绿色木霉葡聚糖内切酶EGIII基因在大肠肝菌中的表达、定点突变及其动力学特性的研究

将绿色木霉葡聚糖内切酶EGIII基因亚克隆到表达载体pET-22b(+),构建重组质粒pET-egl3,转化到大肠杆菌BL21(DE3).利用金属亲和层析对重组EGIII进行纯化,纯化后酶比活力达到6 U/mg蛋白,最适反应温度为60 ℃,最适pH为4.0.同时对EGIII催化区的氨基酸残基R130和E218进行定点饱和突变,各筛选到一株酶活有提高的突变子R130P和E218F,其比活力为野生型EGIII的2.8倍和3.45倍.突变酶E218F的Km提高了一倍,催化效率Kcat提高了5.4倍;而R130P的Km和Kcat没有明显变化.两个突变酶的最适酶解温度和pH分别都提高至65 ℃和4.4.     

绿色木霉葡聚糖内切酶EGⅢ基因在大肠杆菌中的表达、定点突变及其动力学特性的研究

将绿色木霉葡聚糖内切酶EGⅢ基因亚克隆到表达载体pET-22b（＋）,构建重组质粒pET-egl3,转化到大肠杆菌BL21（DE3）。利用金属亲和层析对重组EGⅢ进行纯化,纯化后酶比活力达到6u／mg蛋白,最适反应温度为60℃,最适pH为4．0。同时对EGⅢ催化区的氨基酸残基R130和E218进行定点饱和突变,各筛选到一株酶活有提高的突变子R130P和E218F,其比活力为野生型EGⅢ的2．8倍和3．45倍。突变酶E218F的Km提高了一倍,催化效率Kcat提高了5．4倍;而R130P的Km和Kcat没有明显变化。两个突变酶的最适酶解温度和pH分别都提高至65℃和4．4。     

定点突变对酰胺水解酶DamH可溶性表达和酶活的影响

摘要:【目的】DamH是一种具有酯酶活性的酰胺水解酶,其非活性中心氨基酸残基的突变对重组酶可溶性表达和比酶活产生一定的影响。拟探索DamH的活性中心氨基酸残基构成,并对其非活性中心氨基酸残基突变对可溶性表达和比酶活的影响进行研究。【方法】通过重叠延伸的方法对DamH可能的活性中心氨基酸S149、E244和H274以及非活性中心氨基酸D165及N192进行定点突变,通过静息细胞测活验证了S149、E244和H274 在催化2-氯-N-(2’-甲基-6’-乙基苯基)乙酰胺(CMEPA)水解反应中的作用,通过Ni2+- NTA亲和层析对D165及N192突变子进行纯化,对突变株和野生型比酶活进行比较。【结果】研究表明S149A使DamH的CMEPA 水解酶活性下降为野生型的5%,E244A和H274A突变导致其失去活性;D165P和N192P突变影响到DamH的可溶性表达,表达量分别为野生型的28.2%和20.8%,突变子N192P、D165P比酶活分别为野生型比酶活的55.5%和49.7%。【结论】DamH催化酯类底物和芳基酰胺类底物可能共用同一活性中心S149、E244和H274,其两个α螺旋的转角处氨基酸侧链极性和刚性结构的改变对可溶性表达以及活性有很大的影响。     

简单节杆菌3-甾酮-△1 -脱氢酶基因的克隆表达及定点突变研究

目的:将来源于简单节杆菌的3-甾酮-△~1-脱氢酶(3-ketosteroid-Delta(1)-dehydrogenase,KSDD)在大肠杆菌中进行表达,获得具有活性的脱氢酶;利用计算机预测KSDD的三级结构,并通过定点突变确定酶的关键位点以期优化脱氢酶的活性及性质。方法:克隆简单节杆菌编码KSDD的基因ksdd构建原核表达载体,以Escherichia coli BL21(DE3)为表达宿主构建重组菌并诱导表达,HPLC法检测重组酶催化4-AD脱氢的转化率;通过SWISS-MODEL同源建模分析KSDD结构,对预测的催化关键位点氨基酸残基进行定点突变并研究突变后重组酶的活性变化。结果:成功构建了表达脱氢酶KSDD的重组菌E.coli pET-22-ksdd,21℃下诱导表达后,重组酶对4-AD的转化率为27%;通过SWISS-MODEL同源建模预测出脱氢酶结构并对4个关键位点进行定点突变设计,获得突变子Y120R、Y320L、Y488F和G492Y。突变子Y120R和Y488F失活,证明其为酶的活性位点;突变子Y320L的转化率与野生型基本一致,但37℃反应条件下稳定性有所提高;突变子G492Y对4-AD的转化率是野生型的1.2倍,37℃条件下稳定性有所提高,是突变后氨基酸位点疏水性增加和周围静电作用改变所导致。结论:目前对简单节杆菌3-甾酮-△~1-脱氢酶结构分析及催化机理相关的研究较少,本研究验证了KSDD的活性位点,优化了酶的稳定性,为进一步对酶的性质进行定向改造打下了基础。     

Myxococcus sp.V11海藻糖合酶TreS II分子改造 *

来源于黏细菌Myxococcus sp.V11的海藻糖合酶(trehalose synthase, EC 2.4.1.245)TreS II可通过转糖苷作用将麦芽糖转化成为海藻糖,在酶法生产海藻糖上显示出一定的应用潜力,但TreS II对热敏感,在60℃保温3h,酶活性丧失,限制了其应用范围.目的:拟探索TreS II影响热稳定性的氨基酸残基构成,通过对可能的氨基酸位点进行定点突变,以期获得耐热性的突变子,扩大TreS II应用范围.方法: 通过PCR介导的方法对TreS II可能影响到热稳定性的氨基酸Q3,A283,W374,R449和Y537进行定点突变,以野生型重组酶为对照,比较突变型与野生型的最适反应温度和最适反应pH,通过测定不同温度下保存不同时间后的残留酶活,检测突变子的耐热效果.结果: 研究表明突变子Q3D,A283R,W374D,R449Q和Y537H的比酶活与野生型无显著差异,且最适pH 和最适反应温度也未发生改变;A283R,Y537H在60℃条件下,3h后活性剩余68%;Q3D,W374D,R449Q在温度60℃时,3h后活性剩余35%.结论: TreS II分子结构中与金属离子结合的几个氨基酸残基的改变对蛋白质分子的耐热性具有显著影响.     

N13D、S40E点突变提高木聚糖酶XYNB的热稳定性

对来源于Streptomyces olivaceoviridis的高比活木聚糖酶XYNB进行同源建模和序列比较,设计了N13D、S40E的定点突变,以期改善中温酶XYNB的热稳定性。突变酶N13D、S40E分别在毕赤酵母中表达,经纯化后与野生型酶XYNB(同样经毕赤酵母表达后纯化)进行酶学性质比较,结果表明,突变酶N13D和S40E在70℃处理5min,热稳定性比XYNB分别提高了24.76%和14.46%;突变酶N13D的比活性比XYNB提高了22%。在其他性质方面突变酶N13D、S40E与野生型酶XYNB基本相似。通过对木聚糖酶XYNB的定点突变,提高了该酶的热稳定性,并为结构与功能的进一步研究提供了材料。     

嗜热革节孢GH1 BGL1进口端位点对酶活性及葡萄糖耐受性的影响

糖苷水解酶第一家族(GH1)β-葡萄糖苷酶(BGL1)有葡萄糖耐受性,进口端位点对酶活性及葡萄糖耐受性有很大影响,但具体作用机制尚不清楚。对嗜热革节孢GH1 BGL1进口端的W168、L173、F348、W349、C169、F180、D237、Y179、A260、H307、N335和E437这12个氨基酸残基进行定点突变,将突变酶与野生酶(WT)在毕赤酵母中表达,表达产物纯化后进行酶活性和葡萄糖耐受性测定。与WT相比,所有突变酶活性均有所降低,其中W168H、N335F和W349G几乎丧失活性。突变F180H、D237S、A260N和H307Y的Km低于WT,所有突变的kcat都降低。除L173Q外,其余突变都保持葡萄糖耐受性,在高浓度(400 mmol/L)葡萄糖时,Y179F和D237S酶活受到显著抑制。本研究表明,进口端位点对酶活性及葡萄糖耐受性均具有一定影响,催化活性通道的结构特异性可能是葡萄糖耐受机制。     

亚热带山区土壤未培养微生物L-赖氨酸脱羧酶Ldc1E中关键氨基酸残基的功能鉴定

本研究旨在探讨L-赖氨酸脱羧酶Ldc1E关键氨基酸在底物识别和催化过程中的作用;通过生物信息学方法选择突变位点,并利用直接定点突变技术,完成了6个关键氨基酸残基突变和功能鉴定研究。突变酶D692N最适温度和pH值分别为40℃和6.5。突变酶D692N比野生型Ldc1E对高温具有更强的耐受性,在40℃～55℃温浴1 h后剩余酶活力达到35%以上,在60℃温浴1 h后仍然保留20%的酶活力;而野生型酶Ldc1E在50℃以上温浴1 h后几乎失活。此外,50 mmol/L DMSO、5 mmol/L Al~(3+)和Ca~(2+)对突变酶的酶活力有激活作用,而Al3+对野生型酶Ldc1E具有明显抑制作用。突变酶D692N的分子动力学常数K_m升高了1.78倍,k_(cat)下降了20.2倍。突变酶S221A、H245A、D330A、H366A、F607Y经检测酶催化活性丧失。研究结果表明氨基酸残基位点D692对酶与底物的结合具有重要影响;而S221、H245、D330、H366、F607是Ldc1E酶活性能够体现的关键氨基酸位点,不可替换。本研究为探究L-赖氨酸脱羧酶的结构与功能关系提供理论参考。     

溶葡球菌酶的定点突变与PEG巯基定点修饰

为了建立聚乙二醇 (PEG) 巯基定点修饰溶葡球菌酶的方法,并检验假定连接区的突变与修饰对酶活的影响,对溶葡球菌酶的假定连接区进行了巯基聚乙二醇定点修饰研究。通过分析溶葡球菌酶的结构特征,选择两个结构域之间的氨基酸 (133-154aa) 进行定点突变引入半胱氨酸残基。使用单甲氧基聚乙二醇马来酰亚胺 (mPEG-MAL) 进行定点修饰,对修饰后的酶进行纯化并测定酶活性。结果表明定点突变的半胱氨酸残基PEG修饰效率高、产物单一,运用简便的Ni2+-NTA柱亲和层析法实现了一步分离,获得了高纯度的目标蛋白,但在连接区进行定点突变及PEG定点修饰后的酶活有不同程度的降低,表明假定连接区部分位点的PEG修饰会对溶葡球菌酶的催化活性产生一定影响。     

利用DREAM设计和同源重组进行一步定点突变

目的：建立基于DREAM设计和同源重组的简便、快速定点突变方法。方法：设计两条包含突变的反向PCR（inverse PCR）引物,使其5'端互补从而产生同源重组,同时使用DREAM设计方案在上述引物中引入限制性内切酶位点以便突变子筛选。用能扩增长片段的高保真耐热 DNA聚合酶扩增全长的质粒DNA,直接转化大肠杆菌。转化到细菌中的全长质粒DNA PCR产物可利用其末端同源序列发生同源重组而环化。利用引入的酶切位点方便地进行突变子的筛选。结果：我们用该方法成功地对长度大于7 kb的质粒进行了定点突变。结论：本定点突变无需任何突变试剂盒和特殊的试剂,只需一步反应即可完成;利用DREAM设计使克隆筛选简便可靠,高保真耐热DNA聚合酶可保证多数突变子克隆不发生意外突变,而该酶扩增长片段的能力使该方法适合于大多数质粒不经亚克隆直接突变。     

Enzymatic properties of mutant Escherichia coli tryptophan synthase alpha-subunits

Thirty-nine mutant tryptophan synthase alpha subunits have been purified and analyzed (in the presence of the beta 2-subunit) for their enzymatic (kcat, Km) behavior in the reactions catalyzed by the alpha 2.beta 2 complex, the fully constituted form of this enzyme. The mutant alpha subunits, obtained by in vitro random, saturation mutagenesis of the encoding trpA gene, contain single amino acid substitutions at sites within the first 121 residues of the alpha polypeptide. Four categories of altered residues have been tentatively assigned roles in the catalytic functions of this enzyme: 1) catalytic residues (Glu49 and Asp60); 2) residues involved in substrate binding or orientation (Phe22, Thr63, Gln65, Tyr102, and Leu105); 3) residues involved in alpha.beta subunit interactions (Gly51, Pro53, Asp56, Asp60, Pro62, Ala67, Phe72, Thr77, Pro78, Tyr102, Asn104, Leu105, and Asn108); and 4) residues with no apparent catalytic roles. Catalytic residue alterations result in no detectable activity in the alpha-subunit specific reactions. Substrate binding/orientation roles are detected enzymatically primarily as rate defects; alterations only at Tyr102 result in apparent Km effects. alpha.beta interaction roles are detected as rate defects in all tryptophan synthase reactions plus Km increases for the alpha-subunit substrate, indole-3-glycerol phosphate, only when L-serine is present at the beta 2-subunit active site. A substitution at only one site, Asn104, appears to be unique in its potential effect on intersubunit channeling of indole, the product of the alpha-subunit specific reaction, to the beta 2-subunit active site.     

Identification of glutamic acid 646 as a zinc-coordinating residue in endopeptidase-24.11.

Neutral endopeptidase (EC 3.424.11, NEP) is a membrane-bound zinc-metallopeptidase. The substrate specificity and catalytic activity of NEP resemble those of thermolysin, a bacterial zinc-metalloprotease. Comparison of the primary structure of both enzymes suggests that several amino acids present in the active site of thermolysin are also found in NEP. Using site-directed mutagenesis of the cDNA encoding the NEP sequence, we have already shown that His residues 583 and 587 are two of the three zinc ligands. In order to identify the third zinc ligand, we have substituted Val or Asp for Glu616 or Glu646. Val616 NEP showed the same kinetic parameters as the non-mutated NEP. In contrast, the mutant Val646 NEP was almost completely devoid of catalytic activity and unable to bind the tritiated inhibitor [3H]N-[2(R,S)-3-hydroxyaminocarbonyl-2-benzyl-1-oxypropyl]gl ycine, the binding of which is dependent on the presence of the zinc ion. Replacing Glu for Asp at position 646 conserved the negative charge, and the mutant enzyme exhibited the same Km value as the non-mutated enzyme, but kCat was decreased to less than 3% of the value of the non-mutated enzyme. When compared to the non-mutated enzyme Asp646 NEP showed a higher susceptibility to chelating agents, but bound the tritiated inhibitor with the same affinity. Taken together, these observations strongly suggest that Glu646 of NEP is the third zinc-coordinating residue and is equivalent to Glu166 in thermolysin.     

Assignment of the nucleotide binding sites and the mechanism of substrate inhibition of Escherichia coli adenylate kinase

Site-directed mutagenesis of key amino acids of adenylate kinase has been used to suggest a new model for the location of the AMP and ATP binding sites. Phe-86 and Tyr-133, which are in close contact with the inhibitor Ap5A according to previous crystallographic results, have been independently changed to tryptophan and other amino acids. The Phe-86----Trp mutant had a 3- to 6-fold change in the Km for ATP and a 44-fold increase in the Km for AMP with a simultaneous loss of AMP substrate inhibition. Thus Phe-86 is probably in close contact with bound AMP. The Tyr-133----Trp mutant showed no large effects on enzyme kinetics and suggests that the previous assignment of Ap5A occupying natural adenosine binding sites is probably incorrect. A temperature-sensitive Leu-107----Gln mutant showed a 6-fold decrease in the Km for ATP and no effect on AMP binding, suggesting that this amino acid is near the ATP binding site. Changes in the fluorescence of single tryptophan-containing mutant enzymes provided specific information about AMP and ATP binding. The fluorescence results are consistent with the kinetic studies, and also suggest that AMP substrate inhibition is caused by the formation of an abortive complex that prevents the release of product.     

Mutational analysis of human DNase I at the DNA binding interface: implications for DNA recognition,catalysis, and metal ion dependence.

Human deoxyribonuclease I (DNase I), an enzyme used to treat cystic fibrosis patients, has been systematically analyzed by site-directed mutagenesis of residues at the DNA binding interface. Crystal structures of bovine DNase I complexed with two different oligonucleotides have implicated the participation of over 20 amino acids in catalysis or DNA recognition. These residues have been classified into four groups based on the characterization of over 80 human DNase I variants. Mutations at any of the four catalytic amino acids His 134, His 252, Glu 78, and Asp 212 drastically reduced the hydrolytic activity of DNase I. Replacing the three putative divalent metal ion-coordinating residues Glu 39, Asp 168, or Asp 251 led to inactive variants. Amino acids Gln 9, Arg 41, Tyr 76, Arg 111, Asn 170, Tyr 175, and Tyr 211 were also critical for activity, presumably because of their close proximity to the active site, while more peripheral DNA interactions stemming from 13 other positions were of minimal significance. The relative importance of these 27 positions is consistent with evolutionary relationships among DNase I across different species, DNase I-like proteins, and bacterial sphingomyelinases, suggesting a fingerprint for a family of DNase I-like proteins. Furthermore, we found no evidence for a second active site that had been previously implicated in Mn2+-dependent DNA degradation. Finally, we correlated our mutational analysis of human DNase I to that of bovine DNase I with respect to their specific activity and dependence on divalent metal ions.     

Directed mutagenesis of apecific active site residues on Fibrobacter succinogenes 1,3-1,4-beta -D-glucanase significantly affects catalysis and enzyme structural stability

The functional and structural significance of amino acid residues Met(39), Glu(56), Asp(58), Glu(60), and Gly(63) of Fibrobacter succinogenes 1,3-1,4-beta-d-glucanase was explored by the approach of site-directed mutagenesis, initial rate kinetics, fluorescence spectroscopy, and CD spectrometry. Glu(56), Asp(58), Glu(60), and Gly(63) residues are conserved among known primary sequences of the bacterial and fungal enzymes. Kinetic analyses revealed that 240-, 540-, 570-, and 880-fold decreases in k(cat) were observed for the E56D, E60D, D58N, and D58E mutant enzymes, respectively, with a similar substrate affinity relative to the wild type enzyme. In contrast, no detectable enzymatic activity was observed for the E56A, E56Q, D58A, E60A, and E60Q mutants. These results indicated that the carboxyl side chain at positions 56 and 60 is mandatory for enzyme catalysis. M39F, unlike the other mutants, exhibited a 5-fold increase in K(m) value. Lower thermostability was found with the G63A mutant when compared with wild type or other mutant forms of F. succinogenes 1,3-1,4-beta-d-glucanase. Denatured wild type and mutant enzymes were, however, recoverable as active enzymes when 8 m urea was employed as the denaturant. Structural modeling and kinetic studies suggest that Glu(56), Asp(58), and Glu(60) residues apparently play important role(s) in the catalysis of F. succinogenes 1,3-1,4-beta-d-glucanase.     

Activation of methionine by Escherichia coli methionyl-tRNA synthetase

In the present work, we have examined the function of three amino acid residues in the active site of Escherichia coli methionyl-tRNA synthetase (MetRS) in substrate binding and catalysis using site-directed mutagenesis. Conversion of Asp52 to Ala resulted in a 10,000-fold decrease in the rate of ATP-PPi exchange catalyzed by MetRS with little or no effect on the Km's for methionine or ATP or on the Km for the cognate tRNA in the aminoacylation reaction. Substitution of the side chain of Arg233 with that of Gln resulted in a 25-fold increase in the Km for methionine and a 2000-fold decrease in kcat for ATP-PPi exchange, with no change in the Km for ATP or tRNA. These results indicate that Asp52 and Arg233 play important roles in stabilization of the transition state for methionyl adenylate formation, possibly directly interacting with complementary charged groups (ammonium and carboxyl) on the bound amino acid. Primary sequence comparisons of class I aminoacyl-tRNA synthetases show that all but one member of this group of enzymes has an aspartic acid residue at the site corresponding to Asp52 in MetRS. The synthetases most closely related to MetRS (including those specific for Ile, Leu, and Val) also have a conserved arginine residue at the position corresponding to Arg233, suggesting that these conserved amino acids may play analogous roles in the activation reaction catalyzed by each of these enzymes. Trp305 is located in a pocket deep within the active site of MetRS that has been postulated to form the binding cleft for the methionine side chain.(ABSTRACT TRUNCATED AT 250 WORDS)     

Alteration of specific activity and stability of thermostable neutral protease by site-directed mutagenesis.

On the basis of three-dimensional information, many amino acid substitutions were introduced in the thermostable neutral protease (NprM) of Bacillus stearothermophilus MK232 by site-directed mutagenesis. When Glu at position 143 (Glu-143), which is one of the proposed active sites, was substituted for by Gln and Asp, the proteolytic activity disappeared. F114A (Phe-114 to Ala), Y110W (Tyr-110 to Trp), and Y211W (Tyr-211 to Trp) mutant enzymes had higher activity (1.3- to 1.6-fold) than the wild-type enzyme. When an autolysis site, Tyr-93, was replaced by Gly and Ser, the remaining activities of those mutant enzymes were higher than that of the wild-type enzyme.