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Multiplex microRNA imaging in living cells using DNA-capped-Au assembled hydrogels

机译:使用DNA封端的Au组装水凝胶在活细胞中进行多重microRNA成像

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摘要

Non-invasively imaging multiplex microRNAs (miRNAs) in living cells is pivotal to understanding their physiological functions and pathological development due to the key regulatory roles of miRNAs in gene expression. However, developing smart delivery systems with large gene loading capacity, biocompatibility and responsiveness remains a significant challenge. Herein, we successfully incorporated DNA-capped Au nanoparticles (NPs) and their complementary fluorescent DNA sequences into a porous 3D hydrogel network (AuDH), in which hairpin-locked DNAzyme strands and active metal ions were loaded (AuDH/Mn+/H) for simultaneously imaging multiplex miRNAs in living cells. After transfection into cells, the specific miRNAs trigger the strand-displacement reaction and sequentially activate the DNAzyme-assisted target recycling, leading to a strong increase in the corresponding fluorescence intensity for imaging. This enables simultaneous assessment of the abundance of multiplex cancer-related miRNAs, even if at a very low expression level, in different cells through the different fluorescence intensities due to the dual signal amplification, and the change in abundance of miRNAs induced by siRNA or miRNA mimics in living cells can also be efficiently monitored. The versatile and responsive DNA hydrogel system holds great potential for miRNA biomedical applications.
机译:由于miRNA在基因表达中的关键调控作用,因此活细胞中的非侵入性成像多重microRNA(miRNA)对于了解其生理功能和病理发展至关重要。然而,开发具有大的基因负载能力,生物相容性和响应能力的智能传递系统仍然是一个重大挑战。在这里,我们成功地将DNA封端的Au纳米颗粒(NPs)及其互补的荧光DNA序列整合到了多孔3D水凝胶网络(AuDH)中,其中装载了发夹状锁定的DNAzyme链和活性金属离子(AuDH / M n + / H)同时在活细胞中成像多重miRNA。转染入细胞后,特定的miRNA触发链置换反应并顺序激活DNAzyme辅助的靶标回收,从而导致用于成像的相应荧光强度大大增加。通过双重信号放大,通过不同的荧光强度,即使在非常低的表达水平下,这也能够同时评估不同细胞中多种与癌症相关的miRNA的丰度,以及由siRNA或miRNA诱导的miRNA丰度的变化活细胞中的模拟物也可以得到有效监测。多功能且反应灵敏的DNA水凝胶系统在miRNA生物医学应用方面具有巨大潜力。

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