利用微流控分析开发可靠和经济的核酸应用技术,利用MicroRNAs在低资源环境下诊断筛查人类粪便中的结肠癌

F. Ahmed, M. Gouda, Nancy C. Ahmed
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引用次数: 1

摘要

采用公开市场上易于获得的廉价供应品的分离方法,既可靠又经济,例如在低资源研究环境(LRRS)中基于微流体技术的核酸扩增技术(NAAT),符合ASSURED指南,对于开发使用微(mi)RNA分子在粪便中进行无创诊断结肠癌筛查至关重要。将基于微流体的MiRNA粪便检测与可靠的滚动圈扩增/检测方法相结合,用于MiRNA分子的定量,产生了一种经济、敏感、特异的等温方法,用于lrs中MiRNA的无创定量检测。科学家和工程师们已经对mirna产生了兴趣,他们已经加强了他们的努力,将新兴的简单检测工具应用于量化这些18- 26nt长的小分子的重要生物分析挑战。一些提议的方法结合了新材料,如简单的离心机和基于微流控技术的方法,而另一些则利用这些分子的有趣的生物学特性,如形成分支RCA结构,允许在原子摩尔“aM”浓度水平上检测这些生物标记分子,在LRRS中使用低成本提取和等温扩增方法。我们一直对研究结直肠癌(CRC)很感兴趣,因为它是世界上第三大最常见的恶性肿瘤,并且可以从患者身上无创性地获得粪便。我们的研究重点是结肠癌(CC),因为它在美国比直肠癌(RC)更常见。我们方法的创新之处在于在LRRS的非侵入性粪便样本中探索性地使用价格合理的定量miRNA分析,其提取的易碎总RNA在粪便排泄后不久由市买试剂盒稳定,因此它不会破碎,然后进行定量标准化分析测试,既不需要劳动密集型,也不需要昂贵的仪器。为了开发一组新的miRNA基因,用于早期左、右散发性结肠癌的无创诊断筛查,比目前市场上任何其他结肠癌筛查方法都更经济,并且具有更高的敏感性和特异性。为了显示在LRRS中使用简单方法所提出的定量miRNA测试的临床敏感性和特异性,miRNA结果将与FOBT、结肠镜检查和病理数据相关联。标准化建立了检测的性能标准(样品选择,最佳样品运行条件,保存和储存),以确保在任何实验室,任何训练有素的人员,在全球任何地方资源匮乏的实验室环境中,检测都能以相同的方式进行。
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Use of Microfluidic Assays to Develop Reliable and Economic Nucleic Acid Application Technologies, Employing MicroRNAs for the Diagnostic Screening of Colon Cancer in Human Stool in Low-Resource Settings
Isolation methods that employ readily-available inexpensive supplies on the open market, which are reliable, as well as economical, such as nucleic acid amplification techniques (NAAT) based on microfluidic technology in low-resource research settings (LRRS) that meets the ASSURED guidelines are essential to develop a noninvasive diagnostic colon cancer screen in stool using micro(mi)RNA molecules. A combination of a microfluidic-based MiRNA stool test with a reliable rolling circle amplification/detection method applied to the quantification of miRNA molecules, result in an affordable sensitive and specific isothermal method for the noninvasive quantitative detection of miRNAs in LRRS. Scientists and engineers have become interested in miRNAs, and they have intensified their efforts to apply emerging simple detection tools to the important bioanalytical challenge of quantifying these small 18-26 nt long molecules. Some of the proposed approaches incorporate novel material, such as simple centrifuges and methods based on microfluidic technology, while others utilize the interesting biological properties of these molecules, such as forming branched RCA structures, allowing for the detection of these biomarker molecules at an attomolar "aM" concentration level, using low cost extraction and isothermal amplification methods in LRRS. We have been interested in studying colorectal cancer (CRC) because it is the 3rd most common malignancy worldwide, and stool can be obtained noninvasively from the patients. We have focused in this research on colon cancer (CC) because it is more common in the USA than rectal cancer (RC). The innovation of our approach lies in the exploratory use of an affordable, quantitative miRNA profiling in noninvasive stool samples in LRRS, whose extracted fragile total RNA is stabilized shortly after excretion from stool by commercially available kits, so it does not ever fragment, followed by quantitative standardized analytical tests that are neither labor intensive, nor require expensive instrumentation, in order to develop apanel of novel miRNA genes for the noninvasive diagnostic screening of early left and right sporadic colon cancers, more economically, and with higher sensitivity and specificity than any other colon cancer screening test currently available on the market. To show the clinical sensitivity and specificity of the proposed quantitative miRNA test using simple methodologies in LRRS,the miRNA results are to be correlated with FOBT, colonoscopy, and pathology data. Standardization establishes test’s performance criteria (sample selection, optimal sample running conditions, preservation and storage), in order to ensure that the assay will perform the same way in any laboratory, by any trained personnel, anywhere in low-resource laboratory settings worldwide.
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