungal chitinases and proteinases need to break down the insect's cuticle. Both enzyme classes support the infection process by weakening the chitin barrier and by producing nutritional cleavage products for the fungus. In a second step, the pathogen can now mechanically penetrate the weakened cuticle and reach the insect's hemolymph where it starts proliferating. The critical enzymes chitinase and proteinase are also excreted into the supernatants of fungal cultures and can be used as indicators of virulence. Chromogenic assays adapted for 96-well microtiter plates that measure these enzymes provide a sensitive, fast, and easy screening method for evaluating the potential biocontrol activity of fungal isolates and may be considered as an alternative to laborious and time-consuming bioassays. Furthermore, monitoring fungal enzyme production in dependence of time, nutrient sources, or other factors can facilitate in establishing optimal growth and harvesting conditions for selected isolates with the aim of achieving maximum biocontrol activity.

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Rights statement

© Springer Science+Business Media New York 2016

Language

  • English

Does this contain Māori information or data?

  • No

Publisher

Humana Press

Journal title

Microbial-based biopesticides: methods and protocols

ISBN

9781493963652||9781493963676

Citation

Cheong, P., Glare, T. R., Rostas, M., & Haines, S. R. (2016). Measuring chitinase and protease activity in cultures of fungal entomopathogens. In T. R. Glare & M. E. Moran-Diez (Eds.), Microbial-based biopesticides: methods and protocols. Methods in Molecular Biology, vol. 1477 (pp. 177–189). doi:10.1007/978-1-4939-6367-6_14

Report number

FBP 67547

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