One-step fabrication of mesoporous sulfur-doped carbon nitride for highly selective photocatalytic transformation of native lignin to monophenolic compounds

Photocatalytic selective transform native lignin into valuable chemicals is an attractive but challenging task. Herein, we report a mesoporous sulfur-doped carbon nitride (MSCN-0.5) which is prepared by a facile one-step thermal condensation strategy. It is highly active and selective for the cleavage Cα?C_β bond in β?O?4 lignin model compound under visible light radiation at room temperature, achieving 99% substrate conversion and 98% C_α?C_β bond cleavage selectivity. Mechanistic studies revealed that the C_β?H bond of lignin model compounds activated by holes and generate key C_β radical intermediates, further induced the C_α?C_β bond cleavage by superoxide anion radicals (^?O₂^?) to produce aromatic oxygenates. Waste Camellia oleifera shell (WCOS) was taken as a representative to further understand the reaction mechanisms on native lignin. 33.2 mg of monophenolic compounds (Vanillin accounted for 22% and Syringaldehyde for 34%) can be obtained by each gram of WCOS lignin, which is 2.5 times as that of the pristine carbon nitride. The present work offers useful guidance for designing metal-free heterogeneous photocatalysts for C_α?C_β bond cleavage to harvest monophenolic compounds.     

Urchin-like Nb2O5 hollow microspheres enabling efficient and selective photocatalytic C–C bond cleavage in lignin models under ambient conditions

Selective cleavage of robust C?C bonds to harvest value-added aromatic oxygenates is an intriguing but challenging task in lignin depolymerization. Photocatalysis is a promising technology with the advantages of mild reaction conditions and strong sustainability. Herein, we show a novel urchin-like Nb₂O₅ hollow microsphere (U-Nb₂O₅ HM), prepared by one-pot hydrothermal method, are highly active and selective for Cα?C_β bond cleavage of lignin β-O-4 model compounds under mild conditions, achieving 94% substrate conversion and 96% C?C bond cleavage selectivity. Systematic experimental studies and density functional theory (DFT) calculations revealed that the superior performance of U-Nb₂O₅ HMs arises from more exposed active sites, more efficient free charge separation and the active (001) facet, which facilitates the activation of C_β?H bond of lignin models and generate key C_β radical intermediates by photogenerated holes, further inducing the C_α?C_β bond cleavage to produce aromatic oxygenates. This work could provide some suggestions for the fabrication of hierarchical photocatalysts in the lignin depolymerization system.     

Organic amine mediated cleavage of Caromatic–Cα bonds in lignin and its platform molecules

The activation and cleavage of C–C bonds remains a critical scientific issue in many organic reactions and is an unmet challenge due to their intrinsic inertness and ubiquity. Meanwhile, it is crucial for the valorization of lignin into high-value chemicals. Here, we proposed a novel strategy to enhance the C_aromatic–C_α bond cleavage by pre-functionalization with amine sources, in which an active amine intermediate is first formed through Markovnikov hydroamination to reduce the dissociation energy of the C_aromatic–C_α bond which is then cleaved to form target chemicals. More importantly, this strategy provides a method to achieve the maximum utilization of the aromatic nucleus and side chains in lignin or its platform molecules. Phenols and N,N-dimethylethylamine compounds with high yields were produced from herbaceous lignin or the p-coumaric acid monomer in the presence of industrially available dimethylamine (DMA).

Pre-functionalization with amine sources mediated the cleavage of C_aromatic–C_α bonds to produce two valuable chemicals with high yields, for the full utilization of the aromatic rings and side-chains in lignin and its platform molecules.     

Depolymerization and hydrodeoxygenation of lignin to aromatic hydrocarbons with a Ru catalyst on a variety of Nb-based supports

Efficient conversion of lignin to aromatic hydrocarbons via depolymerization and subsequent hydrodeoxygenation is important. Previously, we found that NbO_x species played a key role in the activation and cleavage of C–O bonds in lignin and its model compounds. In this study, commercial niobic acid (HY-340), niobium phosphate (NbPO-CBMM) and lab-made layered niobium oxide (Nb₂O₅-Layer) were chosen as supports to study the effect of Brönsted and Lewis acids on the activation of C–O bonds in lignin conversion. A variety of Ru-loaded, Nb-based catalysts with different Ru particle sizes were prepared and applied to the conversion of p-cresol. The results show that all the Ru/Nb-based catalysts produce high mole yields of C₇–C₉ hydrocarbons (82.3–99.1%). What's more, Ru/Nb₂O₅-Layer affords the best mole yield of C₇–C₉ hydrocarbons and selectivity for C₇–C₉ aromatic hydrocarbons, of up to 99.1% and 88.0%, respectively. Moreover, it was found that Lewis acid sites play important roles in the depolymerization of enzymatic lignin into phenolic monomers and the cleavage of the C–O bond of phenols. Additionally, the electronic state and particle size of Ru are significant factors which influence the selectivity for aromatic hydrocarbons. A partial positive charge on the metallic Ru surface and a smaller Ru particle size are beneficial in improving the selectivity for aromatic hydrocarbons.     

Lignin-degrading enzyme fromPhanerochaete chrysosporium

The extracellular fluid of ligninolytic cultures of the white-rot wooddestroying fungus,Phanerochaete chrysosporium Burds., contains an enzyme that degrades lignin model compounds as well as lignin itself (1). Like ligninolytic activity, the enzyme appears during idiophasic metabolism, which is triggered by nitrogen starvation. The enzyme has been purified to homogeneity by DEAE-Biogel A chromatography, as assessed by SDS polyacrylamide gel electrophoresis, isoelectric focusing, and gel filtration chromatography. These techniques also revealed a molecular weight of 42,000 daltons, and an isoelectric point of 3.4. The purified enzyme exhibits low substrate specificity. It is an oxygenase, but requires hydrogen peroxide for activity. The activity is optimum at 0.15 mM H₂O₂; at concentrations above 0.5 mM, H₂O₂is inhibitory. Model compound studies have shown that the enzyme catalyzes cleavage between Cα and Cß in compounds of the type aryl-CαHOH—CßHR-(R = -aryl or -O-aryl), and in the Cα-hydroxyl-bearing propyl side chains of lignin. This cleavage produces an aromatic aldehyde moiety from the Cα-portion, and a Cß-hydroxylated moiety from the Cα-portion. Cleavage between Cα and Cß in arylglycerol-Β-aryl ether structures leads indirectly to cleavage of the Β-aryl ether linkage, which is the most abundant intermonomer linkage in lignin. The Cß-hydroxyl oxygen comes from molecular oxygen, and not from H₂O₂, as determined by¹⁸O isotope studies. The pH optimum for these reactions is between 2.5 and 3.0; no activity is observed above pH 5. Formation of the expected aldehydes from spruce and birch lignins, and partial depolymerization of the lignins results from the action of the purified enzyme. In addition to Cα—Cß cleavage, the enzyme catalyzes aromatic alcohol oxidation, aryl methylene oxidation, hydroxylation at Cα and Cß in models containing a Cα—Cß double bond, intradiol cleavage in phenylglycol structures, and phenol oxidations.     

Co-biomass degradation of fluoranthene by marine-derived fungi; Aspergillus aculeatus and Mucor irregularis: Comprehensive process optimization,enzyme induction and metabolic analyses

The application and relevance of marine-derived fungi in the mycoremediation of environment polluted with polycyclic aromatic hydrocarbons (PAHs) is promising whilst limiting environmental hazards. The present study investigated the fluoranthene degradation efficiency of marine-derived fungal co-culture, Aspergillus aculeatus (AA) and Mucor irregularis (MI) in batch processes (Plackett-Burman experiments) enhanced with the addition of surfactants and solid-state substrates. Further optimization studies done through fractional factorial design revealed that the co-culture exhibited 98.4% fluoranthene degradation capacity after 7 days of incubation. The role played by enzymes was revealed with 93, 85 and 71% induction of laccase, lignin peroxidase and manganese peroxidase respectively during fluoranthene degradation. The Gas Chromatography-Mass Spectrometry analysis revealed the formation of five metabolites; 1,2- dihydroxyfluoranthene, 9H-fluorene-1,9-dicarboxylic acid, benzene-1,2,4-tricarboxylic acid, benzene-1,3-dicarboxylic acid and benzoic acid after fluoranthene degradation by AA + MI co-culture which was used in predicting a metabolic pathway. The findings of this study elucidated the promising potentials of marine-derived fungal co-biomass in the eco-friendly remediation of polycyclic aromatic hydrocarbons thus promoting green technology.     

Destruction of aspen wood by the fungusPhanerochaete sanguinea quantitative1H and13C NMR spectroscopies of biologically degraded lignin

The lignin of mechanically ground aspen wood and lignins isolated from aspen wood attacked by the fungusPhanerochaete sanguinea have been investigated by quantitative¹H and¹³C NMR spectroscopies. It has been shown that the biodestruction of the lignin takes place through the cleavage of alkyl-aryl and aryl-aryl bonds and is accompanied by demethylation (demethoxylation) reactions, and the oxidation of C_α and C_γ atoms. In addition to reactions in which the C—C bonds are cleaved, the formation of ether bonds has been observed. An interconnection has been shown between the variations in the amount of functional groups, fragments, and the bonds in biolignins and the loss in mass of the wood. A method is proposed for evaluating the carbohydrate content in lignin preparations using the NMR method.     

Beech Lignin—Proposal of a Constitutional Scheme

The high molecular weight material lignin consists of phenylpropane units linked together by a variety of bond types. During the past eight years, two newly developed degradation procedures have permitted the first direct determinations of the nature of these bonds. The first procedure affords a very mild partial hydrolysis of benzyl ether bonds. Eleven dimeric, trimeric, and tetrameric degradation products were obtained in this way from spruce and beech lignin: they exhibited three different kinds of bonds between the C₉ structural units, and their structures have all been elucidated. In the second procedure, the most important kind of bond in lignin, i. e. the arylglycerol-β-aryl ether bond, can be subjected to directed cleavage under mild conditions after introduction of a suitable neighboring group. On application to beech lignin, 91 % of the material was degraded giving monomeric to tetrameric phenols. Complete structural elucidation of the twenty dimeric phenols isolated and a knowledge of their relative yields and the yields of the other fractions obtained by gel filtration permitted a structural scheme to be set up for beech lignin in which the C₉ structural units are linked together by no less then ten different kinds of bonds. The structural scheme, which can be readily explained biogenetically, has the same elemental composition as natural beech lignin. Further support for the structural scheme comes from a comparison of the ¹³C-NMR spectrum of natural beech lignin and a ¹³C-NMR spectrum calculated for the proposed structure on the basis of about fifty lignin model substances.     

On the kinetics of polymer degradation in solution—VII. Laser flash photolysis of poly-α-methylstyrene in solution

Poly-α-methylstyrene (PαMS) was degraded in CHCl₃ and CCl₄ solution by flash photolysis (λ = 265 nm). The degradation, as detected by light scattering measurements, is caused by the attack on PαMS by solvent radicals, assumed to be formed mainly by energy transfer processes. The direct effect did not lead to detectable main chain cleavage as evidenced by experiments with PαMS dissolved in dioxane or methylene chloride. The time dependence of the decrease of the light scattering intensity (LSI) after the flash was measured. The observed first order lifetime τ(LSI) corresponds to the lifetime of lateral macroradicals P′ that decompose by main chain cleavage (k = 3.5 × 10² sec^?1). Molecular oxygen reacts with the lateral macroradicals with k = (5.5 ± 0.5) 10⁵ M^?1 sec^?1. Only a minor portion of the product of this reaction (PO₂′) decays by main chain scission. Thus O₂ inhibits main chain scission significantly. By addition of cyclohexane and ethyl mercaptan, the main chain cleavage is inhibited. τ(LSI) was not affected by these compounds in the concentration range investigated ([C₆H₁₂]: up to 8.4 M; [C₂H₅SH]: up to 3 × 10^?3 M), indicating that they reacted with solvent radicals which otherwise attack the polymer forming lateral macroradicals.     

Glycosides of marine invertebrates. XXVI. Holothurin A from the Pacific Ocean holothurianHolothvria squamifera. Isolation of the native aglycone

The known triterpene tetraoside holothurin A has been isolated from the Pacific Ocean holothurianHolothuria squamifera. By using two independent methods — enzymatic cleavage and two-stage Smith degradation — 22,25-epoxyholost-9(11)-ene-3β,12α,17α-triol, C₃₀H₄₆O₆, which is the native aglycone of holothurin A, was obtained. The structure of the native aglycone has been established on the basis of the results of IR, mass, and PMR spectroscopy.     

Convenient synthesis of chiral lignin model compounds via optical resolution: four stereoisomers of guaiacylglycerol-β-guaiacyl ether and both enantiomers of 3-hydroxy-1-(4-hydroxy-3-methoxyphenyl)-2-(2-methoxyphenoxy)-propan-1-one (erone)

Guaiacylglycerol-β-guaiacyl ether (GGE) is one of the most important phenolic compound for studying the chemistry and biochemistry of lignin. GGE contains two asymmetric carbons at the alpha and beta positions of its side chain; therefore, theoretically it can exist as four different stereoisomers. It has been proposed that a Gram-negative bacterium, Sphingobium sp. SYK-6 (formerly referred as Sphingomonas paucimobilis SYK-6), degrades GGE enantiospecifically via cleavage of the ether bond. The cleavage was thought to proceed in two steps, each catalyzed by a different enantiospecific enzyme. In the first step, the alcohol residue at the alpha position of the side chain in GGE was thought to be oxidized enantiospecifically by four distinct Cα-dehydrogenases (LigD, LigN, LigL and LigO), to produce two enantiomers of 3-hydroxy-1-(4-hydroxy-3-methoxyphenyl)-2-(2-methoxyphenoxy)-propan-1-one (erone). To study this enantiospecific degradation step by the four dehydrogenases, we synthesized all four stereoisomers of GGE and both enantiomers of erone and separated them into enantiopure samples. The stereoisomers and our synthetic methods to prepare them are useful both for microbial and chemical investigations of lignin degradation.     

Cotton Stalk Pretreatment Using <Emphasis Type="Italic">Daedalea flavida</Emphasis>, <Emphasis Type="Italic">Phlebia radiata</Emphasis>, and <Emphasis Type="Italic">Flavodon flavus</Emphasis>: Lignin Degradation,Cellulose Recovery,and Enzymatic Saccharification

Lignocellulolytic enzyme activities of selective fungi Daedalea flavida MTCC 145 (DF-2), Phlebia radiata MTCC 2791 (PR), and non-selective fungus Flavodon flavus MTCC 168 (FF) were studied for pretreatment of cotton stalks. Simultaneous productions of high LiP and laccase activities by DF-2 during early phase of growth were effective for lignin degradation 27.83 ± 1.25 % (w/w of lignin) in 20-day pretreatment. Production of high MnP activity without laccase in the early growth phase of PR was ineffective and delayed lignin degradation 24.93 ± 1.53 % in 25 days due to laccase production at later phase. With no LiP activity, low activities of MnP and laccase by FF yielded poor lignin degradation 15.09 ± 0.6 % in 20 days. Xylanase was predominant cellulolytic enzyme produced by DF-2, resulting hemicellulose as main carbon and energy source with 83 % of cellulose recovery after 40 days of pretreatment. The glucose yield improved more than two fold from 20-day DF-2 pretreated cotton stalks after enzymatic saccharification.     

Biodegradation of cotton straw byPleutorus florida

Cotton straw is an unutilized waste product containing 25% lignin, thus making it unsuitable for use as animal feed. This material was found to be an excellent substrate for the growth of the edible mushroomPleurotus florida. A growth-promoting flavonoid was isolated from the water-soluble fraction of the straw (Platt et al., 1983). After 3 wk of fungal growth on native cotton straw, an 18% decrease in dry weight occurred. Lignin (insoluble in 72% H₂SO₄) was degraded from the 8th d of growth up to a total of 65% of the original content after 21 d. Prior to lignin degradation, sugars and other water-soluble materials were removed and laccase activity (substrate, 2,6-dimethoxyphenol) was detected. This activity disappeared after the eighth day of growth. In all our experiments it appears that laccase activity precedes the onset of lignin degradation. Cellulase activity reached a maximum after 8 d of fungal growth and immediately disappeared. Total fungal activity was estimated by measuring hydrolysis of fluorescein diacetate (FDA), which indicated a gradual increase during the first 8 d and then reached a plateau. Release of glucose from the straw by commercial cellulase increased with duration of fungal growth from 28 (Μ/g/h^-1 to 250 Μg/g/h^-1. These results are corroborated by information from artificial rumen experiments showing an increase of in vitro dry matter digestability from 26 to 38%. In comparison, on washed straw, FDA and laccase activity was three-fold smaller. Final dry weight reduction was 10.1%, while total lignin loss was only 33% of the original lignin content. It seems that the water-soluble materials are responsible for the rapid growth, increased enzymatic activity, and total degradation of cotton straw byP. florida.     

Structure and Action Mechanism of Ligninolytic Enzymes

Lignin is the most abundant renewable source of aromatic polymer in nature, and its decomposition is indispensable for carbon recycling. It is chemically recalcitrant to breakdown by most organisms because of the complex, heterogeneous structure. The white-rot fungi produce an array of extracellular oxidative enzymes that synergistically and efficiently degrade lignin. The major groups of ligninolytic enzymes include lignin peroxidases, manganese peroxidases, versatile peroxidases, and laccases. The peroxidases are heme-containing enzymes with catalytic cycles that involve the activation by H₂O₂ and substrate reduction of compound I and compound II intermediates. Lignin peroxidases have the unique ability to catalyze oxidative cleavage of C–C bonds and ether (C–O–C) bonds in non-phenolic aromatic substrates of high redox potential. Manganese peroxidases oxidize Mn(II) to Mn(III), which facilitates the degradation of phenolic compounds or, in turn, oxidizes a second mediator for the breakdown of non-phenolic compounds. Versatile peroxidases are hybrids of lignin peroxidase and manganese peroxidase with a bifunctional characteristic. Laccases are multi-copper-containing proteins that catalyze the oxidation of phenolic substrates with concomitant reduction of molecular oxygen to water. This review covers the chemical nature of lignin substrates and focuses on the biochemical properties, molecular structures, reaction mechanisms, and related structures/functions of these enzymes. Reference to a company and/or products is only for purposes of information and does not imply approval of recommendation of the product to the exclusion of others that may also be suitable. All programs and services of the US Department of Agriculture are offered on a nondiscriminatory basis without regard to race, color, national origin, religion, sex, age, marital status, or handicap.     

Chemical Characterization of Kraft Lignin Prepared from Mixed Hardwoods

Chemical characterization of kraft lignin (KL) from mixed hardwoods (Acacia spp. from Vietnam and mixed hardwoods (mainly Quercus spp.) from Korea) was conducted for its future applications. To compare the structural changes that occurred in KL, two milled wood lignins (MWLs) were prepared from the same hardwood samples used in the production of KL. Elemental analysis showed that the MWL from acacia (MWL-aca) and mixed hardwood (MWL-mhw) had almost similar carbon content, methoxyl content, and C₉ formula. KL had high carbon content but low oxygen and methoxyl contents compared to MWLs. The C₉ formula of KL was determined to be C₉H_7.29O_2.26N_0.07S_0.12(OCH₃)_1.24. The M_w of KL and MWLs was about 3000 Da and 12,000–13,000 Da, respectively. The structural features of KL and MWLs were investigated by Fourier transform infrared spectroscopy (FT-IR) and nuclear magnetic resonance spectrometry (¹H, ¹³C NMR). The analyses indicated that KL underwent severe structural modifications, such as γ-carbon cleavage, demethylation, and polycondensation reactions during kraft pulping, which resulted in increased aromatic content and decreased aliphatic content. The main linkages in lignin, β-O-4 moieties, were hardly detected in the analysis as these linkages were extensively cleaved by nucleophilic attack of SH^- and OH^- during pulping.     

Enzymes involved in cellulose and lignin degradation

A detailed presentation was given of the discovered and studied enzymes involved in degradation of cellulose and lignin by the white-rot fungus,Sporotrichum pulverulentum (Phanerochaete chrysosporium). The fungus utilizes, for the degradation of cellulose: (a) Five different endo-1,4-Β-glucanases (b) One exo-1,4-Β-glucanase (acting synergistically with the endoglucanases) (c) Two 1,4-Β-glucosidases The regulation, induction, and catabolite repression of the endoglucanases have been studied in depth and the results of these studies were also presented. In addition to the hydrolytic enzymes,S. pulverulentum also produces the oxidative enzyme cellobiose oxidase that is of importance for cellulose degradation. Another unconventional enzyme is cellobiose: quinone oxidoreductase, which is of importance for both cellulose and lignin degradation. It reduces quinones from the lignin under oxidation of cellobiose from the cellulose. It has recently been discovered thatS. pulverulentum produces two acidic proteases of importance for cellulose degradation since they enhance the endoglucanase activity, particularly in young cultures of the fungus grown on cellulose. The enzymes involved in lignin degradation are not known nearly as well as these involved in cellulose degradation. However, extracellular phenol oxidases, laccase, and peroxidase have been shown to be involved in and necessary for lignin degradation to take place. A phenol oxidase-less mutant ofS. pulverulentum cannot degrade lignin unless a phenol oxidase is added to the medium. Recently, an enzyme splitting the α—Β bond in the propane side chain has been discovered by Kirk and coworkers. Several enzymes involved in the metabolism of vanillic acid, always a metabolite in lignin degradation, have been discovered and studied in our laboratory. Presentations of the enzymes for decarboxylation, demethoxylation, methanol oxidation, ring cleavage, and intracellular quinone reduction by NAD(P)H: quinone oxidoreductase were given. A discussion of possibilities for a specific enzymic primary attack on the native lignin, as well as of the likeliness for an unspecific radical nature of this attack, was also given.     

Influences of Proline and Cysteine Residues on Fragment Yield in Matrix-Assisted Laser Desorption/Ionization In-Source Decay Mass Spectrometry

Matrix-assisted laser desorption/ionization in-source decay produces highly informative fragments for the sequencing of peptides/proteins. Among amino acids, cysteine and proline residues were found to specifically influence the fragment yield. As they are both frequently found in small peptide structures for which de novo sequencing is mandatory, the understanding of their specific behaviors would allow useful fragmentation rules to be established. In the case of cysteine, a c?/w fragment pair originating from Xxx–Cys is formed by side-chain loss from the cysteine residue. The presence of a proline residue contributes to an increased yield of ISD fragments originating from N–C_α bond cleavage at Xxx₁–Xxx₂Pro, which is attributable to the cyclic structure of the proline residue. Our results suggest that the aminoketyl radical formed by MALDI-ISD generally induces the homolytic N–C_α bond cleavage located on the C–terminal side of the radical site. In contrast, N–C_α bond cleavage at Xxx–Pro produces no fragments and the N–C_α bond at the Xxx₁–Xxx₂Pro bond is alternatively cleaved via a heterolytic cleavage pathway.      

Gas-phase CαCβ double bond cleavage in the dissociation of protonated 2-benzylidenecyclopentanones: Dissociative proton transfer and intramolecular proton-transport catalysis

Among gas-phase dissociation reactions, double bond cleavage reaction appears to happen extremely rare, especially in the case of CC double bond. In the dissociation reaction of protonated 2-benzylidenecyclopentanones in tandem mass spectrometry, the formation of benzyl cations was observed, resulting from the cleavage of C^α=C^β double bonds, which is different from the general cleavage route seen in most α, β-unsaturated ketone cases. A combined experimental and theoretical investigation on intramolecular hydrogen transfers was carried out to illustrate the mechanisms. The external proton is initially localized on the carbonyl oxygen (the thermodynamically-preferred protonation site). Upon collisional activation, the mobile proton stepwise migrates to the C^α position to achieve the reduction and subsequent cleavage of the C^α=C^β double bond. The stepwise proton transfer is achieved via intramolecular proton-transport catalysis with the assistance of the phenyl ring. The ortho position of the phenyl accepts the proton from the carbonyl oxygen via a 1,6-H shift, and then donates it to the C^α stepwise. The conventional 1,3-H shift from the carbonyl oxygen to the C^α position can be excluded in this case due to its significant energy barrier. Further isotope-labeling experiments are applied to confirming the reaction mechanism. Last but not least, the scope-expansion experiments indicates that the aromatic and cycloalkanonyl moieties play a crucial roles in the cleavage reaction of C^α=C^β double bond.     

Ligninolytic Fungal Laccases and Their Biotechnological Applications

Lignin is amorphous in nature, lacks stereoregularity, and is not susceptible to hydrolytic attack. Despite its resistant nature, it is however degraded by various microorganisms, particularly, white-rot fungi. Such fungi are capable of extracellular production of lignin peroxidase, manganese peroxidase, and laccase, the three major enzymes associated with ligninolysis. Though all white-rot fungi do not produce all the three enzymes, laccase occupies an important place in ligninolysis. Laccase belongs to a diverse group of enzymes called oxidoreductases and is also known as benzenediol: oxygen oxidoreductase. They have low substrate specificity. The copper-containing enzyme laccase has been detected in a variety of organisms such as bacteria, fungi, plants, and insects. Mostly, these are extracellular proteins, although intracellular laccases have also been detected in some fungi and insects. Fungal laccases are believed to play a variety of roles, such as, morphogenesis, pathogenesis, and lignin degradation. As an oxidase, laccase is used in many agricultural, industrial, and medicinal applications. Current investigations are focused on laccase-based biooxidation, biotransformation, biosensor, and enzymatic synthesis of organic compounds. By enhancing laccase production using different physiochemical parameters, better understanding of the mechanism for the reactions of interest, and optimizing the catalytic activity of laccase, it can be used in a better way in diverse fields of biotechnology.     

Valorization of Rice Straw via Hydrotropic Lignin Extraction and Its Characterization

Rice straw hydrotropic lignin was extracted from p-Toluene sulfonic acid (p-TsOH) fractionation with a different combined delignification factor (CDF). Hydrotropic lignin characterization was systematically investigated, and alkaline lignin was also studied for the contrast. Results showed that the hydrotropic rice straw lignin particle was in nanometer scopes. Compared with alkaline lignin, the hydrotropic lignin had greater molecular weight. NMR analysis showed that β-aryl ether linkage was well preserved at low severities, and the unsaturation in the side chain of hydrotropic lignin was high. H units and G units were preferentially degraded and subsequently condensed at high severity. High severity also resulted in the cleavage of part β-aryl ether linkage. ³¹P-NMR showed the decrease in aliphatic hydroxyl groups and the increasing carboxyl group content at high severity. The maximum weight loss temperature of the hydrotropic lignin was in the range of 330–350 °C, higher than the alkaline lignin, and the glass conversion temperature (T_g) of the hydrotropic lignin was in the range of 107–125 °C, lower than that of the alkaline lignin. The hydrotropic lignin has high β-aryl ether linkage content, high activity, nanoscale particle size, and low T_g, which is beneficial for its further valorization.