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用于蛋白质固定化金属亲和色谱的新型α-氨基苯丙氨酸四唑配体。

New alpha-amino phenylalanine tetrazole ligand for immobilized metal affinity chromatography of proteins.

作者信息

Lei Genhu, Liu Liting, Xiong Xiaohu, Wei Yinmao, Zheng Xiaohui

机构信息

Department of Chemistry, Northwest University, Xi'an, China.

出版信息

J Sep Sci. 2008 Sep;31(16-17):3002-8. doi: 10.1002/jssc.200700520.

Abstract

A new chelating compound has been developed for use in the immobilized metal affinity chromatographic (IMAC) separation of proteins. The bidentate ligand, alpha-amino phenylalanine tetrazole, 4, was synthesized via a five-step synthesis from N-fluorenylmethoxycarbonyl phenylalanine and then immobilized onto silica through the epoxide coupling procedure. The binding behavior of the resulting IMAC sorbent, following chelation with Zn2+ to a density of 183 micromol Zn2+ ions/g silica, was characterized by the retention of proteins in the pH range of 5.0-8.0, and by the adsorption behavior of lysozyme with frontal chromatography at pH 6.0 and 8.0. The prepared column showed the separation ability to four test proteins and the retention time of these proteins increased with an increase in pH. From the derived isotherms, the adsorption capacity, qm, for the binding of lysozyme to immobilized Zn2+-alpha-amino phenylalanine tetrazole-silica was found to be 1.21 micromol/g at pH 6.0 and 1.20 micromol/g sorbent at pH 8.0, respectively, whilst the dissociation constants KD at these pH values were 5.22x10(-6) and 3.49x10(-6) M, respectively, indicating that the lysozyme was retained more stable under alkaline conditions, although the binding capacity in terms of micromole protein per gram sorbent remained essentially unchanged.

摘要

一种新型螯合化合物已被开发用于蛋白质的固定化金属亲和色谱(IMAC)分离。双齿配体α-氨基苯丙氨酸四唑(4)由N-芴甲氧羰基苯丙氨酸经五步合成得到,然后通过环氧偶联法固定在硅胶上。所得IMAC吸附剂在与Zn2+螯合至密度为183 μmol Zn2+离子/克硅胶后,其结合行为通过在pH 5.0 - 8.0范围内蛋白质的保留情况以及在pH 6.0和8.0下用前沿色谱法测定溶菌酶的吸附行为来表征。制备的柱对四种测试蛋白质显示出分离能力,并且这些蛋白质的保留时间随pH值的增加而增加。从推导的等温线可知,溶菌酶与固定化Zn2+-α-氨基苯丙氨酸四唑-硅胶结合时,在pH 6.0时的吸附容量qm为1.21 μmol/克,在pH 8.0时为1.20 μmol/克吸附剂,而在这些pH值下的解离常数KD分别为5.22×10(-6)和3.49×10(-6) M,这表明尽管每克吸附剂结合的微摩尔蛋白质的结合容量基本保持不变,但溶菌酶在碱性条件下保留得更稳定。

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