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首页> 外文期刊>Scientific reports. >Tailoring recombinant lipases: keeping the His-tag favors esterification reactions, removing it favors hydrolysis reactions
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Tailoring recombinant lipases: keeping the His-tag favors esterification reactions, removing it favors hydrolysis reactions

机译:量身定制重组脂肪酶:保持His-tag有利于酯化反应,去除His-tag有利于水解反应

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We determined the effect of the His-tag on the structure, activity, stability and immobilization of LipC12, a highly active lipase from a metagenomic library. We purified LipC12 with a N-terminal His-tag and then removed the tag using tobacco etch virus (TEV) protease. Circular dichroism analysis showed that the overall structure of LipC12 was largely unaffected by His-tag removal. The specific hydrolytic activities against natural and artificial substrates were significantly increased by the removal of the His-tag. On the other hand, His-tagged LipC12 was significantly more active and stable in the presence of polar organic solvents than untagged LipC12. The immobilization efficiency on Immobead 150 was 100% for both forms of LipC12 and protein desorption studies confirmed that the His-tag does not participate in the covalent binding of the enzyme. In the case of immobilized LipC12, the His-tag negatively influenced the hydrolytic activity, as it had for the free lipase, however, it positively influenced the esterification activity. These results raise the possibility of tailoring recombinant lipases for different applications, where the His-tag may be retained or removed, as appropriate for the desired activity.
机译:我们确定了His标签对LipC12(一种来自宏基因组库的高活性脂肪酶)的结构,活性,稳定性和固定化的影响。我们纯化了带有N端His-tag的LipC12,然后使用烟草蚀刻病毒(TEV)蛋白酶去除了标签。圆二色性分析表明,LipC12的整体结构在很大程度上不受His-tag去除的影响。通过去除His标签,显着提高了对天然和人工底物的比水解活性。另一方面,His标记的LipC12在存在极性有机溶剂时比未标记的LipC12更具活性和稳定性。两种形式的LipC12在Immobead 150上的固定效率均为100%,蛋白质解吸研究证实,His标签不参与酶的共价结合。在固定化LipC12的情况下,His-tag对水解活性有负面影响,就像对游离脂肪酶一样,但是对酯化活性有正面影响。这些结果提高了为不同应用定制重组脂肪酶的可能性,其中His标签可以保留或去除,以适合所需的活性。

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