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吸附在浓银胶上的小牛胸腺DNA的表面增强拉曼光谱。

Surface-enhanced Raman spectra of calf thymus DNA adsorbed on concentrated silver colloid.

作者信息

Ke Weizhong, Zhou Dianfeng, Wu Jianzhong, Ji Kang

机构信息

Analysis and Test Center, Jiangsu Provincial Key Laboratory for Photoelectric Technology, Nanjing Normal University, Nanjing 210097, P.R.China.

出版信息

Appl Spectrosc. 2005 Apr;59(4):418-23. doi: 10.1366/0003702053641487.

DOI:10.1366/0003702053641487
PMID:15901326
Abstract

Raman and surface-enhanced Raman scattering (SERS) spectra of calf thymus DNA were investigated. We have carried out improvements to the silver colloid preparation method of Lee and Meisel in two respects. In one method, the silver sol was boiled with rapid stirring for over two hours. In the second method, the silver sol was concentrated by centrifugation before adding it to the DNA solution. The resulting hydrosol could be stored for 15 months because of its high stabilization. Structural information with respect to the phosphate backbone, deoxyribose, and four bases of DNA could be obtained before and after the DNA solutions were added to the concentrated Ag colloid substrate. The intensities of almost all characteristic bands assigned to various groups of the components of DNA were enhanced to a remarkable degree. The enhancement effect of the DNA solution at neutral pH 7.0 was obviously much better than that at acidic pH 3.4 or at alkaline pH 8.5. Intensity increases of the SERS bands of the DNA solution with time were observed. The SERS signals obtained 16 hours after the interaction of the Ag colloid with the DNA solution were much better than the SERS signals obtained just after the mixed liquid was prepared. This method can be widely used to store the Ag colloid for long times and to obtain the SERS spectra of DNA molecules, and it can further be used to study the adsorption behavior of solute biomacromolecules in different solvents.

摘要

研究了小牛胸腺DNA的拉曼光谱和表面增强拉曼散射(SERS)光谱。我们在两个方面对Lee和Meisel的银胶体制备方法进行了改进。一种方法是在快速搅拌下将银溶胶煮沸两个多小时。第二种方法是在将银溶胶加入DNA溶液之前通过离心进行浓缩。所得的水溶胶由于其高稳定性可以储存15个月。在将DNA溶液加入浓缩的Ag胶体底物之前和之后,可以获得关于DNA的磷酸骨架、脱氧核糖和四种碱基的结构信息。几乎所有归属于DNA各组分不同基团的特征带的强度都有显著增强。DNA溶液在中性pH 7.0时的增强效果明显优于在酸性pH 3.4或碱性pH 8.5时的效果。观察到DNA溶液的SERS带强度随时间增加。Ag胶体与DNA溶液相互作用16小时后获得的SERS信号比刚制备混合液后获得的SERS信号要好得多。该方法可广泛用于长时间储存Ag胶体并获得DNA分子的SERS光谱,还可进一步用于研究溶质生物大分子在不同溶剂中的吸附行为。

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