ISOLATION AND CHARACTERIZATION OF LIGNIN PEROXIDASE FROM TROPICAL RESUPINATE WHITE ROT FUNGI

Abstract

Resupinate white rot fungi are abundant throughout tropical regions. They play an important role on wood decaying in the forest, but little is known about their characteristics. In this study, tropical resupinate fungi were collected from dead-wood stumps in seven provinces of Thailand. Twenty-five specimens were successfully isolated and identified into specific or generic levels. Characterization study revealed several unique characters of these tropical resupinate white rot fungi including the potential source of lignin peroxidase which scarcely found in typical white rot fungi, thermotolerant ability, selective delignification property. Among these fungi, Phanerochaete sordida Sk7 showed a remarkable biodegradation characters by efficiently biodegrade structurally diverse substances. A comparative study on decolorization ability of a model azo dye, reactive black 5 under various physicochemical parameters between P. sordida Sk7 and the reference fungus, Phanerochaete chrysosporium suggested greater biodegradation ability of P. sordida Sk7 over a wide range of pHs, temperatures and dye concentrations. The decolorization mechanism of P. sordida Sk7 occurred through degradation activity of laccase and lignin peroxidase rather than mycelial biosorption. None of residual dye and phytotoxic natures of the dye were detected in its metabolites which indicated the successful treatment. Therefore, this fungus was purposed as a good candidate of white rot fungus for bioremediation and biopulping aspects. Since a great biodegradation ability of this fungus was proved, enzymatic degradation system of this fungus was considered. Lignin peroxidase was found to play significant role in its degradation system. Therefore, lignin peroxidase from this fungus was further purified and characterized and it was found to be stable over pH 3-6 and temperature ranging from 10 to 50 ◦C. A full-length of lignin peroxidase cDNA was obtained and found to be highly similar with LiP isosyme H8 from P. chrysosporium.