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New approach in RNA quantification using arginine-affinity chromatography: potential application in eukaryotic and chemically synthesized RNA

机译:使用精氨酸亲和色谱法进行RNA定量的新方法:在真核和化学合成RNA中的潜在应用

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摘要

The knowledge of RNA’s role in biological systems and the recent recognition of its potential use as a reliable biotherapeutic tool increase the demand for development and validation of analytical methods for accurate analysis of RNA. Affinity chromatography is a unique technique because of the versatility of applications reliant on the affinity ligand used. Recently, an arginine-based matrix has been effectively applied in the purification of RNA because of the specific recognition mechanism for RNA molecules. This interaction is suggested to be due to the length of arginine side chain and its ability to produce good hydrogen bonding geometries, which promote multi-contact with RNA backbone or RNA bases, based on RNA folding. Thus, this work presents the development and validation of an analytical method with ultraviolet detection for the quantification of RNA using affinity chromatography with arginine amino acid as immobilized ligand. The method was validated according to International and European legislation for bioanalytical methods. The results revealed that the proposed method is suitable for the reliable detection, separation, and quantification of RNA, showing that the method is precise and accurate for concentrations up to 200 ng/μL of RNA. Furthermore, the versatility of the methodology was demonstrated by its applicability in the quantification of RNA from different eukaryotic cells and in crude samples of chemically synthesized RNA. Therefore, the proposed method demonstrates a potential multipurpose applicability in molecular biology RNA-based analysis and RNA therapeutics.
机译:对RNA在生物系统中的作用的了解以及对RNA作为一种可靠的生物治疗工具的潜在用途的最新认识增加了对开发和验证用于精确分析RNA的分析方法的需求。亲和色谱法是一种独特的技术,因为其应用的多样性取决于所使用的亲和配体。近来,基于精氨酸的基质由于对RNA分子的特异性识别机制而被有效地用于RNA的纯化。认为这种相互作用是由于精氨酸侧链的长度及其产生良好的氢键几何结构的能力,该结构基于RNA折叠促进与RNA主链或RNA碱基的多次接触。因此,这项工作提出了使用精氨酸作为固定配体的亲和层析,通过紫外检测定量RNA的分析方法的开发和验证。该方法已根据国际和欧洲法规对生物分析方法进行了验证。结果表明,该方法适用于RNA的可靠检测,分离和定量,表明该方法对于浓度高达200 ng /μL的RNA是精确而准确的。此外,该方法的多功能性通过其在定量来自不同真核细胞和化学合成RNA的粗样品中的RNA的适用性得到证明。因此,提出的方法证明了在分子生物学基于RNA的分析和RNA治疗方法中潜在的多用途性。

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