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Nanoplasmonic probes of RNA folding and assembly during pre-mRNA splicing

机译:Nanoplasmonic探针的RNA折叠和组装在pre-mRNA拼接

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摘要

RNA splicing plays important roles in transcriptome and proteome diversity. Herein, we describe the use of a nanoplasmonic system that unveils RNA folding and assembly during pre-mRNA splicing wherein the quantification of mRNA splice variants is not taken into account. With a couple of SERS-probes and plasmonic probes binding at the boundary sites of exon-2/intron-2 and intron-2/exon-3 of the pre-mature RNA of the beta-globin gene, the splicing process brings the probes into the plasmonic bands. For plasmonic probes, a plasmon shift increase of similar to 29 nm, corresponding to intron removal and exon-2 and exon-3 connection to form the mRNA molecule, is measured by plasmonic coupling. The increased scattering intensity and surface-enhanced Raman scattering (SERS) fingerprinting reveal the clear dynamics of pre-mRNA splicing. Moreover, a time-resolved experiment of individual RNA molecules exhibited a successful splicing and an inhibited splicing event by 33 mu M biflavonoid isoginkgetin, a general inhibitor of RNA splicing. The results suggest that the RNA splicing is successfully monitored with the nanoplasmonic system. Thus, this platform can be useful for studying RNA nanotechnology, biomolecular folding, alternative splicing, and maturation of microRNA.
机译:RNA剪接扮演重要的角色转录组和蛋白质组多样性。描述nanoplasmonic系统的使用揭示在pre-mRNA RNA折叠和组装拼接在mRNA的量化拼接变异不考虑。SERS-probes和电浆调查绑定exon-2 / intron-2边界的网站的和intron-2 / exon-3实际对RNA的β球蛋白基因剪接过程带来了探讨了电浆。探针,等离子体的转变增加类似于29日nm,相应的去除内含子和exon-2和exon-3连接形成了信使rna分子,是衡量电浆耦合。和表面增强拉曼散射强度散射(ser)指纹图谱显示清晰动态pre-mRNA拼接。单个RNA的时间分辨实验分子成功的拼接和展出抑制由33个μM biflavonoid剪接事件isoginkgetin,抑制剂的RNA拼接。拼接成功的监测nanoplasmonic系统。有用的研究RNA的纳米技术,生物分子折叠、可变剪接成熟的微rna。

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