基因工程手段提高磷脂酰丝氨酸合成酶活性的研究

为了提高目的蛋白磷脂酰丝氨酸合成酶(PSS)的表达,使用rTaq酶从E coli K12总DNA中PCR扩增获得磷脂酰丝氨酸合成酶基因片段,将其重组于高效表达载体pET28b质粒,转入相应表达菌株进行表达,收集菌体超声破碎获得含PSS的粗酶液,使用两相反应体系进行生物转化,HPLC-ELSD手段进行酶活检测。结果显示,重组菌株中PSS的酶活力比对照有所提高,同时获得酶活力提高的突变基因pssE210G。将突变基因重组于更高效的表达载体pBAD-MCS,转入相应宿主菌株表达。结果显示E.coli TOP10(pBAD-MCS-pss)表达的酶活性明显优于E.coli BL21(pET28b-pss)中表达的酶活性。以上实验结果表明,将目的基因重组于高效表达质粒有助于提高酶活力;组合到不同的表达质粒,酶活提高程度不同;磷脂酰丝氨酸合成酶基因第73位氨基酸发生突变,对其酶结构和酶活力有直接的影响。     

磷脂酰丝氨酸合成酶基因的克隆及在枯草芽孢杆菌中的表达

应用 PCR技术从 Escherichia coli K12 Sgal- (ExPASy P23830) 中扩增到大小为 1350bp编码磷脂酰丝氨酸合成酶的 DNA片段,将其插入枯草芽孢杆菌诱导型表达载体 pBES,获得重组质粒 pBES-pss后转化 Bacillus subtilis DB104。经蔗糖诱导后,该磷脂酰丝氨酸合成酶在 Bacillus subtilis DB104 (pBES-pss)中获得胞外分泌表达,SDS-PAGE分析发现目的蛋白分子量约为 52kDa,酶联比色法检测酶活力为 1.50U/mL,提高了磷脂酰丝氨酸合成酶的表达产量,为工业化发酵生产磷脂酰丝氨酸合成酶奠定了良好的基础。     

阿维链霉菌来源的磷脂酰丝氨酸合成酶基因的克隆及其在毕氏酵母中的异源表达

本文旨在构建阿维链霉菌(Streptomyces avermitilis)来源的磷脂酰丝氨酸合成酶基因(pss)的重组质粒,研究其在毕氏酵母中的异源分泌型表达。利用PCR技术克隆阿维链霉菌来源的pss基因,再通过电转化方法将重组质粒pOG-01转入毕氏酵母KM71中,构建重组工程菌KP1。实验结果表明,阿维链霉菌来源的磷酯酰丝氨酸合成酶基因在毕氏酵母KM71中成功表达,2 mL菌体上清催化50 mmol/L卵磷脂,转酯反应的转化率为58%,酶活为4.83 U/mL。     

PSS定点突变及酶活研究

磷脂酰丝氨酸可在磷脂酰丝氨酸合成酶(PSS)催化下由磷脂酰胆碱和L-丝氨酸生成。通过生物信息学手段对磷脂酰丝氨酸合成酶蛋白质结构进行解析和研究分析,获得2个可突变位点F139和P272,通过Overlap PCR法进行定点突变,测定突变序列,并进行酶活测定。结果显示,PSS位点F139突变为L139、M139,位点P272突变为A272,能提高酶活力,说明蛋白质结构解析结合氨基酸定点突变技术,可以改善重组酶的活力。     

氨基脱氧分支酸合成酶对Corynebacterium glutamicum SYPS-062积累L-丝氨酸的影响

为阐明氨基脱氧分支酸合成酶(ADC合成酶)在Corynebacterium glutamicum SYPS-062体内积累L-丝氨酸过程中的作用,通过交叉PCR以及同源重组的方法敲除叶酸途径关键酶ADC合成酶的编码基因pabAB,构建了叶酸缺陷型菌株Corynebacterium glutamicum SYPS-062△pabAB,同时构建pabAB基因增强表达重组菌C.glutamicum SYPS-062(pJC Ⅰ-pabAB).分别考察了ADC合成酶对菌株生长的影响、对L-丝氨酸降解途径关键酶丝氨酸羟甲基转移酶(SHMT)的影响以及其对L-丝氨酸积累的影响.结果表明,与出发菌株相比,增强表达基因pabAB重组菌的ADC合成酶的酶活力提高了33%.SHMT酶的酶活力提高了30%,其最大比生长速率(μm)提高了48%,单位细胞产酸率(Yp/x)降低了36.2%;而敲除基因pabAB重组菌的ADC合成酶的酶活力降低了61%.SHMT酶的酶活力降低了20%,最大比生长速率降低了32%,单位细胞产酸率提高了12%.     

磷脂对乙酰胆碱酯酶的稳定性及磷酸化作用的影响

采用重组的方法,磷脂能显著地提高纯化的黄姑鱼肌肉乙酰胆碱酯酶在水溶液中保存的稳定性。牛脑磷脂酰丝氨酸及牛脑磷脂酰胆碱重组酶,在4℃条件下保存,皆有比对照更高的稳定性。酶与牛脑磷脂酰胆碱重组后,再分别于室温及37℃放置50天,其活力不下降。而对照的活力分别下降为重组前活力的1/2及1/4。在某些稀释条件下,牛脑及牛脊髓磷脂酰丝氨酸重组酶的活性迅速下降。稀释液中钙离子的存在,能阻止这种磷脂对酶的抑制作用。而磷脂酰胆碱重组酶及对照酶皆无此种在稀释条件下的活力迅速下降的现象。牛脑磷脂酰胆碱与酶的重组还能提高对氧磷与酶的反应活性。该重组酶与对氧磷反应的双分子速度常数高达9.0×10~8M~(-1)分~(-1)。因此,此种磷脂酰胆碱重组酶是酶分析法测定极低浓度有机磷化合物的一种较好的酶源。     

磷脂对乙酰胆碱酯酶的稳定性及磷酸化作用的影响

采用重组的方法,磷脂能显著地提高纯化的黄姑鱼肌肉乙酰胆碱酯酶在水溶液中保存的稳定性。牛脑磷脂酰丝氨酸及牛脑磷脂酰胆碱重组酶,在4℃条件下保存,皆有比对照更高的稳定性。酶与牛脑磷脂酰胆碱重组后,再分别于室温及37℃放置50天,其活力不下降。而对照的活力分别下降为重组前活力的1/2及1/4。在某些稀释条件下,牛脑及牛脊髓磷脂酰丝氨酸重组酶的活性迅速下降。稀释液中钙离子的存在,能阻止这种磷脂对酶的抑制作用。而磷脂酰胆碱重组酶及对照酶皆无此种在稀释条件下的活力迅速下降的现象。牛脑磷脂酰胆碱与酶的重组还能提高对氧磷与酶的反应活性。该重组酶与对氧磷反应的双分子速度常数高达9.0×10~8M~(-1)分~(-1)。因此,此种磷脂酰胆碱重组酶是酶分析法测定极低浓度有机磷化合物的一种较好的酶源。     

重组磷脂酰丝氨酸合成酶的分离纯化及酶学性质研究

利对重组枯草芽孢杆菌(pBES-pss)表达的磷脂酰丝氨酸合成酶进行分离纯化及酶学性质研究.pBES-pss发酵后的粗酶液经硫酸铵盐析、中空纤维膜除盐浓缩、SP-Sepharose HP离子交换层析和Sephadex G-75凝胶层析,基本获得电泳纯的重组磷脂酰丝氨酸合成酶,比活力可达13.62 U/mg,分子量约为53 kD.酶学性质研究表明,该酶催化卵磷脂水解反应的最适pH8.0,最适温度为35℃.稳定性研究表明:该酶在pH 6.5～9.5 区间和低于45℃温度下稳定.表面活性剂及金属离子对该酶水解活性的影响结果表明,SDS、Tween20、Tween80对该酶有抑制作用,Triton X-100对该酶有增强作用;Mg2+、Zn2+、K+对该酶有抑制作用,Ca2+、Mn2+和EDTA对该酶有增强作用.     

异戊二烯合成酶(IspS)在大肠杆菌中的表达及其产异戊二烯的研究

将来源于银白杨的异戊二烯合成酶基因按照大肠杆菌密码子偏爱性进行优化,克隆到表达载体pACYCDu-et-1上,在大肠杆菌BL21(DE3)中异源表达,采用镍柱亲和层析纯化重组蛋白并测定其异戊二烯合成酶活性,通过摇瓶发酵实验对重组菌产异戊二烯进行进一步研究。结果显示:银白杨异戊二烯合成酶在大肠杆菌中能够高效表达,经过镍柱纯化后,电泳检测到特异性表达条带;该重组异戊二烯合成酶能够催化异戊二烯的合成,重组菌的异戊二烯产量可达到60μg/L。     

布氏锥虫苯丙氨酰-tRNA合成酶在大肠杆菌中的克隆、表达、纯化及活性测定

苯丙氨酰-tRNA合成酶是布氏锥虫蛋白合成过程中的一类重要酶,以其为靶点的抑制剂可能发展成为新一代的抗锥虫药物,但此前并没有分离锥虫苯丙氨酸-tRNA合成酶的报道。本研究用大肠杆菌成功克隆表达并纯化了布氏锥虫苯丙氨酰-tRNA合成酶并进行了活性测定。首先通过PCR方法从布氏锥虫细胞基因组中分别扩增出苯丙氨酰-tRNA合成酶的α亚基、β亚基的基因,依次克隆入pCOLADuet共表达载体,然后在大肠杆菌BL21(DE3)RIPL中进行了成功表达,并采用Ni-Bind亲和层析对其进行了纯化,最后用免疫印迹进行了鉴定。此外还采用放射性同位素方法进行了酶活性测定,这为下一步进行布氏锥虫苯丙氨酰-tRNA合成酶抑制物的设计和体外筛选奠定了良好的基础。     

Production of D-p-hydroxyphenylglycine by N-carbamoyl-D-amino acid amidohydrolase-overproducing Escherichia coli strains.

The N-carbamoyl-D-amino acid amidohydrolase (D-carbamoylase) gene from Agrobacterium radiobacter NRRL B11291 has been successfully cloned and expressed in Escherichia coli. Subcloning of the D-carbamoylase gene into different types of vectors and backgrounds of E. coli strains showed that the optimal expression level of D-carbamoylase was achieved in a ColE1-derived plasmid with a 150-fold increase in specific enzyme activity compared to that in a pSC101-derived plasmid. In addition, the recombinant plasmids were very stable in the E. coli strain ATCC11303 but not in JCL1258 tested here. Employing the recombinant E. coli strain DH5alpha/pAH61 for D-p-hydroxyphenylglycine production showed that the cell was capable of transforming N-carbamoyl-D-hydroxylphenylglycine to D-p-hydroxyphenylglycine with a molar conversion yield of 100% and a production rate of 1.9 g/(L h). In comparison with A. radiobacter NRRL B11291, this productivity approximates a 55-fold increase in D-hydroxyphenylglycine production. This result suggests the potential application of recombinant E. coli strains for the transformation reaction.     

Intracellular distribution of enzymes of phospholipid metabolism in several gram-negative bacteria.

Cell-free extracts of Salmonella typhimurium, Serratia marcescens, Enterobacter aerogenes, and Micrococcus cerificans contained the following enzymatic activities related to phospholipid metabolism: cytidine 5'-diphospho-1,2-diacyl-sn-glycerol (CDP-diglyceride):l-serine O-phosphatidyltransferase (phosphatidylserine synthase), phosphatidylserine decarboxylase, CDP-diglyceride:sn-glycero-3-phosphate phosphatidyltransferase (phosphatidylglycerophosphate synthase), phosphatidylglycerophosphate phosphatase, and CDP-diglyceride hydrolase. The intracellular distribution of these enzymatic activities as determined by sucrose density gradient centrifugation of cell-free extracts was shown to be similar in each species investigated. The phosphatidylserine decarboxylase, phosphatidylglycerophosphate synthase, and CDP-diglyceride hydrolase activities were all associated with the cell envelope fraction, whereas the phosphatidylserine synthase activity was associated mainly with the ribosomal fraction. These enzymatic activities are comparable and have an intracellular distribution similar to those found in Escherichia coli cell-free extracts. Therefore, the pathways established for phospholipid biosynthesis in E. coli can also account for the synthesis of the major phospholipids (phosphatidylethanolamine and phosphatidylglycerol) in several other gram-negative organisms. In addition, the unusual ribosomal association of the phosphatidylserine synthase from E. coli (Raetz and Kennedy, J. Biol. Chem. 247:2008-2014, 1972) appears to be a general property for this activity in several other bacterial species.     

新型抗结核分枝杆菌药物筛选模型的建立

为建立基于酶水平和细胞水平的新型抗结核分枝杆菌（Mycobacterium tuberculosis）药物的筛选模型,以M.tuberculosis H37Rv基因组DNA为模板,PCR特异性扩增异柠檬酸裂解酶（ICL）基因,构建表达载体,在E.coli BL21（DE3）中高效表达,使用N i2＋亲和层析柱纯化重组ICL,检测其活性。优化ICL酶反应条件,考察待筛选样品溶剂对酶活性的影响,建立ICL抑制剂酶水平筛选模型;考察与优化耻垢分枝杆菌（Mycobacterium smegma）在以乙酸盐为唯一碳源的培养基中的生长状况,建立基于M.sm egma的乙醛酸代谢途径抑制剂的细胞水平筛选模型;利用上述2种筛选模型对1 060种可能具有拮抗活性的微生物代谢样品进行初筛和复筛,两者筛选结果正相关性较好。     

不同来源的谷氨酸棒杆菌氨基脱氧分支酸合成酶的活性分析

分别以高产L-丝氨酸的谷氨酸棒杆菌(Corynebacterium glutamicum)SYPS-062与模式菌株谷氨酸棒杆菌(Corynebacterium glutamicum) ATCC 13032的基因组DNA为模板,运用PCR技术扩增出氨基脱氧分支酸合成酶(ADC synthase)的编码基因pabAB。实验结果表明：来源于SYPS-062和ATCC 13032的pabAB片段全长均为1863bp,编码620个氨基酸。两片段存在16个碱基的差异,引起了7个氨基酸的突变。将pabAB连接表达载体pET-28a(+),构建表达质粒pET-28a-pabAB,并转化E.coli BL21(DE3),在IPTG诱导下,E.coli BL21(DE3)(pET-28a-pabAB)高效表达分子量约为67kDa的可溶性蛋白。表达产物带有His-tag标记,选用Ni柱对表达产物进行纯化,纯化后酶活测定结果表明,来源于SYPS-062氨基脱氧分支酸合成酶的比酶活低于ATCC 13032达46.6%。     

枯草芽孢杆菌C-36内切葡聚糖酶基因的克隆及其在大肠杆菌中融合表达

以自行分离筛选出的天然枯草芽孢杆菌（Bacillus subtilis）C-36的染色体DNA为模板,PCR扩增得到含有内切葡聚糖酶基因的DNA片段,将其克隆到pMD-18T载体中,序列分析表明,克隆得到的DNA片段全长1602bp,编码一个含有499个氨基酸的多肽。与其他芽孢杆菌内切葡聚糖酶基因序列比对,其核苷酸同源率为90％～93％,其编码的氨基酸序列的同源性在90％～98％,已将此基因注册GenBank（DQ782954）。将含内切葡聚糖酶基因的重组克隆质粒进行亚克隆,用Kpn I和EcoR I双酶切后,与相同酶切的表达载体pET-32a相连接,并导入大肠杆菌BL21中表达。蛋白质电泳实验结果表明在6．47×10^4处有表达蛋白带。经测定表达蛋白比酶活力达99．02U／mL,为出发菌C-36（63．78U／mL）的1．55倍。     

Solubilization of microsomal-associated phosphatidylserine synthase and phosphatidylinositol synthase from Saccharomyces cerevisiae

Membrane-associated cytidine 5'-diphospho-1,2-diacyl-sn-glycerol (CDP-diacylglycerol):L-serine O-phosphatidyltransferase (phosphatidylserine synthase, EC2.7.8.8.) and CDP-diacylglycerol:myo-inositol phosphatidyltransferase (phosphatidylinositol synthase, EC 2.7.8.11) were solubilized from the microsomal fraction of Saccharomyces cerevisiae. A variety of detergents were examined for their ability to release phosphatidylserine synthase and phosphatidylinositol synthase activities from the microsome fraction. Both enzymes were solubilized from the microsome fraction with Renex 690 in yield over 80% with increase to specific activity of 1.6-fold. Both solubilized enzymatic activities were dependent on manganese ions and Triton X-100 for maximum activity. The pH optimum for each reaction was 8.0. The apparent Km values for CDP-diacylglycerol and serine for the phosphatidylserine synthase reaction were 0.1 and 0.25 mM, respectively. The apparent Km values for CDP-diacylglycerol and inositol for the phosphatidylinositol synthase reaction were 70 microM and 0.1 mM, respectively. Thioreactive agents inhibited both enzymatic activities. Both solubilized enzymatic activities were thermally inactivated at temperatures above 30 degrees C.     

CDP-2,3-Di-O-geranylgeranyl-sn-glycerol:L-serine O-archaetidyltransferase (archaetidylserine synthase) in the methanogenic archaeon Methanothermobacter thermautotrophicus

CDP-2,3-di-O-geranylgeranyl-sn-glycerol:L-serine O-archaetidyltransferase (archaetidylserine synthase) activity in cell extracts of Methanothermobacter thermautotrophicus cells was characterized. The enzyme catalyzed the formation of unsaturated archaetidylserine from CDP-unsaturated archaeol and L-serine. The identity of the reaction products was confirmed by thin-layer chromatography, fast atom bombardment-mass spectrum analysis, and chemical degradation. The enzyme showed maximal activity in the presence of 10 mM Mn2+ and 1% Triton X-100. Among various synthetic substrate analogs, both enantiomers of CDP-unsaturated archaeols with ether-linked geranylgeranyl chains and CDP-saturated archaeol with ether-linked phytanyl chains were similarly active toward the archaetidylserine synthase. The activity on the ester analog of the substrate was two to three times higher than that on the corresponding ether-type substrate. The activity of D-serine with the enzyme was 30% of that observed for L-serine. A trace amount of an acid-labile, unsaturated archaetidylserine intermediate was detected in the cells by a pulse-labeling experiment. A gene (MT1027) in M. thermautotrophicus genome annotated as the gene encoding phosphatidylserine synthase was found to be homologous to Bacillus subtilis pssA but not to Escherichia coli pssA. The substrate specificity of phosphatidylserine synthase from B. subtilis was quite similar to that observed for the M. thermautotrophicus archaetidylserine synthase, while the E. coli enzyme had a strong preference for CDP-1,2-diacyl-sn-glycerol. It was concluded that M. thermautotrophicus archaetidylserine synthase belongs to subclass II phosphatidylserine synthase (B. subtilis type) on the basis of not only homology but also substrate specificity and some enzymatic properties. The possibility that a gene encoding the subclass II phosphatidylserine synthase might be transferred from a bacterium to an ancestor of methanogens is discussed.     

重组Rhodobacter sphaeroides hemA表达的调控

RhodobactersphaeroideshemA编码5氨基乙酰丙酸合酶(ALAS),催化磷酸吡哆醛依赖性琥珀酰CoA和甘氨酸缩合成ALA.将R.spaeroideshemA导入E.coli进行表达,当hemA具有与lac启动子相同的转录方向时,ALAS有活性.lac启动子与hemA之间的距离会影响ALAS在不同培养基上的表达.E.coli宿主菌对ALAS表达、ALA产量有显著影响,在实验所用6种菌株中,E.coliDH1是最佳宿主菌(P<0.05).ALAS表达还与碳源有关,琥珀酸为碳源时,重组ALAS活性最高(P<0.05),以乳酸为碳源时,ALAS活性很低.重组ALAS活性也受培养基pH值影响,pH6.5时,活性最高(P<0.05).