Abstract
This study assessed the decolorization of reactive red 120 (RR120) by Alcaligenes faecalis subsp. phenolicus strain isolated from the bark borer insect (Indarbela tetraonis) tunnel developed in Peltophorum pterocarpum. The optimal parameters for the dye of decolorization 0.1 mg/L of dye were pH 7, temperature 35°C, fructose (0.4% w/v) as the carbon supply (0.4% w/v), peptone (0.2% w/v) as the nitrogen source (0.4% w/v), 12 hours of static conditions, and 0.3 ml of inoculums. Cell suspension, sodium alginate (3%, w/v), and PVA (5%, w/v) immobilized cell beads (10 beads 0.5 mm in size) were used in the batch continuous reactor for complete bio-decolorization of RR120. The batch reactor was subjected to 5 cycles of batches for 3 days of constant use. Under optimal conditions, the batch mode achieved more than 99% dye decolorization and fabric color removal in less than 48 hours of contact. When the control and dye-decolorized media were analyzed using UV spectroscopy, the absorbance of the control medium was higher than that of the decolorized media. GC-MS and FTIR analysis revealed the basic compounds and functional groups of the parent RR120 dye. This strain decolored 76.51% of AB 113, 96.8% of orange II, 98.47% of congo red, 98.3% of RR120, 97.92% of phenol red individual dyes, and 94.72% of the dye mixture at 12 hours. A. faecalis subsp. Phenolicus strains produced positive results in the qualitative analytical test of exopolysaccharides (EPS) and plant growth-promoting rhizobacteria (PGPR) production. The RR120 was decolorized in the presence of heavy metal ions by A. faecalis sub-sp. Phenolicus bacteria.
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