易错PCR提高华根霉脂肪酶的热稳定性

为了提高华根霉Rhizopus chinensis CCTCC M201021脂肪酶的热稳定性,运用定向进化-易错PCR的方法,经两轮易错PCR引入突变,利用fast-blue RR顶层琼脂法对突变文库进行筛选,第一轮易错PCR后筛选到2株突变菌株,第二轮筛选到4株突变株。第二轮最佳突变株Ep2-4,其中3个氨基酸发生了突变：A129S、P168L和V329A。该突变酶ep2-4在60 ℃下半衰期相对原始酶r27RCL提高5.4倍,T50值提高7.8 ℃。酶学性质研究表明,突变酶ep2-4在热稳定性提高的基础上,仍保有良好的催化活性。蛋白质三维结构模拟显示,突变A129S可以和Gln133形成氢键,增加了酶表面的亲水性和极性;P168L可以与邻近的Leu164形成疏水键,导致突变酶的热稳定性提高。     

基于易错PCR技术的短小芽孢杆菌YZ02脂肪酶基因BpL的定向进化

利用易错PCR技术对短小芽胞杆菌(Bacillus pumilus)YZ02脂肪酶基因BpL进行两轮定向进化研究, 分别获得最佳突变株BpL1-7和BpL2-1369, 其脂肪酶活力比出发酶分别提高了2倍和6倍。序列分析表明, 突变体BpL2-1369有4个碱基发生了突变: T61C/C147T/A334G/T371A, 其中有3个碱基突变导致了氨基酸的改变。通过SWISS-MODEL数据库模拟脂肪酶的结构显示, 3个突变氨基酸分别位于第1个a螺旋的第3个氨基酸、第4和第5个b折叠之间的转角以及第5个b折叠的第1个氨基酸位置。将野生型脂肪酶基因BpL和进化后的基因BpL2-1369的高效表达产物经Ni-Agarose柱和Sephadex-G75纯化后, 酶学性质测定表明: 突变脂肪酶的比活力比野生型脂肪酶提高了1.31倍, Km值由8.24 mmol/L降低至7.17 mmol/L; 在pH>8.0时的稳定性较野生型脂肪酶有所提高。     

基于易错PCR技术的短小芽孢杆菌YZ02脂肪酶基因BpL的定向进化

利用易错PCR技术对短小芽胞杆菌(Bacillus pumilus)YZ02脂肪酶基因BpL进行两轮定向进化研究, 分别获得最佳突变株BpL1-7和BpL2-1369, 其脂肪酶活力比出发酶分别提高了2倍和6倍。序列分析表明, 突变体BpL2-1369有4个碱基发生了突变: T61C/C147T/A334G/T371A, 其中有3个碱基突变导致了氨基酸的改变。通过SWISS-MODEL数据库模拟脂肪酶的结构显示, 3个突变氨基酸分别位于第1个a螺旋的第3个氨基酸、第4和第5个b折叠之间的转角以及第5个b折叠的第1个氨基酸位置。将野生型脂肪酶基因BpL和进化后的基因BpL2-1369的高效表达产物经Ni-Agarose柱和Sephadex-G75纯化后, 酶学性质测定表明: 突变脂肪酶的比活力比野生型脂肪酶提高了1.31倍, Km值由8.24 mmol/L降低至7.17 mmol/L; 在pH>8.0时的稳定性较野生型脂肪酶有所提高。     

易错PCR技术提高黑曲霉N25植酸酶活力的研究

利用易错PCR技术对黑曲霉(Aspergillus niger)N25的植酸酶基因phyA进行定向进化研究,突变基因产物重组于表达载体pET32a(+)中,并导入大肠杆菌BL21(DE3)构建突变体文库,经筛选获得了最佳突变菌株pET32a-phyAep,其植酸酶活力比出发酶提高了41.8%。突变酶的酶学性质研究发现,与野生酶相比,它的热稳定性,最适温度和最适pH值无显著变化。     

基于易错PCR的假密环菌Armillariella tabescens MAN47β-甘露聚糖酶耐高温定向进化

本研究利用易错PCR技术突变假密环菌Armillariella tabescens MAN47β-甘露聚糖酶野生型基因,PCR产物与大肠杆菌-酿酒酵母穿梭表达载体pYCα上连接,在大肠杆菌DH5α中扩增后电转入酿酒酵母Saccharomyces cerevisiae,构建了库容为10_4的初级突变体库,筛选得到耐高温最佳突变株M262.DNS法测得80℃处理30 min后最大酶活力为25 U/mL,较之野生型最适条件酶活力提高了4.3倍.序列分析表明,突变体有3个碱基发生了突变:T343A/C827T/T1139C,相应的氨基酸改变为Ser115Thr/Thr276Met/Val380Ala,利用SWISS-MODEL数据库同源建模显示,这3个突变氨基酸分别位于第4个13折叠的第6个氨基酸、第6个α螺旋的第1个氨基酸、第10个α螺旋和第11个β折叠之间的转角.     

基于易错PCR的假密环菌Armillariella tabescens MAN47 b-甘露聚糖酶耐高温定向进化

本研究利用易错PCR技术突变假密环菌Armillariella tabescens MAN47 β-甘露聚糖酶野生型基因,PCR产物与大肠杆菌-酿酒酵母穿梭表达载体pYCα上连接,在大肠杆菌DH5α中扩增后电转入酿酒酵母Saccharomyces cerevisiae,构建了库容为104的初级突变体库,筛选得到耐高温最佳突变株M262。DNS法测得80oC处理30min后最大酶活力为25U/mL,较之野生型最适条件酶活力提高了4.3倍。序列分析表明,突变体有3个碱基发生了突变:T343A/C827T/T1139C,相应的氨基酸改变为Ser115Thr/Thr276Met/Val380Ala,利用SWISS-MODEL数据库同源建模显示,这3个突变氨基酸分别位于第4个β折叠的第6个氨基酸、第6个α螺旋的第1个氨基酸、第10个α螺旋和第11个β折叠之间的转角。     

应用易错PCR技术提高环糊精葡萄糖基转移酶的可溶性表达

【目的】对嗜热脂肪芽孢杆菌CHB1的环糊精葡萄糖基转移酶(CGTase)基因进行定向进化,筛选得到胞外酶活性和可溶性表达定量提高的突变酶。【方法】采用易错PCR技术向环糊精葡萄糖基转移酶基因中随机引入突变,建立酶基因突变文库,筛选获得胞外酶活性和可溶性表达定量提高的突变体,并对突变酶进行诱导表达、纯化及部分酶学性质研究。【结果】通过筛选获得CGTase胞外酶活性和可溶性表达定量提高的突变菌株ds-6和ep-9,其胞外α-环化活力分别是原始酶的1.72倍和2.18倍,可溶性表达量提高了1倍。序列分析表明,突变体ep-9有3个碱基发生了变化:G2005A/A2037G/T2081G,其中有2个碱基突变导致了氨基酸的改变。SWISS-MODEL数据库模拟CGTase的结构表明,2个突变氨基酸分别位于无规卷曲和β-转角/折叠之间的转角中。酶学性质测定表明:突变CGTase的β-环化比活力是原始酶的2.44倍,总环化比活力提高了34%,K_m值由4.3 g/L降低到3.74 g/L;在pH稳定性方面较原始酶有所提高。单碱基定点突变证实突变体ep-9可溶性表达水平及胞外酶活性提高的关键突变是G2005A。【结论】本试验表明:基于易错PCR技术获得嗜热芽孢杆菌CHB1的CGTase的胞外酶活和可溶性表达定向进化,G2005A突变对于提高CGTase的可溶性表达及胞外酶活起关键作用,这对认识CGTase的构效关系以及进一步改造该酶分子、扩大酶的生产应用具有重要意义。     

基于体外分子进化技术提高弯曲芽孢杆菌CCTCC 2015368 β-淀粉酶的热稳定性

运用体外分子进化技术易错PCR方法,高通量筛选热稳定性提高的弯曲芽孢杆菌Bacillus flexus CCTCC2015368β-淀粉酶突变体。利用LB琼脂淀粉板显色、96-孔板DNS法测酶活和酶标仪检测等,最终筛选到了一株热稳定性显著提高的突变体D476N。野生型和突变体D476N分别纯化后,酶学性质测定表明:突变体D476N的最适pH为6.5,与野生型相比降低了0.5。突变体D476N和野生型的最适温度均为55℃,突变体D476N在55℃下的半衰期为35 min,比野生型提高了95%。突变体D476N的T_(50)值比野生型提高4℃。突变体D476N的K_m值为97.98μmol/L,是野生型(85.86μmol/L)1.14倍;突变体稳定性提高的同时,催化活力相对于野生型有略微下降。通过SWISS-MODEL同源模拟野生型和突变体D476N的三维结构,并通过PyMol软件分析,发现突变后的氨基酸残基Asn476位于蛋白质表面的loop环上,通过MOE软件计算,D476N的分子自由能(ΔG)为106.01kcal/mol,比野生酶降低10.3%,这一结果与蛋白质分子自由能和热稳定性呈负相关的理论相符。     

基于易错PCR的黄曲霉毒素解毒酶体外分子定向进化

运用定向进化-易错PCR方法,提高黄曲霉毒素解毒酶的活力及稳定性,并结合辣根过氧化物酶 (HRP)-隐性亮绿 (RBG) 快速高通量筛选系统,构建了库容约为104的突变体库。经过两轮易错PCR,最终分别获得了耐高温70 ℃突变酶A1773、pH 4.0稳定性的突变酶A1476,pH 4.0和pH 7.5均表现稳定性的突变酶A2863,其酶活力比野生酶分别提高了6.5倍、21倍和12.6倍。经序列分析表明,发现突变酶A1773发生了Glu127Lys和Gln613Arg突变;突变酶A2863发生了Gly73     

定向进化-易错PCR方法提高华根霉Rhizopus chinensis CCTCC M201021脂肪酶的活力

运用定向进化-易错PCR的方法,提高了华根霉Rhizopus chinensis CCTCC M201021脂肪酶的活力。经过两轮易错PCR和pNPP顶层琼脂法筛选,从第一轮和第二轮突变库中分别筛选获得最佳突变株1-11和2-28,脂肪酶酶活与野生菌株相比分别提高2倍和4倍。基因比对结果表明,突变脂肪酶2-28有4个氨基酸发生了突变:A129S、K161R、A230T、K322R。蛋白质分子空间结构模拟显示,突变A129S、K161R、A230T位于脂肪酶分子表面。突变A230T增强了α-螺旋盖结构的稳定性。突变K322R处在loop上,靠近脂肪酶底物结合区域,与邻近的Asp(带负电)形成盐桥。静电引力将该loop向底物进入酶活性中心的通道口反方向牵引,使底物分子更易进入酶活性中心。酶学性质研究表明,突变株2-28脂肪酶的Km值比出发菌株下降了10%,Kcat值提高为原来的2.75倍。     

Improved activity and pH stability of E. coli ATCC 11105 penicillin acylase by error-prone PCR

Penicillin G acylase is the key enzyme used in the industrial production of β-lactam antibiotics. This enzyme hydrolyzes penicillin G and related β-lactam antibiotics releasing 6-aminopenicillanic acid, which is an intermediate in the production of semisynthetic penicillins. To improve the enzymatic activity of Escherichia coli penicillin acylase, sequential rounds of error-prone polymerase chain reaction were applied to the E. coli pac gene. After the second round of evolution, the best mutant M2234 with enhanced activity was selected and analyzed. DNA sequence analyses of M2234 revealed that one amino acid residue (K297I), located far from the center of the catalytic pocket, was changed. This mutant (M2234) has a specific activity 4.0 times higher than the parent enzyme and also displayed higher stability at pH 10.     

通过易错PCR提高鼠伤寒沙门氏菌丙氨酸消旋酶催化活性

[目的] 通过易错PCR技术提高鼠伤寒沙门氏菌中丙氨酸消旋酶的催化活性。[方法] 利用易错PCR技术构建丙氨酸消旋酶基因alr_St的突变体文库,采用缺陷菌株UT5028筛选突变体基因,以D-氨基酸氧化酶偶联法检测各突变蛋白的活性,通过凝胶过滤层析法分析酶蛋白寡聚化状态,并采用HPLC检测酶蛋白的动力学参数。[结果] 经过易错PCR及定点突变技术最终获得了3个催化活性有所提高的突变体A3V、Y343H和A3VY343H,酶学特性分析发现,与野生型蛋白StAlr相比,突变体Y343H仅对底物L/D-丝氨酸的催化效率略有提高,k_cat/K_m值分别是StAlr的2.01和3.68倍;而突变体A3V则对底物L/D-丙氨酸或L/D-丝氨酸的K_m、k_cat和k_cat/K_m值均有较大幅度的改变,其k_cat/K_m值分别是StAlr的105.51、97.36、4.63和10.73倍。凝胶过滤层析结果显示,突变体A3V在蛋白含量极低时就呈现出单体和二聚体共存状态,且随着蛋白含量的增加,其向二聚体状态迁移的速率最为明显。[结论] 丙氨酸消旋酶StAlr的第3位点是影响其催化活性和低聚合状态的关键位点。     

Characterization of thermostable lipase from thermophilic Geobacillus sp. TW1

A novel lipase-producing thermophilic strain TW1, assigned to Geobacillus sp. TW1 based on 16S rRNA sequence, was isolated from a hot spring in China. Based on this strain, a lipase gene encoding 417 amino acids was cloned. Subsequently, the lipase gene was expressed in Escherichia coli and purified as a fusion protein with glutathione S-transferase. The results showed that the recombinant lipase had an activity optimum at 40 degrees C and pH at 7.0-8.0. It was active up to 90 degrees C at pH 7.5, and stable over a wide pH ranging from 6.0 to 9.0. The recombinant lipase was stable in 1 mM enzyme inhibitors (EDTA, 2-ME, SDS, PMSF or DTT), as well as in 0.1% detergents (Tween 20, Chaps or Triton X-100). Its catalytic function was enhanced in the presence of Ca(2+), Mg(2+), Zn(2+), Fe(2+) or Fe(3+), but inhibited by Cu(2+), Mn(2+), and Li(+). By comparison with the crude lipase, the recombinant lipase had similar properties and was characteristic of thermostable enzymes. Our study presented a rapid overexpression and purification of the lipase gene from thermophile, aimed at improving the enzyme yield for industrial applications.     

Zinc in lipase L1 from Geobacillus stearothermophilus L1 and structural implications on thermal stability

Lipase L1 from Geobacillus stearothermophilus L1 contains an unusual extra domain, making a tight intramolecular interaction with the main catalytic domain through a Zn2+-binding coordination. To elucidate the role of the Zn2+, we disrupted the Zn2+-binding site by mutating the zinc-ligand residues (H87A, D61A/H87A, and D61A/H81A/H87A/D238A). The activity vs. temperature profiles of the mutant enzymes showed that the disruption of the Zn2+-binding site resulted in a notable decrease in the optimal temperature for maximal activity from 60 to 45-50 degrees C. The mutations also abolished the Zn2+-induced thermal stabilization. The wild-type enzyme revealed a 34.6-fold increase in stabilization with the addition of Zn2+ at 60 degrees C, whereas the mutant enzymes exhibited no response to Zn2+. Additional circular dichroism spectroscopy studies also confirmed the structural stabilizing role of Zn2+ on lipase L1 at elevated temperatures.     

N-terminal purification tag alters thermal stability of the carboxylesterase EstGtA2 from G. thermodenitrificans by impairing reversibility of thermal unfolding

The novel thermostable carboxylesterase EstGtA2 from G. thermodenitrificans (accession no. AEN92268) was functionally expressed and purified using an N-terminal fusion tag peptide. We recently reported general properties of the recombinant enzyme. Here we report preliminary data on thermal stability of EstGtA2 and of its tagged form. Conformational stability was investigated using circular dichroism and correlated with residual activity measurements using a colorimetric assay. The tag peptide had no considerable impact on the apparent melting temperature: T(m) value = 64.8°C (tagged) and 65.7°C (cleaved) at pH 8. After thermal unfolding, the tag-free enzyme rapidly recovered initial activity at 25°C (1.2 Umg(-1)), which was corroborated by substantial refolding (83%) as determined by far-UV CD transitions. However, after thermal unfolding, the purification tag drastically decreased specific activity at 25°C (0.07 Umg(-1)). This was corroborated by the absence of refolding transition. Although the purification tag has no undesirable impact on activity before thermal unfolding as well as on Tm, it drastically hinders EstGtA2 refolding resulting in a major loss of thermal stability.     

High level expression of thermostable lipase from Geobacillus sp. strain T1

A thermostable extracellular lipase of Geobacillus sp. strain T1 was cloned in a prokaryotic system. Sequence analysis revealed an open reading frame of 1,251 bp in length which codes for a polypeptide of 416 amino acid residues. The polypeptide was composed of a signal peptide (28 amino acids) and a mature protein of 388 amino acids. Instead of Gly, Ala was substituted as the first residue of the conserved pentapeptide Gly-X-Ser-X-Gly. Successful gene expression was obtained with pBAD, pRSET, pET, and pGEX as under the control of araBAD, T7, T7 lac, and tac promoters, respectively. Among them, pGEX had a specific activity of 30.19 Umg(-1) which corresponds to 2927.15 Ug(-1) of wet cells after optimization. The recombinant lipase had an optimum temperature and pH of 65 degrees C and pH 9, respectively. It was stable up to 65 degrees C at pH 7 and active over a wide pH range (pH 6-11). This study presents a rapid cloning and overexpression, aimed at improving the enzyme yield for successful industrial application.     

A general model of error-prone PCR

In this paper, we generalize a previously-described model of the error-prone polymerase chain reaction (PCR) reaction to conditions of arbitrarily variable amplification efficiency and initial population size. Generalisation of the model to these conditions improves the correspondence to observed and expected behaviours of PCR, and restricts the extent to which the model may explore sequence space for a prescribed set of parameters. Error-prone PCR in realistic reaction conditions is predicted to be less effective at generating grossly divergent sequences than the original model. The estimate of mutation rate per cycle by sampling sequences from an in vitro PCR experiment is correspondingly affected by the choice of model and parameters.