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硅壳/金核纳米粒子:关联壳厚度与聚集时的等离子体红移。

Silica shell/gold core nanoparticles: correlating shell thickness with the plasmonic red shift upon aggregation.

机构信息

Department of Chemistry and Chemical Biology, McMaster University, 1280 Main Street West, Hamilton, Ontario, Canada L8S 4M1.

出版信息

ACS Appl Mater Interfaces. 2011 Oct;3(10):3942-7. doi: 10.1021/am200825f. Epub 2011 Sep 14.

DOI:10.1021/am200825f
PMID:21882833
Abstract

Differences in the wavelengths of the surface plasmon band of gold nanoparticles (AuNP)--before and after particle aggregation--are widely used in bioanalytical assays. However, the gold surfaces in such bioassays can suffer from exchange and desorption of noncovalently bound ligands and from nonspecific adsorption of biomolecules. Silica shells on the surfaces of the gold can extend the available surface chemistries for bioconjugation and potentially avoid these issues. Therefore, silica was grown on gold surfaces using either hydrolysis/condensation of tetraethyl orthosilicate 1 under basic conditions or diglyceroxysilane 2 at neutral pH. The former precursor permitted slow, controlled growth of shells from about 1.7 to 4.3 nm thickness. By contrast, 3-4 nm thick silica shells formed within an hour using diglyceroxysilane; thinner or thicker shells were not readily available. Within the range of shell thicknesses synthesized, the presence of a silica shell on the gold nanoparticle did not significantly affect the absorbance maximum (~5 nm) of unaggregated particles. However, the change in absorbance wavelength upon aggregation of the particles was highly dependent on the thickness of the shell. With silica shells coating the AuNP, there was a significant decrease in the absorbance maximum of the aggregated particles, from ~578 to ~536 nm, as the shell thicknesses increased from ~1.7 to ~4.3 nm, because of increased distance between adjacent gold cores. These studies provide guidance for the development of colorimetric assays using silica-coated AuNP.

摘要

金纳米粒子(AuNP)表面等离子体带的波长在粒子聚集前后会产生差异,这种差异被广泛应用于生物分析检测中。然而,在这些生物分析检测中,金表面可能会发生非共价结合配体的交换和脱附,以及生物分子的非特异性吸附。金表面的二氧化硅壳可以扩展用于生物偶联的可用表面化学,并可能避免这些问题。因此,使用正硅酸乙酯 1 在碱性条件下水解/缩合或二甘油氧基硅烷 2 在中性 pH 值下在金表面上生长了二氧化硅壳。前者允许壳从约 1.7nm 至 4.3nm 的厚度缓慢、受控地生长。相比之下,使用二甘油氧基硅烷在一小时内形成了 3-4nm 厚的二氧化硅壳;较薄或较厚的壳不易获得。在所合成的壳厚度范围内,金纳米粒子上二氧化硅壳的存在不会显著影响未聚集粒子的吸收最大值(约 5nm)。然而,粒子聚集时吸收波长的变化高度依赖于壳的厚度。随着二氧化硅壳包覆 AuNP,当壳厚度从约 1.7nm 增加到约 4.3nm 时,聚集粒子的吸收最大值从约 578nm 显著降低到约 536nm,这是因为相邻金核之间的距离增加了。这些研究为使用包覆二氧化硅的 AuNP 进行比色分析检测提供了指导。

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