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用于蛋白质识别的大孔分子印迹整体聚合物柱的液相色谱法。

Macroporous molecularly imprinted monolithic polymer columns for protein recognition by liquid chromatography.

机构信息

Key Laboratory of Separation Science for Analytical Chemistry, National Chromatographic R.&.A Center, Dalian Institute of Chemical Physics, the Chinese Academic of Sciences, Dalian, P. R. China.

出版信息

J Sep Sci. 2010 Sep;33(17-18):2757-61. doi: 10.1002/jssc.201000350.

Abstract

Macroporous cytochrome c (cyc)-imprinted monolithic polyarylamide columns were prepared, and applied for the template protein recognition by HPLC. With cyc (18.8 mg) as template, the imprinted monolithic materials were in situ polymerized in an HPLC column tube, with methacrylamide (450 mg), methacrylic acid (15.8 mg), piperazine diacrylamide (720 mg) and ammonium sulfate (390 mg) dissolved in 5 mL of phosphate buffer (pH 7.4), initiated by ammonium persulfate and TEMED. After the reaction, cyc was removed with acetic acid (10%, v/v) containing 10% w/v SDS. The non-imprinted monolithic column was prepared under the same procedure except without cyc. Retention of cyc and its competitive protein, lysozyme (lys), on molecular-imprinting polymer (MIP) and non-imprinted polymer columns was studied. When the pH value of mobile phase was 4.0, on MIP column, the retention factors of cyc and lys were 2.0 and 1.3, respectively. However, those on non-imprinted polymer column were very similar, both as 1.1. Even in competitive environment, a mixture of cyc and lys could be separated on MIP column under gradient elution, with resolution as 1.2. These results indicate that protein-imprinted monolithic polymer columns could offer obvious affinity and specific recognition to the template protein.

摘要

大孔细胞色素 c(cyc)印迹整体聚芳酰胺柱的制备及其在 HPLC 中模板蛋白识别的应用。以 cyc(18.8mg)为模板,在 HPLC 柱管中原位聚合印迹整体材料,将丙烯酰胺(450mg)、甲基丙烯酸(15.8mg)、哌嗪二丙烯酰胺(720mg)和硫酸铵(390mg)溶解在 5ml 磷酸盐缓冲液(pH7.4)中,由过硫酸铵和 TEMED 引发。反应后,用含 10%v/vSDS 的乙酸(10%,v/v)去除 cyc。在相同的程序下制备非印迹整体柱,但不含有 cyc。研究了印迹聚合物(MIP)和非印迹聚合物柱上 cyc 和溶菌酶(lys)的保留情况。当流动相的 pH 值为 4.0 时,在 MIP 柱上,cyc 和 lys 的保留因子分别为 2.0 和 1.3,而在非印迹聚合物柱上则非常相似,均为 1.1。即使在竞争环境下,cyc 和 lys 的混合物也可以在梯度洗脱下在 MIP 柱上分离,分辨率为 1.2。这些结果表明,蛋白质印迹整体聚合物柱可以对模板蛋白提供明显的亲和力和特异性识别。

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