A biotinylated photocleavable polyethylenimine (B-PC-PEI) was designed and synthesized for the capture and controlled release of nucleic acids from solid supports. B-PC-PEI was synthesized via a 3-step reaction process and verified by 1H NMR and mass spectrometry. In aqueous solution, the o-nitrobenzyl group within B-PC-PEI was efficiently cleaved by 5 min of 365 nm light exposure from a distance of 20 cm (9 mW/cm2). When coupled to streptavidin-coated beads, the PEI domain of Cy5-labeled B-PC-PEI was released by 365 nm light exposure. In contrast, a Cy5-labeled biotinylated PEI (B-PEI) was used as a control and negligible fluorescence loss was observed. Cy5-labeled siRNA was electrostatically captured to streptavidin-coated beads preabsorbed with B-PC-PEI or B-PEI, and flow cytometry demonstrated significant loss of fluorescence from the bead surface after 5 min of light exposure only for B-PC-PEI, demonstrating controlled release of siRNA from the bead surface. Finally, the release of the Cy5-labeled siRNA into the supernatant was quantified. The release of Cy5-siRNA into the supernatant was significantly greater after 5 min of light exposure for B-PC-PEI/streptavidin beads compared to 0 min exposure and remained unchanged for B-PEI/streptavidin beads. B-PC-PEI facilitates capture and triggered release of surface-tethered nucleic acids with light exposure and is fully compatible with streptavidin-based applications.
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机译:设计并合成了生物素化的光裂解聚乙烯亚胺(B-PC-PEI),用于捕获和控制从固体支持物中释放核酸。 B-PC-PEI通过三步反应过程合成,并通过 1 1 H NMR和质谱进行验证。在水溶液中,距离20 cm(9 mW / cm 2 )的365 nm光线暴露5分钟,B-PC-PEI中的邻硝基苄基被有效裂解。当与抗生蛋白链菌素包被的微珠偶联时,Cy5标记的B-PC-PEI的PEI结构域通过365 nm曝光而释放。相反,将Cy5标记的生物素化PEI(B-PEI)用作对照,观察到的荧光损失可忽略不计。 Cy5标记的siRNA被静电捕获到预先吸附有B-PC-PEI或B-PEI的链霉亲和素包被的珠子上,流式细胞仪证明仅在B-PC-PEI暴露5分钟后,珠子表面的荧光显着减少,证明了siRNA从微珠表面的受控释放。最后,定量Cy5标记的siRNA向上清液中的释放。与曝光0分钟相比,B-PC-PEI /链霉亲和素珠暴露5分钟后,Cy5-siRNA在上清液中的释放显着更大,而对于B-PEI /链霉亲和素珠则保持不变。 B-PC-PEI可以在光线照射下促进表面连接的核酸的捕获和触发释放,并且与基于链霉亲和素的应用完全兼容。
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