03 October 2021 1 3K Report

We have been using the Enz Check lysozyme assay and are assuming the cells are not intact but in pieces. However over time and especially with vortexing or pipetting to mix substrate, I would think the cell wall pieces would get smaller and this would affect your estimation of lysozyme activity - less substrate, and probably more background? Is this correct? If so what are the recommendations on mixing these cells?

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