纯化方式对麦麸酯酶农药检测效能的影响

为探讨麦麸酯酶应用于农残检测的可行性,采用固蓝B染色体系,以酶活抑制率为指标,研究了经Sephadex G-200凝胶过滤层析、双水相萃取、硫酸铵分段盐析3种方式纯化后的麦麸酯酶对6种农药的敏感性及最低检测限(LOD)。结果显示,经Sephadex G-200凝胶过滤层析、双水相萃取、硫酸铵分段盐析后的麦麸酯酶对6种农药的LOD范围分别是0.003～0.193 mg/L、0.005～0.116 mg/L和0.039～0.386 mg/L。其中,经凝胶过滤层析和双水相萃取后的麦麸酯酶对6种农药的敏感性相对于粗酶液均有不同程度的提高,而经硫酸铵分段盐析后的麦麸酯酶对6种农药的敏感性低于粗酶液。该研究为麦麸酯酶应用于农药残留检测奠定了一定的技术基础。     

培养液中纤维素酶的分离纯化

目的:为了研究纤维素酶的特性,使之利用纤维素从而促进纤维素资源化,减少环境污染,该文选用作者实验室筛选出的菌株K7-2培养产生纤维素酶,进行了纤维素酶的分离纯化。方法:将菌株K7-2在30℃、150r/min摇床培养3d,于5 000r/min离心30min,取上清液即为粗酶液,经硫酸铵分级沉淀、Sephadex G-75凝胶过滤层析、DEAE-Sephadex A-25离子交换层析方法进行分离纯化。结果:分离纯化后的酶活是0.0904U/ml,比活力提高4.1120倍。结论:这为进一步研究此纤维素酶的组份、结构和理化特性奠定了基础。     

短芽孢杆菌低温弹性蛋白酶酶学特性分析

旨在从短芽孢杆菌(Bacillus brevis)XZE116发酵液中分离纯化低温弹性蛋白酶,并对酶学性质进行研究。利用硫酸铵分级盐析、DEAE-Sepharose阴离子交换层析和Sephadex G-75分子筛凝胶过滤层析等方法进行纯化。结果显示,分离纯化到了均一的酶蛋白,酶纯度提高了37.21倍,回收率为35.3%。SDS-PAGE及Sephadex G-75分子筛凝胶过滤层析显示酶蛋白为单亚基蛋白,分子量是32.6 kD。最适作用温度25℃。在pH7.5-10.5范围内酶活性及稳定性较高,最适作用pH9.0,Mg2+对酶有明显激活作用。丝氨酸蛋白酶特异性抑制剂强烈抑制酶活性,表明所纯化到的弹性蛋白酶属于丝氨酸蛋白酶。酶对阴离子表面活性剂(0.1%SDS)、阳离子表面活性剂(0.1%CTAB)和非离子型表面活性剂(1%Tween80)均具有很强的稳定性。鉴于短芽孢杆菌XZE116弹性蛋白酶具有以上优良酶特性,它在肉品嫩化领域具有潜在的应用价值。     

意大利蜜蜂N-乙酰-β-D-氨基葡萄糖苷酶的分离纯化及性质分析

【目标】N-乙酰-β-D-氨基葡萄糖糖苷酶(NAGase)是一种重要的几丁质分解酶,能从N-乙酰葡萄糖苷的非还原端催化去除β-1,4-N-乙酰-D-氨基葡萄糖残基,参与了昆虫外骨骼的蜕皮过程。研究蜜蜂该酶的特征有助于阐明其在蜜蜂发育过程中的作用机制。【方法】采用40%-70%硫酸铵分级沉淀、DEAE-纤维素离子交换层析和葡聚糖G-100凝胶过滤层析的方法从意大利蜜蜂Apis mellifera ligustica幼虫体内分离纯化NAGase。以对-硝基苯-N-乙酰-β-D-氨基葡萄糖苷(pNP-NAG)为底物检测该酶的活力,用native PAGE和SDS-PAGE检测酶的纯度。IEF-PAGE测定该酶等电点。葡聚糖G-200凝胶过滤层析测定酶的总分子量。【结果】结果显示,纯化的NAGase酶的比活力为803. 09 U/mg,总分子量为77. 3 kD。结合SDS-PAGE表明该酶由两个具有相同分子量(39 k D)的亚基组成。该酶等电点为4. 8。酶水解底物pNP-NAG的过程遵循米氏方程,米氏常数(Km)和最大反应速度(Vm)分别为0. 11 mmol/L和17. 65μmol/L·min。该酶水解反应的最适pH和最适温度分别为pH 5. 5和60℃。酶催化pNP-NAG反应的活化能为64. 8 k J/mol。Pb2+,Cu2+,Zn2+和Al3+对该酶有不同程度的抑制作用。【结论】本研究描述了意大利蜜蜂NAGase的分离纯化方法及其理化性质,为进一步进行蜜蜂NAGase的结构解析和功能研究奠定基础。     

HaSNPV几丁质酶的分离纯化与毒理学研究

利用重组工程菌GS115-pPIC 9k-ChiA 4.0发酵几丁质酶粗液,经(NH₄)₂SO₄盐析、透析、DEAE Sepharose Fast Flow离子交换层析以及Sephadex G-100凝胶过滤层析分离纯化,获得电泳纯的棉铃虫单粒包埋型核型多角体病毒(HaSNPV)几丁质酶,回收率为19.64%,纯化17.74倍;经HaSNPV几丁质酶毒理学研究,通过触杀作用和胃毒作用,几丁质酶使小菜蛾幼虫细胞液化,导致死亡,其作用效果与几丁质酶浓度和作用时间成正比,且胃毒作用大于触杀作用;经小麦根腐、烟草赤星、番茄灰霉和苹果炭疽等植物病原真菌的抑菌实验,表明几丁质酶可以通过酶解真菌细胞壁中的几丁质达到抑菌作用。     

一种来源于蜗牛酶的β-葡萄糖苷酶的纯化

通过DEAE-Sepharose离子交换分段层析、DEAE-Sepharose离子交换梯度层析和Sephadex G-100凝胶过滤层析三种方法的联用,从中华白玉蜗牛消化酶中提纯出一种β-葡萄糖苷酶。该酶在SDS-PAGE上呈单一蛋白质条带。应用SDS-PAGE和凝胶过滤层析测定其分子量,提示该酶是由4个分子量为110~115 kD的相同亚基组成的同源四聚体。pNPG为底物的动力学参数Km和Vmax分别为0.182 mmol/L和0.189μmol/(min.mg)。     

银杏种仁中抗菌蛋白的纯化及性质

银杏果仁提取上清液经硫酸铵沉淀、CM—52离子交换柱层析和Sephadex G-50凝胶过滤层析后分离纯化出一种抗菌蛋白。SDS—PAGE分析结果表明,此蛋白分子量为13000,对热稳定;氨基酸组分分析表明,该蛋白含18种不同氨基酸,尤富含丙氨酸(Ala)和精氨酸(His)等,缺乏半胱氨酸(Cys);纯化的蛋白对黄瓜镰刀孢菌(Fusarium oxysporum)、瓜类炭疽菌(Colletotrichum orbiculare)、小麦全蚀病菌(Gaeumannomyces graminis)等真菌有很强的抑制作用,而且对金黄色葡萄球菌(Staphylococcus aureus)、大肠杆菌(Escherichia Coli)等细菌也有一定的抑制作用。     

东亚飞蝗主要过敏原的分析、鉴定与纯化

通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳(SDS-PAGE)分离东亚飞蝗Locusta migratoria manilensis(Meyen)的蛋白质组分并测定其分子量,收集过敏病人血清,采用免疫印迹(Western—blotting)法鉴定其过敏原成分,通过凝胶过滤层析对东亚飞蝗过敏原进行分离纯化。结果表明:东亚飞蝗蛋白粗提液条带大概有30条左右,其中主带大约有10条,相对分子量约为13、15、25、28、40、45、55、70、100、110ku,其中蛋白含量最丰富的约在70ku左右。免疫印迹结果显示,蝗虫过敏条带主要有5条,相对分子量分别约为19、29、38、70、130ku。通过凝胶过滤层析对东亚飞蝗过敏原进行分离纯化,得到了一个高纯度相对分子质量约为70ku东亚飞蝗过敏原,并且发现了一个相对分子质量约为130ku的蝗虫新过敏原。本研究为临床上蝗虫食物变态反应性疾病的诊断和治疗奠定基础。     

烟草磷酸吡哆醛水解酶的分离纯化与表征

采用硫酸铵沉淀、DEAE-Sepharose Fast Flow阴离子交换、Sephadex G-100凝胶过滤和SP Sephadex C-25阳离子交换柱层析等步骤,对烟草磷酸吡哆醛水解酶进行了分离纯化。结果表明:该酶被纯化了119.6倍,得率为28.49%,经凝胶过滤和SDS-PAGE测得该酶的全分子量为49.6kDa,亚基分子量约为25kDa;该酶最适温度为50℃,最适反应pH为5.5;Mg2+、Ca2+、Mn2+等对该酶有激活作用,金属离子螯合剂EDTA对酶有抑制作用,加入Mg2+后抑制作用得到解除;在最适反应条件下,测得反应底物磷酸吡哆醛(PLP)和磷酸吡哆胺(PMP)的Km值分别为0.23mmol/L和0.56mmol/L。     

猪血超氧化物歧化酶分离纯化工艺改进及其抗氧化活性研究

以新鲜猪血为原料,首次利用改进的新工艺提取分离超氧化物歧化酶,经过溶血,热变,丙酮沉淀,超滤浓缩,SephadexG-75凝胶过滤层析和DEAE-sepharose-fast flow离子交换层析纯化,冷冻干燥等步骤,得到高纯度酶,并对酶的相关性能进行研究。试验结果显示产品粗酶活性在3 000 U/mg左右,分别经SephadexG-75和DEAE-sepharose-fast flow层析纯化后,酶活分别达到5 585 U/mg和6 148 U/mg产品得率分别为13.4%和10.32%,SDS-PAGE凝胶电泳显示为单一条带达到电泳纯,其分子量在31 kD附近,其临苯三酚抗氧化活性明显。     

Enzymic synthesis of useful chito-oligosaccharides utilizing transglycosylation by chitinolytic enzymes in a buffer containing ammonium sulfate

A chitinase purified from culture filtrates of Trichoderma resei KDR-11 efficiently catalyzed a transglycosylation reaction on tetra-N-acetylchitotetraoside in a buffer medium containing ammonium sulfate, converting the tetrasaccharide into hexa-N-acetylchitohexaose (39.6%) and di-N-acetylchitobiose (55.7%) as the major products. Sugar-chain elongation from di-N-acetylchitobiose as the initial substrate to hexa-N-acetyl-chitohexaose and hepta-N-acetylchitoheptaose was also efficiently induced through lysozyme catalysis in the presence of ammonium sulfate at high (30%) concentration. In this case, the addition of ammonium sulfate to the reaction system resulted in a remarkable increase of the hexamer and heptamer productions, which are desirable as biologically active oligosaccharides.     

Two-step purification of Bacillus circulans chitinase A1 expressed in Escherichia coli periplasm

A protein purification procedure was developed to efficiently and effectively purify the target enzyme, chitinase A1 of Bacillus circulans WL-12, from Escherichia coli DH5alpha carrying the chiA gene with its natural promoter in the plasmid pNTU110. Chitinase A1 was purified to apparent homogeneity from E. coli periplasm with a final recovery of 90.6%. Two main steps were included in this protein purification procedure, ammonium sulfate precipitation (40% saturation) and anion-exchange chromatography at pH 6.0 using Q Ceramic HyperD column. The yield of chitinase A1 was estimated at 95 microg/L. A polyclonal antibody against chitinase A1 was raised by immunizing BALB/c mice with chitinase A1 purified from E. coli DH5alpha(pNTU110). As indicated by Western blot analysis, a 3000-fold diluted antibody detected purified chitinase A1 from E. coli DH5alpha(pNTU110) in an amount of at least 1 ng and specifically detected chitinase A1 produced by B. circulans WL-12.     

疏绵状嗜热丝孢菌热稳定几丁质酶的纯化及其性质研究

采用硫酸铵沉淀、DEAE SepharoseFastFlow阴离子层析、Phenyl Sepharose疏水层析等步骤获得了凝胶电泳均一的疏绵状嗜热丝孢菌 (Thermomyceslanuginosus)几丁质酶。经SDS PAGE和凝胶过滤层析测得纯酶蛋白的分子量在 4 8～ 4 9 .8kD之间。该酶反应的最适温度和最适pH分别为 5 5℃和 4 5 ,在pH4 5条件下 ,该酶在 5 0℃以下稳定 ;6 5℃的半衰期为 2 5min ;70℃保温 2 0min后 ,仍保留 2 4 %的酶活性。其N 端氨基酸序列为AQGYLSVQYFVNWAI。金属离子对几丁质酶的活性影响较大 ,Ca2 、Na 、K 、Ba2 对酶有激活作用 ;Ag 、Fe2 、Cu2 、Hg2 对酶有显著的抑制作用 ;以胶体几丁质为底物的Km 和Vmax值分别为 9 .5 6mg mL和 2 2 . 12 μmol min。抗菌活性显示 ,该酶对供试病原菌有不同程度的抑制作用。     

海洋微生物几丁质酶分离纯化及其抗真菌活性

以实验室筛选的海洋产几丁质酶短芽胞杆菌属（Bacillus brevis sp．）菌株Bspl,经往复式摇床振荡培养96h后,发酵液先后采取了75％的硫酸铵盐析、透析、几丁质亲和层析、SDS—PAGE等方法对几丁质粗酶液进行分离纯化和鉴定。几丁质亲和层析一步纯化后,经过SDS—PAGE电泳测定该酶的分子量为23ku,其比活力为86．65．纯化倍数为1．707、产率为32．1％。纯化的几丁质酶能抑制病原真菌的生长,对病原真菌的拮抗作用具有广谱性。同时研究了几丁质酶的稳定性,以胶态几丁质为底物,分离的几丁质酶在pH7．5,55．0℃左右具有最大酶活性;Zn^2＋、Cu^2＋和Hg^2＋能强烈抑制几丁质酶活性;Ni^＋和EDTA抑制20％-40％;然而5mmol／LCo^2＋可以使几丁质酶活性提高1．4倍;Mg^2＋、Ca^2＋等也能使酶活性增加。     

产气肠杆菌几丁质酶的分离纯化及性质研究

从自然罹病死亡的草原毛虫(Gynephorap ruoergnesis)体内分离到一株产气肠杆菌(Enterobacter aerogenes),它在几丁质的诱导下能产生较高活性的几丁质酶。发酵液经硫酸铵盐析、DEAE纤维素柱层析和Sephadex G-100柱层析分离出几丁质酶。用SDSPAGE测得该酶的分子量为425kD。水解几丁质的Km值为2.88mg/mL-1。酶反应的最适温度为55℃,最适pH值为60,金属离子对几丁质酶活性影响较大,其中Zn2+、Ba2+、Ca2+和Mn2+对酶有较强的激活作用,而Hg2+、Co2+和Mg2+则有较强的抑制作用。     

Purification and characterization of chitinase from Streptomyces sp. M-20

Chitinase (EC 3.2.1.14) was isolated from the culture filtrate of Streptomyces sp. M-20 and purified by ammonium sulfate precipitation, DEAE-cellulose ion-exchange chromatography, and Sephadex G-100 gel filtration. No exochitinase activity was found in the culture filtrate. The molecular mass of the purified chitinase was 20 kDa, estimated by a sodium dodecyl sulfate-polyacrylamide gel electrophoresis, and was confirmed by activity staining with Calcofluor White M2R. Chitinase was optimally active at pH of 5.0 and at 30 degrees C. The enzyme was stable from pH 4 to 8, and up to 40 degrees C. Among the metals and inhibitors that were tested, the Hg(+), Hg(2+), and p-chloromercuribenzoic acid completely inhibited the enzyme activity. The chitinase activity was high on colloidal chitin, chitotriose, and chitooligosaccharide. The purified chitinase showed antifungal activity against Botrytis cinerea, and lysozyme activity against the cell wall of Botrytis cinerea.     

Purification and characterization of extracellular chitinase from Aeromonas schubertii

A locally isolated stain Aeromonas schubertii was cultured and induced by powdered chitin for the production of chitinases. Extracellular proteins were purified by ammonium sulfate precipitation, dialysis to remove salts, and then preparative isoelectric focusing (IEF) to yield several chitinases. The purified enzymes were analyzed by SDS–PAGE (sodium dodecyl sulfate–polyacrylamide gel electrophoresis) with and without glycol chitin and were found to be SDS-resistant. The chitinase present in the highest abundance was the one with an estimated molecular weight of 75 kDa. The Michaelis constant and turnover number were determined to be 0.29 mM and 1 s⁻¹, respectively, for this enzyme using colloidal chitin azure as the substrate. However, the ethanol treatment of this enzyme could significantly increase its chitinolytic activity. Other chitinases obtained in the same IEF fraction were determined to have molecular weights of ca. 30, 38, and 110 kDa. Since the proteins with highest chitinase activity were collected from IEF fraction tube with pH value of 4.8, those chitinase were believed to be acidic. An activity assay method using colloidal chitin azure as the substrate was recommended since it possessed a broader range of linearity in comparison with conventional reducing sugar equivalent method.     

Electrophoretic Studies of Alkaline Proteinases from Strains of Aspergillus flavus Group

Entevobacter sp. G-1 which produces chitinolytic and chitosanolytic enzymes, was previously isolated in our laboratory. One major chitinase, designated ChiA, was purified 42.9-fold from a culture filtrate of Entevobacter sp. G-L To purify the chitinase, ammonium sulfate fractionation, DEAE-Sephadex A-50 column chromatography, and gel filtration on Sephadex G-100 column chromatography were used. The ChiA protein had a molecular weight of 60,000 estimated by SDS polyacrylamide gel electrophoresis and an isoelectric point of 6.6. The optimal pH and optimal temperature of ChiA against colloidal chitin were pH 7.0, and 40°C, respectively. The purified ChiA degraded colloidal chitin mainly to GlcNAc₂ with a small amount of GlcNAc₃ and GlcNAc₄. ChiA hydrolyzed flaked chitin, colloidal chitin, and ethylenglycol chitin, but did not hydrolyze carboxymethyl cellulose (CMC), nor >90% deacetylated flaked chitosan. The chitinase activity was 42% inhibited by 10mm EDTA, but was not inhibited by Ca²⁺ (<50 mm) or NaCl (<400 mm). The purified ChiA hydrolyzed colloidal chitin and chitin-related compounds in an endo splitting manner.     

Purification, Characterization, and Antifungal Activity of Chitinase from Streptomyces venezuelae P10

Streptomyces venezuelae P₁₀ could produce extracellular chitinase in a medium containing 0.6% colloidal chitin that was fermented for 96 hours at 30°C. The enzyme was purified to apparent homogeneity with 80% saturation of ammonium sulfate as shown by chitin affinity chromatography and DEAE-cellulose anion-exchange chromatography. Sodium dodecyl sulfate–polyacrylamide gel electrophoresis (SDS-PAGE) of the enzyme showed a molecular weight of 66 kDa. The chitinase was characterized, and antifungal activity was observed against phytopathogens. Also, the first 15 N-terminal amino-acid residues of the chitinase were determined. The chitin hydrolysed products were N-acetylglucosamine and N, N’-diacetylchitobiose.