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用于溶细胞多糖单加氧酶的连续比色活性分析——关键评估和实际考虑因素。

Continuous photometric activity assays for lytic polysaccharide monooxygenase-Critical assessment and practical considerations.

机构信息

Department of Food Science and Technology, Institute of Food Technology, University of Natural Resources and Life Sciences, Vienna, Austria.

Department of Food Science and Technology, Institute of Food Technology, University of Natural Resources and Life Sciences, Vienna, Austria.

出版信息

Methods Enzymol. 2023;679:381-404. doi: 10.1016/bs.mie.2022.08.054. Epub 2022 Dec 30.

DOI:10.1016/bs.mie.2022.08.054
PMID:36682872
Abstract

Lytic polysaccharide monooxygenase (LPMO) is a monocopper-dependent enzyme that cleaves glycosidic bonds by using an oxidative mechanism. In nature, they act in concert with cellobiohydrolases to facilitate the efficient degradation of lignocellulosic biomass. After more than a decade of LPMO research, it has become evident that LPMOs are abundant in all domains of life and fulfill a diverse range of biological functions. Independent of their biological function and the preferred polysaccharide substrate, studying and characterizing LPMOs is tedious and so far mostly relied on the discontinuous analysis of the solubilized reaction products by HPLC/MS-based methods. In the absence of appropriate substrates, LPMOs can engage in two off-pathway reactions, i.e., an oxidase and a peroxidase-like activity. These futile reactions have been exploited to set up easy-to-use continuous spectroscopic assays. As the natural substrates of newly discovered LPMOs are often unknown, widely applicable, simple, reliable, and robust spectroscopic assays are required to monitor LPMO expression and to perform initial biochemical characterizations, e.g., thermal stability measurements. Here we provide detailed descriptions and practical protocols to perform continuous photometric assays using either 2,6-dimethoxyphenol (2,6-DMP) or hydrocoerulignone as colorimetric substrates as a broadly applicable assay for a range of LPMOs. In addition, a turbidimetric measurement is described as the currently only method available to continuously monitor LPMOs acting on amorphous cellulose.

摘要

溶细胞多糖单加氧酶(LPMO)是一种单铜依赖性酶,通过氧化机制切割糖苷键。在自然界中,它们与纤维二糖水解酶协同作用,促进木质纤维素生物质的有效降解。经过十多年的 LPMO 研究,已经明显看出 LPMO 在所有生命领域都很丰富,并具有多种不同的生物学功能。无论其生物学功能和首选多糖底物如何,研究和表征 LPMO 都很繁琐,迄今为止主要依赖于基于 HPLC/MS 的方法对可溶反应产物的不连续分析。在没有合适底物的情况下,LPMO 可以进行两种非途径反应,即氧化酶和过氧化物酶样活性。这些徒劳的反应已被利用来建立易于使用的连续光谱测定法。由于新发现的 LPMO 的天然底物通常未知,因此需要广泛适用、简单、可靠和稳健的光谱测定法来监测 LPMO 的表达并进行初始生化特性分析,例如热稳定性测量。在这里,我们提供了详细的描述和实用的方案,使用 2,6-二甲氧基苯酚(2,6-DMP)或愈创木酚氢醌作为比色底物进行连续光度测定,这是一种广泛适用于一系列 LPMO 的测定方法。此外,还描述了浊度测量作为目前唯一可连续监测作用于无定形纤维素的 LPMO 的方法。

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