Exploiting Purine as an Internal Standard for SERS Quantification of Purine Derivative Molecules Released by Bacteria

次黄嘌呤 嘌呤 化学 嘌呤代谢 生物分子 拉曼散射 拉曼光谱 色谱法 代谢组学 核酸 嘌呤类似物 组合化学 分析化学(期刊) 纳米技术 生物化学 材料科学 光学 物理
作者
Ho‐Wen Cheng,Hsin-Mei Tsai,Yuh‐Lin Wang
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:95 (46): 16967-16975 被引量:4
标识
DOI:10.1021/acs.analchem.3c03259
摘要

Surface-enhanced Raman scattering (SERS) is a highly sensitive technique used in diverse biomedical applications including rapid antibiotic susceptibility testing (AST). However, signal fluctuation in SERS, particularly the widespread of signals measured from different batches of SERS substrates, compromises its reliability and introduces potential errors in SERS-AST. In this study, we investigate the use of purine as an internal standard (IS) to recalibrate SERS signals and quantify the concentrations of two important purine derivatives, adenine and hypoxanthine, which are the most important biomarkers used in SERS-AST. Our findings demonstrate that purine IS effectively mitigates SERS signal fluctuations and enables accurate prediction of adenine and hypoxanthine concentrations across a wide range (5 orders of magnitude). Calibrations with purine as an IS outperform those without, exhibiting a 10-fold increase in predictive accuracy. Additionally, the calibration curve obtained from the first batch of SERS substrates remains effective for 64 additional substrates fabricated over a half-year period. Measurements of adenine and hypoxanthine concentrations in bacterial supernatants using SERS with purine IS closely align with the liquid chromatography–mass spectrometry results. The use of purine as an IS offers a simple and robust platform to enhance the speed and accuracy of SERS-AST, while also paving the way for in situ SERS quantification of purine derivatives released by bacteria under various stress conditions.

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