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用于通过快速灵敏的芯片移动反应边界电泳滴定法荧光测定总蛋白含量的延迟信号。

Retardation signal for fluorescent determination of total protein content via rapid and sensitive chip moving reaction boundary electrophoretic titration.

作者信息

Wang Houyu, Shi Yongting, Yan Jian, Dong Jingyu, Li Si, Xiao Hua, Xie Haiyang, Fan Liu-Yin, Cao Cheng-Xi

机构信息

Laboratory of Bioseparation and Analytical Biochemistry, State Key Laboratory of Microbial Metabolism, School of Life Science and Biotechnology, Shanghai Jiao Tong University , Shanghai 200240, China.

出版信息

Anal Chem. 2014 Mar 18;86(6):2888-94. doi: 10.1021/ac403963f. Epub 2014 Feb 25.

DOI:10.1021/ac403963f
PMID:24512429
Abstract

A novel concept and theory of moving reaction boundary (MRB) retardation signal (RMRB) was advanced for determination of total protein content via MRB electrophoretic titration (MRBET). The theoretical results revealed that the retardation extent of boundary displacment, viz., the RMRB value, was as a function of protein content. Thus, the RMRB value of a sample could be used to determine its total protein content according to the relevant calibration curve. To demonstrate the concept and theoretical results, a novel microdevice was designed for the relevant experiments of MRBET. The microdevice has 30 identical work cells, each of which is composed of five ultrashort single microchannels (5 mm). In the microdevice, fluorescein isothiocyanate (FITC) was used to denote MRB motion and RMRB value for the first time, the polyacrylamide gel (PAG) containing protein sample was photopolymerized in microchannels, and the MRB was created with acid or alkali and target protein sample. As compared to the classic Kjeldahl method and conventional MRBET performed in glass tube, the developed titration chip has the following merits: good sensitivity (0.3-0.4 μg/mL vs 150-200 μg/mL of protein concentration, 0.6-0.8 ng vs 30-2000 μg of absolute protein content), rapid analysis (20-60 s vs 15-200 min), and portable low-power (15 V vs 200 V).

摘要

提出了一种通过移动反应边界(MRB)延迟信号(RMRB)测定总蛋白含量的新概念和理论,即MRB电泳滴定法(MRBET)。理论结果表明,边界位移的延迟程度,即RMRB值,是蛋白质含量的函数。因此,样品的RMRB值可根据相关校准曲线用于测定其总蛋白含量。为了验证这一概念和理论结果,设计了一种新型微器件用于MRBET的相关实验。该微器件有30个相同的工作单元,每个单元由五个超短单微通道(5毫米)组成。在该微器件中,首次使用异硫氰酸荧光素(FITC)来表示MRB运动和RMRB值,将含有蛋白质样品的聚丙烯酰胺凝胶(PAG)在微通道中光聚合,并用酸或碱与目标蛋白质样品产生MRB。与经典凯氏定氮法和在玻璃管中进行的传统MRBET相比,所开发的滴定芯片具有以下优点:灵敏度高(蛋白质浓度为0.3 - 0.4μg/mL,而经典方法为150 - 200μg/mL;绝对蛋白质含量为0.6 - 0.8ng,而经典方法为30 - 2000μg)、分析速度快(20 - 60秒,而经典方法为15 - 200分钟)以及便携低功耗(15V,而经典方法为200V)。

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