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首页> 外文期刊>RSC Advances >Selective binding of matrix metalloproteases MMP-9 and MMP-12 to inhibitor-assisted thermolysin-imprinted beads
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Selective binding of matrix metalloproteases MMP-9 and MMP-12 to inhibitor-assisted thermolysin-imprinted beads

机译:基质金属蛋白酶MMP-9和MMP-12与抑制剂辅助的嗜热菌蛋白酶印迹珠的选择性结合

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Protein-imprinted polymers have been synthesized to recognize and specifically bind selected proteins. However, protein imprinting requires substantial amounts of pure protein to efficiently obtain imprinted polymers for large scale applications, e.g. protein purification by affinity chromatography. In the absence of large quantities of a pure protein of interest, an alternative strategy was developed. In this case study, neutral metalloprotease thermolysin was selected as a commercially available surrogate for imprinting polymer beads. Phosphoramidon-assisted thermolysin-imprinted beads were synthesized. During rebinding experiments, it was shown that these beads specifically bind to thermolysin. In addition, it was shown that these beads also bind in CHO cell culture supernatant to the matrix metalloprotease-9 and -12 (MMP-9, -12). Therefore, these beads can be applied as a selective sorbent for the rare metalloproteases MMP-9 and MMP-12 to remove these proteases from CHO cell culture supernatants. The high selectivity of thermolysin-imprinted beads can be extended to other proteases of the family of metalloproteases, and is not limited to thermolysin. This innovative approach is suitable to address the challenges in the field of protease purification and isolation from biotechnologically relevant media.
机译:已经合成了蛋白质印迹聚合物,以识别并特异性结合选定的蛋白质。然而,蛋白质印迹需要大量的纯蛋白质,以有效地获得用于大规模应用的印迹聚合物,例如,聚合物。通过亲和色谱法纯化蛋白质。在缺乏大量目标纯蛋白质的情况下,开发了另一种策略。在本案例研究中,选择中性金属蛋白酶嗜热菌蛋白酶作为印迹聚合物珠的市售替代品。合成了磷酰胺辅助的嗜热菌素印迹珠。在重新结合实验中,表明这些珠粒特异性结合嗜热菌素。另外,显示这些珠在CHO细胞培养上清液中也结合至基质金属蛋白酶9和-12(MMP-9,-12)。因此,这些珠子可用作稀有金属蛋白酶MMP-9和MMP-12的选择性吸附剂,以从CHO细胞培养上清液中除去这些蛋白酶。印有嗜热菌素的珠的高选择性可以扩展至金属蛋白酶家族的其他蛋白酶,并且不限于嗜热菌素。这种创新的方法适合解决蛋白酶纯化和从生物技术相关介质中分离的挑战。

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