胆固醇氧化酶PsCO_4异源表达、纯化及酶学性质分析

胆固醇氧化酶专一性催化胆固醇为胆甾-4-烯-3-酮,广泛的应用于临床以及食品加工行业。本论文将来源于Pimelobacter simplex的胆固醇氧化酶PsCO_4,分别转化到大肠杆菌宿主BL21(DE3)、Rosetta(DE3)和C41(DE3)中,在不同温度(15℃、25℃、37℃)及IPTG诱导浓度(0.01mmol/L、0.1mmol/L、0.5mmol/L)下异源表达Ps CO_4。结果表明,转入Rosetta(DE3)菌株的PsCO_4蛋白,在IPTG浓度为0.1mmol/L、15℃下经18h诱导表达,PsCO_4可溶性表达量最高(0.63mg/ml)。异源表达的胆固醇氧化酶PsCO_4最适温度为30℃,最适pH为7.5。通过TLC,GC-MS检测出Ps CO_4催化胆固醇生成胆甾-4-烯-3-酮。以胆固醇和β-谷甾醇、豆甾醇和孕烯醇酮为底物,测定PsCO_4对四种底物的催化反应动力学参数,胆固醇k_(cat)/K_m为0.08s~(-1)·μM~(-1)分别高于β-谷甾醇(0.04s~(-1)·μM~(-1))、豆甾醇(0.005s~(-1)·μM~(-1))和孕烯醇酮(0.02s~(-1)·μM~(-1))。     

甲基丙二酰辅酶A 变位酶表达载体的构建及初步表达

目的:克隆表达甲基丙二酰辅酶A变位酶(MCM)蛋白,为进一步研究相关基因突变对功能的影响机制奠定基础。方法:自人外周血淋巴细胞中提取总RNA、逆转录,并与pET32a构建融合蛋白原核表达载体;优化蛋白表达诱导条件;经SDS-PAGE、WesternBlot检测目的蛋白的表达。结果:经酶切鉴定并经测序证实获得全长2210bp的甲基丙二酰辅酶A变位酶基因(MUT),并成功构建融合蛋白原核表达载体,SDS-PAGE在102 kDa处获得目的条带,Western Blot检测确定为MCM表达蛋白。结论:成功克隆表达出MCM表达蛋白。     

热带假丝酵母长链二(脂)酰辅酶A合成酶的形成及性质

热带假丝酵母(Candida tyopicalis)具有不同碳链的二(脂)酰CoA合成酶的活力,原始菌No．1230的十二二酰CoA合成酶的活性较其突变株U3-21。高近一倍。生长碳源对酶的形成有一定的影响。十二二酰CoA合成酶需有ATP、CoASH才显示活性。酶作用的最适pH在6—8,最适温度为30℃。该酶耐热性极差,50℃,5分钟酶活全部丧失。ADP、AMP、KF、Zn2+ 及 8-羟基喹啉、2,4-二硝基苯酚、高浓度的EDTA和尿素对酶活性有抑制作用。     

硬脂酰辅酶A去饱和酶与脂代谢调控

硬脂酰辅酶A去饱和酶（stearoyl-coenzyme A desaturase,SCD）是催化饱和脂酰辅酶A生成单不饱和脂酰辅酶A的关键酶,在不同的组织中有多种亚型分布。高热量饮食、运动、激素等因素均影响SCD的基因表达水平。对SCD蛋白表达水平和活性的调控会直接影响生物体内饱和脂肪酸（saturated fatty acid,SFA）与单不饱和脂肪酸（monounsaturated fatty acid,MUFA）的比例,从而进一步影响整个机体的脂质代谢,进而与细胞应激反应及胰岛素敏感性直接相关。因此,SCD逐渐成为代谢疾病治疗的一个潜在的靶分子。     

长链脂酰辅酶A合成酶家族与恶性肿瘤

脂肪酸代谢紊乱容易导致癌症的发生。长链脂酰辅酶A合成酶家族(long chain acyl-coenzyme A synthetase family,ACSLs)负责激活长链脂肪酸,在脂肪酸代谢中发挥重要作用。但在癌细胞中,其调控作用经常被解除,细胞内脂肪酸的分布、种类和数量发生改变,进而导致癌症和其他代谢性疾病的发生。ACSLs 在哺乳动物中包括5种亚型,分别为ACSL1、3、4、5和6。ACSL1在甘油三脂的合成和分配中发挥重要作用;ACSL3有助于脂滴的形成,脂滴对维持脂质稳态具有重要作用;ACSL4的表达与类固醇激素相关,在铁死亡途径中发挥重要作用;ACSL5可以催化外源性脂肪酸的代谢,但不能催化从头合成脂肪酸的代谢;ACSL6在脑内的脂肪酸代谢及生殖器官中精子发生和卵巢功能维持等方面发挥重要作用。ACSLs的调控因子包括转录因子、共激活因子、激素受体、蛋白激酶和小的非编码RNA等。它们通过介导脂肪酸代谢,广泛参与线粒体介导的能量代谢,内质网应激和肿瘤炎性微环境等。此外,ACSLs还作为独立预后因素,成为各种癌症临床诊断和治疗的生物标志物和治疗靶点。近年来,越来越多的研究表明,ACSL家族在癌症的发生发展进程中发挥重要作用。本文从ACSL基因家族,ACSLs与恶性肿瘤及基于ACSLs脂代谢的肿瘤治疗方面进行阐述,为后续ACSL基因家族的研究及肿瘤的靶向治疗提供理论依据和候选分子靶标。     

琥珀酰辅酶A转移酶的表达纯化及抗体制备

目的:琥珀酰辅酶A转移酶(SCOT)是酮体代谢过程中的关键限速酶,此酶缺陷多由SCOT基因突变引起,患者多有酮症酸中毒表现。为了进一步研究SCOT的功能,采用原核表达系统表达并纯化重组SCOT,制备SCOT多克隆抗体。方法:选择蛋鸡、肉鸡模式生物为研究对象,通过生物信息学对其抗原性和属间同源性进行分析,通过RT-PCR从鸡的骨骼肌cDNA中扩增了SCOT基因N端半长片段,克隆到表达载体pET28b中,在大肠杆菌BL21(DE3)中诱导表达,并用镍离子螯合柱(Ni-NTA)纯化重组SCOT;用纯化的重组SCOT免疫小鼠后得到多克隆抗体。结果:Western印迹表明,制备的SCOT抗体具有较高的特异性,可特异性识别鸡的SCOT蛋白,同时可特异性识别小鼠和人的相应SCOT蛋白。结论:SCOT多克隆抗体的制备为后续在鸡、鼠和人中研究SCOT基因提供基础。     

聚苹果酸聚合途径中苹果酰辅酶A连接酶基因的克隆、表达及酶学性质

【目的】研究出芽短梗霉聚苹果酸聚合途径中苹果酰辅酶A连接酶基因及其酶学特性。【方法】通过设计兼并引物,采用IPCR技术从出芽短梗霉CCTCC M2012223的基因组中扩增得到苹果酰辅酶A连接酶基因的cDNA全长序列,构建表达载体,通过大肠杆菌异源表达,Ni-NTA柱层析纯化酶蛋白,分析其酶学特性。【结果】获得苹果酰辅酶A连接酶基因序列全长为1498 bp,编码440 aa,含有4个外显子和3个内含子。该重组酶最适反应温度为25℃,最适反应pH值为8.0,高浓度底物ATP明显对酶活性具有抑制作用,单体选择性表明对底物草酸、草酰乙酸、丁酸、丙二酸也具有很好催化活性。【结论】成功从出芽短梗霉CCTCC M2012223中克隆获得聚苹果酸聚合途径的苹果酰辅酶A连接酶基因,为聚苹果酸聚合途径解析及新型可降解材料创制奠定基础。     

一种新型亮氨酸5-羟化酶NmLEH的异源表达、纯化及酶学性质分析 *

羟基化氨基酸是一种新型氨基酸衍生物,可广泛用作化工材料的前体物及医药合成的中间体。将来源于Nostoc minutum的新型L-亮氨酸5-羟化酶 (NmLEH) 通过重组质粒在大肠杆菌中异源表达。结果表明,在BL21(DE3) 宿主细胞中,诱导温度为25℃,IPTG诱导浓度为0.5mmol/L,诱导10h时,蛋白质表达量最高 (0.45mg/ml);通过Ni-亲和层析和凝胶过滤层析两步分离纯化获得了高度纯化的重组NmLEH蛋白;对NmLEH的酶学性质进行了表征,该酶的最适反应温度为25℃,最适pH 为7.5,在pH 7.0~9.0较为稳定,最适底物为亮氨酸和甲硫氨酸;同源序列分析表明NmLEH属于亚铁和α-酮戊二酸依赖性双加氧酶家族[Fe(II)/αKG-Dos],并预测了该酶的保守催化活性位点(H150、D152、H236);通过同源建模得到了该蛋白质的模拟结构,分析了该蛋白质催化活性中心的形成机制。     

油茶脂酰辅酶A脱氢酶基因的克隆与表达分析

以国审油茶(Camellia oleifera)良种‘华硕’种子为材料,在已构建的转录组和表达谱数据库基础之上,采用RACE技术,克隆获得油茶脂酰辅酶A脱氢酶基因的全长c DNA序列,命名为Co ACAD(基因登录号KJ910338)。该基因c DNA全长为2702 bp,含有2487 bp的开放读码框,编码828个氨基酸,分子量为92.4113 k D,理论等电点p I为8.47,具有2个比较明显的跨膜区和酪氨酸蛋白激酶活性位点LVHGDFRIDNLVF,存在5个亚结构域;在Co ACAD基因c DNA全长序列的基础上构建表达载体,其中原核表达载体在宿主细胞BL21(DE3)中成功诱导表达,获得表观分子量约为93 k D的目的蛋白;实时荧光定量PCR分析表明,Co ACAD基因在果实膨大期和成熟期上调表达,预示着Co ACAD基因可能在种子发育过程中参与能量供应过程的调控。     

脂酰辅酶A长链合成酶3及其相关疾病

脂滴(lipid droplets)是细胞内脂质贮存和调节细胞脂质稳态的重要细胞器,其表面具有多种脂滴相关蛋白质。长链酰基辅酶A合成酶家族的成员脂酰辅酶A长链合成酶3(acyl CoA long chain synthetase 3,ACSL3)即脂滴相关蛋白质的一种,也是生物合成过程中必需的酶之一。ACSL3广泛分布于大多数细胞中的脂滴表面,其在脂滴的合成、自噬的调节和细胞铁死亡等多种病理生理过程中发挥着不同的作用。此外,多项研究表明,ACSL3还广泛参与到多种疾病的发生发展,包括动脉粥样硬化、非酒精性脂肪肝病、糖尿病和肿瘤等。当前,国内对ACSL3的研究相对集中于ACSL3与动物育种和生长的关系,而对ACSL3在脂质代谢中的作用机制及其与疾病的关系鲜有报道。本文基于国内外对ACSL3的研究,对该基因的结构、在细胞脂代谢中的作用机制及其相关疾病进行归纳,进一步探究ACSL3在脂滴的合成、自噬、铁死亡过程中的作用,为防治动脉粥样硬化、非酒精性脂肪肝病、糖尿病(glucose)等多种ACSL3相关疾病提供新的理论依据。     

Alteration of substrate specificity of valine dehydrogenase from Streptomyces albus

The catabolism of branched chain amino acids, especially valine, appears to play an important role in furnishing building blocks for macrolide and polyether antibiotic biosyntheses. To determine the active site residues of ValDH, we previously cloned, partially characterized, and identified the active site (lysine) of Streptomyces albus ValDH. Here we report further characterization of S. albus ValDH. The molecular weight of S. albus ValDH was determined to be 38 kDa by SDS-PAGE and 67 kDa by gel filtration chromatography indicating that the enzyme is composed of two identical subunits. Optimal pHs were 10.5 and 8.0 for dehydrogenase activity with valine and for reductive amination activity with -ketoisovaleric acid, respectively. Several chemical reagents, which modify amino-acid side chains, inhibited the enzyme activity. To examine the role played by the residue for enzyme specificity, we constructed mutant ValDH by substituting alanine for glycine at position 124 by site-directed mutagenesis. This residue was chosen because it has been considered to be important for substrate discrimination by phenylalanine dehydrogenase (PheDH) and leucine dehydrogenase (LeuDH). The Ala-124–Gly mutant enzyme displayed lower activities toward aliphatic amino acids, but higher activities toward L-phenylalanine, L-tyrosine, and L-methionine compared to the wild type enzyme suggesting that Ala-124 is involved in substrate binding in S. albus ValDH.     

Probing the catalytic roles of n2-site glutamate residues in Escherichia coli glutamine synthetase by mutagenesis.

The contribution of metal ion ligand type and charge to catalysis and regulation at the lower affinity metal ion site (n2 site) of Escherichia coli glutamine synthetase (GS) was tested by mutagenesis and kinetic analysis. The 2 glutamate residues at the n2 site, E129 and E357, were changed to E129D, E129H, E357H, E357Q, and E357D, representing conservative and nonconservative alterations. Unadenylylated and fully adenylylated enzyme forms were studied. The Mn(2+)-KD values, UV-cis and fluorescence emission properties were similar for all mutants versus WTGS, except E129H. For kinetic determinations with both Mn2+ and Mg2+, nonconservative mutants (E357H, E129H, E357Q) showed lower biosynthetic activities than conservative mutants (E129D, E357D). Relative to WTGS, all the unadenylylated Mn(2+)-activated enzymes showed reduced kcat/Km values for ATP (> 7-fold) and for glutamate (> 10-fold). Of the unadenylylated Mg(2+)-activated enzymes, only E129D showed kinetic parameters competitive with WTGS, and adenylylated E129D was a 20-fold better catalyst than WTGS. We propose the n2-site metal ion activates ADP for departure in the phosphorylation of glutamate by ATP to generate gamma-glutamyl phosphate. Alteration of the charge density at this metal ion alters the transition-state energy for phosphoryl group transfer and may affect ATP binding and/or ADP release. Thus, the steady-state kinetic data suggest that modifying the charge density increases the transition-state energies for chemical steps. Importantly, the data demonstrate that each ligand position has a specialized spatial environment and the charge of the ligand modulates the catalytic steps occurring at the metal ion. The data are discussed in the context of the known X-ray structures of GS.     

Alteration of a single amino acid changes the substrate specificity of dihydroflavonol 4-reductase

Many plant species exhibit a reduced range of flower colors due to the lack of an essential gene or to the substrate specificity of a biosynthetic enzyme. Petunia does not produce orange flowers because dihydroflavonol 4-reductase (DFR) from this species, an enzyme involved in anthocyanin biosynthesis, inefficiently reduces dihydrokaempferol, the precursor to orange pelargonidin-type anthocyanins. The substrate specificity of DFR, however, has not been investigated at the molecular level. By analyzing chimeric DFRs of Petunia and Gerbera, we identified a region that determines the substrate specificity of DFR. Furthermore, by changing a single amino acid in this presumed substrate-binding region, we developed a DFR enzyme that preferentially reduces dihydrokaempferol. Our results imply that the substrate specificity of DFR can be altered by minor changes in DFR.     

Structural principles of the wide substrate specificity of <Emphasis Type="Italic">Thermoactinomyces vulgaris</Emphasis> carboxypeptidase T. reconstruction of the carboxypeptidase B primary specificity pocket

Site-directed mutagenesis in the active site of Thermoactinomyces vulgaris carboxypeptidase T (CpT), which is capable of hydrolyzing both hydrophobic and positively charged substrates, resulted in five mutants: CpT1 (A243G), CpT2 (D253G/T255D), CpT3 (A243G/D253G/T255D), CpT4 (G207S/A243G/D253G/T255D), and CpT5 (G207S/A243G/T250A/D253G/T255D). These mutants step-by-step reconstruct the primary specificity pocket of carboxypeptidase B (CpB), which is capable of cleaving only positively charged C-terminal residues. All of the mutants retained the substrate specificity of the wild-type CpT. Based on comparison of three-dimensional structures of CpB and the CpT5 model, it was suggested that the lower affinity of CpT5 for positively charged substrates than the affinity of CpB could be caused by differences in nature and spatial location of Leu247 and Ile247 and of His68 and Asp65 residues in CpT and CpB, respectively, and also in location of the water molecule bound with Ala250. An additional hydrophobic region was detected in the CpT active site formed by Tyr248, Leu247, Leu203, Ala243, CH3-group of Thr250, and CO-groups of Tyr248 and Ala243, which could be responsible for binding hydrophobic substrates. Thus, notwithstanding the considerable structural similarity of CpT and pancreatic carboxypeptidases, the mechanisms underlying their substrate specificities are different.     

Purification, characterization, and mass spectrometric sequencing of a medium chain acyl-CoA synthetase from mouse liver mitochondria and comparisons with the homologues of rat and bovine

Medium chain acyl-CoA synthetases catalyze the first reaction of amino acid conjugation of many xenobiotic carboxylic acids and fatty acid metabolism. This paper reports studies on purification, characterization, and the partial amino acid sequence of mouse liver enzyme. The medium chain acyl-CoA synthetase was isolated from mouse liver mitochondria. The purified enzyme catalyzes this reaction not only for straight medium chain fatty acids but also for aromatic and arylacetic acids. Maximal activity was found with hexanoic acid. High activities were obtained with benzoic acid having methyl, pentyl, and methoxy groups in the para- or meta-positions of the benzene ring. However, the enzyme was less active with valproic acid and ketoprofen. Salicylic acid exhibited no activity. The medium chain acyl-CoA synthetases from mouse and bovine liver mitochondria were subjected to in-gel tryptic digestion, followed by LC-MS/MS sequence analysis. The amino acid sequence of each tryptic peptide of mouse liver mitochondrial medium chain acyl-CoA synthetase differed from that from bovine liver mitochondria only in one or two amino acids. LC-MS/MS analysis provided the information about these differences in amino acid sequences. In addition, we compared the properties of this protein with the homologues from rat and bovine.     

酿酒酵母表达和纯化功能性的铁载体合成蛋白PchE

【目的】利用酿酒酵母表达系统,通过乙醇脱氢酶启动子异源表达细菌源的铁载体合成蛋白PchE,并与来源于枯草芽孢杆菌的泛酰化酶Sfp同宿主共表达,探索真核表达体系表达具有生化活性的细菌源蛋白。【方法】从大肠杆菌BAP1染色体上扩增sfp基因,将pchE基因及串联的pchE与sfp基因分别构建到酵母-大肠杆菌穿梭质粒pXW55中,各自转化酿酒酵母BJ5464-npg A表达,经过亲和层析和离子交换层析纯化蛋白,利用HPLC检测细菌源与酵母源表达的PchE在体外重构生化反应中的催化活性。【结果】利用酿酒酵母表达系统可以获得高纯度的原核蛋白PchE。真菌源的泛酰化基因NpgA和细菌源的Sfp,均可泛酰化修饰PchE,合成中间产物HPT-Cys。【结论】在酿酒酵母Saccharomyces cerevisiae BJ5464-npgA表达系统中,首次证明真菌源的泛酰化基因NpgA和细菌源的Sfp,均可泛酰化修饰细菌源的非核糖体肽合酶。比较酵母和细菌宿主的目标蛋白表达,证明酵母表达的巨大蛋白PchE的纯度更高,非特异性条带减少,推测酵母宿主可能更适合表达纯化功能性的巨型蛋白质。     

Engineering the substrate specificity of Escherichia coli asparaginase. II. Selective reduction of glutaminase activity by amino acid replacements at position 248

The use of Escherichia coli asparaginase II as a drug for the treatment of acute lymphoblastic leukemia is complicated by the significant glutaminase side activity of the enzyme. To develop enzyme forms with reduced glutaminase activity, a number of variants with amino acid replacements in the vicinity of the substrate binding site were constructed and assayed for their kinetic and stability properties. We found that replacements of Asp248 affected glutamine turnover much more strongly than asparagine hydrolysis. In the wild-type enzyme, N248 modulates substrate binding to a neighboring subunit by hydrogen bonding to side chains that directly interact with the substrate. In variant N248A, the loss of transition state stabilization caused by the mutation was 15 kJ mol(-1) for L-glutamine compared to 4 kJ mol(-1) for L-aspartic beta-hydroxamate and 7 kJ mol(-1) for L-asparagine. Smaller differences were seen with other N248 variants. Modeling studies suggested that the selective reduction of glutaminase activity is the result of small conformational changes that affect active-site residues and catalytically relevant water molecules.     

海因酶热稳定性及底物特异性研究进展

海因酶是在微生物中广泛分布的能水解5-取代海因衍生物制备光学纯氨基酸的关键生物催化剂,在各种氨基酸的酶法生产中具有良好的应用前景。着重概述了海因酶的热稳定性、底物特异性研究及应用,并讨论了其发展方向。     

Leu254 residue and calcium ions as new structural determinants of carboxypeptidase T substrate specificity

New determinants of Thermoactinomyces vulgaris carboxypeptidase T (CPT) substrate specificity--structural calcium ions and Leu254 residue--were found by means of steady-state kinetics and site-directed mutagenesis. The removal of calcium ions shifted the selectivity profile of hydrolysis of tripeptide substrates with C-terminal Leu, Glu, and Arg from 64/1.7/1 to 162/1.3/1. Substitution of the hydrophobic Leu254 in CPT for polar Asn did not change hydrolysis efficiency of substrates with C-terminal Leu and Arg, but resulted in more than 28-fold decrease in activity towards the substrate with C-terminal Glu. It is shown that the His68 residue is not a structural determinant of CPT specificity.