This study used methods such as ammonium sulfate precipitation, DEAE-cellulose 52 anion exchange resin and trypsin-Sepharose 4B affinity columns to purify and extract trypsin inhibitor from Phaseolus coccineus (PCTI). 15% SDS-PAGE and MALDI-TOF mass spectrometers were used to analyze the molecular weight of PCTI, which was 8.92 kDa, belonging to Bowman-Birk-type proteinase inhibitor. Further investigation on the nature of PCTI found that its residue activity for inhibiting trypsin was still maintained above 80% when its temperatures reached 80℃ and 100℃, showing its high tolerance to temperature. PCTI's residue activity for inhibiting trypsin was also maintained above 80% when it was treated by buffer solutions with different pH values, suggesting that its structural stability would not change in regard to pH values. When treated with different concentrations of DTT (a reducing agent), PCTI's residue activity for inhibiting trypsin decreased with increasing DTT concentration, showing that the maintenance of the conformational stability of PCTI active site was significantly correlated to disulfide bonds inside the molecule. The mole ratio of PCTI to trypsin is one to one. The enzyme kinetics Lineweaver-burk double reciprocal plot and Dixon plots analysis show that the inhibition effect of PCTI on trypsin is of competitive inhibition, with the inhibition constant (ki) being 8.96 x 10^(-9) M.