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                            Original Research
                            
                            
                            6.
                            
                            
                            Real time RT-PCR assay for detection of different 
                            serotypes of FMDV in Egypt - Laila El-Shehawy, A. M. H. Azab, W. Mossad, Ehab El-Sayed, 
                            A. Ismail, Wafaa Deghady
                            Vet World. 2012; 5(12): 732-737
              
               
              
              doi: 
              10.5455/vetworld.2012.7
32-737
              
              
               
              
              
              
   
 
              
               
               
               
              
              
              Abstract
              
              
                            Aim: 
                            The present study indicated that rRT-PCR could be 
                            provided for the detection of FMDV in infected, 
                            contact and carrier cattle and also provide a rapid 
                            sensitive tool aiming to aid in rapid disease 
                            detection and control. Foot and Mouth disease virus 
                            serotypes O1 and A still existing in Egypt. In 
                            January 2012, sever outbreaks struck the animal 
                            population in most Egyptian governorates. The 
                            causative virus was identified as FMDV SAT2. 
                            Material and Methods: Five samples of tongue 
                            epithelium (ET) and five oesophageal-pharyngeal (OP) 
                            fluid samples were collected from FMD suspected 
                            cattle in infected farm at El-Fayoum and 20 OP 
                            samples from in-contact cattle at the same farm in 
                            addition to 30 OP samples from apparently healthy 
                            cattle at three different localities in El-Fayoum 
                            governorate (12 from Fayoum; 9 from Sinoras and 9 
                            from Edsa) in order to detect carrier cattle. All of 
                            these samples were collected during November and 
                            December 2011 and January 2012. 
              
                             Results: All 
                            the ET and OP samples were inoculated on BHK cell 
                            culture and baby mice. The obtained results were 
                            identified using complement fixation test in 
                            addition to real-time reverse transcriptase 
                            polymerase chain reaction (rRT-PCR). In the infected 
                            farm at El-Fayoum FMDV type SAT2 was detected in 
                            cattle which are considered as the first 
                            introduction of this type while FMDV type O and SAT2 
                            were detected in the in-contact cattle in the same 
                            farm. The sensitivity of rRT-PCR was cleared in the 
                            in-contact cattle as 13 out of 20 OP samples were 
                            positive to FMDV by rRT-PCR while 11 out of 20 OP 
                            samples were positive to FMDV by CFT. The OP samples 
                            collected from apparently healthy cattle from Fayoum, 
                            Sinoras and Edsa localities in Fayoum governorate 
                            demonstrate the circulation of the FMDV type A, O 
                            and the recent SAT2 in carrier cattle which threaten 
                            cattle population in Fayoum governorate. Also the 
                            sensitivity of real time RT-PCR over the CFT in 
                            detection of FMDV carrier cattle was clearly noticed 
                            in these localities as 19 out of 30 OP samples were 
                            positive by rRT-PCR while in contrast there were 
                            only 16 out of 30 samples positive by CFT. 
              
                             
                            Conclusion: In conclusion, this study 
                            demonstrates that real-time RT-PCR currently used at 
                            the WRL for FMD provides an extremely sensitive and 
                            rapid additional procedure for improved laboratory 
                            diagnosis of FMD especially in-contact and carrier 
                            cases. The rRT-PCR generated results in less than 
                            one day from test commencement, in contrast to up to 
                            four days to define some positive and all negative 
                            samples by combined use of CFT and virus isolation. 
                            This is an important feature when definitive 
                            diagnostic results are required in a short timescale 
                            during emergencies. Also this study demonstrates the 
                            current situation of FMDV circulating in EL-Fayoum 
                            governorate and the introduction of new SAT2 
                            serotype beside type A and O. 
              
                             Keywords: FMDV, 
                            Typing, Isolation, OP, ET, SAT-2, rRT-PCR, Carrier, 
                            Cattle