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首页> 外文期刊>ACS applied materials & interfaces >Aptamer-Based Fluorescent Biosensing of Adenosine Triphosphate and Cytochrome c via Aggregation-Induced Emission Enhancement on Novel Label-Free DNA-Capped Silver Nanoclusters/Graphene Oxide Nanohybrids
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Aptamer-Based Fluorescent Biosensing of Adenosine Triphosphate and Cytochrome c via Aggregation-Induced Emission Enhancement on Novel Label-Free DNA-Capped Silver Nanoclusters/Graphene Oxide Nanohybrids

机译:基于Aptamer的腺苷三磷酸腺苷和细胞色素C的荧光生物溶解在新的无标记DNA封端的无碱纳米蛋白/石墨烯纳米胺上的聚集诱导的发射增强

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摘要

Four fluorescent DNA-stabilized fluorescent silver nanoclusters (DNA AgNCs) were designed and synthesized with differences in lengths of cytosine-rich DNA strand (as the stabilizing agent) and target-specific strand DNA-AgNCs DNA aptamers for adenosine triphosphate (ATP) and cytochrome c (Cyt c). After their nanohybrid formation with graphene oxide (GO), it was unexpectedly found that, depending on the composition of the base and length of the strand DNA aptamer, the fluorescence intensity of three of the nanohybrids significantly enhanced. Our experimental observations and quantum mechanical calculations provided an insight into the mechanisms underlying the behavior of DNA AgNCs/GO nanohybrids. The enhanced fluorescence was found to be attributed to the aggregation-induced emission enhancement (AIE) characteristic of the DNA AgNCs adsorbed on the GO surface, as confirmed evidently by both fluorescence and transmission electron microscopies. The AIE is a result of hardness and oxidation properties of GO, which lead to enhanced argenophilic interaction and thus to increased Ag(I) DNA complex shell aggregation. Consequently, two of the DNA-AgNCs/GO nanohybrids were successfully extended to construct highly selective, sensitive, label-free, and simple aptasensors for biosensing of ATP (LOD = 0.42 nM) and Cyt c (LOD = 2.3 nM) in lysed Escherichia coli DH5 alpha cells and mouse embryonic stem cells, respectively. These fundamental findings are expected to significantly influence the designing and engineering of new AgNCs/GO-based AIE biosensors.
机译:设计并合成了四种荧光DNA稳定的荧光银纳米蛋白(DNA AGNC),富含细胞苷的DNA链(作为稳定剂)和靶特异性链DNA-AGNCS DNA适体的腺苷三磷酸(ATP)和细胞色素的差异C(cyt c)。用石墨烯氧化物(GO)形成纳米冬次形成后,意外地发现,取决于链DNA适体的碱基和长度的组成,三种纳米冬小的荧光强度显着增强。我们的实验观察和量子力学计算提供了对DNA Agncs / Go纳米布麦的行为的机制的洞察。发现增强的荧光归因于吸附在去谱上的DNA AgNC的聚集诱导的发射增强(AIE)特征,如通过荧光和透射电子显微镜明显证明的。 AIE是GO的硬度和氧化性质的结果,这导致增强的嗜好的嗜好相互作用,因此增加了Ag(i)DNA复合壳聚集。因此,成功地扩展了两种DNA-AgNC / Go纳米胺,以构建高度选择性,敏感,无标记的,并且在裂解的大肠杆菌中的ATP(LOD = 0.42nm)和Cyt c(Lod = 2.3nm)的生物沉积的简单Aptasensors Coli DH5α细胞和小鼠胚胎干细胞。这些基本发现预计会显着影响新的AGNCS / GOIE生物传感器的设计和工程。

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