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首页> 外文期刊>Analytica chimica acta >Self-assembling protein platform for direct quantification of circulating microRNAs in serum with total internal reflection fluorescence microscopy
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Self-assembling protein platform for direct quantification of circulating microRNAs in serum with total internal reflection fluorescence microscopy

机译:自组装蛋白平台,可通过全内反射荧光显微镜直接定量检测血清中的循环微RNA

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摘要

MicroRNA (miRNA) has recently emerged as a new and important class of cellular regulators. Strong evidences showed that aberrant expression of miRNA is associated with a broad spectrum of human diseases, such as cancer, diabetes, cardiovascular and psychological disorders. However, the short length and low abundance of miRNA place great challenges for conventional techniques in the miRNA quantification and expression profiling. Here, we report a direct, specific and highly sensitive yet simple detection assay for miRNA without sample amplification. A self-assembled protein nanofibril acted as an online pre-concentrating sensor to detect the target miRNA. Locked nucleic acid (LNA) of complimentary sequence was served as the probe to capture the target miRNA analyte. The quantification was achieved by the fluorescence intensity measured with total internal reflection fluorescence microscopy. A detection limit of 1 pM was achieved with trace amount of sample consumption. This assay showed efficient single-base mismatch discrimination. The applicability of quantifying circulating mir-196a in both normal and cancer patient's serums was also demonstrated.
机译:MicroRNA(miRNA)最近已经成为一种新的重要的细胞调节剂。有力的证据表明,miRNA的异常表达与多种人类疾病有关,例如癌症,糖尿病,心血管和心理疾病。但是,miRNA的短长度和低丰度对miRNA定量和表达谱分析中的常规技术提出了巨大挑战。在这里,我们报告了无需样品扩增的miRNA的直接,特异性和高灵敏度但简单的检测方法。自组装的蛋白质纳米原纤维充当在线预浓缩传感器,以检测目标miRNA。互补序列的锁定核酸(LNA)用作捕获目标miRNA分析物的探针。通过用全内反射荧光显微镜法测量的荧光强度实现定量。痕量样品消耗实现了1 pM的检测限。该测定法显示有效的单碱基错配鉴别。还证明了在正常和癌症患者血清中定量循环mir-196a的适用性。

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