首页> 外文期刊>RSC Advances >Bark depolymerization during submerged fermentation using monofloral honey, a natural mediator substitute, and integration between laccases vs. bark biopolymers, characterized by Py-GC-MS
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Bark depolymerization during submerged fermentation using monofloral honey, a natural mediator substitute, and integration between laccases vs. bark biopolymers, characterized by Py-GC-MS

机译:使用单花蜂蜜(天然介质替代物)进行深层发酵期间的树皮解聚,漆酶与树皮生物聚合物之间的整合(以Py-GC-MS为特征)

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Due to increasing waste production and disposal problems arising from synthetic polymer production, there is a critical need to substitute materials with biodegradable and renewable resources. Attempts to use laccases as a catalyst to enhance the catalytic properties of enzymes have shown them to be a promising solution for bark depolymerization. In this study, eight different fungal strains were tested for laccase enzyme production during submerged fermentation (SF), and the Pleurotus species were shown to be the best producers among the competing fungal strains. P. pulmonarius mainly produces laccase enzyme in production medium (PM) at initial conditions of pH 5.5 and 30 degrees C. Bark depolymerization was conducted in SF and we identified polyphenols/polyaromatic compounds after four weeks when the PM was induced with 50 mg per 100 mL of each bark during the lag-phase. During SF where honey was used as a natural mediator substitute (NMS) in the PM, laccase activities were about 1.5 times higher than those found in comparable cultures without honey in the PM. These samples were analyzed by GC-MS/ MS. The laccase enzyme was purified using UNO (R) sphere Q-1 anion exchange chromatography and the molecular weight was determined to be similar to 50 kDa on 10% SDS-PAGE. The laccase kinetic parameters V-max, K-m, and turnover number (K-cat) were found to be 76.9 mu M min(-1), 909 mM and 739 min(-1), respectively, from a Lineweaver-Burk plot. Furthermore, laccases are suitable for biotechnological applications that transform bark biomass into high value bark biopolymers/biochemicals. The differences observed among the identified aromatic compound MS/MS profiles were due to the utilization of two different bark species. Py-GC-MS analysis of bark showed differing effects of fungal activity on bark composition. Polyphenolics were separated in reverse-phase mode using HPLC with a pinnacle DB Biphenyl, C18 column, and UV detector. Two recognition wavelengths of 290 and 340 nm were selected to improve the separation of each single compound in monofloral honey and bark-fermented samples. This study is novel because it replaces natural mediators (NM) with monofloral honey in PM and bark materials impregnated with honey, and studies the effects of fungi-derived laccases on bark biopolymers.
机译:由于合成聚合物生产引起的废物生产和处置问题增加,因此迫切需要用可生物降解和可再生资源替代材料。尝试使用漆酶作为催化剂来增强酶的催化性能已显示它们是用于树皮解聚的有前途的解决方案。在这项研究中,测试了八种不同的真菌菌株在深层发酵(SF)过程中产生漆酶的能力,而平菇物种被证明是竞争真菌菌株中最好的生产者。 P. pulmonarius主要在pH 5.5和30摄氏度的初始条件下在生产培养基(PM)中产生漆酶。在SF中进行树皮解聚,当PM诱导为100 mg 50 mg时,我们在四周后鉴定出多酚/多芳族化合物。滞后阶段每个树皮的毫升数。在SF中,蜂蜜被用作PM中的天然介质替代物(NMS)期间,漆酶活性比在PM中不含蜂蜜的类似培养物中的漆酶活性高约1.5倍。通过GC-MS / MS分析这些样品。使用UNO(R)球Q-1阴离子交换色谱法纯化漆酶,并在10%SDS-PAGE上测定分子量类似于50 kDa。根据Lineweaver-Burk图,发现漆酶动力学参数V-max,K-m和周转数(K-cat)分别为76.9μMmin(-1),909 mM和739 min(-1)。此外,漆酶适用于将树皮生物质转化为高价值的树皮生物聚合物/生化物质的生物技术应用。在鉴定的芳族化合物MS / MS谱图中观察到的差异是由于利用了两种不同的树皮。皮的Py-GC-MS分析显示真菌活性对树皮组成的影响不同。使用高效液相色谱仪(具有顶峰DB Biphenyl,C18色谱柱和UV检测器)以反相模式分离多酚类化合物。选择两个识别波长290和340 nm,以改善单花蜂蜜和树皮发酵样品中每种化合物的分离。这项研究是新颖的,因为它在PM和浸有蜂蜜的树皮材料中用单花蜂蜜代替了天然介质(NM),并且研究了真菌衍生的漆酶对树皮生物聚合物的影响。

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