پديد آورندگان :
Ghaleh Golab Behbahan N. نويسنده , Asasi K. نويسنده , Afsharifar A. R. نويسنده , Pourbakhsh S. A. نويسنده
چكيده لاتين :
Mycoplasmas were isolated from tracheal and air sac samples of the suspected flocks to have mycoplasmosis and cultured on Freyיs medium. Forward and reverse primers were selected on the basis of known sequences of Mycoplasma gallisepticum (MG) and Mycoplasma synoviae (MS) 16S rRNA genes.These primers successfully amplified a 780 bp fragment of the target DNA in MG. Restriction fragment
length polymorphism (RFLP) by three restriction enzymes (REs), HpaI, Hpall, and MboI was performed for each PCR product. According to the RFLP results, 55 samples were detected as MG; no MS was detected.
The PCR results were confirmed by sequencing of a selected amplicons. Results showed that PCR and RFLP are rapid and useful for diagnosis of both cultured as well as field samples of suspected flocks to have
infection with MG. In addition, PCR could be performed with at least 100 CFU of MG per each PCR reaction.
