HPLC Retention Behavior of Oligonucleotides on an Anion-Exchange HPLC with a High Concentration of Urea

IF 1.2 4区 化学 Q4 BIOCHEMICAL RESEARCH METHODS Chromatographia Pub Date : 2023-11-04 DOI:10.1007/s10337-023-04291-y
Kunio Kawamura, Yoshimi Maruoka
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Abstract

Roles of short RNA molecules in the emergence process of primitive life-like system and physiological activities have been extensively studied from the viewpoint of both fundamental and applicational areas. The discovery of catalytic functions of short RNA molecules suggests that the most primitive life-like systems have emerged from a chemical network consisting of short functional RNA molecules that existed. However, the quantitative analysis of such short RNA, including ribozymes, micro-RNA, and small non-coding RNA consisting of less than approximately 100 nucleotide units is difficult to perform using conventional techniques, such as gel electrophoresis (GE) and high-performance liquid chromatography (HPLC). Both GE and HPLC are complementarily used for different purposes related to oligonucleotide analysis. Recently, the HPLC method’s usefulness with a high urea concentration has been demonstrated for short oligonucleotides. In this study, the HPLC separation behavior in the presence of a high urea concentration is studied using a Tosoh DNA-NPR anion-exchange column (diameter 2.0 mm, length 100 mm along with a guard column) with a buffer containing 0.02 M Tris and 7.5 M urea at pH 9.0 and a buffer containing 1.5 M NaCl, 0.02 M Tris, and 7.5 M urea at pH 9.0 mixed with a linear gradient at a flow rate of 0.15 mL min−1 at 35 °C. Different sequences of oligonucleotides are collected to know how the influence of secondary structure formation can be reduced. Molecular modeling of the secondary structure is applied to evaluate the HPLC retention behaviors of oligonucleotides on an anion-exchange column. This study provides valuable information for selecting the elution conditions for separating the RNA and DNA oligonucleotides and preheating treatment.

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高浓度尿素阴离子交换高效液相色谱法的寡核苷酸保留行为
短 RNA 分子在原始类生命系统的产生过程和生理活动中的作用已从基础和应用两个领域得到广泛研究。短 RNA 分子催化功能的发现表明,最原始的类生命系统是由存在的短功能 RNA 分子组成的化学网络产生的。然而,使用凝胶电泳(GE)和高效液相色谱(HPLC)等传统技术很难定量分析这类短 RNA,包括核酶、微 RNA 和由小于约 100 个核苷酸单位组成的小型非编码 RNA。凝胶电泳和高效液相色谱可互补使用,用于与寡核苷酸分析相关的不同用途。最近,HPLC 方法在高尿素浓度下对短寡核苷酸的实用性已得到证实。本研究使用 Tosoh DNA-NPR 阴离子交换柱(直径 2.0 mm,长 100 mm,带保护柱),在 pH 9.0、含 0.02 M Tris 和 7.5 M 尿素的缓冲液中,以及在 pH 9.0、含 1.5 M NaCl、0.02 M Tris 和 7.5 M 尿素的缓冲液中,以 0.15 mL/min-1 的流速、线性梯度进行分离,研究了高浓度尿素存在下的 HPLC 分离行为。收集不同序列的寡核苷酸,以了解如何减少二级结构形成的影响。二级结构的分子建模被用于评估寡核苷酸在阴离子交换柱上的高效液相色谱保留行为。这项研究为选择分离 RNA 和 DNA 寡核苷酸的洗脱条件和预热处理提供了有价值的信息。
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来源期刊
Chromatographia
Chromatographia 化学-分析化学
CiteScore
3.40
自引率
5.90%
发文量
103
审稿时长
2.2 months
期刊介绍: Separation sciences, in all their various forms such as chromatography, field-flow fractionation, and electrophoresis, provide some of the most powerful techniques in analytical chemistry and are applied within a number of important application areas, including archaeology, biotechnology, clinical, environmental, food, medical, petroleum, pharmaceutical, polymer and biopolymer research. Beyond serving analytical purposes, separation techniques are also used for preparative and process-scale applications. The scope and power of separation sciences is significantly extended by combination with spectroscopic detection methods (e.g., laser-based approaches, nuclear-magnetic resonance, Raman, chemiluminescence) and particularly, mass spectrometry, to create hyphenated techniques. In addition to exciting new developments in chromatography, such as ultra high-pressure systems, multidimensional separations, and high-temperature approaches, there have also been great advances in hybrid methods combining chromatography and electro-based separations, especially on the micro- and nanoscale. Integrated biological procedures (e.g., enzymatic, immunological, receptor-based assays) can also be part of the overall analytical process.
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