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通过环介导等温扩增检测病原体特异性抗体。

Detection of pathogen-specific antibodies by loop-mediated isothermal amplification.

作者信息

Burbulis Ian E, Yamaguchi Kumiko, Nikolskaia Olga V, Prigge Sean T, Magez Stefan, Bisser Sylvie, Reller Megan E, Grab Dennis J

机构信息

VTT/MSI Molecular Sciences Institute, Berkeley, California, USA.

Department of Pathology, The Johns Hopkins University School of Medicine, Baltimore, Maryland, USA.

出版信息

Clin Vaccine Immunol. 2015 Apr;22(4):374-80. doi: 10.1128/CVI.00811-14. Epub 2015 Feb 4.

DOI:10.1128/CVI.00811-14
PMID:25651920
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4375353/
Abstract

Loop-mediated isothermal amplification (LAMP) is a method for enzymatically replicating DNA that has great utility for clinical diagnosis at the point of care (POC), given its high sensitivity, specificity, speed, and technical requirements (isothermal conditions). Here, we adapted LAMP for measuring protein analytes by creating a protein-DNA fusion (referred to here as a "LAMPole") that attaches oligonucleotides (LAMP templates) to IgG antibodies. This fusion consists of a DNA element covalently bonded to an IgG-binding polypeptide (protein L/G domain). In our platform, LAMP is expected to provide the most suitable means for amplifying LAMPoles for clinical diagnosis at the POC, while quantitative PCR is more suitable for laboratory-based quantification of antigen-specific IgG abundance. As proof of concept, we measured serological responses to a protozoan parasite by quantifying changes in solution turbidity in real time. We observed a >6-log fold difference in signal between sera from vaccinated versus control mice and in a clinical patient sample versus a control. We assert that LAMPoles will be useful for increasing the sensitivity of measuring proteins, whether it be in a clinical laboratory or in a field setting, thereby improving acute diagnosis of a variety of infections.

摘要

环介导等温扩增技术(LAMP)是一种通过酶促反应复制DNA的方法,鉴于其高灵敏度、特异性、速度以及技术要求(等温条件),在即时医疗(POC)的临床诊断中具有很大的实用性。在此,我们通过创建一种蛋白质-DNA融合体(在此称为“LAMPole”),将寡核苷酸(LAMP模板)连接到IgG抗体上,从而使LAMP适用于蛋白质分析物的检测。这种融合体由一个与IgG结合多肽(蛋白L/G结构域)共价结合的DNA元件组成。在我们的平台中,LAMP有望为在POC进行临床诊断时扩增LAMPole提供最合适的方法,而定量PCR更适合基于实验室对抗原特异性IgG丰度的定量分析。作为概念验证,我们通过实时定量溶液浊度的变化来测量对原生动物寄生虫的血清学反应。我们观察到,接种疫苗的小鼠血清与对照小鼠血清之间以及临床患者样本与对照样本之间的信号差异超过6个对数级。我们断言,LAMPole将有助于提高蛋白质检测的灵敏度,无论是在临床实验室还是在现场环境中,从而改善对各种感染的急性诊断。

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