颗粒状固定化青霉素酰化酶的研究

将巨大芽孢杆菌 (Bacillusmegaterium)胞外青霉素酰化酶通过共价键结合到聚合物载体EupergitC颗粒环氧基团上 ,制成的颗粒状固定化青霉素酰化酶表现活力达 1 40 0 μ/g左右。固定化酶水解青霉素的最适 pH8 0 ,最适温度为 55℃。在pH6 0～ 8 5、温度低于 40℃时固定化酶活力稳定。在 pH8 0、温度 37℃时 ,固定化酶对青霉素的表现米氏常数Ka为 2×1 0 - 2 mol/L ;苯乙酸为竞争性抑制剂 ,抑制常数Kip为 2 8× 1 0 - 2 mol/L ;6 APA为非竞争性抑制剂 ,抑制常数Kia为 0 1 2 5mol/L。固定化酶水解青霉素 ,投料浓度为 8% ,在使用 2 0 0批后 ,保留活力 80 %左右 ,6 APA收率平均达 89 48%。     

固定化青霉素酰化酶的研究

将巨大芽孢杆菌胞外青霉素酰化酶通过共价键连接到醋酸纤维素载体上,制成的固定化青霉素酰化酶的表观活力达2000 u／g左右(PDAB法)。水解lO％(w／v)的青霉素G钾盐落液,使用30批,保留活力70％以上。6-氨基青毒烷酸(6-APA)总收率平均达88．37％。固定化青霉素酰化酶水解青霉素G的最适pH为9．95,最适温度为55℃,表观米氏常数为1.093×10-2mol／L,在pH 5．8-10．7,温度45℃以下酶的活力稳定。     

固定化青霉素G酰化酶水解头孢菌素G制备7—ADCA的研究

用聚丙烯腈纤维固定化青霉素酰化酶水解头孢菌素G制备7-ADCA,固定化酶对头孢菌素G的最适pH为9.0,最适温度50℃。在37℃、pH8.0固定化酶对头孢菌素G的表观米氏常数为1.67×10~(-2)mol/L。最大反应速度为3.01mmol·g~(-1)·min~(-1)。头孢菌素G溶液浓度在2％以上时,对固定化酶有明显的抑制作用。固定化酶水解头孢菌素G的最佳投料浓度为5％～6％,水解时用酶量以每克头孢菌素G投300U以上为好。按上述条件水解头孢菌素G,操作25批后固定化酶保留活力77.8％,7-ADCA平均收率92.68％。     

固定化尖镰孢菌细胞的某些酶学特性

尖镰孢菌(Fusariun oxysporum)33—11是一株青霉素V酰化酶的高产菌株。用二醋酸纤维素固定的该菌细胞裂解青霉素V最适的Ph范围为7．4至7.6;最适的反应温度为45℃至48℃;其酶活性受8-羟基喹啉和EDTA的可逆抑制,Mg²⁺、Zn^2-和Mn^2-离子则有激活作用。采用问歇式搅拌裂解青霉素V,测得0．6rnm颗粒度固定化细胞的表观km值为11．7mmol／L。裂解青霉素V的反应活化能为33kJ／mol;底物抑制常数Ks为1950mmol/L;苯氧乙酸和6-APA的抑制常数分别为220mmol／L和270mm0I／L,在裂解反应中．前者是竞争性抑制剂,后者是非竞争性抑制剂。     

高产天冬氨酸酶的大肠杆菌细胞的固定化

用聚乙烯醇凝胶包埋具有高活力天冬氨酸酶的大肠杆菌(Escherichia coli)No.1细胞。该酶的表现活力高达1638 00u／g湿细胞,酶活力的回收率为97．5％。固定化细胞和游离细胞天冬氨酸酶的最适pH均为8．0,最适温度分别为40—45℃和40—55℃。二价金属离子Mn2+、Mg2+、Ca2+和Fe2+对热钝化的天冬氨酸酶活力具有保护作用。在37—45℃下,两种细胞的热稳定性相同。二者在pH6．0的柠檬酸缓冲液中比较稳定。固定化细胞在1mol／L、pH8．0的底物溶液(内含Mn2+1mmol／L)中于4℃冰箱保存6个月,天冬氨酸酶的活力保持不变。用固定化细胞柱连续生产L-天冬氨酸,底物转化为产物的转化率达95％以上;产物的总 收率为91．1％。固定化细胞柱连续运转40天,天冬氨酸酶活力仍保持最初酶活力的90％。     

尖镰孢青霉素V酰化酶的纯化及性质

通过硫酸铵沉淀、硅藻土吸附、DEAD-纤维素离子交换层析和Sephadex G-200凝胶过滤,由尖镰孢(Fusarium oxysporum)FP941培养滤液中得到了聚丙烯酰胺凝胶电泳均一的青霉素V酰化酶。酶作用最适pH为7.0,最适温度为50℃。酶在pH6.0—8.0和42℃以下稳定。酶作用青霉素V的米氏常数Km为4.65×10~(-3)mol/L;苯氧乙酸是酶的竞争性抑制剂,抑制常数Ki为23.87×10~(-3)mol/L;6-氨基青霉烷酸是酶的非竞争性抑制剂,抑制常数Ki为30.01×10~(-3)mol/L。某些金属离子对酶有抑制作用,Fe~(2+)最强,其次是Hg~(2+)和Cu~(2+)。用SDS凝胶电泳测定酶亚基分子量为77600;用分子筛测定自然酶分子量为148000。     

腈水合酶转化反应的影响因子

棒状杆菌(corynebactcrium sp.)ZBB-21腈水合酶能高效地将丙烯腈转化为丙烯酰胺,其转化反应的最遣PH为8．0,最适转化反应温度为25℃。反应体系中加入微量的K+、Na+、Mg2+和Fe3+对酶的转化反应有明显的促进作用。过量丙烯腈(浓度为0．3mol／L以上)对酶活性有抑制作用,转化产物丙烯酰胺及其结构类似物丙烯酸是腈水合酶的竞争性抑制剂,其抑制常数K．分别为0．06mol／L和0．70mol,L,游离氰离子(CN-)的存在严重抑制丙烯酰胺的形成(K;=1．25 x 10-3mol／L)。     

产气气杆菌茁霉多糖酶的研究I．酶的提纯和性质

产气气杆菌(Aerobacter aerogenes) 10016的茁霉多糖酶(pullulanase E．C．3．2．1．41)用Sephadex G100凝胶过滤、聚丙烯酰胺垂直板型凝胶电泳进行纯化,得到了聚丙烯酰胺凝胶电泳均一的纯酶。纯酶作用的最适温度为50℃,最适pH为5．3—5．8,耐热性较差,50℃ 4小时后仅存活力10％。纯酶在pH4．3一8．6稳定。酶作用于糯米淀粉的米氏常数Km为2.0×10-2克／毫升。用聚丙烯酰胺薄屡凝胶等电聚焦测定酶的等电点pI为3．8,用SDS凝胶电泳测定酶的分子量为51,000—52,000;此酶是一种糖蛋白;含糖总量为6．5—7．0％;纯酶能专一性的水解茁霉多糖、糯米淀粉,也能分解糊精,而不作用于糖原、纤维二糖以及环状糊精。     

固定化诺卡氏菌细胞生产L(+)酒石酸的研究

用明胶包埋酒石酸诺卡氏菌(Nocardia tartaricans SWl3—57)得到顺式环氧琥珀酸开环水解酶活力较高的固定化细胞。固定化细胞的最适温度为30～45℃,而游离细胞的最适温度为35～45℃。两者的最适pH均为8．0～9．0,固定化细胞的表观米氏常数Km为0．256mol／L,而游离细胞有底物抑制作用,在底物浓度小于0．45mol／L时Km为0．246mol／L。用固定化细胞装柱(y=100ml),pH8．S,温度37℃,稀释速率D=0．25h^-1,以0．5mol／L浓度顺式环氧琥珀酸钠溶液为底物,连续运转53d,平均产L(+)酒石酸66．95g／L,克分子转化率为92．09％,反应器生产能力达到16．58g／L·h。     

聚丙烯腈纤维固定化青霉素酰化酶合成头孢氨苄的研究

将巨大芽孢杆菌胞外青霉素酰化酶通过共价键结合到聚丙烯腈纤维的衍生物上。制成的丝状固定化青霉素酰化酶表现活力达 1 5 3U g(湿重 )。固定化酶合成头孢氨苄的最适pH为 6 5 ,最适温度为 40℃。 7 ADCA的投料浓度以 4%为好 ,7 ADCA与PGME的投料量比率为1∶2 ,最佳用酶量为 1 70U g 7 ADCA。在pH6 5、温度 3 0℃时 ,固定化酶对 7 ADCA的表观米氏常数K7 ADCA为 0 1 6 2mol L ,对PGME的表观米氏常数KPGME为 0 3 6 4mol L ,最大反应速度Vmax为0 0 4 6 2mol·L- 1·min- 1,用固定化酶合成头孢氨苄 ,使用 5 0次保留酶活力 83 9%     

活性炭吸附固定化粪产碱杆菌青霉素G酰化酶

目的：以活性炭为载体固定化粪产碱杆菌来源的青霉素G酰化酶,考察固定化酶的性质。方法：对影响酶固定化的因素优化筛选,确定有显著影响的因素：pH、离子强度、酶量、固定化时间进行L934的正交实验,获得最佳固定化条件,并对固定化酶的最适反应温度、pH及批次稳定性进行研究。结果：最佳固定化条件为：载体0.3g,酶量5mL,总反应体系为12mL,离子强度1mol/L,温度4℃,pH 7.0,固定化40h;最高固定化酶活性为135.9U/g湿载体。固定化酶性最适反应温度为55℃,最适pH为10,重复使用12次后没有活性损失。结论：活性炭吸附固定化青霉素G酰化酶的活性高,批次反应稳定,具有工业应用潜力。     

固定化青霉素V酰化酶的制备及性质

尖镰孢(Fusarium oxysporum)FP941青霉素V酰化酶经γ氧化铝吸附洗脱、硫酸铵沉淀和脱盐处理后,固定在环氧丙烯聚合物载体上,湿固定化酶表现活力为217 IU/g,固定化产率为53%。固定化酶作用最适温度为55℃,最适pH为80;在pH50～110及50℃以下稳定;37℃使用25次后,酶活力保留90%。     

Enzymatic splitting of penicillin V for the production of 6-APA using immobilized penicillin V acylase

Penicillin V acylase from Fusarium sp. SKF 235 was immobilized on several cation-exchange resins, of which Amberlite CG-50 was preferred. Maximum activity of the immobilized penicillin V acylase was 250 to 280 IU/g dry beads. The pH and temperature optima of the enzyme shifted from 6.5 to 6.8 and 55°C to 60°C, respectively, as a result of immobilization. However, the K _m for penicillin V remained at 10mm. Parameters for producing 6-aminopenicillanic acid were investigated and the immobilized penicillin V acylase was used for 68 cycles in a stirred tank reactor.     

An efficient immobilizing technique of penicillin acylase with combining mesocellular silica foams support and <Emphasis Type="Italic">p</Emphasis>-benzoquinone cross linker

To improve the performance of covalently immobilized penicillin acylase (PA), the immobilization was carried out in mesocellular silica foams (MCFs) using p-benzoquinone as cross linker. The characterizations of the immobilized enzyme were studied carefully. The results showed that the relative activity of the immobilized PA was increased to 145% of that of free enzyme. The activity was 3.7 folds of that of PA on the silica nanoparticles. The enzyme in MCFs presented a turnover equal to that of free enzyme. It was also found that the optimum pH of the immobilized PA shifted to pH 7.5 and the optimum reaction temperature rose from 45 to 50 degrees C. Furthermore, the stability of PA was ameliorated greatly after immobilization. Fourier transform infrared spectroscopy showed no major secondary structural change for PA confined in MCFs. The proposed covalent immobilizing technique would rank among the potential strategies for efficient immobilization of PA.     

漆酶在磁性壳聚糖微球上的固定及其酶学性质研究

以磁性壳聚糖微球为载体,戊二醛为交联剂,共价结合制备固定化漆酶。探讨了漆酶固定化的影响因素,并对固定化漆酶的性质进行了研究。确定漆酶固定化适宜条件为：50 mg磁性壳聚糖微球,加入10mL 0.8mg/mL 漆酶磷酸盐缓冲液（0.1mol/L,pH 7.0）,在4℃固定2h。固定化酶最适pH为3.0, 最适温度分别为10℃和55℃,均比游离酶降低5℃。在pH 3.0,温度37℃时,固定化酶对ABTS的表观米氏常数为171.1μmol/L。与游离酶相比,该固定化漆酶热稳定性明显提高,并具有良好的操作和存储稳定性。     

Immobilization of oxalate decarboxylase to Eupergit and properties of the immobilized enzyme

Oxalate decarboxylase, an oxalate degradation enzyme used for medical diagnosis and decreasing the oxalate level in the food or paper industry, was covalently immobilized to Eupergit C. Different immobilization parameters, including ratio of enzyme to support, ammonia sulfate concentration, pH, and incubation time, were optimized. Under the condition of enzyme/support ratio at 1:20, pH 9, with 1.5?mol/L (NH(4))(2)SO(4), room temperature, and shaking at 30?rpm for 24?hr, activity recovery of immobilized Oxdc reached 90% with an apparent specific activity of 0.44?U/mg support. The enzymatic properties of immobilized Oxdc were investigated and compared with those of the soluble enzyme. Both shared a similar profile of optimum conditions; the optimum pH and temperature for soluble and immobilized Oxdc were 3.5 and 50°C, respectively. The immobilized enzyme was more stable at lower pH and higher temperatures. The kinetic parameters for soluble and immobilized enzyme were also determined.     

Increase in conformational stability of enzymes immobilized on epoxy-activated supports by favoring additional multipoint covalent attachment*

Epoxy supports (Eupergit C) may be very suitable to achieve the multipoint covalent attachment of proteins and enzymes, therefore, to stabilize their three-dimensional structure. To achieve a significant multipoint covalent attachment, the control of the experimental conditions was found to be critical. A three-step immobilization/stabilization procedure is here proposed: 1) the enzyme is firstly covalently immobilized under very mild experimental conditions (e.g. pH 7.0 and 20 degrees C); 2) the already immobilized enzyme is further incubated under more drastic conditions (higher pH values, longer incubation periods, etc.) to "facilitate" the formation of new covalent linkages between the immobilized enzyme molecule and the support; 3) the remaining groups of the support are blocked to stop any additional interaction between the enzyme and the support. Progressive establishment of new enzyme-support attachments was showed by the progressive irreversible covalent immobilization of several subunits of multi-subunits proteins (all non-covalent structures contained in crude extracts of different microorganism, penicillin G acylase and chymotrypsin). This multipoint covalent attachment enabled the significant thermostabilization of two relevant enzymes, (compared with the just immobilized derivatives): chymotrypsin (5-fold factor) and penicillin G acylase (18-fold factor). Bearing in mind that this stabilization was additive to that achieved by conventional immobilization, the final stabilization factor become 100-fold comparing soluble penicillin G acylase and optimal derivative. These stabilizations were observed also when the inactivations were promoted by the enzyme exposure to drastic pH values or the presence of cosolvents.     

黄曲霉毒素解毒酶的固定化及其性质的研究

黄曲霉毒素是农作物常见的受污染的霉菌毒素,毒性大,稳定性高,是潜在的肝癌致癌物,对人的危害较大。该毒素的解毒与去毒一直是受到关注的问题。黄曲霉毒素解毒酶对黄曲霉毒素有特殊的去毒和降解作用,但是该酶的稳定性离解决实际问题尚有一段距离。报道了对黄曲霉毒素解毒酶的固定化,并对固定化处理后酶的稳定性、性质、催化活性、解毒活性进行了测定。结果表明,通过固定化操作酶的解毒活性被保留下来,酶的酸碱稳定性、热稳定性、放置稳定性等均得到显著的提高。