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用于从复杂生物流体中提取扩增就绪核酸的有限资源可制备壳聚糖磁性颗粒。

Limited-resource preparable chitosan magnetic particles for extracting amplification-ready nucleic acid from complex biofluids.

机构信息

Department of Chemistry, Bennett University, Greater Noida, Uttar Pradesh 201310, India.

Department of Medicine, Medical College and Hospital, Kolkata, West Bengal, India.

出版信息

Analyst. 2021 Dec 20;147(1):165-177. doi: 10.1039/d1an01150b.

Abstract

Extraction and concentration of pure nucleic acid from complex biofluids are the prerequisite for nucleic acid amplification test (NAAT) applications in pathogen detection, biowarfare prevention, and genetic diseases. However, conventional spin-column mediated nucleic acid extraction is constricted by the requirement for costly power-intensive centralized lab infrastructure, making it unsuitable for limited-resource settings. Significant progress in lab-on-a-chip devices or cartridges (, Cepheid GeneXpert®) that integrate nucleic acid extraction and amplification has been made, but these approaches either require additional equipment or are costly. Similarly, their complexities make them difficult to fabricate in low-resource settings by the end-user themselves. The application of magnetic particles such as silica-coated iron oxide beads for nucleic acid extraction is relatively instrument-free, rapid, user-friendly, and amenable to automation. But, they rely on hazardous chaotropic salt chemistry and ethanol desalting that could limit their efficacy for downstream NAATs. Recent advances in several types of novel material (, polyamine) coated magnetic bead-based chaotropic salt-free extraction methods offer a possible solution to this problem. However, these materials also involve multistep synthesis impermissible in limited-resource settings. To offer a possible instrument-free magnetic particle-based nucleic acid extraction doable at limited-resource settings, we investigated the nucleic acid capture ability of two chitosan-coated magnetic particles that are preparable by minimally trained personnel using only a water bath and a magnetic stirrer within 6-8 h. We quantitatively probed the efficiency of the passive (without any electrical shaking or vortex-aided) DNA magnetocapture (, binding to chitosan magnetic particles, physical separation from its sample of origin, and release from the particles) using UV. To explore their suitability towards clinically relevant sensitive downstream NAATs, 100-1000 copies (, in the order of zeptomole) of () or human genomic DNA from aqueous solution, crude cell lysate, and fetal bovine serum were extracted by them and then successfully detected using quantitative real-time loop-mediated isothermal amplification (LAMP) or real-time polymerase chain reaction (PCR). Alongside, their suitability with gel-based LAMP, colorimetric LAMP, and (on beads) LAMP was also probed. The required optimization of the amplification methods has been discussed. Overall, the turnaround time for the magnetocapture combined with NAAT was 1.5-2 h and is thus expected to aid in rapid clinical decision making. With the ease of preparation, reproducibility, and compatibility with downstream NAATs, we anticipate that these magnetic particles would facilitate the expansion and decentralization of nucleic acid-based diagnosis for limited-resource settings.

摘要

从复杂的生物流体中提取和浓缩纯核酸是核酸扩增测试 (NAAT) 应用于病原体检测、生物战预防和遗传疾病的前提。然而,传统的基于离心柱的核酸提取受到昂贵的、需要大量电力的集中式实验室基础设施的限制,因此不适合资源有限的环境。在微流控芯片设备或试剂盒(例如 Cepheid GeneXpert®)中已经取得了核酸提取和扩增的重大进展,但这些方法要么需要额外的设备,要么成本高昂。同样,它们的复杂性使得它们难以由最终用户在资源有限的环境中自行制造。用于核酸提取的磁性颗粒(如硅涂层氧化铁珠)的应用相对无仪器、快速、用户友好且适合自动化。但是,它们依赖于危险的离液盐化学和乙醇脱盐,这可能会限制它们在下游 NAAT 中的效果。几种新型材料(例如多胺)涂覆的基于磁性珠的无离液盐提取方法的最新进展为解决这个问题提供了可能的解决方案。然而,这些材料也涉及多步合成,这在资源有限的环境中是不允许的。为了提供一种在资源有限的环境中可行的、无仪器的基于磁性颗粒的核酸提取方法,我们研究了两种壳聚糖涂覆的磁性颗粒的核酸捕获能力,这两种磁性颗粒可以由经过最少培训的人员在 6-8 小时内使用水浴和磁力搅拌器制备。我们使用 UV 定量探测了 DNA 磁捕获的效率(即无需任何电振动或涡旋辅助)(结合到壳聚糖磁性颗粒上、从其原始样品中物理分离以及从颗粒上释放)。为了探索它们在临床相关的敏感下游 NAAT 中的适用性,我们用它们从水溶液、粗细胞裂解物和胎牛血清中提取了 100-1000 个拷贝(在飞摩尔范围内)()或人基因组 DNA,并成功地使用定量实时环介导等温扩增 (LAMP) 或实时聚合酶链反应 (PCR) 进行了检测。同时,还探测了它们与凝胶基 LAMP、比色 LAMP 和(在珠子上)LAMP 的适用性。已经讨论了扩增方法的优化需求。总体而言,磁捕获与 NAAT 的组合时间为 1.5-2 小时,因此有望有助于快速临床决策。由于制备简便、重现性好且与下游 NAAT 兼容,我们预计这些磁性颗粒将促进资源有限环境中基于核酸的诊断的扩展和分散。

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