壳聚糖–精氨酸树脂固定化胰凝乳蛋白酶及其性质

以自制的多孔、具柔性亲水手臂的壳聚糖–精氨酸树脂为载体,戊二醛为交联剂固定胰凝乳蛋白酶,确定了酶与载体的最佳比例为20 mg酶/g湿树脂,交联剂的最佳用量为10 mL 1.0%戊二醛/1.5 g湿树脂,交联时间为60 min,所得固定化酶的活力回收率达68.95%。固定化胰凝乳蛋白酶的Km为8.36 mg/mL,比游离酶增大1.52倍,其酶促反应10 min达到最大速率,具有接近游离酶的催化时间进程曲线;其最适温度为70 ℃,比游离酶升高10 ℃;其最适pH值为5.92,比游离酶酸性偏移2个pH值。此外,固定化胰凝乳蛋白酶具有良好的热稳定性和贮存稳定性,75 ℃时的半衰期为8 h,4 ℃时的半衰期为46天。     

海藻酸钙凝胶包埋乳酸氧化酶催化DL-乳酸生产丙酮酸

研究了用海藻酸钠包埋、戊二醛交联法固定耻垢分枝杆菌(Mycobacterium Srnegmatis)生成乳酸氧化酶的最佳条件,比较了原酶与固定化酶的酶学性质.将1mL酶液和1 mL质量分数为3%的海藻酸钠溶液的混合液,用注射器滴加到20 mL0.2 mol/L.的CaCl2溶液中,25℃静置固化2 h后,过滤洗涤,将同体转移至20 mL质量分数为0.2%戊二醛溶液中37℃交联2 h后,过滤、洗涤和干燥得到球状同定化酶.固定化酶的活力回收率为39.8%.酶学性质研究表明,此固定化酶的热稳定性较好,游离酶在65 ℃保温l h酶蛋白完全变性失活,而固定化酶在65℃保温1 h仍可保持86%的酶活力;其最适酶促反应温度可由37℃升至55℃,最适反应pH=7.4保持不变;在不加保护剂的条件下,4℃放置50 d后游离酶仅保持40%以上的酶活力,而固定化酶能保持80%以上的酶活力.该固定化乳酸氧化酶用于催化氧化DL-乳酸生产丙酮酸,3 h后丙酮酸产率可达75%,连续循环使用5次固定化酶活力仍保持85%.     

固定化葡萄糖氧化酶的制备及稳定性研究

选用自制的磁性纳米四氧化三铁为酶固定化的载体,通过交联法来固定葡萄糖氧化酶。通过对酶固定化过程中一系列因素的研究,确定出酶固定化的最佳工艺为:交联剂戊二醛与浓度为0.7 mg/mL酶液的体积比为1:4,固定化时间为0.5 h,固定化温度为室温(≤20 ℃),固定化所用缓冲液pH=7。采用比色法测定其酶活力。结果表明葡萄糖氧化酶经过固定化后,其酶活力较游离酶显著增加。固定化酶的热稳定性、酸碱稳定性、存储稳定性都有很大的提高。     

以HPD-750大孔树脂为载体材料固定化果胶酶

HPD-750树脂是中极性大孔吸附树脂,生物相容性好,机械性能稳定,具有较大的比表面积,可用于固定化酶载体材料。本文以HPD-750大孔树脂为载体固定化果胶酶,研究各因素对固定化酶的影响,并采用正交试验对固定化条件进行优化。结果表明,当pH为4.0、固定化温度为45℃、固定化时间为4h、加酶量为0.16g/mL时,固定化酶活力可达5146U/mg。以HPD-750大孔树脂为载体材料制备的固定化酶相较于游离酶具有更好的酸碱稳定性和热稳定性。在循环使用10次后,酶活力依然保留80%以上;4℃储藏25d之后,其酶活力仍保留60%以上。与D311大孔树脂、聚丙烯酰胺和海藻酸钠微球制备的固定化酶相比,HPD-750大孔树脂固定化酶的活性、操作稳定性、机械稳定性和储存稳定性都较好。该结果说明,HPD-750大孔树脂可作为固定化酶较好的载体材料。     

化学修饰木瓜蛋白酶的固定化及性质研究

在底物保护和无底物保护下,用丁二酸酐对木瓜蛋白酶进行化学修饰,以三硝基苯磺酸法测定修饰酶的平均氨基修饰度,以棉布为载体,戊二醛为交联剂,对修饰前后的木瓜蛋白酶分别进行固定化.考察了温度、pH和表面活性剂SDS对化学修饰的固定化木瓜蛋白酶活力的影响,并与固定化天然木瓜蛋白酶进行了比较.研究表明,化学修饰固定化木瓜蛋白酶的最适反应温度为80℃;最适pH为9.0;在SDS浓度为20mg/mL时酶活也仍能保持在40%左右;米氏常数为187g/L.与天然的固定化酶相比,化学修饰的固定化木瓜蛋白酶的热稳定性、耐碱性和耐洗涤性得到了显著提高.     

棘孢曲霉β-葡萄糖苷酶Ⅰ在毕赤酵母中的表达及烷基糖苷的催化合成

将来自棘孢曲霉(Aspergillus aculeatus NO. F-50)的β-葡萄糖苷酶Ⅰ在毕赤酵母中分泌表达. 初步研究表明, 目的蛋白得到较好表达, 以对硝基酚-β-D-葡萄糖苷(4-Nitrophenyl-β-D-glucopyranoside, pNPG)为底物, 重组β-葡萄糖苷酶Ⅰ酶促反应的最适温度为65 ℃, 最适pH为5.0, 50 ℃下反应发酵上清液中的酶活力可达33.8 U/mL, 蛋白表达量最高可达0.388 mg/mL. 该重组酶可通过逆水解或转糖苷反应催化合成烷基糖苷. 在有机-水双相反应体系中, 初步优化了pH 值、 含水量、 葡萄糖浓度及酶量等条件. 结果表明, 在优化的反应条件下, 丁基、 己基、 辛基和癸基葡萄糖苷最大产率分别为51.4%, 28.8%, 6.9%和3.0%.     

海藻酸钠固定化根霉脂肪酶的制备及其性质

 研究了以海藻酸钠为载体,用包埋法制备固定化德氏根霉(Rhizopus delemar)脂肪酶的条件. 将酶粉和海藻酸钠溶于pH 5.0的HAc-NaAc缓冲溶液,用注射器将此混合液滴入到0.05 mol/L无菌CaCl2溶液中,静置固化45 min, 经过滤、洗涤和干燥后得到球状固定化酶. 固定化酶的活力回收约为34.1%. 酶学性质研究表明,此固定化酶的热稳定性较好. 游离酶在 60 ℃下保温1 h已完全丧失活力,而固定化酶在100 ℃下保温1 h仅损失36.2%的活力,在100 ℃下保温6 h仍可保持46.8%的酶活力. 酶经固定化后,其橄榄油水解反应的最适温度由40 ℃上升至90 ℃, Km值由13.8 mg/ml下降为8.1 mg/ml. 常见有机溶剂对固定化酶的活力影响较小. 将该固定化脂肪酶用于非水溶剂中正戊酸异戊酯的合成,重复使用6次后,固定化酶仍保持95%的酶活力.     

壳聚糖固定化乳酸脱氢酶的制备及酶学性质研究

以磁性壳聚糖作为载体,戊二醛作为交联剂,对乳酸脱氢酶(LDH)进行固定化.固定化的最适条件为:戊二醛浓度6%,pH值7.5,酶的偶联时间2 h.对游离及固定化LDH酶学性质的研究表明,酶促反应的最适pH值为9.2,最适温度分别为37℃和50℃,对乳酸的表观米氏常数分别为1.6 mmol/L和0.9 mmol/L.游离酶和固定化酶在40℃放置150 min后,其活力分别为最初的56.5%和76.1%.固定化酶在4℃贮存4周后,活力仍保留50%以上.固定化酶在室温下与底物重复反应6次后,活力仍保留60%以上,说明固定化酶具有较好的热稳定性、贮存稳定性和复用性.     

黑曲霉脂肪酶的耦合固定化及特性

研究了吸附-絮凝耦合的方法固定脂肪酶的工艺条件.结果表明:在33℃下,用0.03mol/L的磷酸二氢钾?氢氧化钠缓冲液控制体系pH为7.0,酶与树脂(质量比1∶8)作用吸附1h后,用0.2mL絮凝剂聚丙烯酰胺(w(PAM)=0.5%)处理,得到活力较高的固定化脂肪酶.固定化酶最适pH9.0,最适温度为45℃,活力为405U/g,酶活回收率可以达到40%.固定化脂肪酶制备简便,可重复使用,稳定性较高.     

乙烯对脂肪酶活力的直接作用及机理初探

研究了乙烯对脂肪酶活力的直接作用及其机理. 结果表明: 低浓度乙烯能使脂肪酶催化三油酸甘油酯的水解活力提高; 当乙烯浓度为0.9834 mmol•L^－1时, 酶活力提高13.0%. 高浓度乙烯降低脂肪酶活力; 当乙烯浓度为7.9669 mmol•L^－1时, 酶活力下降24.5%. 加入乙烯的酶最适温度向高温偏移10～15 ℃, 而酶的最适pH值不变. 在pH＝7.9时, 乙烯使酶活力升高较大, pH为4.5～7.5, 8.5, 9.5～11时酶的活力降低. 加入乙烯的酶与对照相比, 其紫外吸收和荧光发射强度均有较大幅度增加, 荧光偏振度、比旋光度和粘度显著下降. DSC分析表明: 在低温范围内酶的可逆吸热峰值温度明显高于对照, 而热焓变低于对照; 在高温范围内酶的不可逆吸热峰值温度和热焓变都低于对照. 这些结果证实了乙烯可以直接影响酶的微环境和构象. 乙烯对脂肪酶的直接作用机制可能是通过改变酶的微环境以及渗入到酶分子内部改变酶构象而引起酶活力的改变.     

Molecular Basis for Stereospecific Hydrolysis of Ethyl Mandelate by Thermophilic Esterase

The stereospecific hydrolysis of mandelate can be effectively catalyzed by hyperthermophilic acylpeptide esterase APE 1547(Aeropyrum pernix esterase 1547). APE 1547 used in this reaction showed a remarkable stereodiscrimination in favour of R-mandelic acid(99% e.e.) with an enantiomeric ratio E>200. The results of computer simulation are consistent with the experimental results. It can be inferred that the R-substrate adopted a binding mode productive of the reaction due to the formation of the hydrogen bond at the active site of APE 1547.     

Effect of Calcium Cation on Thermophilic Acylamino Acid-releasing Enzyme Ape1547 from Aeropyrum pernix K1

The gene of enzyme(Ape1547) was cloned from hyperthermophilic archaeon Aeropyrum pernix K1 and expressed in Escherichia coil.The effect of calcium cation on the properties of Ape1547 was studied.Ape1547 exhibits both peptidase activity and esterase activity.The fluorescence spectrum shows that calcium cation quenches the fluorescence of the enzyme through static quenching mechanism,indicating that calcium cation was bound to the enzyme.Based on the study of calcium cation on CD ellipticity of Ape1547 by cir...     

Enhanced Activity and Enantioselectivity of a Hyperthermophilic Esterase from Archaeon Aeropyrum pernix K1 by Acetone Treatment

To improve the activity and enantioselectivity of hyperthermophilic archaeon Aeropyrum pernix K1 esterase (APE1547) and its mutants, they were purified by acetone-treated method. It was found that the acetone treatment not only caused APE1547 and its mutants to display higher activity and enantioselectivity but also saved more than 90% of time spent in purifying them by Ni-chelating column. In hydrolysis of p-nitrophenyl caprylate, the acetone-treated APE1547 and mutant A containing the following substitutions R11G, L36P, V225A, I551L, and A564T showed 5.7- and 6.9-fold active increase, respectively. In the resolution of 2-octanol acetate, the acetone-treated mutant A had a 9-fold enantioselective increase relative to that purified by Ni-chelating column. In addition, the impact of pH, temperature, and chemical reagents on activity of APE1547 and mutant A was discussed in this paper.     

Acylation of Quercetin with a Novel Thermophilic Esterase as Biocatalyst

The regioselective acylation of quercetin catalyzed by a novel thermophilic esterase(APE1547)from the archaeon Aeropyrum pernix K1 was successfully conducted in organic solvents.The effects of acyl don...     

Enzyme catalytic promiscuity: asymmetric aldol addition reaction catalyzed by a novel thermophilic esterase in organic solvent

The asymmetric aldol addition of 2-butanone and 4-nitrobenzaldehyde catalyzed by a novel thermophilic esterase (APE1547) from the archaeon Aeropyrum pernix K1 was successfully conducted in organic solvents. APE1547 exhibited a good enzyme activity and enantioselectivity in the reaction. The effects of organic solvent, temperature, water content, and substrate concentration were investigated. The reaction provided optically active secondary alcohol with satisfying enantioselectivity (71.2 %ee) and enzyme activity (38.1 µmol/g/h) under the optimum conditions. A high yield (68.7%) could be obtained when the reaction time was approximately 120 h.     

超嗜热酯酶APE1547中特殊位置氢键对酶活力和热稳定性的影响

探讨了APE1547蛋白的β-推进器结构中第3和第4“叶片”间的侧链氢键(Thr127-Gly154, Leu182-Arg145-Glu122)对蛋白质的作用.     

Study on a Specific Site Tyr~(444) on a Hyperthermophilic Enzyme APE1547

Hyperthermophilic enzyme APE1547 is an extremely thermostable recombinant protein from thermophilic archaeon Aeropyrum pernix K1. The Tyr444 located in the catalytic domain adjacent to the catalytic amino acid Ser445 and formed hydrogen bond with Ile567. To study the effect of Tyr444 on the activity of APE1547,site-directed mutagenesis was applied. Two mutant enzymes T444S and T444G were created. Comparison of the mutant enzymes with wide enzyme,the thermostability of mutants T444S and T444G decreased by 10...     

Denaturing Effects of Urea and Guanidine Hydrochloride on Hyperthermophilic Esterase from Aeropyrum pernix K1

Introduction Esterases(EC3.1.1.x)representadiversegroup ofhydrolasescatalyzingthecleavageandformationof esterbonds.Theyarewidelydistributedinanimals,plantsandmicroorganisms.Becauseoftheiractivities inbothaqueousandnonaqueoussolventsystems,ester aseshavebe…     

离子液体中酶促Michael加成反应的研究

以离子液体作为反应介质,研究了嗜热酯酶APE1547在不同离子液体中催化咪唑与丙烯酸乙酯的Mi-clasel加成反应,并对反应条件进行了优化.在最适反应条件下,Michael加成反应产率可达98.8%,另外发现嗜热酯酶APE1547在该反应体系中可重复使用8次,其催化性能没有明显下降.     

Clone,Purification and Characterization of Thermostable Aminopeptidase ST1737 from Sulfolobus tokodaii

The aminopeptidase gene from thermophilic archaea Sulfolobustokodaii was cloned and expressed in Escherichia coli BL21 codon-plus(DE3). To overexpress the aminopeptidase, the vector pET32a was constructed, in which the target gene was fused with the genes of histidine-tag and thioredoxin(Trx). The expressed protein was purified using Ni²⁺-column affinity chromatography and ion exchange chromatography and cleft with enterokinase(EK) to obtain the purified aminopeptidase(ST1737). The biochemical and enzymic properties of the expressed ST1737 were characterized. The results show that its optimal pH and temperature are 8 and 80 ℃, respectively. The half-life of ST1737(0.2 mg/mL) is about 85 h at 90 ℃, indicating that the enzyme exhibits an excellent thermostability. The activity of ST1737 could still maintain over 85% after its treatment at 25 ℃ in different buffers with a pH range of from 6.0 to 10.5 for 24 h, demonstrating that ST1737 is stable in neutral or slight alkali environment. The enzyme shows a high activity for the substrates, such as unmodified peptide Asp-Ala, while the pNPC₈ shows an optimal esterase substrate specificity. These results indicate that the enzyme is a bifunctional enzyme, and different from the aminopeptidase reported before.