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Development of Immunochromatographic Assay for Determination of Tetracycline in Human Serum

机译:免疫层析法测定人血清中四环素的进展

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摘要

Determining antibiotic concentration in human blood provides useful pharmacokinetic information. Commonly used methods such as ELISA require a long time to obtain results and thus cannot be applied when information is needed immediately. In this study, a novel antibody-based lateral flow technique was developed for tetracycline detection in human serum. Contrary to tests developed to analyze food samples, the features of work with serum as analyzed probe were studied for the first time here. The application of labeled and unlabeled specific antibodies was compared. For this purpose, specific and anti-species antibodies were labeled with gold nanoparticles and used for antigen–antibody interaction on the membrane surface with observed staining in the test zone. For both schemes, optimal conditions were established to provide the best sensitivity. The developed assay has a limit of visual detection as low as 35 and 11 ng/mL for the direct and indirect labeled antibodies, respectively. The limit of instrumental detection is from 0.4 to 3.5 ng/mL for diluted and undiluted sera. The use of indirect antibody labeling showed a small increase in sensitivity compared to traditional direct antibody labeling. The developed method showed no cross-reactivity with antibiotics of other classes. The method was used to test samples of serum. The results showed high correlation with the data obtained by ELISA (R2 = 0.98968). The assay provides a quick assessment of the amount of antibiotics in the blood and keeps them under control throughout the duration of therapy.
机译:测定人血中的抗生素浓度可提供有用的药代动力学信息。 ELISA等常用方法需要很长时间才能获得结果,因此在立即需要信息时无法应用。在这项研究中,开发了一种基于抗体的新型侧向流动技术,用于检测人血清中的四环素。与开发用于分析食物样品的测试相反,这里首次研究了以血清作为分析探针的工作特性。比较了标记的和未标记的特异性抗体的应用。为此,将特异性和抗物种抗体用金纳米颗粒标记,并用于膜表面的抗原-抗体相互作用,并在测试区域观察到染色。对于这两种方案,都建立了最佳条件以提供最佳灵敏度。对于直接和间接标记的抗体,开发的检测方法的视觉检测极限分别低至35和11 ng / mL。稀释和未稀释血清的仪器检测极限为0.4至3.5 ng / mL。与传统的直接抗体标记相比,间接抗体标记的使用显示出灵敏度的小幅提高。所开发的方法与其他种类的抗生素没有交叉反应。该方法用于测试血清样品。结果与酶联免疫吸附测定的数据高度相关(R 2 = 0.98968)。该测定法可快速评估血液中的抗生素数量,并在整个治疗过程中使它们保持受控状态。

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