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Development of Double-Stranded siRNA Labeling Method Using Positron Emitter and Its In Vivo Trafficking Analyzed by Positron Emission Tomography

机译:正电子发射体双链siRNA标记方法的发展及其正电子发射断层成像分析的体内运输

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Pharmacokinetic study of small interfering RNA (siRNA) is an important issue for the development of siRNAs for use as a medicine. For this purpose, a novel and favorable positron emitter-labeled siRNA was prepared by amino group-modification using N-succinimidyl 4-[fluorine-18] fluorobenzoate ([~(18)F]SFB), and real-time analysis of siRNA trafficking was performed by using positron emission tomography (PET). Naked [~(18)F]-labeled siRNA or cationic liposome/[~(18)F]-labeled siRNA Complexes were administered to mice, and differential biodistribution of the label was imaged by PET. The former was cleared quite rapidly from the bloodstream and excreted from the kidneys; but in contrast, the latter tended to accumulate in the lungs. We also confirmed the biodistribution of fluorescence-labeled naked siRNA and cationic liposome/siRNA complexes by use of a near-infrared fluorescence imaging system. As a result, a similar biodistribution was observed, although quantitative data were obtained only by planar positron imaging system (PPIS) analysis but not by fluorescence in vivo imaging. Our results indicate that PET imaging of siRNA provides important information for the development of siRNA medicines.
机译:小干扰RNA(siRNA)的药代动力学研究是开发用作药物的siRNA的重要课题。为此,通过使用N-琥珀酰亚胺基4- [氟-18]氟苯甲酸酯([〜(18)F] SFB)进行氨基修饰,制备了新颖且有利的正电子发射体标记的siRNA,并对siRNA进行了实时分析。使用正电子发射断层扫描(PET)进行贩运。将裸露的[〜(18)F]标记的siRNA或阳离子脂质体/ [〜(18)F]标记的siRNA复合物施用于小鼠,并通过PET对标记的不同生物分布进行成像。前者从血液中迅速清除,并从肾脏排泄。但与此相反,后者往往会在肺中积累。我们还证实了通过使用近红外荧光成像系统,荧光标记的裸siRNA和阳离子脂质体/ siRNA复合物的生物分布。结果,观察到相似的生物分布,尽管仅通过平面正电子成像系统(PPIS)分析获得了定量数据,而没有通过体内荧光成像获得定量数据。我们的结果表明,siRNA的PET成像为siRNA药物的开发提供了重要的信息。

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