Phosphorus Release and Regeneration Following Laboratory Lysis of Bacterial Cells.

Front Microbiol

Department of the Geophysical Sciences, University of Chicago, Chicago, IL, United States.

Published: April 2021

The availability of phosphorus limits primary production in large regions of the oceans, and marine microbes use a variety of strategies to overcome this limitation. One strategy is the production of alkaline phosphatase (APase), which allows hydrolysis of larger dissolved organic phosphorus (DOP) compounds in the periplasm or at the cell surface for transport of orthophosphate into the cell. Cell lysis, driven by grazing and viral infection, releases phosphorus-containing cell components, along with active enzymes that could persist after lysis. The importance of this continued enzymatic activity for orthophosphate regeneration is unknown. We used three model bacteria - K-12 MG1655, sp. WH7803, and sp. MED4 - to assess the impact of continued APase activity after cell lysis, via lysozyme treatment, on orthophosphate regeneration. Direct release of orthophosphate scaled with cell size and was reduced under phosphate-starved conditions where APase activity continued for days after lysis. All lysate incubations showed post-lysis orthophosphate generation suggesting phosphatases other than APase maintain activity. Rates of DOP hydrolysis and orthophosphate remineralization varied post-lysis among strains. K-12 MG1655 rates of remineralization were 0.6 and 1.2 amol cellhr under deplete and replete conditions; WH7803 lysates ranged from 0.04 up to 0.3 amol cellhr during phosphorus deplete and replete conditions, respectively, while in MED4 lysates, rates were stable at 0.001 amol cellhr in both conditions. The range of rates of hydrolysis and regeneration underscores the taxonomic and biochemical variability in the process of nutrient regeneration and further highlights the complexity of quantitatively resolving the major fluxes within the microbial loop.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC8060472PMC
http://dx.doi.org/10.3389/fmicb.2021.641700DOI Listing

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