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目的：建立基于核酸序列分析的快速、准确、低成本的甲型 H1N1 流感病毒检测方法。方法：通过优化焦测序反应体系中 ATP 硫酸化酶和荧光素酶的浓度，建立高灵敏的焦测序反应体系；将该体系应用于低成本、小型化的便携式生物发光分析仪，焦测序分析流感病毒 M、 NP、HA 基因片段的核酸序列。结果：优化后的焦测序反应体系可检测低至 10 fmol 的 DNA 样本，检测灵敏度较传统焦测序提高了 10 倍以上。对两例样本进行检测，根据所测得的 M、NP、 HA 基因特异性片段序列，可以确认其均为甲型 H1 N1 感染；另外，对 M2 蛋白阻断剂耐药性标志位点（ S31N 突变）的测定结果显示该病毒存在 S31N 突变，为 M2 蛋白阻断剂耐药型。结论：高灵敏焦测序体系结合便携式生物发光分析仪成功实现了对甲型 H1N1 流感病毒快速、准确的低成本检测。

英文摘要:

Objectivre:To establish a rapid, accurate and low-cost influenza A (H1 N1 ) virus detection method based on nucleic acid sequence analysis.Methods:A highly sensitive pyrosequencing system was establised by optimizing the concentrations of ATP sulfurylase and luciferase respectively; the nucleic acid sequences of M， NP， HA gene fragments of influenza virus were analysed with a low-cost and portable bioluminescence analyzer by coupling the highly sensitive pyrosequencing system.Results:Compared with conventional pyrosequencing system, the sensitivity of the proposed method increased more than 10 times, and as low as 1 0 fmol of DNA samples can be detected. Based on the pyrosequencing results of the M, NP, HA genes, we confirmed the infection of influenza A (H1 N1 ) virus in the two samples. The sequencing results of the gene coding M2 protein inhibitor drug resistance marker (S31N mutation) proved the presence of S31 N mutation, indicating that the virus is M2 protein inhibitor-resistant.Conclusion:A rapid, accurate and low-cost detection method of influenza A (H1N1 ) virus was established by combining the highly sensitive pyrosequencing system with a portable bioluminescence analyzer.

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