中国生漆化学成分研究

生漆作为天然高分子材料在我国应用已有6000多年的历史.其主要化学成分为漆酚、漆酶和漆多糖.提取分离并研究这些物质的化学组成、生物活性功能是多年来生漆化学研究的热点之一.总结了20多年来国内外关于漆酚、漆酶和漆多糖分离提取方法及漆多糖生物活性的最新研究进展.     

真菌漆酶在绿色化学中的研究进展

漆酶主要是由真菌分泌的一类胞外多铜氧化酶,因其具备多功能特性而被广泛地应用于绿色环境化学。漆酶能够以分子氧作为电子接受体,催化氧化多种酚类和非酚类底物形成自由基中间体,随后这些自由基中间体涉及到氧化耦合或键断裂,最终导致底物发生氧化、分解或聚合反应。目前,主要采用包埋、吸附、共价绑定和交联结合等方法制备固定化漆酶,以增强漆酶在实际环境中的催化活性、稳定性和循环再利用功效。概述了真菌漆酶的分子组成、结构特性及其催化氧化不同底物的作用机理,系统地比较了漆酶的固定化技术及其利弊,重点阐述了漆酶在有机污染物去除、合成染料脱色、造纸废水、食品加工、生物传感器和环境质量指示器等领域的研究进展,旨在为拓展和开发真菌漆酶在绿色环境化学中的多功能应用提供新的理论依据和指导思想。     

一色齿毛菌漆酶的酶学特性及染料脱色研究

染料由于具有复杂的化学结构通常难以降解。本文从白腐菌一色齿毛菌LS0547中纯化出胞外漆酶并用于染料脱色实验。SDS-PAGE结果显示纯化的漆酶分子量大小为63.7kDa。漆酶氧化底物ABTS的最适pH为2.2,最适温度为50℃。叠氮钠可强烈抑制漆酶活性,半胱氨酸和二硫苏糖醇可部分抑制漆酶活性。漆酶氧化ABTS,丁香醛连氮和2,6-二甲氧基苯酚的米氏常数分别为0.217,0.306和0.199mmol/L。粗酶和纯化的漆酶用于不同化学结构的染料的脱色研究,结果表明一色齿毛菌纯化漆酶可快速对RB亮蓝进行脱色,偶氮胭脂红和结晶紫的脱色效果低于RB亮蓝,测试的三种染料均可在没有介体存在的条件下被漆酶脱色,显示出一色齿毛菌漆酶在染料废水处理中的应用前景。     

灵芝(Ganoderma lucidum)漆酶基因的克隆及其序列分析

漆酶(laccase EC1·10·3·2)是一种含Cu的多酚氧化酶,自从1883年日本学者吉田首次从漆树汁液中发现以来,漆酶特别是真菌漆酶一直是生物学、化学和环境科学等领域十分活跃的研究热点,在纸浆的生物漂白[1,2],有毒污染物的降解[3~5]等方面有较大的应用价值.根据其来源主要分为漆树漆酶和真菌漆酶两大类,由一个结构相似的基因家族所编码,目前,至少有40个以上的真菌漆酶基因被克隆和测序[6~9],最近也有从细菌中克隆到漆酶基因的报道[10~12].我国幅员辽阔,具有十分丰富的真菌资源,但是我国对漆酶的研究与发达国家相比还十分落后,对于漆酶基因资…     

漆酶介导生物体内酚类氧化偶联的基本原理及其在绿色合成中的应用

漆酶(Laccase,p-diphenol dioxygen oxidoreductases,EC 1.10.3.2)是一类包含三核铜簇位点的多酚氧化还原酶,广泛存在于细菌、真菌、高等植物和昆虫体内。该类酶不仅能够促进生态系统中高分子木质素和腐殖质聚合物的生物分解,还可以催化有机体内单酚和多酚类化合物参与黑色素、木质素、黄酮类和角质层等功能酚聚合物的生物合成。漆酶介导有机物的分解代谢和合成代谢机制有益于生态环境中碳循环和生物形态发生变化。在生物体内,漆酶催化天然酚类单电子氧化形成苯氧活性自由基或醌类中间体,随后这些活性中间体发生自我偶联或交叉偶联反应,生成多种结构复杂的大分子C-C、C-O-C或C-N-C功能聚合产物。因此,通过人工模拟漆酶催化生物体内的绿色合成代谢机理和路径,合理设计和定向改造漆酶在生物体外催化酚类底物偶联形成大分子功能聚合产物的结构和特性,有望为拓展和研发漆酶在绿色合成化学中的多功能应用提供丰富的参考价值和新颖的见解思路。     

三种重要木质素降解酶研究进展

就三种重要木质素降解酶：LiP、MnP和漆酶在自然界的分布,化学组成、结构特征、降解机制、分子生物学等进行综述,并探讨了其作用协同性。     

汽爆秸秆漆酶协同作用提取木质素

组分分离是秸秆炼制的关键技术。本文建立了汽爆耦合漆酶协同作用工艺,研究其对秸秆物理形态、化学组成以及木质素碱提取过程的影响。研究结果表明汽爆破坏秸秆表面致密结构,提高比表面积,促进漆酶对秸秆木质素的氧化作用;红外分析表明,漆酶破坏了汽爆秸秆中半纤维素酯键,且愈创木基吸收峰减弱,漆酶削弱了木质素与纤维素间相互作用;汽爆漆酶协同作用后的秸秆木质素提取率提高约20%(70℃,120 min)。Nuclei Growth模型分析温和条件下秸秆木质素提取过程,动力学结果表明,汽爆漆酶协同预处理增加了汽爆秸秆木质素碱提过程中反应起始作用位点,并提高了该过程对温度的敏感性。汽爆-漆酶协同预处理是一种有效的分离木质素的方法,将在木质纤维素原料的生物炼制中发挥重要作用。     

真菌漆酶异源表达研究进展

由于漆酶能够氧化芳香类化合物和其它一些非芳香类有机物,具有广泛的底物特异性,因此在纸浆漂白、纺织品染料脱色、有毒废弃物的去除、生物修复和生物传感器等方面具有巨大的应用潜力。但是缺少大量廉价的酶源供应阻碍了漆酶商业化的应用,解决这个问题的一个主要方法就是通过漆酶的异源表达来获得大量的漆酶。综述了真菌漆酶在酵母表达系统和丝状真菌表达系统中表达的研究结果,着重总结了影响漆酶异源表达的因素和提高漆酶表达的策略。     

一种pH稳定的黄色漆酶的快速纯化和性质特征

通过丙酮沉淀和 DEAE- cellulose DE52 柱层析, 快速、有效地从一株白腐菌 Trametes sp. SQ01 的发酵液中纯化了漆酶。纯化的漆酶并非传统漆酶那样呈现蓝色, 而是一种黄色蛋白。以 ABTS 为底物时, 该酶的最适 pH 和温度分别是 pH 4.5 和 70°C, Km 为 0.029 mmol/L。T. SQ01 漆酶在 pH 3.0~11.0时, 酶活相对稳定, 在 pH 5.0 时最为稳定, 是目前报道的 pH 稳定性最好的漆酶。低浓度的金属离子(1 mmol/L) Cu2+、Mg2+ 、Ca2+ 和Co2+ 对漆酶有促进作用, 而高浓度(5 mmol/L)的Co2+、Zn2+、 Mn2+、Mg2+ 却抑制漆酶酶活。SDS 对该酶有激活作用, 当其浓度为1 mmol/L时, 漆酶相对酶活达到128%。DTT对漆酶强烈抑制, 即使是浓度为1 mmol/L, 亦可完全抑制漆酶酶活。纯化后的漆酶对亮蓝(RBBR) (100 mg/L)的脱色能力显著, 0.5 U/mL 的漆酶在 10 min内即可达到 80%的脱色率。T. sp. SQ01 漆酶的快速纯化以及高效脱色的能力表明该酶在染料脱色降解方面有着广阔的应用前景。     

漆酶的性质、功能、催化机理和应用

漆酶是一种结合多个铜离子的蛋白,是铜蓝氧化酶蛋白家族的一员。本文叙述漆酶的分子结构、底物特异性及其物理化学特性,并讨论漆酶的酶促反应机理和生物学功能,包括植物漆酶参与细胞壁的形成以及漆酶与病原菌毒力的关系。本文还着重介绍了漆酶在环境生物修复方面的应用。     

Improved recovery of active recombinant laccase from maize seed

Lignolytic enzymes such as laccase have been difficult to over-express in an active form. This paper describes the expression, characterization, and application of a fungal laccase in maize seed. The transgenic seed contains immobilized and extractable laccase. Fifty ppm dry weight of aqueously extractable laccase was obtained, and the remaining solids contained a significant amount of immobilized laccase that was active. Although a portion of the extractable laccase was produced as inactive apoenzyme, laccase activity was recovered by treatment with copper and chloride. In addition to allowing the apoenzyme to regain activity, treatment with copper also provided a partial purification step by precipitating other endogenous corn proteins while leaving >90% of the laccase in solution. The data also demonstrate the application of maize-produced laccase as a polymerization agent. The apparent concentration of laccase in ground, defatted corn germ is approximately 0.20% of dry weight.     

Association of laccase activity with conidiation in an aflatoxigenic strain of Aspergillus parasiticus

Abstract The relationship between laccase activity and asexual development in Aspergillus parasiticus was established. A. parasiticus produced a laccase activity similar to that reported for Aspergillus nidulans . Laccase activity appeared only in conidiating cultures and was absent from vegetative cultures. Shaking of the cultures inhibited conidiation and suppressed laccase activity. The composition of the media affected the degree of conidiation and the specific activity of laccase. Ammonium sulphate as sole nitrogen source was suppressive, whereas glutamate was highly stimulatory to both conidiation and laccase production. The addition of citrate was also stimulatory to conidia production and, to a lesser degree, laccase activity. There appears to be no quantitative correlation between laccase activity and the number of conidia produced.     

三相鼓泡塔生物反应器培养云芝菌合成漆酶

为了提高云芝菌发酵生产漆酶的效率,提出了一种利用自絮凝菌丝球在三相鼓泡塔生物反应器中重复分批发酵产漆酶的新方法。在优化后的产酶条件下,考察维生素C的添加浓度对漆酶活力的影响,并通过在培养基中添加维生素C进行漆酶多批次培养。研究结果表明,维生素C的添加浓度为1.50mmol/L时,可使漆酶活力提高2.6倍。连续进行了10批培养,每批最大漆酶的活力均在1000 U/mL以上,最高酶活出现在第五批为1919.6 U/mL,总培养时间达25 d。此方法所得漆酶对染料靛蓝具有明显的脱色降解作用,在介体1-羟基苯并三唑（HBT）用量0.10%,漆酶用量100 U/L条件下作用40 min时,靛蓝脱色率达到96.7%。该方法采用的三相鼓泡塔生物反应器性能稳定、菌丝球可重复使用,该方法有利于漆酶的高效、规模化生产。     

The reversible depletion and reconstitution of a copper ion in Coprinus cinereus laccase followed by spectroscopic techniques

The specific activities of crude and purified Coprinus cinereus laccase preparations could be enhanced by a factor of 10-12 by activation with copper ions. The copper to protein contents of purified non-activated laccase were 2.3 ± 0.1 compared to 3.3 ± 0.1 in purified activated laccase indicating that only a fraction of the laccase can be activated. Purified laccase not activated with copper ions shows in isoelectric focusing four bands in order of decreasing pI in a ratio 1/5/3/1 where only bands I and II had laccase activity. Purified activated laccase showed only three bands (I, II and III) in the ratio 5/4/1 all with some laccase activity. The pH profile of the activity for activated and non-activated laccase showed identical behavior indicating that the active forms were the same. The change in UV-Vis around 330 nm following the depletion and reconstitution of the enzyme combined with activity measurements supports the reversibility of the selective removal and insertion of copper ions at the type 2 site. The circular dichroism spectrum of activated purified laccase has characteristic changes around 350 nm relative to non-activated laccase indicative of changes at the type 2/type 3 sites. The difference between the electron paramagnetic resonance spectra of non-activated and activated C. cinereus laccase indicates that a fraction of the non-activated purified laccase contained a copper(II) signal with a coupling constant between a type 1 and a type 2 copper(II). This electron paramagnetic resonance signal could be explained by an induced asymmetry in the type 3 site due to a missing type 2 copper ion.     

Study on Remediation-improvement of 2,4-Dichlorophenol Contaminated Soil by Organic Fertilizer Immobilized Laccase

ABSTRACT

In this paper, laccase is immobilized by the cross-linking method, using organic fertilizer as a carrier and glutaraldehyde as a cross-linking agent. Here, the optimal conditions of laccase immobilization were explored and the optimal operating conditions and stabilities of free laccase and immobilized laccase were also studied. Then, free laccase and immobilized laccase were applied to the soil remediation. Meanwhile, the effect of soil improvement treated with immobilized laccase was studied through ecological evaluation. The results showed that the optimal conditions for laccase immobilization were: the volume fraction of glutaraldehyde was 5%, the amount of enzyme added was 15 mL, and the immobilization time was 6 h. Under the same conditions, thermal stability and acid-base stability of immobilized laccase were better than free laccase. Under the optimal conditions, using laccase to treat 2,4-dichlorophenol in the soil, it was found that the free laccase group degraded 44.4% within 5 days, while the immobilized laccase group degraded 58.6%. Although both the degradation trends and route are the same, the degradation effect of the latter is obviously better. Ecological evaluation showed that organic fertilizer carrier had an impact on soil physical and chemical properties and soil enzymes, playing a positive role in soil ecological security and improving the soil.     

A comparison of entrapped and covalently bonded laccase: Study of its leakage,reusability, and the catalytic efficiency in TEMPO-mediated glycerol oxidation

This article presents the comparison for reusability and leakage between entrapped and covalently bonded laccase and their performances towards the selective oxidation of glycerol. The reusability of immobilized laccase enzyme was studied by reacting a batch of immobilized laccase with ABTS for 15 cycles. The investigation of the leakage of immobilized laccase was carried out by storing the immobilized laccase in acetate buffer solution for 32 days. The data show that the retained enzyme activities of entrapped and covalently bonded enzyme after being reused for eight cycles were well above 60% and the leakages after storing for a month in the acetate buffer at 4?°C were well below 15%. The entrapped laccase coupled with TEMPO was found to perform better and gave a two-fold higher yield of glyceraldehyde and glyceric acid in the selective oxidation of glycerol compared to covalently bonded laccase. Hence, physical entrapment of laccase would be a suitable immobilization method in the laccase-mediated selective oxidation of glycerol.     

应用Coriolus vericolor 菌丝球脱色染料及印染废水的研究

对白腐真菌（Coriolus vericolor）产生漆酶进行了研究。发现该菌产漆酶的最适初始pH值为4．5。提高微量元素浓度或添加藜芦醇都可使C.versiclor的产酶能力增加,添加Tween80会有一定的抑制作用。采用C.versicolor菌丝球进行重复分批产酶试验,结果表明菌丝球的稳定性很好,同一批菌丝球可连续利用14次,平均每批酶活力可保持在6．72U／mL,产酶能力优于聚氨酯泡沫固定化菌丝。将粗酶液用要料的脱色降解试验,在酶活力为3．3IU／mL,酸性橙浓度为500mg/L条件下,经过24h反应,脱色率达到98．5％;对含弱酸大红和卡布龙红的印染废水进行脱色试验,脱色率也达到了93％。     

Laccase stabilization by covalent binding immobilization on activated polyvinyl alcohol carrier

AIMS: Attempts were made to immobilize laccase from Panus conchatus. METHODS AND RESULTS: The laccase was immobilized on carboxylated polyvinyl alcohol (PVA) activated by N-hydroxysuccinimide (N-HSI) in aqueous solution at different pHs, temperatures, and with different reaction times. An optimum condition for laccase immobilization is at pH 3.2, 40 degrees C and 12 h, respectively. Immobilization of laccase increased optimal pH for reaction with 2, 2'-azinobis (3-ethylbenzthiazoline-6-solfonate) (ABTS) and pH stability. Immobilized laccase proved to be reacted consecutively 17 times with only a 50% decrease on activity and be used in removal of 2,4,6-trichlorophenol (TCP). CONCLUSIONS: It was possible to immobilize the laccase on carboxylated polyvinyl alcohol by activation with N-hydroxysuccinimide in HAc-NaAc buffer. The immobilized laccase is both stable and reusable. SIGNIFICANCE IMPACT OF THE STUDY: The results indicate that this immobilized laccase can be used in the removal of poisonous effluent from pulp bleaching mills.     

Expression of the Pycnoporus cinnabarinus laccase gene in Aspergillus niger and characterization of the recombinant enzyme.

Pycnoporus cinnabarinus laccase lac1 gene was overexpressed in Aspergillus niger, a well-known fungal host producing a large amount of homologous or heterologous enzymes for industrial applications. The corresponding cDNA was placed under the control of the glyceraldehyde-3-phosphate dehydrogenase promoter as a strong and constitutive promoter. The laccase signal peptide or the glucoamylase preprosequence of A. niger was used to target the secretion. Both signal peptides directed the secretion of laccase into the culture medium as an active protein, but the A. niger preprosequence allowed an 80-fold increase in laccase production. The identity of the recombinant protein was further confirmed by immunodetection using Western blot analysis and N-terminal sequencing. The molecular mass of the mature laccase was 70 kDa as expected, similar to that of the native form, suggesting no hyperglycosylation. The recombinant laccase was purified in a three-step procedure including a fractionated precipitation using ammonium sulfate, and a concentration by ultrafiltration followed by a Mono Q column. All the characteristics of the recombinant laccase are in agreement with those of the native laccase. This is the first report of the production of a white-rot laccase in A. niger.     

Extracellular laccase activity and transcript levels of putative laccase genes during removal of the xenoestrogen technical nonylphenol by the aquatic hyphomycete Clavariopsis aquatica

We investigated the influence of potential laccase inducers with environmental relevance on extracellular laccase activity and removal of the xenoestrogen technical nonylphenol (tNP) by the aquatic hyphomycete Clavariopsis aquatica. Concomitantly, we identified two putative laccase gene fragments (Icc1 and Icc2) and have followed their expression during removal of tNP under different conditions. Our results indicate a significant effect of copper on extracellular laccase activity in supernatants of fungal cultures. Laccase activity was highest in the presence of copper when added together with vanillic acid, followed by copper when used alone. Only slight laccase activities were recorded in the presence of only vanillic acid, whereas in the absence of either compound laccase activities were negligible. Laccase activity was well correlated with the removal efficiency of tNP, indicating the involvement of laccase in tNP bioconversion. Overall, Icc2 was less expressed than Icc1. The expression of Icc1 and Icc2 correlated only partially with the measured laccase activity, suggesting the existence of cell-associated laccase fractions not detectable in fungal culture supernatants and/or the existence of additional laccase genes.