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利用单克隆抗体对鼻分泌物中呼吸道合胞病毒多肽进行定量分析。

Quantification of respiratory syncytial virus polypeptides in nasal secretions by monoclonal antibodies.

作者信息

Hendry R M, Godfrey E, Anderson L J, Fernie B F, McIntosh K

出版信息

J Gen Virol. 1985 Aug;66 ( Pt 8):1705-14. doi: 10.1099/0022-1317-66-8-1705.

DOI:10.1099/0022-1317-66-8-1705
PMID:3894575
Abstract

An indirect enzyme-linked immunosorbent assay (ELISA) which uses monoclonal antibody as solid-phase immunosorbent was developed to measure specific polypeptides of respiratory syncytial virus (RSV). The assay was used to examine 43 nasopharyngeal (NP) aspirates from RSV-positive infants that had been examined previously for RSV by culture, direct immunofluorescence, and polyclonal antibody ELISA. Frozen NP aspirates were serially diluted and examined for the 66K mol. wt. fusion glycoprotein (F), the 84K large surface glycoprotein (G) and the 41K nucleoprotein (N) by monoclonal capture ELISA. F protein was detected in all 43 specimens, G protein was detectable in 20 (47%) and N protein in 22 (51%) of 43 NP aspirates. In specimens with detectable G and N proteins, F was detected by endpoint titration at approximately tenfold greater dilutions than either G or N. In 19 sequential NP aspirates from five patients with RSV infection, F was present in higher titre throughout infection. In 20 cases, matching cell culture isolates were examined by immunofluorescence with strain-specific monoclonal antibodies. Three of 20 isolates showed strain-specific differences by their lack of reaction with anti-G monoclonal antibody. Titration of the 20 cell culture isolates by monoclonal antibody capture ELISA showed the relative amount of F and N proteins to be equal in all cases, whereas levels of G protein tended to be slightly lower. Reconstruction experiments with NP aspirates demonstrated that degradation of F and N proteins did not occur in NP aspirates, but that G protein antigenicity appeared to be affected by nasal secretions. When compared with cell culture-grown material, nasal secretions contained abundant F protein but a surprisingly low concentration of N protein.

摘要

开发了一种间接酶联免疫吸附测定法(ELISA),该方法使用单克隆抗体作为固相免疫吸附剂来检测呼吸道合胞病毒(RSV)的特定多肽。该测定法用于检测43份来自RSV阳性婴儿的鼻咽(NP)吸出物,这些吸出物之前已通过培养、直接免疫荧光和多克隆抗体ELISA检测过RSV。将冷冻的NP吸出物进行系列稀释,并通过单克隆捕获ELISA检测66K分子量的融合糖蛋白(F)、84K大表面糖蛋白(G)和41K核蛋白(N)。在所有43份标本中均检测到F蛋白,在43份NP吸出物中的20份(47%)可检测到G蛋白,22份(51%)可检测到N蛋白。在可检测到G和N蛋白的标本中,通过终点滴定法检测到F的稀释倍数比G或N大约高十倍。在来自5名RSV感染患者的19份连续NP吸出物中,F在整个感染过程中均以较高滴度存在。在20例病例中,用菌株特异性单克隆抗体通过免疫荧光检查匹配的细胞培养分离株。20株分离株中有3株因与抗G单克隆抗体无反应而显示出菌株特异性差异。通过单克隆抗体捕获ELISA对20株细胞培养分离株进行滴定显示,在所有情况下F和N蛋白的相对量相等,而G蛋白水平往往略低。用NP吸出物进行的重建实验表明,NP吸出物中未发生F和N蛋白的降解,但G蛋白抗原性似乎受到鼻分泌物的影响。与细胞培养生长的材料相比,鼻分泌物中含有丰富的F蛋白,但N蛋白浓度出奇地低。

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