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基于纳米粒子等离子体纳米间隙的多肽空间限制 SERS 分析。

Intra-nanoparticle plasmonic nanogap based spatial-confinement SERS analysis of polypeptides.

机构信息

College of Chemistry and Chemical Engineering, Central South University, Changsha 410083, China.

College of Chemistry and Chemical Engineering, Central South University, Changsha 410083, China.

出版信息

Talanta. 2024 Jun 1;273:125899. doi: 10.1016/j.talanta.2024.125899. Epub 2024 Mar 9.

DOI:10.1016/j.talanta.2024.125899
PMID:38484502
Abstract

Sensing and characterizing water-soluble polypeptides are essential in various biological applications. However, detecting polypeptides using Surface-Enhanced Raman Scattering (SERS) remains a challenge due to the dominance of aromatic amino acid residues and backbones in the signal, which hinders the detection of non-aromatic amino acid residues. Herein, intra-nanoparticle plasmonic nanogap were designed by etching the Ag shell in Au@AgNPs (i.e., obtaining AuAg cores) with chlorauric acid under mild conditions, at the same time forming the outermost Au shell and the void between the AuAg cores and the Au shell (AuAg@void@Au). By varying the Ag to added chloroauric acid molar ratios, we pioneered a simple, controllable, and general synthetic strategy to form interlayer-free nanoparticles with tunable Au shell thickness, achieving precise regulation of electric field enhancement within the intra-nanogap. As validation, two polypeptide molecules, bacitracin and insulin B, were successfully synchronously encapsulated and spatial-confined in the intra-nanogap for sensing. Compared with concentrated 50 nm AuNPs and Au@AgNPs as SERS substrates, our simultaneous detection method improved the sensitivity of the assay while benefiting to obtain more comprehensive characteristic peaks of polypeptides. The synthetic strategy of confining analytes while fabricating plasmonic nanostructures enables the diffusion of target molecules into the nanogap in a highly specific and sensitive manner, providing the majority of the functionality required to achieve peptide detection or sequencing without the hassle of labeling.

摘要

在各种生物应用中,感测和表征水溶性多肽至关重要。然而,由于信号中芳香族氨基酸残基和骨架的主导地位,使用表面增强拉曼散射(SERS)检测多肽仍然具有挑战性,这阻碍了对非芳香族氨基酸残基的检测。在此,通过在温和条件下用氯金酸刻蚀 Au@AgNPs(即获得 AuAg 核)中的 Ag 壳,设计了纳米粒子内等离子体纳米间隙,同时形成最外层的 Au 壳和 AuAg 核与 Au 壳之间的空隙(AuAg@void@Au)。通过改变 Ag 与添加的氯金酸的摩尔比,我们开创了一种简单、可控和通用的合成策略,形成了具有可调 Au 壳厚度的无夹层纳米粒子,实现了纳米间隙内电场增强的精确调节。作为验证,两种多肽分子,杆菌肽和胰岛素 B,成功地同时被封装并空间限制在纳米间隙内用于感测。与集中的 50nm AuNPs 和 Au@AgNPs 作为 SERS 底物相比,我们的同时检测方法提高了测定的灵敏度,同时有利于获得更全面的多肽特征峰。在制造等离子体纳米结构的同时限制分析物的合成策略,以高度特异性和灵敏的方式使目标分子扩散到纳米间隙中,提供了实现肽检测或测序所需的大部分功能,而无需繁琐的标记。

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