Abstract This study involved the investigations of lysozyme refolding and aggregates refolding by direct dilution. The renaturation of active protein and aggregate was determined by activity measurement, absorbance at 280nm, together with Congo Red binding assay, ThT fluorescence, TEM and optical measurement. To understand the competition behavion between the protein refolding and aggregation, we investigated the effect of different constituents of renaturation buffer on refolding performance by direct dilution method. Experiments results showed that low concentration urea addition in the renaturation process could suppress protein aggregation to stimulate the pathway of correct refolding at high protein concentration. Chang [2004] proved that the maximum refolding efficiency occurred in 60 minute with renaturation buffer while maintaining [GSSG]/[GSH]≧1 the ratio A280/A260 above 0.3 for various protein concentrations. Subsequently, the refolding experiments of renaturation buffer with various combination of [GSSG]/[GSH] and urea concentration were carried out for 6 days. The results showed that activity recovery increased gradually from 65% to 96% by 10-fold dilution at the concentration 1.2mM/1.2mM [GSSG]/[GSH] and 2M Urea of renaturation buffer during 6day incubation.