RecBCD is a trimeric enzyme complex that initiates homologous recombinational repair in E. coli. RecBCD complex contains single-stranded DNA nuclease and two DNA helicases. In these two helicases, RecB is a 3'-to-5' single-stranded DNA translocase and RecD is a 5'-to-3' one. Formation of RecBCD trimeric complex was shown to stimulate both 3'-to-5' and 5'-to-3' translocation activities, implying interaction and coordination of RecB and RecD helicases in the trimeric complex. ATP hydrolysis is coupled to the unwinding and translocation process during the catalytic step of DNA helicases, so most DNA helicases are ATPases. Here, we used total internal reflection fluorescence microscopy to directly observe and analyze individual Cy3-labeled ATP binding and turnover events during RecBCD unwinding at the single-molecule level. This allows us to characterize ATPase activities of both RecB and RecD as well as their coordination.Comparison of Cy3-ATP bound time between RecBCD and RecBCD* K177Q shows different ATP bound time.Though we can only measure one ATP bound time of wild type RecBCD, we found positive correlation of ATP concentration and ATP bound time. It implies the coordination between RecB and RecD synchronizes both ATPase catalytic rates.