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Rapid detection of respiratory viruses by shell vial culture and direct staining by using pooled and individual monoclonal antibodies.

机译:通过贝壳小瓶培养快速检测呼吸道病毒并使用合并的单个单克隆抗体直接染色。

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摘要

The Bartels respiratory virus panel detection kit is an indirect fluorescent-antibody (IFA) method that uses pooled and individual antisera for tissue culture confirmation of seven respiratory viruses. We evaluated these reagents for detecting viral antigen in shell vial cultures and by direct staining of cells from respiratory specimens. The isolation from 254 specimens of respiratory viruses in shell vial cultures compared with standard tube cultures was highly sensitive (94%) and specific (97.3%). The numbers of viral isolates detected in three consecutive years of testing with shell vial cultures were 68 of 254 (26.8%), 101 of 381 (26.5%), and 122 of 430 (28.4%). IFA direct staining of all 1,065 specimens resulted in 183 (17.2) being uninterpretable because of inadequate numbers of cells or interfering fluorescence. The sensitivity and specificity of the interpretable IFA direct stains in comparison with shell vial cultures were 85.9 and 87.1%, respectively. For detection of 881 adequate specimens, Bartels respiratory syncytial virus IFA direct staining compared with an Ortho Diagnostics Systems direct fluorescent-antibody test for respiratory syncytial virus RSV was highly sensitive (95.5%) and specific (97%). Shell vial cultures combined with Bartels IFA reagents are a rapid alternative to standard tube cultures. Bartels IFA direct staining with individual antisera provides useful same-day screening of respiratory specimens, but the antiserum pool was not effective in screening for positive specimens because of excessive amounts of nonspecific fluorescence.
机译:Bartels呼吸道病毒面板检测试剂盒是一种间接荧光抗体(IFA)方法,使用合并的单个抗血清对7种呼吸道病毒进行组织培养确认。我们评估了这些试剂,用于检测贝壳小瓶培养物中的病毒抗原,并通过直接对呼吸道标本中的细胞进行染色。与标准试管培养相比,从小瓶培养物中的254种呼吸道病毒标本中分离出的细菌具有很高的敏感性(94%)和特异性(97.3%)。在连续三年进行的带壳小瓶培养的测试中,病毒分离物的数量为254个中的68个(26.8%),381个中的101个(26.5%)和430个中的122个(28.4%)。所有1065个样本的IFA直接染色导致183(17.2)因细胞数量不足或荧光干扰而无法解释。与外壳小瓶培养相比,可解释的IFA直接染色的敏感性和特异性分别为85.9%和87.1%。为了检测881个适当的标本,Bartels呼吸道合胞病毒IFA直接染色与Ortho Diagnostics Systems直接荧光抗体检测呼吸道合胞病毒RSV相比具有很高的敏感性(95.5%)和特异性(97%)。带Bartels IFA试剂的带壳小瓶培养物是标准试管培养物的快速替代方法。 Bartels IFA用单独的抗血清直接染色可对呼吸道标本进行有用的当日筛查,但由于过量的非特异性荧光,抗血清库在筛查阳性标本方面无效。

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