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使用蛋白A的固相免疫电子显微镜与直接电子显微镜和酶联免疫吸附测定法在粪便中检测轮状病毒的比较。

Comparison of solid-phase immune electron microscopy by use of protein A with direct electron microscopy and enzyme-linked immunosorbent assay for detection of rotavirus in stool.

作者信息

Svensson L, Grandien M, Pettersson C A

出版信息

J Clin Microbiol. 1983 Nov;18(5):1244-9. doi: 10.1128/jcm.18.5.1244-1249.1983.

Abstract

A total of 525 stool specimens collected during 1 year were examined for the presence of rotavirus by direct electron microscopy (EM), enzyme-linked immunosorbent assay (ELISA), and a solid-phase immune electron microscope method (SPIEM) utilizing protein A-coated grids for anchoring of specific viral antisera. Rotavirus was seen in 187 specimens; SPIEM detected 183 (97.8%), whereas direct EM and ELISA detected 161 (86%) and 166 (88.7%), respectively. No false-positive reactions were seen by ELISA. The sensitivity of the methods was evaluated by coded investigation of a dilution series of a positive sample, with a negative fecal specimen as diluent. SPIEM was approximately 30 times more sensitive than direct EM and 10 times more sensitive than ELISA. A study was done to compare the elapsed time for recognition of rotavirus by SPIEM and EM in 25 randomly selected positive specimens. All virus-positive specimens were detected within 2 min by SPIEM, whereas up to 9 min was required for direct EM. SPIEM with protein A is a highly sensitive method, useful for rapid detection of viruses in clinical specimens. Due to the direct visualization of virus particles by electron microscopy, there is no requirement for monospecific antisera for the method.

摘要

在1年的时间里共收集了525份粪便标本,采用直接电子显微镜(EM)、酶联免疫吸附测定(ELISA)以及利用蛋白A包被的网格固定特异性病毒抗血清的固相免疫电子显微镜方法(SPIEM)检测其中是否存在轮状病毒。在187份标本中发现了轮状病毒;SPIEM检测出183份(97.8%),而直接EM和ELISA分别检测出161份(86%)和166份(88.7%)。ELISA未出现假阳性反应。通过以阴性粪便标本作为稀释剂对阳性样本的稀释系列进行编码研究来评估这些方法的敏感性。SPIEM的敏感性比直接EM高约30倍,比ELISA高10倍。开展了一项研究,比较在25份随机选择的阳性标本中通过SPIEM和EM识别轮状病毒所花费的时间。所有病毒阳性标本通过SPIEM在2分钟内均可检测到,而直接EM则需要长达9分钟。带有蛋白A的SPIEM是一种高度敏感的方法,可用于临床标本中病毒的快速检测。由于通过电子显微镜可直接观察病毒颗粒,该方法无需单特异性抗血清。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4f57/272873/ef7f8a77ec37/jcm00136-0246-a.jpg

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