4.6 Article

A Simple in situ Assay to Assess Plant-Associative Bacterial Nitrogenase Activity

Journal

FRONTIERS IN MICROBIOLOGY
Volume 12, Issue -, Pages -

Publisher

FRONTIERS MEDIA SA
DOI: 10.3389/fmicb.2021.690439

Keywords

nitrogen fixation; symbiosis; diazotroph; acetylene reduction assay; endophyte

Categories

Funding

  1. 1851 Royal Commission for the Exhibition of 1851 Research Fellowship [RF-2019-100238]
  2. Wolfson College, University of Oxford Junior Research Fellowship
  3. Biotechnology and Biological Sciences Research Council [BB/T006722/1, BB/T001801/1, BB/M011224/1]
  4. BBSRC [BB/L011484/1, BB/T006722/1] Funding Source: UKRI

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Utilizing a modified in situ acetylene reduction assay (ARA) with barley as the host, nitrogenase activity in diazotrophic bacteria can be rapidly and reliably assessed, aiding in the identification of high-quality plant-associative diazotrophs.
Assessment of plant-associative bacterial nitrogen (N) fixation is crucial for selection and development of elite diazotrophic inoculants that could be used to supply cereal crops with nitrogen in a sustainable manner. Although diazotrophic bacteria possess diverse oxygen tolerance mechanisms, most require a sub 21% oxygen environment to achieve optimal stability and function of the N-fixing catalyst nitrogenase. Consequently, assessment of N fixation is routinely carried out on free-living bacteria grown in the absence of a host plant and such experiments may not accurately divulge activity in the rhizosphere where the availability and forms of nutrients such as carbon and N, which are key regulators of N fixation, may vary widely. Here, we present a modified in situ acetylene reduction assay (ARA), utilizing the model cereal barley as a host to comparatively assess nitrogenase activity in diazotrophic bacteria. The assay is rapid, highly reproducible, applicable to a broad range of diazotrophs, and can be performed with simple equipment commonly found in most laboratories that investigate plant-microbe interactions. Thus, the assay could serve as a first point of order for high-throughput identification of elite plant-associative diazotrophs.

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