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通过分子印迹琼脂糖凝胶膜进行蛋白质识别

Protein recognition via molecularly imprinted agarose gel membrane.

作者信息

Lin Yuan, Tang Shunqing, Mao Xuan, Bao Lei

机构信息

Institute of Biomedical Engineering, Jinan University, Guangzhou 510632, People's Republic of China.

出版信息

J Biomed Mater Res A. 2008 Jun 1;85(3):573-81. doi: 10.1002/jbm.a.31361.

Abstract

Agarose gel membranes (AGMs), which could selectively recognize bovine serum albumin (BSA) and bovine hemoglobin (Hb), were prepared by molecular imprinting technique under moderate preparation conditions. Four imprinting processes, including gelation without any treatment, second gel-melting, and two glutaraldehyde crosslinking processes of fumigation or direct addition of the crosslinking agent, were developed to investigate the protein-recognition behavior of the AGMs. Results showed that the preparation processes affected the adsorption capacity and selectivity of the imprinted AGMs. Both BSA- and Hb-imprinted AGMs exhibited higher adsorption abilities for the targeted proteins (3.77-5.72 times for BSA, 1.31-2.18 times for Hb) than the nonimprinted ones. And the selectivity of BSA-imprinted AGMs for BSA molecules (the selective factor K = 3.29-4.90) was higher than that of Hb-imprinted AGMs for Hb (K = 0.32-1.17). The optimal adsorption capacity of BSA- and Hb-imprinted AGMs was 25.90 and 117.45 mg/g, respectively, when the membrane was crosslinked by glutaraldehyde with a fumigation process; the optimal selectivity of BSA- and Hb-imprinted AGMs was 4.91 when the membrane was prepared by second gel-melting process, and 0.76 when the membrane was prepared without any treatment. These findings demonstrate that the molecularly imprinted AGMs are hopeful to be used in specific protein analysis.

摘要

在适度的制备条件下,通过分子印迹技术制备了能够选择性识别牛血清白蛋白(BSA)和牛血红蛋白(Hb)的琼脂糖凝胶膜(AGM)。开发了四种印迹过程,包括未经任何处理的凝胶化、二次凝胶熔化以及熏蒸或直接添加交联剂的两种戊二醛交联过程,以研究AGM的蛋白质识别行为。结果表明,制备过程影响了印迹AGM的吸附容量和选择性。与非印迹AGM相比,BSA印迹和Hb印迹的AGM对目标蛋白质均表现出更高的吸附能力(BSA为3.77 - 5.72倍,Hb为1.31 - 2.18倍)。并且BSA印迹AGM对BSA分子的选择性(选择性因子K = 3.29 - 4.90)高于Hb印迹AGM对Hb的选择性(K = 0.32 - 1.17)。当通过熏蒸过程用戊二醛交联膜时,BSA印迹和Hb印迹AGM的最佳吸附容量分别为25.90和117.45 mg/g;当通过二次凝胶熔化过程制备膜时,BSA印迹和Hb印迹AGM的最佳选择性为4.91,而未经任何处理制备膜时最佳选择性为0.76。这些发现表明,分子印迹AGM有望用于特定蛋白质分析。

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