微波辐射高效共价固定青霉素酰化酶

为提高青霉素酰化酶的共价固定化效率, 在微波辐射条件下将酶蛋白共价固定于介孔泡沫硅(MCFs)的孔道中. 通过正硅酸四乙酯水解缩合制备介孔泡沫硅, 再于微波辅助下将青霉素酰化酶共价固定在其孔道中. 以固定化酶相对活力和活力回收为指标, 考察了加酶量、固定化温度、微波辐射时间等条件对酶固定化效率的影响. 实验结果表明: 当加酶量为60 mg/g, 固定化温度为20 ℃, 微波辐射140 s, 固定化酶相对活力达到178.1%, 表观活力为1191.3 U/g(以湿重计). 与常规方法相比, 微波辅助固定化酶时, 固定化酶相对活力提高34.5%, 固定化时间亦大幅缩短至数分钟, 这为青霉素酰化酶的高效共价固定化提供了一条新的途径.     

基于金属有机骨架的固定化氯过氧化物酶的制备和性能评价

30℃水相体系中"一锅法"快速制备固定化氯过氧化物酶（CPO@ZIF-8）,在构筑金属有机沸石咪唑骨架结构（ZIF-8）的同时将氯过氧化物酶（CPO）固定在其三维纳米孔道中.温和的条件为固定化酶制备过程中酶活性的保持提供了前提.结构和性能表征说明酶分子的引入并不改变ZIF-8材料的孔道结构,同时酶分子在CPO@ZIF-8中呈现出在整体骨架材料中的嵌入式均匀分布.与先构筑ZIF-8骨架材料,然后通过表面吸附来固定酶分子的方法相比,通过将酶分子引入整体骨架材料中不仅提高了酶的固载量,更主要的是利用ZIF-8材料的高比表面积提高了固定化CPO的催化效率,同时基于三维孔道提供的刚性屏蔽环境有效改善了CPO在极端反应条件下的热稳定性、酸碱稳定性和对有机溶剂的耐受性.     

胶囊固定化辣根过氧化物酶酶促体系引发丙烯酰胺聚合研究

研究了以海藻酸钠／壳聚糖／海藻酸钠为囊壁材料的胶囊固定化辣根过氧化物酶的制备及其影响因素,并将肢囊固定化辣根过氧化物酶／乙酰丙酮／H2O2酶促体系用于引发丙稀酰胺的聚合。结果表明,作为囊壁材料之一的壳聚糖的平均分子量以1万左右为宜,以柠檬三酸钠溶液为溶芯荆的溶芯时间控制在2～4min时,固定化率可达60％,相对于游离酶,其相对活力约为60％。胶囊固定化辣根过氧化物酶／乙酰丙酮／H2O2酶促体系可引发丙稀酰胺的聚合。     

青霉素酰化酶在甲基丙烯酸缩水甘油酯共聚物上的固定化

 用共价键合法将青霉素酰化酶固定化在珠状多孔的甲基丙烯酸缩水甘油酯（GM）共聚物上，研究了固定化反应时间、温度、pH值和酶液用量对固定化青霉素酰化酶的表观活性、表观偶联效率、活性回收及稳定性的影响．将GM共聚物载体加入到磷酸缓冲液（0．1mol／L，pH10．8）与青霉素酰化酶液（每克干载体用酶液1ml）的混合溶液中，在30℃下反应72h，单位质量（干重）固定化酶的表观活性为348U／g，表观偶联效率为66．7％，活性回收为31．7％．     

介孔材料及其改性材料中酶的固定化研究进展

介孔材料具有高的比表面积、高的孔体积、均一可调的孔径、有序的孔道结构以及易于表面功能化等优点,可广泛用于酶的固定化.介孔材料中酶的固定化方法主要包括物理吸附、物理包埋和化学吸附.综述了介孔材料中不同固定化酶方法的优缺点、酶的固定化影响因素及固定化酶的应用,并对固定化酶的发展前景进行了展望.     

Al-MOF基多级孔Al2O3固定化酶反应器的构筑及构效关系研究

针对生物酶在固相载体负载后存在的催化活性与稳定性之间“此消彼长”的问题, 本工作采用“自牺牲模板”策略以铝基金属有机骨架材料(Al-MOF)为前驱体设计制备多级孔Al₂O₃ (MHAl₂O₃)材料, 再以“聚多巴胺(PDA)”仿生膜对材料表面进行功能化修饰后用以固载辣根过氧化物酶(HRP). 通过调节前驱体的煅烧温度来实现载体孔径大小的调控, 探讨了载体的孔道限域效应对固定化酶反应器催化活性的影响, 所得固定化酶反应器的热稳定性和重复使用性显著提高. 为了解析固定化酶反应器的构效关系, 采用酶动力学和热动力学参数研究了固定化酶反应器催化过程中酶与底物的相互作用, 结果表明固载后酶分子对底物的亲和性和专一性得到提升. 将固定化酶反应器用于模拟废水中苯胺黑药的催化降解时, 表现出非常高效的催化效率.     

介孔材料的修饰及固定青霉素酰化酶的稳定性研究

利用扩孔剂的作用合成出较大孔径(12 nm)的介孔材料SBA-15, 并进行表面氨基修饰, 以此为载体, 以戊二醛为交联剂, 对青霉素酰化酶进行组装固定, 并对固定化青霉素酰化酶(PGA)的稳定性进行了深入的研究. 实验结果表明, PGA与载体交联后仍保持活性. 热稳定性研究结果表明, 制备的固定化青霉素酰化酶在低于60 ℃时保持稳定; pH在6~11范围内保持稳定; 固定化酶重复使用10次之后, 仍具有高达90%的残留活力.     

介孔材料固定化酶*

本文综述了近年来酶在介孔材料上的固定化研究新进展,重点介绍了水解酶类的脂肪酶、蛋白酶、青霉素G酰化酶等和氧化还原酶类的辣根过氧化物酶、氯过氧化物酶、漆酶等在介孔材料上的固定化研究现状,并对介孔材料固定化酶的发展前景进行了展望。     

高分子载体材料对青霉素酰化酶的固定化作用

介绍了天然高分子材料和合成高分子材料对青霉素酰化酶的固定化作用,着重讨论了高分子材料的制备、性质及其表面修饰对固定化酶活性和使用稳定性的影响。     

固定化青霉素酰化酶新型载体PEI/SiO2的制备及其特性

通过γ-氯丙基三甲氧基硅烷的媒介, 将聚乙烯亚胺(PEI)化学偶联在硅胶微粒表面, 制备了固定化青霉素酰化酶的新型复合载体PEI/SiO2, 最终制得了活性高且稳定性好的固定化青霉素酰化酶. 通过测定复合载体表面PEI的偶合量, 考察了各种反应条件对复合载体制备的影响规律; 通过红外光谱与电导滴定法测定, 对复合载体表面的化学结构与组成进行了表征; 为探索复合载体PEI/SiO2固定化酶的作用机理, 测定了复合载体在固定化酶前的ζ电位. 研究结果表明, 通过氯丙基硅烷偶联剂的媒介, 聚胺大分子PEI可以充分地被化学偶联在SiO2表面, 键合量可达到15%. 偶联反应的适宜条件: 反应温度90-94 ℃; 反应时间5h; PEI的质量浓度0.45-0.50 g/mL. 由于PEI分子链中含有大量氨基, 少量的共价键联与大量的物理吸附相结合, 既可使青霉素酰化酶被快速稳定地固定化, 又能很好地保持酶的构象, 使其具有较高的催化活性与活力回收率, 而且具有良好的连续操作稳定性, 重复使用15次, 固定化酶的活性可稳定地保持在初活性的87.5%水平上.     

介孔材料MCFs的合成及组装青霉素酰化酶的性质研究

介孔材料由于具有纳米级规则孔道和巨大的比表面积而在催化、吸附及分离等方面存在较大的应用价值．近年来,由介孔分子筛如MCM-41和SBA-15州等组装功能性材料已成为研究的热点．酶作为高效催化剂有许多优点,但在溶液中易失活,使用后无法回收,有的酶在溶液中还存在自水解问题：将酶组装在介孔材料中制成固定化酶则可解决上述问题．目前已成功地将辣根过氧化物酶     

青霉素酰化酶在含铁MCM-41介孔分子筛上的固定化研究

制备了具有长程有序结构、孔径分布狭窄的含铁MCM-41介孔分子筛，利用直接法和共价结合法将青霉素酰化酶固定在分子筛表面。结果表明，两种方法制备的固定化酶对青霉素G水解反应的表观活性分别为782U/g和256U／g；经6次连续操作使用，二者保持初始活性的49．4％和81．2％，后者的操作稳定性好于前者。共价结合法制备的固定化酶活性较低，是由于Fe—MCM-41表面修饰后比表面积和孔径明显减小所致。     

乙烯基Ia3d介孔硅分子筛的环氧化及其固定化青霉素酰化酶(英文)

采用直接共聚法合成表面含有乙烯基的具有立方相Ia3d结构的介孔硅分子筛(V-ClMS),然后对乙烯基团进行环氧化制备得到表面环氧基功能化的介孔硅分子筛(E-CIMS),采用X射线衍射、N2吸附-脱附、透射电镜、热重分析和13C固体核磁共振对制备的介孔硅分子筛进行了表征.结果表明,表面含有乙烯基的V-ClMS介孔硅分子筛能被一步成功合成,并易于发生环氧化而获得表面环氧基功能化的E-CIMS介孔硅分子筛.将E-CIMS介孔硅分子筛作为载体用于固定化青霉素G酰化酶(PGA),研究了表面环氧基团对固定化PGA初活性和操作稳定性的影响.结果表明,随着表面环氧基团数量的增加,介孔硅分子筛孔径减小,表面疏水性增加,导致载酶量和初活性减小.但介孔硅分子筛表面适量的环氧基团能增强E-CIMS介孔硅分子筛与PGA之间的相互作用,从而提高固定化PGA的操作稳定性.     

含氨基和环氧基双功能基的聚合物刷磁性微球的制备及对青霉素G酰化酶的固定化

在内部分散超顺磁性Fe3O4纳米粒子的二乙烯苯交联聚丙烯酸微球表面引入原子转移自由基聚合(ATRP)引发剂,引发聚合向微球表面分别引入P(GMMA-r-DMAEMA-r-GMA)、P(GMMA-r-DMAEMA)和P(GMMA-r-GMA)无规共聚物刷(GMMA为甲基丙烯酸甘油单酯,DMAEMA为甲基丙烯酸-N,N-二甲氨基乙酯,GMA为甲基丙烯酸缩水甘油酯),聚合物刷中GMMA链节的作用是使聚合物刷具有亲水性,DMAEMA引入氨基,GMA引入环氧基.研究了青霉素G酰化酶在这些载体上的固定化和其酶活性.结果表明,同时引入环氧基和氨基的P(GMMA-r-DMAEMA-r-GMA)刷磁性微球固定化青霉素G酰化酶的活性和活性收率都最高,其固定化动力学比只含环氧基P(GMMA-r-GMA)刷磁性微球的好.固定化酶比自由酶更耐热,固定化酶的最佳pH值比自由酶的略高,固定化酶重复使用10次后其活性保留70%.     

含环氧基亲水性固定化青霉素酰化酶共聚载体的合成与性能研究

环氧基团可以在温和条件下与酶分子的氨基反应使其固定于载体表面.选用含有活性环氧基团的甲基丙烯酸缩水甘油酯(GMA)和亲水性的N-乙烯吡咯烷酮(NVP)两种单体,以N,N′-亚甲基双丙烯酰胺(MBAA)为交联剂,甲醇水溶液作致孔剂,液体石蜡为主介质,通过反相悬浮聚合技术成功地合成了亲水性大孔GMA-NVP-MBAA三元共聚物载体(GNM).通过调节交联剂的用量和单体NVP与GMA的比例,可以调节载体的孔径、比表面积及在水中的溶胀性能.将巨大芽孢杆菌青霉素酰化酶共价偶联于平均孔径为16.5nm、表面环氧基含量为0.906mmol/g的GNM共聚物载体,制成固定化酰化酶,其表观活性高达625U/g,水解青霉素G钾盐的最适宜温度为50℃,pH值为8.0.固定化酶在4℃保存40d,活性保持不变.经3次使用后,活性达到稳定值(601U/g左右),再经12次使用,活性几乎保持不变.     

Methodology for the immobilization of enzymes onto mesoporous materials

Cytochrome c and xylanase were adsorbed onto two mesoporous materials, SBA-15 (a pure silicate) and MSE (an organosilicate), with very similar physical properties but differing chemical compositions. A methodical order was developed whereby the influences of surface area, pore size, extent of order, particle size, surface potentials, isoelectric points, pH, and ionic strength on immobilization were explored. In silico studies of cytochrome c and xylanase were conducted before any immobilization experiments were carried out in order to select compatible materials and probe the interactions between the adsorbents and the mesoporous silicates. The stabilities of the mesoporous materials at different pH values and their isoelectric points and zeta potentials were determined. Electrostatic attraction dominated protein interactions with SBA-15, while weaker hydrophobic interactions are more prominent with MSE for both cytochrome c and xylanase. The ability of the immobilized protein/enzyme to withstand leaching was measured, and activity tests and thermostability experiments were conducted. Cytochrome c immobilized onto SBA-15 showed resistance to leaching and an enhanced activity compared to free protein. The immobilized cytochrome c was shown to have higher intrinsic activity but lower thermostability than free cytochrome c. From an extensive characterization of the surface properties of the silicates and proteins, we describe a systematic methodology for the adsorption of proteins onto mesoporous silicates. This approach can be utilized in the design of a solid support for any protein.     

Immobilization of whole-cell penicillin g acylase by entrapping within polymethacrylamide beads

Escherichia coli ATCC 11105 containing the periplasmic penicillin G acylase was entrapped within a copolymer of methacrylamide andN,N’- methylenebisacrylamide. A solution of monomer that was made up from methacrylamide andN,N’-methylenebisacrylamide dissolved in buffer was mixed with lyophilized cells and ammonium persulfate. This suspension was then pumped drop by drop into in soybean oil supplemented with 0.06% (v/v) 3-(dimethylamino)-propionitril. During submerging in the oil phase, the droplets were hardened and induced to polymerize within the droplets. Particles with a volume ranging from 0.013–0.017 mL per bead containing a biomass concentration up to 38.0 g/L were prepared. The optimal condition for the deacylation of penicillin G to 6-aminopencillanic acid (6-APA) catalyzed by the immobilized whole-cell penicillin G acylase was found to be 45‡C and pH 8.0. Product inhibition of this enzyme by 6-APA could be eliminated by controlling pH value at 8 during the course of penicillin G hydrolysis using a pH-stat. Conversion determined by the pH-stat method were 0.3% higher than that by p-dimethylaminobenzaldehyde method. Cell concentration in the matrix was found to be an important factor influencing the maximum velocity and the specific activity retained in the matrix. A kinetic model, in which the mass transfer resistances as a result of external film mass transfer and pore diffusion were assumed to be negligible, could properly describe the hydrolysis of penicillin G by the cells entrapped within the polymethacylamide beads.     

Immobilized penicillin G acylase as reactor and chiral selector in liquid chromatography

In this paper, the use of penicillin G acylase (PGA) as a biocatalyst and as a chiral selector is described. Penicillin G-acylase is an interesting enzyme used in the manufacture of semisynthetic antibiotics and, in particular, in the production of 6-APA by hydrolysis of penicillin G. Five PGA-based HPLC columns have been prepared by using two different silica supports by employing two immobilization methods, namely "in situ" and "in batch". The effects of the immobilization techniques and of different silica pore size on the catalytic properties of the enzyme as well as the applicability of the PGA-bonded stationary phases as chiral selectors for a number of chiral drugs have been investigated. The HPLC columns based on immobilized PGA combine the hydrolytic activity and the chiral recognition properties of PGA, therefore they have been used for the development of a combined reaction-separation system for chiral and achiral substrates.     

Beaded reactive polymers 3 effect of triacrylates as crosslinkers on the physical properties of glycidyl methacrylate copolymers and immobilization of penicillin G acylase

Various glycidyl methacrylate (GMA) copolymers were synthesized by suspension polymerization, using pentaerythritol triacrylate (PETA), trimethylolpropane triacrylate (TMPTA), and trimethylolpropane trimethacrylate (TRIM) as crosslinking comonomers. These copolymers were evaluated for the immobilization of penicillin G acylase. Broad pore-size distribution that was observed was in the range 5-300 nm. Both surface area and pore volume increased with increase in the mole fraction of crosslinking comonomer (increasing crosslink density). The pore volume of the copolymers was more than doubled by including lauryl alcohol as porogen. Binding of penicillin G acylase (PGA) was quantitative on highly crosslinked copolymers. The expression of bound PGA was better on the relatively more hydrophilic GMA-TMPTA and GMA-PETA copolymer supports compared to the GMA-TRIM copolymers. Among the different copolymers studied, GMA-TMPTA copolymer 7411 exhibited highest activity of immobilized penicillin G acylase (167.4 IU/g) with 35.1% expression.