氨基树脂固定化S-腺苷甲硫氨酸合成酶的研究

以氨基树脂为载体对S-腺苷甲硫氨酸(SAM)合成酶进行固定化,优化了酶的固定化条件并对固定化酶的性质进行了研究。优化的固定化条件为:戊二醛体积分数5%、SAM合成酶添加量20mg·g-1、固定化时间5h。所制备的固定化SAM合成酶的酶活力为476.8U·g-1,酶活力回收率为74.5%。与游离SAM合成酶相比,固定化SAM合成酶的稳定性大幅提高,在50℃孵育5h酶活力仍保留61.2%,而游离SAM合成酶则完全失活;在pH值为6.0~6.5、8.0~9.5的缓冲溶液中,固定化SAM合成酶也更加稳定;固定化SAM合成酶连续催化反应10批次,酶活力保留86.3%;固定化SAM合成酶在4℃储存30d,酶活力保留81.4%。固定化SAM合成酶米氏常数KATPm=0.14mmol·L-1,KLm-Met=0.28mmol·L-1。     

青霉素酰化酶基因工程菌 E.coli A_(56)(pPA22)水解青霉素 G 的动力学

用初速度法测定了青霉素酰化酶基因工程菌 E.coli A_(56)(pPA22)游离细胞和固定化细胞水解青霉素 G 的动力学常数,并进行了动力学模型的检验。该菌体酶活高,米氏常数小,固定化后米氏常数和苯乙酸抑制常数增大,底物抑制常数和6-APA 抑制常数没有变化。通过青霉素 G 裂解过程的考察,验证了青霉裂解动力学模型的适用性及动力学常数测定的可靠性。     

磁性壳聚糖微球的制备及其用于甲酸脱氢酶的固定化

分别采用乳化交联法和共沉淀法制备磁性壳聚糖微球载体,并对形貌结构进行比较,结果表明,采用共沉淀法制备的磁性壳聚糖微球负载Fe3O4的效果好,故将其作为载体固定甲酸脱氢酶。最佳固定化条件:添加酶量9 U.g-1,pH=7.0,固定化时间5 h。游离酶和固定化酶的最适宜反应温度分别为50℃和30℃;游离酶的最适宜pH=7.0,固定化酶的最适宜pH=6.0;将游离酶和固定化酶分别置于60℃恒温水浴放置180 min后,游离酶和固定化酶的相对酶活力分别为0.78%和40.39%;将游离酶和固定化酶置于不同pH的缓冲液中保存1 h后,在强酸(pH=2.0)和强碱(pH=10.0)条件下,固定化酶的相对酶活力分别为11.03%和38.43%,游离酶已全部失活;固定化酶重复使用6次后,相对酶活力为73.53%,表明固定化酶具有较好的热稳定性、酸碱稳定性和操作稳定性。     

陶瓷-壳聚糖复合材料固定真菌漆酶酶学性质研究

以陶瓷为第一载体、壳聚糖为二次载体、戊二醛为交联剂,采用共价结合和吸附联用法制备固定化漆酶,并研究了固定化漆酶的性质.固定化酶最适pH为3.0,最适温度分别为25℃和50℃,均与游离酶相同.在pH 3.0,温度25℃时,固定化酶对ABTS的表观米氏常数为66.64 μmol/L.与游离酶相比,固定化酶的热稳定性明显提高,并具有良好的贮存和操作稳定性.     

AS1.398中性蛋白酶的固定化研究

利用壳聚糖为载体，戊二醛为交联剂，对AS1．398中性蛋白酶进行了固定化研究，固定化反应的最佳条件是采用1％的戊二醛浓度，壳聚糖和戊二醛的交联反应时间为4h，加入酶固定化反应12h，固定化酶的最适温度35℃，最适pH值8．0。得到的固定化酶的活力回收平均为82．5％，固定化酶的稳定性能好于游离酶。     

固定化细胞延胡索酸酶性质的研究

探讨了海灌酸钠固定化普通变形杆菌延胡索酸酶的性质。研究结果表明：酶催化延胡索酸为Ｌ－苹果酸的最适温度为４０℃，最适ｐＨ为７．０。在温度低于４０℃和ｐＨ５。０～８．０的条件下，固定化细胞酶活力稳定性好，显示其热稳定性和ｐＨ稳定性明显优于游离细胞。Ｃｙｓ对固定化细胞酶活力无影响，ＧＳＨ对前激活作用。     

磁性壳聚糖微球的制备及其固定化乳糖酶的研究

采用水热法制备得到磁性Fe_3O_4纳米粒子,以壳聚糖、制备的Fe_3O_4为原料,采用乳化交联法成功制备了磁性壳聚糖微球,并通过SEM、FTIR、VSM、XRD对其进行表征。进一步以制备的磁性壳聚糖微球为载体,采用吸附法制备磁性壳聚糖微球固定化乳糖酶。以酶活力为考察指标,研究了不同固定化条件对制备固定化酶的影响,以及固定化酶的酶学性质。结果表明,乳糖酶的最佳固定化条件为:固定化时间4 h,pH为7.0,乳糖酶酶液浓度为0.6 mg/mL,固定化酶相对于游离酶的pH稳定性和温度稳定性均有一定程度的提高,固定化酶重复使用5次后,酶活仍保留65%以上。     

响应面法优化海藻酸钠固定α-淀粉酶的研究

利用海藻酸钠为载体包埋制备固定化α-淀粉酶,在海藻酸钠浓度,氯化钙浓度和游离酶添加量的单因素实验基础上,采用响应曲面设计对三因素进行优化确定固定化的最优条件。得到的最佳条件为:海藻酸钠浓度为2.48%、氯化钙浓度为2.04%、游离酶浓度为0.23%,在该条件下进行验证实验得到固定化酶的回收率为74%,达到了较高的固定化酶的回收率。     

超氧化物歧化酶的固定化及其酶学性质

目的制备固定化超氧化物歧化酶(SOD),并分析其酶学性质。方法以壳聚糖为载体,戊二醛为交联剂,制备固定化超氧化物歧化酶。以邻苯三酚自氧化法分别测定溶液酶与固定化酶的活力,并计算回收率。对固定化酶的温度和pH稳定性、半衰期、重复使用的回收率及米氏常数(Km)进行测定。结果固定化超氧化物歧化酶活力为333U/g,酶活回收率为86.32%,半衰期为43.8d;固定化酶室温保存5d后,相对酶活力仍保持在80%以上,最适反应温度为45℃,使用一次后回收率为70.12%,重复使用两次后回收率为51.72%;固定化酶与溶液酶在pH6时活性最强,Km分别为0.18mmol/L和0.16mmol/L。结论该固定化酶较溶液酶的稳定性得到提高,便于贮存,在食品、药品、日用品等领域有良好的应用前景。     

明胶膜固定化脲酶的制备及性质

以明胶为载体,戊二醛为交联剂,采用包埋-交联联用法制备了明胶膜固定化脲酶,其酶活力为6 07U/g载体,酶活力收率为66 1%。最优固定化条件是包酶量为10mg酶/g明胶,ρ(明胶)=100g/L,φ(戊二醛)=0 5%。研究了固定化酶的性质,并与游离酶作了比较,游离酶的最适pH=7 0,固定化酶的最适pH=6 5;游离酶的最适温度为60℃,固定化酶的最适温度升至70℃;固定化酶与游离酶的米氏常数Km分别为11 7mM和12 4mM;固定化酶在80℃下180min仍保留初始活力的10%,而游离酶几乎完全失活。固定化酶重复使用20次其活力仅下降15%,4℃下贮存35d后仍保持初始活力的55%。     

Immobilized penicillin G acylase on mesoporous silica: The influence of pore size, pore volume and mesophases

Penicillin G acylase (PGA) was immobilized on KIT-6 and SBA-15 with different pore sizes to study the influence of pore size, pore volume and mesophases on the immobilized enzyme (IME) activity. The results show that the pore size, pore volume, mesophase and surface area have an obvious influence on the IME activity, of which the pore size is the most important factor. The activity of PGA immobilized on KIT-6/130 reaches to 3522 IU/g by dry support, which is higher than that ever reported for carrier-bound penicillin G acylase [A.I. Kallenberg, F. van Rantwijk, R.A. Sheldon, Adv. Synth. Catal. 347 (2005) 905–926]. Because of the covalent immobilization, the operational stability of IME increases.     

介孔分子筛SBA-16固定化木瓜蛋白酶性质的研究

以介孔分子筛SBA-16为载体采用物理吸附的方法对木瓜蛋白酶进行了固定化,研究了固定化条件对酶的相对活性的影响及在不同pH值下游离酶和固载酶的pH稳定性。实验结果表明当1 g载体的給酶量为30 mg,固定化时间为2.5 h,pH值为7.0时,固定化木瓜蛋白酶的相对活性最好。与游离酶相比,固定化酶的pH稳定性有明显改善。     

Improvement in the Cleaning Performance Towards Protein Soils in Laundry Detergents by Protease Immobilization on the Silica Nanoparticles

This work aimed to understand the effect of protease immobilization on silica nanoparticles and how such immobilization affects protease performance as catalysis for enhancing the removal of protein soils. Detergent products contain many components that may affect the free enzyme activity and stability. Various factors such as temperature, pH and humidity are know to affect enzyme activity and cleaning efficiency. Therefore, the effect of enzyme immobilization on the removal of protein based soil was investigated on cotton fabrics as the model soil. The effect of temperature and humidity on the stability of free and immobilized enzyme was compared. It was found that the immobilized enzyme increased cleaning efficiency toward protein soil removal on cotton fabrics, whereas the free enzyme imposed a small effect on the enzymatic activity towards the same soil substrates. In addition, the stability of the immobilized enzyme against temperature and humidity was much higher than its corresponding value by free enzyme.     

A computational method for determination of the mass-transfer coefficient in packed-bed immobilized enzyme reactors

A computational method was developed that determined the mass-transfer coefficient k_L or the volumetric mass-transfer coefficient k_La in packed-bed immobilized enzyme (IME) reactors. To study the performance of this method, two experimental systems were considered where an enzyme was immobilized on a non-porous support surface (surface-IME system) or within a porous support (pore-IME system). The values of k_L and k_La determined in these packed-bed IME reactor systems were successfully expressed in terms of the substrate concentration at the reactor inlet and the liquid flow rate. Furthermore, the correlations obtained for k_L and k_La were used to calculate the unconverted fractions of substrate at the reactor outlet. Comparison showed that the calculated results were in satisfactory agreement with the experimental values.     

天然矿物埃洛石为载体固定α-淀粉酶的工艺和性能

以天然纳米材料埃洛石为载体,通过物理吸附法对α-淀粉酶进行固定.利用红外光谱、扫描电镜、透射电镜等对埃洛石的结构和形貌特征进行测试与表征,同时对埃洛石纳米管固定化α-淀粉酶的条件及固定化酶的酶学性能进行了研究,并与游离酶进行了比较.结果表明:这种具有管状结构的埃洛石硅酸盐矿物是理想的酶载体,酶的固定化效率平均达到37.38%;所得的固定化α-淀粉酶4℃下保存15d后,酶活力仍保持90%以上;固定化α-淀粉酶的热稳定性也明显优于游离酶,连续7批次操作后仍保持56.2%的酶活力.     

α-淀粉酶在MCM-41介孔分子筛上的固定化研究

采用浸渍法将α-淀粉酶固定在介孔分子筛MCM-41上。考察了吸附时间、给酶量和pH对α-淀粉酶固定化性能的影响,并对固定化酶的活性、稳定性和载体结构等进行了研究。结果表明,在固定化时间为11 h,给酶量为70 mg.g-1,pH=5.9的条件下,固定化酶活性回收率可达48%。与游离酶相比,固定化酶的耐热能力增强,温度达到70℃时,固定化酶相对活性可达到75%,而游离酶只有14%;在pH=3.3～8.0的内,固定化酶相对活性为62%～100%,而游离酶的相对活性为5%～100%,固定化酶具有更宽的pH适应性;此外,固定化酶储存稳定性明显增强,并具有一定的可重复操作性,且固定后载体仍然保持了良好的介孔结构。     

Immobilization of organophosphorus hydrolase enzyme by covalent attachment on modified cellulose microfibers using different chemical activation strategies: Characterization and stability studies

The plant cellulose powder was activated by two different methods using 1,4-butanediol diglycidyl ether(BTDE)and 1,1′-Carbonyldiimidazole(CDI) as the chemical coupling agents.Organophosphorus hydrolase(OPH) from Flavobacterium ATCC 27551 was immobilized on any of activated support through covalent bonding.The optimal conditions of affecting parameters on enzyme immobilization in both methods were found, and it was demonstrated that the highest activity yields of immobilized OPH onto epoxy and CDI treated cellulose were 68.32%and 73.51%, respectively.The surface treatment of cellulose via covalent coupling with BTDE and CDI agents was proved by FTIR analysis.The kinetic constants of the free and immobilized enzymes were determined, and it was showed that both immobilization techniques moderately increased the Kmvalue of the free OPH.The improvements in storage and thermal stability were investigated and depicted that the half-life of immobilized OPH over the surface of epoxy modified cellulose had a better growth compared to the free and immobilized enzymes onto CDI treated support.Also, the pH stability of the immobilized preparations was enhanced relative to the free counterpart and revealed that all enzyme samples would have the same optimum pH value for stability at 9.0.Additionally, the immobilized OPH onto epoxy and CDI activated cellulose retained about 59% and 68% of their initial activity after ten turns of batch operation, respectively.The results demonstrated the high performance of OPH enzyme in immobilized state onto an inexpensive support with the potential of industrial applications.     

UV-curable methacrylated/fumaric acid modified epoxy as a potential support for enzyme immobilization

The immobilization procedure of UV-curing coating is simple and causes less loss of enzymatic activity. UV-curable methacrylated/fumaric acid modified cycloaliphatic epoxide is here proposed as a rigid support material for covalent immobilization of α-amylase. The immobilized enzyme is analyzed in terms of bioactivity retention as a function of repeated use ability, pH, storage, as well as stability under various experimental conditions, taking starch as a substrate. The properties of immobilized enzyme were also compared with those of the free enzyme. The highest activity of free enzyme was obtained at pH 7.0 while this value was shifted to pH 7.5 for immobilized system. Optimum catalytic activity was observed at 30 °C, for both free and immobilized enzyme; however, the immobilized enzyme had a higher activity than the free one. The immobilized enzyme that was used 35 times in 8 h in repeated batch experiments demonstrated that about 73% of the enzyme activity was retained. The free enzyme lost all its activity with in 15 days. The retained activity of immobilized enzyme was found to be around 80%. The amount of bound α-amylase was found 94 mg per gram polymeric support material.     

Preparation and characterization of polymer-coated mesoporous silica nanoparticles and their application in Subtilisin immobilization

The preparation and characterization of polymer-coated mesoporous silica nanoparticles (MSNs) and their application in Subtilisin (Alcalase®) immobilization were investigated. For the synthesis of polymer-coated MSNs, acrylic acid (AA) and chitosan (CS) mixture were blended as poly(acrylic acid) (PAA) and CS polymer layer onto MSNs via in-situ polymerization technique. Then, both uncoated MSNs and polymer-coated mesoporous silica nanoparticles (CS-PAA/MSNs) were characterized by taking into account properties such as morphologic pattern, size distribution, surface charge of the particles as well as thermogravimetric stability with SEM, TEM, Zetasizer and TGA analyses. Subtilisin was immobilized onto polymer-coated mesoporous silica nanoparticles via adsorption technique. For optimizing the enzyme immobilization process, the percent enzyme loading depending on the matrix amount, immobilization time and pH were investigated. Then, the activity values of immobilized enzyme and free enzyme were compared at various pH and temperature values. The maximum enzyme activity was achieved at pH 9.0 for both immobilized and free enzyme. Immobilized enzyme showed more stability at higher temperatures compared with free enzyme. Furthermore, the operational and storage stability of immobilized enzyme were determined. The activity of immobilized enzyme was reduced from 100% to 45.83% after five repeated uses. The storage stability of immobilized enzyme was found to be higher than that of free enzyme. The activity of immobilized enzyme was reduced from 100% to 60% after 28 days of storage time. We concluded that the polymer-coated MSNs were a suitable matrix for Subtilisin immobilization compared to uncoated MSNs.     

海藻酸钠-明胶协同固定化S-腺苷甲硫氨酸合成酶的研究

以海藻酸钠和明胶为载体,对S-腺苷甲硫氨酸合成酶进行固定化。再用戊二醛对其进一步交联,增强固定化酶的稳定性。考察了海藻酸钠和明胶质量分数、CaCl2质量分数、酶和载体比例以及交联剂戊二醛体积分数等因素对固定化酶的影响。结果表明,最佳固定化条件为:海藻酸钠质量分数2.0%、明胶质量分数1.0%、CaCl2质量分数4.0%、固定化酶量为2.5 g/L凝胶、戊二醛体积分数0.6%。交联固定化酶热稳定性得到大幅度提高,在50℃下保温5 h仍保留72%的活力,而游离酶则完全失活。交联固定化酶在碱性溶液中的稳定性较高,在pH=8.0～9.0的缓冲液中4℃保温10 h酶活性仍保留87%以上。将交联固定化酶用于S-腺苷甲硫氨酸的合成,连续反应8批次后酶活性仍保留65%。