Literature DB >> 18604983

Determination of lysozyme activity by a fluorescence technique in comparison with the classical turbidity assay.

R Helal1, M F Melzig.   

Abstract

The aim of this comparable study was to evaluate two different methods for the assay of lysozyme activity. Lysozyme activity was assayed by turbidimetric and fluorescence-based methods with hen egg white lysozyme as standard. The standard activity of each assay was calibrated in units of activity per mg under the experimental conditions (37 degrees C) so that direct comparison between these two assays could be made. The turbidimetric assay was performed using a 0.36 mg/ml Micrococcus lysodeikticus suspension and a microtiter plate reader capable of analyzing enzyme kinetics at 450 nm, and the linearity, in the range of 2.3-23.8 units/ml, presented a correlation coefficient (R2) as high as 0.9967. The fluorescence-based assay was performed with EnzChek kit using a suspension of Micrococcus lysodeikticus labeled with fluorescein and a fluorescence microplate reader. The linearity in the range of 0.47-5.28 units/ml, presented a correlation coefficient (R2) as high as 0.9881. Thus, the turbidimetric assay provides a simple rapid accurate and specific method for the determination of lysozyme activity but with relatively low sensitivity in comparison with the fluorescence-based method which was demonstrated to be a high sensitivity assay, and hence a reliable applicable technique to determine lysozyme activity at low levels e.g. in cell culture systems.

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Year:  2008        PMID: 18604983

Source DB:  PubMed          Journal:  Pharmazie        ISSN: 0031-7144            Impact factor:   1.267


  12 in total

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6.  Lipoprotein LprI of Mycobacterium tuberculosis Acts as a Lysozyme Inhibitor.

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7.  In vitro Effects of Selected Saponins on the Production and Release of Lysozyme Activity of Human Monocytic and Epithelial Cell Lines.

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10.  An improved 96-well turbidity assay for T4 lysozyme activity.

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Journal:  MethodsX       Date:  2015-05-18
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