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Manuscript ID : 518283 Visit : 140 Page: 673 - 681

Article Type: Original Research

Detection of Mycoplasma synoviae in clinical samples by VlhA-PCR method

Subject Areas : Veterinary Clinical Pathology

حسین Ansari 1 , S.A Pourbakhsh 2 , نریمان Sheikhi 3 , M.H Bozorgmehri Fard 4 , عباس Ashtari 5

1 - Ph.D Student of Poultry Diseases, Faculty of Specialized Veterinary Sciences, Islamic Azad University- Science & Research Branch, Tehran, Iran
2 - Department of Microbiology, Faculty of Specialized Veterinary Sciences, Islamic Azad University- Science & Research Branch, Tehran, Iran
3 - Department of Clinical Science, Faculty of Specialized Veterinary Sciences, Islamic Azad University- Science & Research Branch, Tehran, Iran
4 - Department of Clinical Science, Faculty of Specialized Veterinary Sciences, Islamic Azad University- Science & Research Branch, Tehran, Iran
5 - Mycoplasma Reference Lab. of Razi Vaccine and Serum Research Institute, Karadj, Iran

Received: 2009-11-12 Accepted : 2010-05-29 Published : 2010-02-20

Keywords: PCR, Clinical samples, Mycoplasma synoviae, VlhA gene,

Abstract :

As one of the major pathogens of avian species, Mycoplasma Synoviae causes significant economic losses to the poultry industry. The main purpose of this study was to detect Mycoplasma Synoviae in clinical samples using the VlhA-PCR method. For serological screening test, 373 serum samples were collected from 25 breeder farms and rapid serum agglutination test conducted which revealed that 143 samples equivalent to 19 breeder farms were positive. For VlhA-PCR assay, 20 of the previously mentioned breeder farms were selected and sterile swab were collected from the palatine cleft, trachea, air sacs and lungs. Three swabs from 3 birds were placed in a test tube containing 1 ml of PBS and transferred to the laboratory for PCR test. Specific primers for VIhA gene were employed in this study. The PCR product from specific primers showed 350-400 bp for all field isolated on electrophoresis gel in 8 farms. VlhA-PCR with high sensitivity could be employed in definitive diagnosis of Mycoplasma Synoviae infection in the laboratory.

References:


  1. حسینی، ا. (1386): تعیین هویت مولکولی مایکوپلاسما سینوویه جدا شده از مرغداری­های صنعتی استان مازندران، رساله دکترای تخصصی بیماری­های طیور، دانشکده دامپزشکی دانشگاه علوم تحقیقات تهران، صفحات: 89-1.
    2.
  2. Ben, B., Abdelmoumen Mardassi, R., Ben Mohamed, I., Gueriri, S. and Boughattasand B. (2005): Duplex PCR  to differentiate between mycoplasma synoviae  and mycoplasma gallisepticum on the basis of conserved species-specific sequence of their hemagglutinin gene,journal of clinical microbiology, pp: 48-958.
    3.
  3. Bradbury, Y. (2001): Avian Mycoplasma. Work shop of European Mycoplasma specialist. World poultry Sci.J., 61: 355-357.
    4.
  4. Fiorentin, L., Mores M., Trevison, I.M. and Antunes, S.C. (2003): Test profiles of broiler breeder flocks housed in farms with endemic Mycoplasma synoviae infection. Brazilian journal of poultry science, pp: 38-49.
    5.
  5. Nathan, J. and Gasser, R. (2007): Classification of mycoplasma synoviae strains using single-strand conformation polymorphism and high-resolution melting-curve andlysis of the VlhA gene single-copy region, Microbiology, 153: 2679-2688.
    6.
  6. Jordan, F., Mark, P., Denis A. and Trevor, F. (2002): Poultry Disease, fifth Edition, p: 178-193
    7.
  7. Kiss, I., Matiz, K., Kaszanitsky, E., Chavez, Y. and Johnsson, K.E. (1997): Detection and identification of avian mycoplasma by polymerase chain reaction and restriction fragment length polymorphism  assay. Vet. Microbial. pp
    8.
  8. Kleven, S.H. (2008): Mycoplasmosis.In: Saif, Y.M., Barnes, H.J., Gilsson, J.R., Fadly, A.M., Mc Dongald, L.R. and swayne, D.E. Diseases of Poultry. 12th.ed. Iowa state university press (A Blackwell Publishing Company). pp: 719-722.
    9.
  9. Lockaby, S.B., Hoerr, F.J., Lauerman, L.H., Smith, B.F., Samoylov, A.M., Toivio-Kinnucan, M.A.and et al (1999): Factors associated with virulence of Mycoplasma synoviae. Avian Dis. Apr-Jun, 43(2): 251-256.
    10.
  10. Lauerman, H., Sharpton, A. (1993): Development and application of a polymerase chain reaction assay for mycoplasma synoviae, avian disease, vol. 37: 829-834.
    11.
  11. Noormohamadi, A.H., Markham, P.F., Kanci, A., Whither, K.G. and Browing, G.F. (2002): A novel mechanism for control of antigenic variation in the hemagglutining gene family of Mycoplasma synoviae. Mol. Microbial. 35: 911-923.
    12.
  12. Noormohamadi, A.H., Hemmatzadeh, F. and Whither, K.G. (2007): Safety and Efficacy of the Mycoplasma Synoviae MS-H Vaccine in Turkeys. Avian Disease Preprint; N/A-N/A.
    13.
  13. OIE terrestrial manual. (2008): Avian mycoplasmosis, chapter 3.5.6. pp: 482-512.
    14.
  14. Ramirez, A., clive J., Naylor, P., Hammond, j. and Bradbury, M. (2006): Development and evaluation of a diagnostic PCR for Mycoplasma synoviae using primers located in The intergenic spacer region dna 23s rRNA gene. Veterinary Microbiology, 118: 76-82.
    15.
  15. Ricardo, M. and Silveria, L.F. (1996): polymerase chain reaction  optimization for mycoplasma  synoviae  diagnosis,avian disease , vol 40:218-222.
    16.
  16. Senties-Cue, G., Shivaprasad, H.L., Chin, R.P. (2005): Systemic Mycoplasma synoviae infection in broiler chickens. Avian Pathol. Apr; 34(2): 137-42.s
    17.
  17. Yang Hong ,Marcarmen Garcia, (2004): Specific Detection and typing of mycoplasma synoviae strains in poultry with pcr and DNA sequence analysiss targeting the Hemagglutinin encoding Gene VlhA, Avian Disease, vol, 48:606-616.
    18.
  18. Yogev, D., Levision, S., Kleven, S.H., Halachmi, D. and Razhn, S. (1998): Ribosomal RNA gene probes to detect intraspecies heterogenecity hn Mycoplasma gallisepticum and Mycoplasma synoviae. Avian Disease; 32: 220-231.
    19.

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