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一种 PET 水解角质酶的生化特性及 NMR 研究。

Biochemical Characterization and NMR Study of a PET-Hydrolyzing Cutinase from .

机构信息

NOBIPOL, Department of Biotechnology and Food Science, NTNU Norwegian University of Science and Technology, 7491 Trondheim, Norway.

Department of Materials and Production, Materials Engineering Group, Aalborg University, 9220 Aalborg Ø, Denmark.

出版信息

Biochemistry. 2023 Apr 18;62(8):1369-1375. doi: 10.1021/acs.biochem.2c00619. Epub 2023 Mar 26.

Abstract

In recent years, the drawbacks of plastics have become evident, with plastic pollution becoming a major environmental issue. There is an urgent need to find solutions to efficiently manage plastic waste by using novel recycling methods. Biocatalytic recycling of plastics by using enzyme-catalyzed hydrolysis is one such solution that has gained interest, in particular for recycling poly(ethylene terephthalate) (PET). To provide insights into PET hydrolysis by cutinases, we have here characterized the kinetics of a PET-hydrolyzing cutinase from (FsC) at different pH values, mapped the interaction between FsC and the PET analogue BHET by using NMR spectroscopy, and monitored product release directly and in real time by using time-resolved NMR experiments. We found that primarily aliphatic side chains around the active site participate in the interaction with BHET and that pH conditions and a mutation around the active site (L182A) can be used to tune the relative amounts of degradation products. Moreover, we propose that the low catalytic performance of FsC on PET is caused by poor substrate binding combined with slow MHET hydrolysis. Overall, our results provide insights into obstacles that preclude efficient PET hydrolysis by FsC and suggest future approaches for overcoming these obstacles and generating efficient PET-hydrolyzing enzymes.

摘要

近年来,塑料的缺点已经显现出来,塑料污染成为一个主要的环境问题。迫切需要寻找新的回收方法来有效管理塑料废物。利用酶催化水解来生物催化回收塑料是一种解决方案,特别是对于回收聚对苯二甲酸乙二醇酯(PET)而言。为了深入了解角质酶对 PET 的水解作用,我们在这里对来自 的 PET 水解角质酶(FsC)在不同 pH 值下的动力学进行了表征,通过 NMR 光谱研究了 FsC 与 PET 类似物 BHET 之间的相互作用,并通过使用时间分辨 NMR 实验直接实时监测产物释放。我们发现,主要是活性位点周围的脂肪族侧链参与了与 BHET 的相互作用,并且 pH 条件和活性位点周围的突变(L182A)可以用于调节降解产物的相对量。此外,我们提出 FsC 对 PET 的低催化性能是由较差的底物结合和较慢的 MHET 水解引起的。总的来说,我们的研究结果为阻碍 FsC 有效水解 PET 的障碍提供了深入的了解,并提出了未来克服这些障碍和生成高效 PET 水解酶的方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c8f3/10116592/ec285d966757/bi2c00619_0002.jpg

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