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Nucleic Acid Sample Preparation Using Spontaneous Biphasic Plug Flow

机译:自发双相塞流法制备核酸样品

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Nucleic acid (NA) extraction and purification has become a common technique in both research and clinical laboratories. Current methods require repetitive wash steps with a pipet that are laborious and time-consuming, making the procedure inefficient for clinical settings. We present here a simple technique that relies on spontaneous biphasic plug flow inside a capillary to achieve sample preparation. By filling the sample with oil, aqueous contaminants were displaced from the captured NA without pipetting wash buffers or use of external force and equipment. mRNA from mammalian cell culture was purified, and polymerase chain reaction (PCR) amplification showed similar threshold cycle values as those obtained from a commercially available kit. Human immunodeficiency virus (HIV) viral-like particles were spiked into serum and a 5-fold increase in viral RNA extraction yield was achieved compared to the conventional wash method. In addition, viral RNA was successfully purified from human whole blood, and a limit of detection of approximately 14 copies of RNA extracted per sample was determined. The results demonstrate the utility of the current technique for nucleic acid purification for clinical purposes, and the overall approach provides a potential method to implement nucleic acid testing in low-resource settings.
机译:核酸(NA)的提取和纯化已成为研究实验室和临床实验室的常用技术。当前的方法需要用移液管进行重复的洗涤步骤,这是费力且费时的,这使得该过程在临床环境中效率低下。我们在这里介绍一种简单的技术,该技术依赖于毛细管内部的自发双相塞流来实现样品制备。通过用油填充样品,无需移取洗涤缓冲液或使用外力和设备即可将水污染物从捕获的NA中移出。纯化了来自哺乳动物细胞培养物的mRNA,聚合酶链反应(PCR)扩增显示的阈值循环值与从市售试剂盒获得的阈值相似。将人免疫缺陷病毒(HIV)病毒样颗粒掺入血清中,与常规洗涤方法相比,病毒RNA提取率提高了5倍。另外,成功地从人全血中纯化了病毒RNA,并确定了每个样品中提取的RNA的大约14个拷贝的检测限。结果证明了当前技术用于临床目的核酸纯化的实用性,并且总体方法提供了一种在低资源环境下实施核酸测试的潜在方法。

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