A specific PCR (polymerase chain reaction) primer pair has been developed using RAPD (random amplified polymorphic DNA) to differentially detect Erwinia carotovora subsp. carotovora (Ecc) and E. chrysanthemi (Ech). A specific 1,200 bp DNA fragment was amplified and cloned from Ecc DNA using OPY2O primer, one of the sixty random primers used in RAPD. Nucleotide sequence of this 1,200 bp DNA showed 83% similarity to Ech rhiN gene, where conserved sequences were displayed in two regions. But in Ech rhiN sequence, there are additional 49 bp nucleotides inserted between these two conserved regions. Herein, a set of primers Ec3F/Ec4R was designed and applied to differentially detect Ecc and Ech by PCR. Using bacterial chromosomal DNA as templates, a distinct 497 bp fragment can be amplified from 225 Ecc strains, and a 548 bp fragment was amplified from 85 Ech strains. No fragment can be amplified from the other seven bacterial species in six genera. Sensitivity of PCR for detecting Ecc and Ech was between 10~50 pg for purified DNA and 1.1×10^1 cfu and 1.2×10^1 cfu for cultured cells, respectively. It took 3-4 hr to detect Ecc and Ech by colony PCR using Ec3F/Ec4R primer set and the target bacteria in infected tissues of cala lily and phalaenopsis. Results presented here suggest that the primer pair Ec3F/Ec4R applied in PCR can be very useful in rapid identification, detection, and differentiation of the soft rot pathogens Ecc and Ech.