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Development of a simple and quick immunochromatography method for detection of anti-HPV-16/-18 antibodies

机译:开发一种用于检测抗HPV-16 / -18抗体的简单快速的免疫色谱方法

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摘要

Immunochromatography (IC) is widely used to detect target molecules in biological fluids. Since this method can be performed without a special technique or device, IC is a convenient way to assess the existence of antibodies or pathogens such as viruses and bacteria, simply and quickly. In this study, we established an IC method to detect serum antibodies against oncogenic human papillomavirus (HPV)-16 and HPV-18 L1 proteins using recombinant L1 proteins produced by silkworms as antigens. Infection of oncogenic HPVs is a major risk factor of cervical cancer, which is one of the most common cancers in women worldwide. We first measured blood sera of two groups by magnetic beads enzyme-linked immunosorbent assay (MB-ELISA). For the first group, sera were collected prospectively from young women who planned to receive HPV vaccination. The second group consisted of children under 20 years of age, non-vaccinated healthy women, vaccinated healthy women, dysplasia, cervical intraepithelial neoplasia III, and cervical cancer patients. We confirmed that standard vaccination doses significantly increased serum HPV antibody concentrations, and the level was sustained at least more than 30 months after vaccination. In contrast, an increase in antibody concentration was not observed in patients with precancerous cervical changes and cervical cancer. We next measured the samples in both groups using the IC method we originally developed, and found that the measurement values of IC highly correlated with those of MB-ELISA. The simple and quick IC method would be a useful tool for rapid monitoring of L1 specific antibody levels in a non-laboratory environment. With less than one drop of serum, our IC can easily detect serum HPV-16/-18 antibodies within 15 minutes, without the need for electronic devices or techniques.
机译:免疫色谱法(IC)被广泛用于检测生物流体中的目标分子。由于无需特殊技术或设备即可执行此方法,因此IC是一种简便,快捷地评估抗体或病原体(例如病毒和细菌)的存在的方法。在这项研究中,我们建立了一种IC方法,以家蚕产生的重组L1蛋白为抗原来检测针对致癌性人乳头瘤病毒(HPV)-16和HPV-18 L1蛋白的血清抗体。致癌性HPV感染是宫颈癌的主要危险因素,宫颈癌是全世界女性中最常见的癌症之一。我们首先通过磁珠酶联免疫吸附测定(MB-ELISA)测量了两组的血液血清。对于第一组,前瞻性地从计划接受HPV疫苗接种的年轻女性中收集血清。第二组包括20岁以下的儿童,未接种疫苗的健康女性,接种疫苗的健康女性,发育不良,宫颈上皮内瘤变III和宫颈癌患者。我们确认标准疫苗接种剂量显着增加了血清HPV抗体浓度,并且该水平在疫苗接种后至少持续了30个月以上。相反,在癌前期宫颈改变和宫颈癌患者中未观察到抗体浓度的增加。接下来,我们使用最初开发的IC方法测量了两组中的样品,发现IC的测量值与MB-ELISA的测量值高度相关。简单快速的IC方法将是在非实验室环境中快速监测L1特异性抗体水平的有用工具。只需不到一滴血清,我们的IC即可在15分钟内轻松检测出血清HPV-16 / -18抗体,而无需电子设备或技术。

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