明胶多孔支架固定化过氧化氢酶

以明胶多孔支架为载体,戊二醛为交联剂成功地制备了固定化过氧化氢酶,并对其固定化酶的性质进行了研究。固定化过氧化氢酶活力回收率可高达51.1%。与游离酶相比较,虽然催化效率有所降低,但是其固定化酶在65℃保存的稳定性有明显提高。固定化酶可重复使用10次后,活力仍保持在初始活力的60%以上,其具有良好的操作稳定性。     

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%。     

大孔树脂D380固定化硫酸软骨素裂解酶

目的以大孔树脂D380为载体,戊二醛为交联剂,进行硫酸软骨素裂解酶(ChSase)的固定化,并考察固定化酶的酶学性质。方法分别考察加酶量、吸附温度、吸附时间、吸附pH值、戊二醛交联浓度、交联时间及交联温度对ChSase固定化效果的影响,并分析该固定化酶的最适反应温度、最适反应pH值、米氏常数(Km)及其操作稳定性。结果ChSase的最佳固定化条件为:加酶量150U/g树脂,吸附温度15℃,吸附时间6h,吸附pH值7.0,戊二醛交联浓度0.01%,交联时间3h,交联温度4℃。以此条件制备的固定化酶,其酶结合效率可达79.1%。该固定化ChSase的最适反应温度为45℃;最适反应pH值为7.0;Km达1.46×10-1g/L,较游离酶高;具有较好的操作稳定性。结论以大孔树脂D380为载体固定化ChSase是可行的,所得固定化酶有较高的使用效率和稳定性,适合于工业化生产。     

海藻酸钠明胶协同固定化黑曲霉脂肪酶

以海藻酸钠明胶为复合载体,采用包埋法制备固定化黑曲霉脂肪酶,考察了海藻酸钠、明胶浓度等因子对固定化效果的影响,比较固定化酶和游离酶对温度、pH等条件的稳定性。结果表明,制备固定化黑曲霉脂肪酶的最优条件为:海藻酸钠、明胶浓度分别为1.25%和0.5%,CaC l2浓度为10%,给酶量为450 IU/g;固定化酶最适温度为35℃,最适pH为9.0,常见有机溶剂和金属离子对固定化酶的活力影响较小。     

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%。     

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。     

以壳聚糖为载体固定化青霉素酰化酶的研究

介绍了以壳聚糖为载体固定化青霉素酰化酶需首先制备壳聚糖颗粒 ,使用戊二醛、甲醛、乙二醛 3种活化剂处理所得的壳聚糖颗粒 ,确定了以戊二醛为活化剂交联其上的氨基共价结合青霉素酰化酶的固定化方法。从戊二醛的浓度、pH值、固定化时间、固定化pH值、酶用量等条件摸索了最佳固定化条件 ,获得了酶活力为4 0 0 0 0U/ (g·h)、回收率为 5 0 %左右的固定化青霉素酰化酶。     

磁性SiO2纳米粒子的制备及其用于漆酶固定化

以氨基修饰的磁性SiO2纳米粒子为载体,通过交联剂戊二醛固定漆酶,对固定化条件进行了优化,比较了固定化酶与游离酶的酶学性质. 结果表明,漆酶固定化的最佳条件为戊二醛浓度8%(w),固定化时间6 h,缓冲液pH值7.0,初始酶液浓度0.15 g/L. 固定化的漆酶的最适pH为4.0,最适温度为20℃. 在60℃条件下保温4 h,固定化漆酶仍能保持酶活力60.9%,在连续10次操作后,酶活力仍能保持55%以上,其热稳定性和操作稳定性均比游离酶高.     

分子筛固定氨基酰化酶Ⅰ的研究

以Y型分子筛为载体,分别采用吸附法、吸附-戊二醛交联法、偶联法和偶联-重氮法4种方法对氨基酰化酶I进行固定化。 研究发现偶联法获得的分子筛固定化酶的活性最高,达0.258 IUmg-1,并对分子筛固定化酶最适pH值、最适反应温度、重复使用性和米氏常数进行了测定;结果表明该载体适合氨基酰化酶I的固定,可以获得较高的酶活力,分子筛固定化酶的最适pH值、最适反应温度都有所拓宽。     

酸性脲酶的固定化研究

以明胶为包埋材料,戊二醛为交联剂固定化粪产碱菌所产的酸性脲酶。对酸性脲酶的固定化条件(包括明胶含量、戊二醛浓度、吸附时间、交联时间和粗酶液用量)及酶学性质(温度和pH值)进行了研究。结果表明,固定化酶的最适宜条件为：明胶的质量分数15％,戊二醛质量分数0.3％,吸附时间4 h,交联时间20 min,粗酶液用量4 mL。...     

固定化黄孢原毛平革菌木素过氧化物酶的研究

用大孔吸附树脂进行黄孢原毛平革菌来源的木素过氧化物酶固定化试验,筛选出固定化效果较好的XAD7HP大孔树脂,研究了其固定化条件。结果表明,当树脂1.0g,酶液pH4.5,加酶量87.2U,吸附温度25℃,吸附4h,戊二醛质量分数0.2%,戊二醛处理时间120min,可获得最佳的固定化效果,固定化酶活力可达到16U/g(对载体)。     

银/二氧化硅复合载体固定木瓜蛋白酶的研究

以沉积了银纳米粒子的二氧化硅微球为载体,戊二醛为交联剂共价固定了木瓜蛋白酶。研究了戊二醛用量以及载体中银纳米粒子质量分数对酶负载率、相对活力和酶活回收率的影响,考察了温度和pH值对固定酶的影响。结果表明,戊二醛的适宜质量分数为5%;当载体的银负载量(质量分数)为0.68%时,固定木瓜蛋白酶活回收率最高,比使用未负载银载体提高了131%;固定酶的最适反应温度为75℃,与游离酶基本相同;最适pH值为7.5,与游离酶相比向碱性方向移动了1个单位。     

<Emphasis Type="Italic">Penicillium</Emphasis> sp. ZD-Z1 chitosanase immobilized on DEAE cellulose by cross-linking reaction

Chitosanase obtained fromPenicillium sp.ZD-Z1 was immobilized on DEAE cellulose with glutaraldehyde by cross-linking reaction. The optimal conditions of immobilization were as follows: 0.1 g DEAE cellulose was treated with 5 ml 5% glutaraldehyde solution; then 2.3 mg chitosanase was immobilized on the carrier. The optimal temperature and pH was 60 °C and 4.0, and the K _m value was 18.87 g/L. Under optimal conditions, the activity of immobilized enzyme is 1.5 U/g, and the recovery of enzyme activity is 81.3%. After immobilization, the optimal temperature and K _m value increased (from 50 °C to 60 °C, from 2.49 g/L to 18.87 g/L), whereas the optimal pH was reduced (from 5.0 to 4.0). The enzyme activity loss was less than 20% after 10 times batch reaction; the immobilized enzyme showed good operation stability.     

氨基硅烷功能化磁性材料固定化琼胶酶的性能

利用3-氨丙基三乙氧基硅烷(APTES)对制备的SiO₂包覆Fe₃O₄复合粒子(Fe₃O₄@SiO₂)进行改性，制备了氨基硅烷功能化磁性材料Fe₃O₄@SiO₂-NH₂，将Fe₃O₄@SiO₂-NH₂作为载体用于固定化琼胶酶。采用SEM、FTIR、VSM对Fe₃O₄@SiO₂-NH₂和固定化琼胶酶进行了表征，对琼胶酶的固定化条件进行了优化，评价了固定化琼胶酶的性能。结果表明，琼胶酶成功固定在载体上。Fe₃O₄@SiO₂-NH₂的磁化饱和强度为48.4 emu/g，固定化琼胶酶的磁化饱和强度为42.8 emu/g...     

Efficient Immobilization of Lecitase in Gelatin Hydrogel and Degumming of Rice Bran Oil Using a Spinning Basket Reactor

Immobilization of Lecitase (Phospholipase A1) in gelatin hydrogel and its stability is studied with a view to utilizing the immobilized enzyme for degumming rice bran oil. Excellent retention of enzyme activity (>80%) is observed in hydrogel containing 43.5% gelatin crosslinked with glutaraldehyde. Compared to the free enzyme which has a broad pH-activity profile (6.5–8.0), the activity of the immobilized enzyme is strongly dependent on pH and has a pH-optimum of pH 7.5. The optimum temperature of enzyme activity increases from 37 to 50 °C. Compared to the free enzyme which loses all its activity in 72 h at 50 °C, the immobilized enzyme retains its activity in full. The immobilized enzyme has been used efficiently in a spinning basket bioreactor for the degumming of rice bran oil with 6 recycles without loss of enzyme activity. The phosphorus content of the oil decreases from 400 ppm to 50–70 ppm in each cycle. After charcoal treatment and dewaxing, a second enzymatic treatment brings down the phosphorus content to <5 ppm.     

Urease immobilized on chitosan membrane: Preparation and properties

Urease was covalently immobilized on glutaraldehyde-pretreated chitosan membranes. The optimum immobilization conditions were determined with respect to glutaraldehyde pretreatment of membranes and to reaction of glutaraldehyde-pretreated membranes with urease. The immobilized enzyme retained 94% of its original activity. The properties of free and immobilized urease were compared. The Michaelis constant was about five times higher for immobilized urease than for the free enzyme, while the maximum reaction rate was lower for the immobilized enzyme. The stability of urease at low pH values was improved by immobilization; temperature stability was also improved. The optimum temperature was determined to be 65°C for the free urease and 75°C for the immobilized form. The immobilized enzyme had good storage and operational stability and good reusability, properties that offer potential for practical application.