Laccase CotA from Bacillus subtilis 168 was successfully displayed on the membrane of Escherichia coli cells using poly-γ-glutamate synthetase A protein (PgsA) from B. subtilis as an anchoring matrix. Further analyses demonstrated that the fusion protein PgsA/CotA efficiently translocates to the cell surface of E. coli with an enzymatic activity of 65 U/10 cells. Surface-displayed CotA was shown to possess improved enzymatic properties compared with those of the wild-type CotA， including higher thermal stability (above 90% activity at 70 °C and nearly 40% activity at 90 °C after 5-h incubation) and stronger inhibitor tolerance (approximately 80 and 65% activity when incubated with 200 and 400 mM NaCl， respectively). Furthermore， the whole-cell system was demonstrated to have high enzymatic activity against anthraquinone dye， Acid Blue 62， triphenylmethane dye， Malachite Green， and azo dye， Methyl Orange with the decolorization percentages of 91， 45， and 75%， after 5-h incubation， respectively.