FLUORESCENT DNA BINDING DYE‐BASED APPROACH FOR MEASURING THE GROWTH OF AN ESCHERICHIA COLI LYSINE AUXOTROPH AND QUANTIFYING LYSINE

Abstract

Microbiological assays for determination of bioavailable lysine appear to have many advantages. However, since the developed assay is based on bacterial growth and considerable optical density (OD) is required to detect distinguishable differences in extent of growth, it can be time consuming. The purpose of this study was to explore the fluorescence as an alternative method to measure bacterial growth instead of OD and examine the possibility to shorten the time required for the lysine assay. An assay based on SYTO 9 green fluorescent DNA binding dye (Live/Dead BacLight Protocol, Molecular Probes) was used to stain all bacteria in a population. Additional experiments were carried out to determine the ability of fluorescence based on SYTO 9 to overcome problems associated with high nonbacterial background that contributes to OD. From this study it appears that using fluorescence based on SYTO 9 green fluorescent staining, the E. coli lysine auxotroph growth assay can be completed in 9 h instead of 11 h and has the advantage of improved detection sensitivity. Problems associated with interference by high background nonbacterial OD can be partially resolved by fluorescence.