检测日本脑炎病毒特异性抗体反应的检测方法的建立和验证。
Development and validation of an assay for detection of Japanese encephalitis virus specific antibody responses.
机构信息
General Sir John Kotelawala Defence University, Colombo, Sri Lanka.
Centre for Dengue Research, University of Sri Jayewardenepura, Nugegoda, Sri Lanka.
出版信息
PLoS One. 2020 Oct 28;15(10):e0238609. doi: 10.1371/journal.pone.0238609. eCollection 2020.
INTRODUCTION
Although immune responses to the Japanese Encephalitis virus (JEV), and the dengue viruses (DENV) have a potential to modulate the immune responses to each other, this has been poorly investigated. Therefore, we developed an ELISA to identify JEV specific, DENV non cross-reactive antibody responses by identifying JEV specific, highly conserved regions of the virus and proceeded to investigate if the presence of JEV specific antibodies associate with dengue disease severity.
METHODOLOGY AND RESULTS
22 JEV specific peptides were identified from highly conserved regions of the virus and the immunogenicity and specificity of these peptides were assessed in individuals who were non-immune to JEV and DENV (JEV-DENV-, N = 30), those who were only immune to the JEV and not DENV (JEV+DENV-, N = 30), those who were only immune to DENV(JEV-DENV+, N = 30) and in those who were immune to both viruses (JEV+DENV+, N = 30). 7/22 peptides were found to be highly immunogenic and specific and these 7 peptides were used as a pool to further evaluate JEV-specific responses. All 30/30 JEV+DENV- and 30/30 JEV+DENV+ individuals, and only 3/30 (10%) JEV-DENV+ individuals responded to this pool. We further evaluated this pool of 7 peptides in patients following primary and secondary dengue infection during the convalescent period and found that the JEV-specific peptides, were unlikely to cross react with DENV IgG antibodies. We further compared this in-house ELISA developed with the peptide pool with an existing commercial JEV IgG assay to identify JEV-specific IgG following vaccination, and our in-house ELISA was found to be more sensitive. We then proceeded to investigate if the presence of JEV-specific antibodies were associated with dengue disease severity, and we found that those who had past severe dengue (n = 175) were significantly more likely (p<0.0001) to have JEV-specific antibodies than those with past non-severe dengue (n = 175) (OR 5.3, 95% CI 3.3 to 8.3).
CONCLUSIONS
As our data show that this assay is highly sensitive and specific for detection of JEV-specific antibody responses, it would be an important tool to determine how JEV seropositivity modulate dengue immunity and disease severity when undertaking dengue vaccine trials.
简介
尽管日本脑炎病毒(JEV)和登革热病毒(DENV)的免疫反应有相互调节的潜力,但这一点尚未得到充分研究。因此,我们开发了一种 ELISA 来鉴定 JEV 特异性、DENV 非交叉反应性抗体反应,方法是鉴定 JEV 病毒高度保守区域的 JEV 特异性肽,并进一步研究 JEV 特异性抗体的存在是否与登革热疾病严重程度相关。
方法和结果
从病毒的高度保守区域鉴定了 22 个 JEV 特异性肽,评估了这些肽在对 JEV 和 DENV 无免疫力的个体(JEV-DENV-,N=30)、仅对 JEV 有免疫力而不对 DENV 有免疫力的个体(JEV+DENV-,N=30)、仅对 DENV 有免疫力而不对 JEV 有免疫力的个体(JEV-DENV+,N=30)和对两种病毒均有免疫力的个体(JEV+DENV+,N=30)中的免疫原性和特异性。发现 7/22 个肽高度免疫原性和特异性,将这 7 个肽作为一个池进一步评估 JEV 特异性反应。所有 30/30 JEV+DENV-和 30/30 JEV+DENV+个体,以及仅 30/30 JEV-DENV+个体(10%)对该池有反应。我们进一步在原发性和继发性登革热感染后的恢复期患者中评估了这 7 个肽的池,并发现 JEV 特异性肽不太可能与 DENV IgG 抗体发生交叉反应。我们进一步将这种基于肽池的内部 ELISA 与现有的商业 JEV IgG 检测进行比较,以确定疫苗接种后的 JEV 特异性 IgG,结果发现内部 ELISA 更敏感。然后,我们研究了 JEV 特异性抗体的存在是否与登革热疾病严重程度相关,发现过去患有严重登革热(n=175)的个体比过去患有非严重登革热(n=175)的个体(OR 5.3,95%CI 3.3 至 8.3)更有可能具有 JEV 特异性抗体。
结论
由于我们的数据表明,该检测方法对 JEV 特异性抗体反应具有高度的敏感性和特异性,因此在进行登革热疫苗试验时,它将是一种确定 JEV 血清阳性如何调节登革热免疫和疾病严重程度的重要工具。
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