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[通过电泳滴定和电容耦合非接触式电导检测法测定人血清总蛋白]

[Determination of human serum total protein via electrophoresis titration and capacitively coupled contactless conductivity detection].

作者信息

Zhang Rui-Hua, Guo Ze-Hua, Zhang Qiang, Zha Gen-Han, Cao Cheng-Xi, Fan Liu-Yin, Liu Wei-Wen

机构信息

School of Electronic Information & Electrical Engineering, Shanghai Jiao Tong University, Shanghai 200240, China.

Student Innovation Center, Shanghai Jiao Tong University, Shanghai 200240, China.

出版信息

Se Pu. 2023 Aug;41(8):707-713. doi: 10.3724/SP.J.1123.2023.04015.

DOI:10.3724/SP.J.1123.2023.04015
PMID:37534558
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10398821/
Abstract

Serum total protein refers to the sum of all proteins in the serum, and its content determination is relevant to human health monitoring and disease diagnosis. However, existing detection techniques present a number of limitations; for example, the Kjeldahl method suffers from the negative effects of interfering substances such as non-protein nitrogen (NPN). Although the electrophoresis titration (ET) method has solved interference problems to some extent, the current ET technique relies on optical detection methods, which increases the tediousness of the operation. This study addresses the challenge of accurate serum total protein detection by combining the traditional ET technique with capacitively coupled contactless conductivity detection (CD). The research contributions of this work are multifold. First, it presents the first development of an ET-CD detection system, which consists of six components: an ET power module, an ET chip, a CD sensing module, a detection module, a data acquisition card, and software. The developed system can capture the conductivity of substances in the channel using the software developed by our laboratory during ET. The detection system can be used to quantify the total protein content in human serum without the addition of specific labeling reagents or using optical detection equipment, and its running time is approximately 300 s. Second, this research proposes the corresponding principle of the system. Under an electric field, ion migration results in different pH levels before and after the boundary, leading to a protein surface charge difference. The maintenance of the electrical neutrality of the substances in the detection channel is related to the protein surface charge; therefore, the ion concentration distribution of the substances in the detection channel changes as the protein surface charge varies. A plot of conductivity as a function of running time showed an "inverted clock shape", first falling and then rising. Owing to the addition of different types and concentrations of proteins, the microenvironment of the entire system changes, resulting in different changes in conductivity. Third, the performance of the detection system was tested using human serum albumin (HSA) standard protein, which was mixed with polyacrylamide gel (PAG) mother liquor, riboflavin, etc., and irradiated under ultraviolet light for 10 min to form a gel. The ET experiments were then carried out. The shape of the conductivity curve was consistent with the proposed principle, and the higher the HSA concentration, the lower the conductivity curve trough, followed by a lagged time of the trough. Quantitative analysis of the conductivity signals showed that the linear range was 0.25-3.00 g/L, with a linearity of up to 0.98. The limit of detection (LOD) was 0.01 g/L, the relative standard deviation (RSD) was 1.90%, and the relative error of the test values was <7.20%, indicating the good detection stability and sensitivity of the system. Clinical samples collected from healthy volunteers were used as target blood samples for serum total protein content measurement using our detection system. Blood samples from a volunteer were used to obtain a standard curve, and the serum samples of other four volunteers were selected for ET-CD and biuret detection. The results showed that the relative errors between the two methods were within 4.43%, indicating the accuracy and reliability of the detection system. The advantages of the ET-CD detection system proposed in this paper are as follows: (i) ET-CD realizes the rapid detection of total serum protein content based on the ET technique; (ii) compared with the traditional protein ET technique, the ET-CD method does not rely on specific labeling components or optical detection equipment, thereby reducing the complexity of the operation; and (iii) the output signal of ET-CD can be used for quantitative analysis with excellent analytical performance and high accuracy. These merits highlight the potential of the developed system for clinical application and biochemical analysis.

摘要

血清总蛋白是指血清中所有蛋白质的总和,其含量测定与人体健康监测和疾病诊断相关。然而,现有的检测技术存在一些局限性;例如,凯氏定氮法受到非蛋白氮(NPN)等干扰物质的负面影响。虽然电泳滴定(ET)法在一定程度上解决了干扰问题,但目前的ET技术依赖光学检测方法,增加了操作的繁琐性。本研究通过将传统的ET技术与电容耦合非接触式电导检测(CD)相结合,应对了准确检测血清总蛋白的挑战。这项工作的研究贡献是多方面的。首先,它首次开发了一种ET-CD检测系统,该系统由六个组件组成:ET电源模块、ET芯片、CD传感模块、检测模块、数据采集卡和软件。在ET过程中,所开发的系统可以使用我们实验室开发的软件捕获通道中物质的电导率。该检测系统无需添加特定标记试剂或使用光学检测设备即可用于定量人血清中的总蛋白含量,其运行时间约为300秒。其次,本研究提出了该系统的相应原理。在电场作用下,离子迁移导致边界前后pH值不同,从而导致蛋白质表面电荷差异。检测通道中物质的电中性维持与蛋白质表面电荷有关;因此,随着蛋白质表面电荷的变化,检测通道中物质的离子浓度分布也会改变。电导率随运行时间的变化曲线呈“倒钟形”,先下降后上升。由于添加了不同类型和浓度的蛋白质,整个系统的微环境发生变化,导致电导率出现不同的变化。第三,使用人血清白蛋白(HSA)标准蛋白对检测系统的性能进行了测试,将其与聚丙烯酰胺凝胶(PAG)母液、核黄素等混合,并在紫外线下照射10分钟以形成凝胶。然后进行ET实验。电导率曲线的形状与所提出的原理一致,HSA浓度越高,电导率曲线的谷值越低,随后谷值出现延迟时间。对电导率信号的定量分析表明,线性范围为0.25 - 3.00 g/L,线性度高达0.98。检测限(LOD)为0.01 g/L,相对标准偏差(RSD)为1.90%,测试值的相对误差<7.20%,表明该系统具有良好的检测稳定性和灵敏度。使用从健康志愿者收集的临床样本作为目标血样,用我们的检测系统测量血清总蛋白含量。使用一名志愿者的血样获得标准曲线,并选择其他四名志愿者的血清样本进行ET-CD和双缩脲检测。结果表明,两种方法之间的相对误差在4.43%以内,表明该检测系统的准确性和可靠性。本文提出的ET-CD检测系统的优点如下:(i)ET-CD基于ET技术实现了血清总蛋白含量的快速检测;(ii)与传统的蛋白质ET技术相比,ET-CD方法不依赖特定的标记组件或光学检测设备,从而降低了操作的复杂性;(iii)ET-CD的输出信号可用于定量分析,具有出色的分析性能和高精度。这些优点突出了所开发系统在临床应用和生化分析中的潜力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb3a/10398821/1939d4c35ea6/cjc-41-08-707-img_4.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb3a/10398821/e03abfcb74c1/cjc-41-08-707-img_1.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb3a/10398821/aa11e2c5ce33/cjc-41-08-707-img_2.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb3a/10398821/dc7ebe5b4cc4/cjc-41-08-707-img_3.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb3a/10398821/1939d4c35ea6/cjc-41-08-707-img_4.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb3a/10398821/e03abfcb74c1/cjc-41-08-707-img_1.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb3a/10398821/aa11e2c5ce33/cjc-41-08-707-img_2.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb3a/10398821/dc7ebe5b4cc4/cjc-41-08-707-img_3.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cb3a/10398821/1939d4c35ea6/cjc-41-08-707-img_4.jpg

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