Aeromonas hydrophila is a gram negative, facultatively anaerobic freshwater bacterium, occurring widely in aquatic environment. It has been indicated as a factor causing diseases in humans and animals. As there was no suitable system to study the gene function in Aeromonas spp. The purpose of this work is to construct vectors which contain replication origin by fuse the vector of E.coli with indigenous plasmids of Aeromonas hydrophila. In order to get indigenous plasmids of Aeromonas, we examined the plasmid carriage rate of a total 70 clinical and environmental Aeromonas isolates. Four clinical Aeromonas species, AH25, AH32, AH35, AH69 and four environmental Aeromonas species carry plasmids. All plasmids were examined after digestion with restriction endonucleases. Restriction endonucleases fragments were sized by comparison with standard marker. Plasmids of clinical Aeromonas species, pAH 32、pAH 35, and environmental Aeromonas species, pAH 132、pAH 169、pAH191, could be digested by restriction endonucleases. The size of these plasmids are 17 Kb、15kb、2.4kb、2.4kb、2.4kb respectively. We had interest in Plasmid, pAH35, which had more restriction endonucleases digestive site than others. For this purpose, we fused vector of E.coli with fragment of indigenous plasmids in Aeromonas hydrophila to construct a replication origin-screening vector. We transformed these plasmids to E.coli to amplify them then transferred these vector into Aeromonas spp by electroporation. Once the recombinant contains a replication origin from plasmid of Aeromonas hydrophila, antibitic trait is used as a selection marker as it is transformed into Aeromonas hydrophila. The plasmid which contains replication origin could be constructed an expressional vector. On the basis of similarity to other genes in the Gene Bank Database, NCBI, we found a fragment named pAH35-3 which similarity to a plasmid pAsa2 of Aeromonas salmonicida subsp. salmonicida strain A449. Plasmid pAsa2 is the type of ColE1-type. We suggest plasmid pAH35 is a ColE1-type plasmid, too. In this work, we investigate the replication origin of this plasmid and try to construct a shuttle vector for this genus. In this work, the replication origin of plasmid pAH35 has not been confirmed.