柱层析纯化犬腺病毒1型抗原包被间接酶联免疫吸附试验的建立

Q4 Immunology and Microbiology Journal of Bacteriology and Virology Pub Date : 2020-03-01 DOI:10.4167/jbv.2020.50.1.017
Dong-Kun Yang, Ha-Hyun Kim, Siu Lee, Miryeon Ji, Bokhee Han, Soobin Oh, B. Hyun
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引用次数: 1

摘要

犬腺病毒1型(CAV-1)会导致犬科成员(包括狗)感染性肝炎。检测CAV-1抗体的间接酶联免疫吸附试验(I-ELISA)是狗血清大通量测试所必需的。我们在2016年2月至2018年10月期间从忠北省和庆北省的狗身上采集了165份血清样本。韩国CAV-1疫苗株CAV1V在Madin–Darby犬肾(MDCK)细胞中繁殖,并通过Nuvia cPrime阴离子交换色谱纯化;该病毒作为I-ELISA抗原。使用病毒中和(VN)方法测量狗血清中的病毒中和抗CAV-1滴度。使用纯化的CAV-1抗原和血清样品优化I-ELISA。该试剂盒用于评估狗血清。比较VN和I-ELISA数据。与VN测定相比,I-ELISA的敏感性、特异性和准确性分别为97.0%、74.2%和92.7%。I-ELISA数据与VN的数据显著相关(r=0.88)。这些结果表明I-ELISA可用于犬血清中CAV-1的血清监测。链霉素(100μg/mL)和抗真菌两性霉素B(0.25μg/mL。CAV-1的CAV1V株,即韩国使用的CAV-1疫苗,被用作病毒抗原。2016年至2018年,共从居住在忠北省和庆北省的狗身上采集了165份血清样本,并在每次测试中使用了这些血清。我们不知道这些狗是否接种了CAV疫苗。在接种后5天检查细胞病变效应(CPE)(DPI)。CAV-1的病毒中和抗体(VNA)滴度是完全抑制CPE的最高血清稀释度的倒数。每个血清样品从1:2稀释到1:256。VNA滴度≥1:2被认为是阳性。使用稀释度为1:20至1:40960的血清板样品在37°C下测定1小时的适当浓度。接下来,将100µL量的抗狗IgG辣根过氧化物酶(HRP)缀合物(KPL,Gaithersburg,MD,USA)添加到微孔板的所有孔中,在上述温度下孵育1小时。洗涤后,将50µL量的2'-2-嗪基双-(3-乙基苯并噻唑啉)底物(ABTS)溶液加入平板中,然后在室温下孵育10分钟。最后,加入停止溶液(1.0%w/v十二烷基硫酸钠)以停止反应。I-ELISA的吸光度在分光光度计(Sunrise ELISA读取器;Tecan,瑞士)中在405nm处测量。在优化的I-ELISA条件下,将在稀释缓冲液(PBS中的1%[w/v]脱脂乳)中稀释100倍的100µL血清加入到包被CAV1V抗原的96孔微孔板中。在37℃孵育1小时后,用含有0.05%吐温20(PBST)的PBS洗涤平板,并与在稀释缓冲液中稀释4000倍的100µL抗狗IgG HRP缀合物在37℃下孵育1 h。洗涤后,将50µL ABTS底物溶液和50µL终止溶液(1.0%[w/v]十二烷基硫酸钠)添加到微孔板的所有孔中。表现出吸收性大于0.4的临界值的血清样品被评价为阳性。I-ELISA的特异性、敏感性和准确性如前所述(15)。
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Development of an Indirect ELISA Featuring Plates Coated with Column Chromatographically Purified Canine Adenovirus Type-1 Antigen
Canine adenovirus type 1 (CAV-1) causes infectious hepatitis in members of the family Canidae, including dogs. An indirect enzyme-linked immunosorbent assay (I-ELISA) that detects CAV-1 antibodies is required for large-throughput tests of dog sera. We collected 165 serum samples from dogs of Chungbuk and Gyeongbuk provinces between February 2016 and October 2018. The Korean CAV-1 vaccine strain CAV1V was propagated in Madin – Darby canine kidney (MDCK) cells and purified via Nuvia cPrime anion-exchange chromatography; the virus served as an I-ELISA antigen. Virus-neutralizing anti-CAV-1 titers in dog sera were measured using the virus neutralization (VN) method. The I-ELISA was optimized using purified CAV-1 antigen and serum samples. This kit was used to evaluate dog sera. The VN and I-ELISA data were compared. The sensitivity, specificity, and accuracy of the I-ELISA were 97.0%, 74.2%, and 92.7% compared to the VN assay, respectively. The I-ELISA data significantly correlated with those of VN (r = 0.88). These results suggest that the I-ELISA is useful for serosurveillance of CAV-1 in dog sera. streptomycin (100 μ g/mL), and the antimycotic amphotericin B (0.25 μ g/mL) at 37 ° C under 5% (v/v) CO 2 , and used for viral antigen production and serological assay. The CAV1V strain of CAV-1, which is the CAV-1 vaccine used in Korea, was employed as a viral antigen. A total of 165 serum samples were collected from dogs residing in Chungbuk and Gyeongbuk provinces from 2016 to 2018, and the sera were used in each test. We do not know if the dogs had been inoculated with the CAV vaccine. checked for cytopathic effect (CPE) over 5 days post inoculation (DPI). The virus-neutralizing antibody (VNA) titer of CAV-1 was the reciprocal of the highest serum dilution that completely inhibited the CPE. Each serum sample was diluted from 1:2 to 1:256. A VNA titer ≥ 1:2 was considered positive. serum panel samples at dilutions of 1:20 to 1:40,960, were used to determine the appropriate concentrations at 37 ° C for 1 h. Next, 100 µ L amounts of anti-dog IgG horseradish peroxidase (HRP) conjugate (KPL, Gaithersburg, MD, USA) were added to all well of the microplate, which was incubated for 1 h at the above temperature. After washing, 50 µ L amounts of 2 ’ 2-azino-bis-(3-ethylbenzothiazoline) substrate (ABTS) solution were added to the plate, which was then incubated for 10 min at room temperature. Finally, stop solution (1.0% w/v sodium dodecyl sulfate) were added to stop the reaction. The absorbance of the I-ELISA was measured at 405 nm in a spectrophotometer (Sunrise ELISA reader; Tecan, Switzerland). Under the optimized I-ELISA conditions, 100 µ L serum diluted 100-fold in dilution buffer (1% [w/v] skim milk in PBS) was added to a 96-well microplate coated with CAV1V antigen. After incubation at 37 ° C for 1 h, the plate was washed with PBS containing 0.05% Tween 20 (PBST) and incubated with 100 µ L anti-dog IgG HRP conjugate diluted 4,000-fold in dilution buffer for 1 h at 37 ° C. After washing, 50 µ L ABTS substrate solution and 50 µ L stop solution (1.0% [w/v] sodium dodecyl sulfate) were added to all wells of the microplate. Serum samples exhibiting absorbances greater than the cutoff of 0.4 were evaluated as positive. The specificity, sensitivity, and accuracy of the I-ELISA were determined as previously reported (15).
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来源期刊
Journal of Bacteriology and Virology
Journal of Bacteriology and Virology Immunology and Microbiology-Immunology
CiteScore
0.80
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发文量
16
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