Raman Spectroscopy as a Real-Time In Situ Analyzer for Cell Culture Bioprocesses

介电谱 拉曼光谱 检出限 循环伏安法 化学 单体 分析化学(期刊) 材料科学 电极 色谱法 电化学 聚合物 光学 物理 物理化学 有机化学
作者
Alexander Pitters,Maryann Cuellar,Pat Wiegand,Sean J. Gilliam,Ian R. Lewis,Bruno Lenain
出处
期刊:New Biotechnology [Elsevier]
卷期号:33: S113-S113 被引量:1
标识
DOI:10.1016/j.nbt.2016.06.1118
摘要

The development of fast and reliable methods for protein determination are of great relevance to a diversity of areas from industry to diagnostics. Molecular Imprinted Materials (MIM) has proved to be an interesting methodology for protein analysis however further studies of the effect of the experimental parameters and starting materials in the performance of the MIM are still required. Caffeic acid (CAF) is employed for the first time as a monomer to tailor a synthetic receptor for a protein target. This was done by bulk-electropolymerization, applying a constant potential of +2.0 V, for 30 s, on a carbon screen-printed electrode, immersed in a solution of protein and CAF prepared in phosphate buffer. Annexin A3 (ANXA3) was selected as protein target due to the fact that this is an emerging biomarker in prostate cancer.The assembly of the protein imprinted material (PIM) was followed by Electrochemical Impedance Spectroscopy (EIS) and Raman Spectroscopy. A non-imprinted material (NIM) was prepared in parallel as control.Square wave voltammetry (SWV) was used to monitor the electrochemical signal of the [Fe(CN)6]3−/[Fe(CN)6]4− redox for the quantification of ANXA3.The optimized PIM-based device showed average detection limits (LOD) of 0.095 ng/mL, a linear behavior against log (concentration) between 0.10, and 200 ng/mL and good selectivity. The NIM-based device showed random behavior against protein concentration. Finally, the PIM-sensor was successfully applied to the analysis of ANXA3 in spiked urine samples.
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