摘要
本试验经培养特性、形态特征、红细胞吸附试验和生长抑制试验等从8株珍禽霉形体中筛选出1株具有代表性的菌株MG—P,将MG—P和标准株MG-S分别建立了HI和Dot-ELISA试验,检测3批120份共 100多种珍禽动物的血清样本,MG—P的阳性检出率为HI 14. 2%(17/20),Dot—ELISA 16.7%(20/120),两法阳性符合率为 85%(17/20);MG—S_6的阳性检出率为HI 9.2%(11/120),Dot—ELISA16. 7%(20/120),两法符合率为 55%(11/20)。以MG—P为检测抗原,将 HI、Dot—ELISA和常规血清平板凝集试验(SPA)比较,结果表明HI具有高特异性和敏感性,而Dot—ELISA和SPA具有较高的非特异性,且 SPA试验重复性差。因此以 MG—P建立的HI试验为检测珍禽霉形体血清抗体的最佳方法。
One strain mycoplasma (MG-P) was selected from eight strains isolated from zoo rare birds by culture property, morphological character, red cell adhesion and growth inhibition. MG-P and MG - Ss were propagated in selected medium and then hyperimmune sera were prepared in poultry. The methods of HI and Dot - ELISA with the two antigens for detection of mycoplasma antibodies were developed and applied in 3 batches 120 samples from zoo poultry. The positive rate with MG-P was 14.2% by HI and 16.7% by Dot-ELISA, while with MG-& were 9.2% and 16.7%, respeceively.The test of sensitivity, specificity and repetition of HI, Dot - ELISA and serum - plate agglutination (SPA) showed that HI had higher specificity and sensitivity, Dot -ELISA and SPA had higher no - specificity and SPA also had lower repetition. According to those results the HI with MG - P was the best method to detect mycoplasma antibody from zoo rarebirds.
