期刊
SEPARATION AND PURIFICATION TECHNOLOGY
卷 315, 期 -, 页码 -出版社
ELSEVIER
DOI: 10.1016/j.seppur.2023.123676
关键词
Nucleic acids; Ionic liquid; Ionic liquid-based support; Multimodal ligand; Purification
Nucleic acids, especially RNA, have been explored as potential biopharmaceuticals for gene therapy. However, their labile nature poses challenges in their production and purification. This study investigates the use of chromatographic silica-based supports functionalized with ionic liquids for RNA purification. The results show promising potential for the development of a more efficient and safer method for RNA isolation.
Nucleic acids have been considered interesting molecules to be used as biopharmaceuticals for the treatment of various diseases, in gene therapy strategies. In particular, RNA arises as the most promising approach because it does not require access to the nucleus of cells to exert its function; however, it is quite challenging due to its labile nature. To increase the possibility of translating RNA-based technology to clinical protocols, the biomanufacturing of RNAs has been intensively exploited in the last few years. However, the standard RNA purification processes remain time-consuming and present limitations regarding recovery yield and purity. This work describes the functionalization of chromatographic silica-based supports with four ionic liquids (ILs) composed of functional moieties that can promote distinct interactions with nucleic acids. After an initial screening to evaluate the binding and elution behavior of nucleic acids in the IL-based supports, SSi[C(3)C(3NH2)Im]Cl has shown to be the most promising for further purification assays. This support was studied for the RNA purification from different samples (clarified or more complex) and has shown to be highly effective, for all the conditions studied. Generally, it is here presented a new method for RNA isolation in a single step, using an IL-based chromatographic support, able to eliminate the usage of hazardous compounds often included in standard RNA extraction protocols.
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