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[分子印迹技术用于复杂生物样品系统分离与识别的研究进展]

[Recent advances of molecular imprinting technology for the separation and recognition of complex biological sample systems].

作者信息

Xie Bao-Xuan, Lyu Yang, Liu Zhen

机构信息

State Key Laboratory of Analytical Chemistry for Life Science, School of Chemistry and Chemical Engineering, Nanjing University, Nanjing 210023, China.

出版信息

Se Pu. 2024 Jun;42(6):508-523. doi: 10.3724/SP.J.1123.2024.01011.

DOI:10.3724/SP.J.1123.2024.01011
PMID:38845512
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11165394/
Abstract

Given continuous improvements in industrial production and living standards, the analysis and detection of complex biological sample systems has become increasingly important. Common complex biological samples include blood, serum, saliva, and urine. At present, the main methods used to separate and recognize target analytes in complex biological systems are electrophoresis, spectroscopy, and chromatography. However, because biological samples consist of complex components, they suffer from the matrix effect, which seriously affects the accuracy, sensitivity, and reliability of the selected separation analysis technique. In addition to the matrix effect, the detection of trace components is challenging because the content of the analyte in the sample is usually very low. Moreover, reasonable strategies for sample enrichment and signal amplification for easy analysis are lacking. In response to the various issues described above, researchers have focused their attention on immuno-affinity technology with the aim of achieving efficient sample separation based on the specific recognition effect between antigens and antibodies. Following a long period of development, this technology is now widely used in fields such as disease diagnosis, bioimaging, food testing, and recombinant protein purification. Common immuno-affinity technologies include solid-phase extraction (SPE) magnetic beads, affinity chromatography columns, and enzyme linked immunosorbent assay (ELISA) kits. Immuno-affinity techniques can successfully reduce or eliminate the matrix effect; however, their applications are limited by a number of disadvantages, such as high costs, tedious fabrication procedures, harsh operating conditions, and ligand leakage. Thus, developing an effective and reliable method that can address the matrix effect remains a challenging endeavor. Similar to the interactions between antigens and antibodies as well as enzymes and substrates, biomimetic molecularly imprinted polymers (MIPs) exhibit high specificity and affinity. Furthermore, compared with many other biomacromolecules such as antigens and aptamers, MIPs demonstrate higher stability, lower cost, and easier fabrication strategies, all of which are advantageous to their application. Therefore, molecular imprinting technology (MIT) is frequently used in SPE, chromatographic separation, and many other fields. With the development of MIT, researchers have engineered different types of imprinting strategies that can specifically extract the target analyte in complex biological samples while simultaneously avoiding the matrix effect. Some traditional separation technologies based on MIP technology have also been studied in depth; the most common of these technologies include stationary phases used for chromatography and adsorbents for SPE. Analytical methods that combine MIT with highly sensitive detection technologies have received wide interest in fields such as disease diagnosis and bioimaging. In this review, we highlight the new MIP strategies developed in recent years, and describe the applications of MIT-based separation analysis methods in fields including chromatographic separation, SPE, diagnosis, bioimaging, and proteomics. The drawbacks of these techniques as well as their future development prospects are also discussed.

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2386/11165394/477ca781c3bd/img_9.jpg
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https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2386/11165394/477ca781c3bd/img_9.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2386/11165394/d2575d1dcd71/img_1.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2386/11165394/3aab3785eab2/img_2.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2386/11165394/98cbe0e5ed7b/img_3.jpg
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https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2386/11165394/0d4ad0eb5274/img_5.jpg
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https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2386/11165394/477ca781c3bd/img_9.jpg
摘要

随着工业生产和生活水平的持续提高,复杂生物样品系统的分析和检测变得越来越重要。常见的复杂生物样品包括血液、血清、唾液和尿液。目前,用于分离和识别复杂生物系统中目标分析物的主要方法是电泳、光谱学和色谱法。然而,由于生物样品由复杂的成分组成,它们会受到基质效应的影响,这严重影响了所选分离分析技术的准确性、灵敏度和可靠性。除了基质效应外,痕量成分的检测也具有挑战性,因为样品中分析物的含量通常非常低。此外,缺乏用于易于分析的样品富集和信号放大的合理策略。针对上述各种问题,研究人员将注意力集中在免疫亲和技术上,旨在基于抗原与抗体之间的特异性识别效应实现高效的样品分离。经过长期发展,该技术现已广泛应用于疾病诊断、生物成像、食品检测和重组蛋白纯化等领域。常见的免疫亲和技术包括固相萃取(SPE)磁珠、亲和色谱柱和酶联免疫吸附测定(ELISA)试剂盒。免疫亲和技术可以成功地减少或消除基质效应;然而,它们的应用受到许多缺点的限制,如成本高、制备过程繁琐、操作条件苛刻和配体泄漏。因此,开发一种能够解决基质效应的有效且可靠的方法仍然是一项具有挑战性的工作。与抗原与抗体以及酶与底物之间的相互作用类似,仿生分子印迹聚合物(MIP)具有高特异性和亲和力。此外,与许多其他生物大分子如抗原和适体相比,MIP具有更高的稳定性、更低的成本和更简单的制备策略,所有这些都有利于它们的应用。因此,分子印迹技术(MIT)经常用于SPE、色谱分离和许多其他领域。随着MIT的发展,研究人员设计了不同类型的印迹策略,这些策略可以在避免基质效应的同时特异性地提取复杂生物样品中的目标分析物。一些基于MIP技术的传统分离技术也得到了深入研究;其中最常见的技术包括用于色谱的固定相和用于SPE的吸附剂。将MIT与高灵敏度检测技术相结合的分析方法在疾病诊断和生物成像等领域受到了广泛关注。在这篇综述中,我们重点介绍了近年来开发的新的MIP策略,并描述了基于MIT的分离分析方法在色谱分离、SPE、诊断、生物成像和蛋白质组学等领域的应用。还讨论了这些技术的缺点及其未来的发展前景。

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