What question did this study set out to answer?

The aim is to clone and purify bacillus nitroreductase and explore its potential applications in biotechnological processes.

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May 8, 2026Open Access

Cloning, purification and possible use of a Bacillus nitroreductase in biotechnological applications

Key Points

The aim is to clone and purify bacillus nitroreductase and explore its potential applications in biotechnological processes.
Enzyme purification and characterization using LC-ESI-MS to analyze reduction products.
Development of an electrochemical detection platform for measuring enzymatic activity.
ANOVA and regression analysis to assess enzyme activity and kinetics.
The enzyme successfully reduced CB1954 and TNT to specific products (2-amino 4,6-DNT).
Electrochemical detection revealed significant cathodic responses to nitrofurazone.
Statistical analysis indicated significant differences in enzyme activity across tested conditions.

Abstract

), respectively. The enzymatic reduction of CB1954 analyzed by LC-ESI-MS gave prominent molecular ions at the expected m/z values of CB1954 (M + H⁺: m/z 253), primary hydroxylamine intermediates (M + H⁺: m/z 239), and amino end-products (M + H⁺: m/z 223). The purified enzyme was also found to biotransform TNT to the product 2-amino 4,6-DNT. In addition, a proof-of-concept electrochemical detection platform based on immobilized nitroreductase produced a measurable cathodic response toward nitrofurazone, demonstrating the enzyme's electrochemical applicability. ANOVA identified significant differences in activity levels among multiple groups, while regression analysis enabled prediction of enzyme responses and characterization of the underlying kinetic patterns in statistical analysis.

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Cloning, purification and possible use of a Bacillus nitroreductase in biotechnological applications

Key Points

Abstract

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