产青霉素酶枯草芽孢杆菌发酵条件的优化

目的:对一株产青霉素酶的重组枯草芽孢杆菌(Bacillus subtilis DB104/pWB-pemp)的摇瓶发酵条件进行优化.方法:利用单因素实验及正交实验等方法考查重组菌摇瓶发酵条件,研究不同浓度的碳源、氮源、金属离子、磷酸盐及不同pH、接种量、装液量和温度等条件对产青霉素酶的影响.结果:重组菌株摇瓶最适发酵条件为pH 7.0、接种量3％、装液量14％、发酵温度37℃,培养基成分为2％蔗糖、3.5％酵母膏、0.1mmol/L镁离子、0.4％磷酸盐.结论:最优条件下,发酵36h,产酶活力达到2227.8U/mL,为先前研究结果(1 580 U/mL)的1.41倍,为重组菌的大规模发酵生产奠定了基础.     

产脂肪酶菌株筛选及柠檬酸杆菌产酶条件优化

脂肪酶可以催化甘油三酯水解成脂肪酸和甘油,已广泛应用在工业领域,而获得产酶微生物是研究的基础。采用油脂平板法筛选出1株脂肪酶产生菌。经16S rRNA序列分析可知,该菌株属于柠檬酸杆菌(Citrobacter werkman and Gillen)。单因素试验对其进行产酶条件优化,优化后产酶条件（g/L）：淀粉2.0,KH₂PO₄ 1.0,K₂HPO₄·3H₂O 2.2,(NH₄)₂SO₄ 1.0,MgSO₄·7H₂O 0.1,牛肉膏2.0,橄榄油10.0 mL,pH 7.5,接种量1.5%(v/v),37 ℃培养43 h。获得最大酶活为384 U/mL,是优化前的13倍。可以利用该菌制备脂肪酶。     

地衣芽孢杆菌TG116胞外蛋白酶产酶条件与酶学性质

【背景】从独角莲中分离得到的地衣芽孢杆菌TG116是一株对植物病原菌具有广谱抗性作用的生防菌株。【目的】优化TG116的产酶条件并探索其酶学性质,进一步了解其抗菌机制。【方法】采用Folin-Phenol显色法与响应曲面法,优化菌株TG116的产酶条件并研究其蛋白酶的酶学性质。【结果】菌株TG116产酶最适条件为:温度40.83°C,p H 8.01,发酵时间53.74 h,增加通气量可以显著提高酶活力。按照优化后的条件培养48 h后,上清液蛋白酶活力从57.46 U/mL达到了254.07 U/mL。酶学性质研究表明:该酶为碱性蛋白酶,最适反应pH为8.5,最适反应温度为50°C,具有良好的温度和pH稳定性,EDTA对酶活具有强烈的抑制作用,金属离子Mg~(2+)、Ca~(2+)、Na~+、Co~(2+)、K~+等对酶活也具有一定的抑制作用。【结论】菌株TG116具有良好的p H与温度稳定性,在实际应用中蛋白酶不易失活,可以分解真菌的细胞壁蛋白成分,破坏细胞壁结构,从而抑制甚至杀死病原菌,达到抗菌作用。     

节杆菌K1108乙内酰脲酶产酶条件研究

研究了乙内酰脲酶产生菌节杆菌K1108的产酶条件。该菌乙内酰脲酶为诱导酶,存在于细胞内,乙内酰脲水解酶和N氨甲酰氨基酸水解酶是同时被诱导产生。最适诱导物为5苄基乙内酰脲,而5吲哚甲基乙内酰脲和5苯基乙内酰脲等不能诱导其酶的产生。筛选到一种安慰诱导物,诱导活性提高了2倍多。对产酶培养基进行了筛选和优化,在最适条件下,K1108产酶能力可达108U/mL。     

甲壳素脱乙酰酶产生菌产酶条件的优化

采用斜面培养和液体发酵培养产甲壳素脱乙酰酶的真菌构巢曲霉,并且研究了产酶条件。结果表明,构巢曲霉的最适产酶条件为：发酵培养基初始pH值为6.5、发酵时间为96h、培养温度为31℃、碳源浓度为2%、氮源浓度为2%、金属离子浓度为0.01mol/L、接种量为6%。     

木聚糖酶高产菌株的鉴定及产酶条件的优化

目的:通过了解木聚糖酶高产菌株A79的遗传背景.并优化其产木聚糖酶的液体发酵条件,为下一步工业化生产和木聚糖酶制剂的研制奠定基础.方法:通过形态观察和18S rDNA基因的分子系统进化分析,对菌株A79进行鉴定;通过单因素和均匀设计试验,优化其产胞外木聚糖酶的液体发酵条件.结果:通过对18S rDNA基因的分子系统进化分析,菌株A79被鉴定为黑曲霉(Asperillus niger A79).其最佳产酶培养基为:玉米芯5.0%,麸皮0.5%.纤维物质1.O%,玉米浆1.1%.(NH4)2SO40.8%,蛋白胨0.8%,CaCO3 0.5%,KH2PO4 0.23%,MgSO4,·7H2O 0.08%,微量元素(MaIldels)0.08%,pH自然.最佳发酵条件为:接种量5%(2.0×107),28℃、250r/min振荡培养96h.结论:经优化培养,酶活力由前期的50 000u/ml提高到90000u/ml,增加了近50%.     

耐底物腈水合酶融合子的产酶条件优化

采用正交设计法对耐底物腈水合酶融合子的发酵条件进行优化,以发酵液起始pH,发酵周期,接种量,装料系数作为考察因素,最终确定最佳发酵条件为:起始pH8.0、发酵周期54h、接种量12％、装液系数12％.在此优化条件下融合子腈水合酶的活力达到1100万U/ml,较优化前提高了83.3％.通过响应面法对发酵培养基配方进行优化研究,采用Plackett-Burman法对8个因素进行了筛选,结果表明,葡萄糖、尿素、磷酸氢二钾、磷酸二氢钾是影响发酵液腈水合酶产量的主效应因子.用最陡爬坡试验及Central composite design设计进一步优化,利用Design-Expert软件进行二次回归分析,得到各因素的最佳浓度为:葡萄糖22.62g/L、尿素9.76g/L、K2HP04 1.22g/L、KH2PO41.268g/L.在此培养基优化配方下融合子腈水合酶的活力达到1280万U/ml,较原配方的酶活提高了16.4％.     

产蛋白酶细菌Bs3210菌株产酶条件的研究

在对我国地带性土壤中产蛋白酶细菌生态分布的研究基础上,获得了一株产酶活力达到1945单位/ml的野生菌株。经鉴定为枯草芽孢杆菌(Bacillus subtnis)、对该菌的产酶条件进行了比较系统的研究。结果表明,王米粉和豆饼粉是该菌良好的碳源和氮源。而有机酸和无机盐对产酶有抑制作用。     

均匀设计法对产几丁质酶细菌C4发酵条件的优化

系统研究了碳源,氮源,起始pH值、培养基装量、培养温度和时间等因素对细菌C4产几丁质酶的影响。结果表明,碳、氮源分别以胶体几丁质、KNO和蛋白胨最好;在起始pH值7．6—8．5,培养基装量为三角瓶体积的12％,培养温度28℃,振荡培养(180r／min)5d时最有利于几丁质酶的产生。在此基础上通过均匀设计法优化了发酵培养基配方。优化后的培养基配方为：胶体几丁质1．5％,蛋白胨0．55％,KNO3 0．3％,MgSO4 0．09％,Tween80 0．005％。在该条件下,几丁质酶活力达2．68U／mL,比在原基础培养条件下的酶活力提高90．1％。     

1株产单宁酶细菌的分离鉴定及产酶条件研究

从富含单宁酸的土壤中分离筛选出1株产单宁酶的细菌,经过菌落形态观察和16S rDNA分子生物学鉴定,该细菌为肺炎克雷伯菌。对该菌所产胞外单宁酶的发酵条件进行了初步研究,得出最佳产酶条件：培养温度37℃,培养时间36 h,培养转速180 r/min,单宁酸含量2 g/L,最佳碳源为葡萄糖,最佳氮源为氯化铵,此时所产单宁酶活力为0.8 U/mL。     

产生物表面活性剂芽孢杆菌培养条件的优化

为了提高生物表面活性剂的表面活性,通过单因素及正交试验对已筛选的产生物表面活性剂芽孢杆菌的培养基及培养条件进行了优化,优化后的培养基成分为可溶性淀粉20 g/L,氯化铵2 g/L,KH2PO46 g/L,K2HPO42 g/L,MgSO4.7H2O 0.3 g/L,NaCl 2 g/L,CaCl20.08 g/L,EDTA 0.4 g/L。培养条件为4%接种量,种龄16 h,初始pH7,培养温度37℃,摇床转速160 r/min,发酵48 h。优化发酵条件后,发酵液表面张力由初始67.5 mN/m降低至24.8 mN/m,生物表面活性剂产量达到1.08 g/L。     

高产磷酯酶C菌株的诱变选育

在前面进行的高产磷酯酶C(PLC)菌株筛选、分类鉴定及其抗血小板功能研究的基础上,对选育出的高产PLC菌株BacilluscereusShenZhen7541进行了紫外线和Co60γ射线诱变处理,以期提高其产PLC的水平,从而有利于PLC的纯化制备。B.cereus7541经过三次紫外线照射及两次Co60γ射线辐射诱变处理,通过分离与卵黄琼脂杯碟法及NPPC法酶活检验筛选,最终获得了三株高产PLC突变菌株9287、9289和5612,其产PLC酶活水平分别达到14.878±1.428u/mL、16.450±0.793u/mL、16.400±0.967u/mL,较原始出发菌株B.cereus7541产酶水平(5.803±0.793u/mL)分别提高了2.879、3.236和3.226倍。经t值检验,三株菌产PLC水平与7541差异均达极显著(P<0.001)。     

A 140-Kilodalton Protein Is Released from Cultured Astrocytes by Phosphatidylinositol Phospholipase C

Astrocytes in culture synthesize a 140-kilodalton (140-kD) protein (protein 140) that is released into the medium on incubation with phosphatidylinositol phospholipase C. This molecule therefore belongs to the class of proteins anchored to the external side of the cell membrane through a glycolipid moiety. Protein 140 is present in astrocyte cultures derived from two different regions of the brain and is not expressed by neurons in vitro. It differs from neuronal cell adhesion molecule 120 or 140 and is probably identical to a protein of 140 kD present in C6 glioma cells.     

磷脂酰肌醇特异性磷脂酶C的异源表达和应用

旨在研究大肠杆菌产磷脂酰肌醇特异性磷脂酶C(PI-PLC)的发酵表达和分离纯化,探究PI-PLC酶切GPI锚定蛋白的效果。依据NCBI数据库中蜡样芽孢杆菌的PI-PLC的基因序列,按照大肠杆菌的密码子偏好性进行密码子优化,合成相应基因序列并构建基因表达载体pGEX-6P-1-PI-PLC。将重组质粒转入受体菌E.coli BL21(DE3)中,通过加入异丙基硫代-β-D-半乳糖苷(IPTG)诱导目的基因PI-PLC表达。经检测,含有GST标签的PI-PLC融合蛋白以可溶蛋白形式存在于菌体破碎上清,分子量约为61 kDa,与预期相符。初步优化诱导表达条件后,发现最佳诱导表达条件为:以接种量5%接种体积分数接种,待菌体生长至OD600nm达到0.5,在16℃条件下以0.3 mmol/L浓度IPTG诱导24 h。利用GST标签对蛋白进行纯化,纯化后的PI-PLC质量浓度为0.52 mg/mL,比酶活为1322.5 U/mg。利用PI-PLC酶液对哺乳动物细胞表面的模式GPI锚定蛋白CD59进行酶切,酶切作用显著。因此,下一步可以将PI-PLC融合蛋白应用于细胞生物学中对GPI-APs的研究和鉴定。     

Phospholipase signaling is modified differentially by phytoregulators in Capsicum chinense J. cells

Plant defense mechanisms respond to diverse environmental factors and play key roles in signaling pathways. The phospholipidic signaling pathway forms part of the plant response to several phytoregulators, such as salicylic acid (SA) and methyl jasmonate (MJ), which have been widely used to stimulate secondary metabolite production in cell cultures.¹ Furthermore, it has been reported that the levels of such phytoregulators as SA and MJ can increase in response to stressful conditions.^2,3 The phospholipidic signal transduction system involves the generation of second messengers by the hydrolysis of phospholipids. In this study, we examined how phospholipidic signaling can be modulated depending on the growth stage of the culture, and we focused on two key lipases having relevant roles in the signaling cascades in plants. An evaluation was made of the effects of SA and MJ on the phospholipase activities in Capsicum chinense Jacq. suspension cells at different phases of the culture cycle. The treatment with SA differentially modified the phospholipase C (PLC) (EC: 3.1.4.3) and phospholipase D (PLD) (EC: 3.1.4.4) activities in a dose-dependent manner that also depended on the day of the culture cycle. In contrast, the treatment with MJ resulted in a biphasic behavior of the PLC and PLD activities. We conclude that the enzymatic activities in the phospholipidic signaling pathways are modified differentially depending on the day of the culture’s growth cycle; accordingly, the response capacity to such environmental factors as phytoregulators is variable at different stages of growth and the physiology of the cells.     

Bacillus sp.fmbJ224发酵产新型抗菌肽培养基的优化研究

采用Plackett-Burman设计(Plackett-Burman Design,PB)法,对影响Bacillus sp．fmbJ224产新型抗菌肽的17个因素进行了筛选。结果表明：影响该菌发酵产新型抗菌肽的主要培养基成分为葡萄糖、NH4NO3、谷氨酸、CaCl2、MnSO4。在此基础上,再采用响应曲面法(Response Surface Methodology,RSM)对其5个显著因子的最佳水平范围进行研究。通过对二次多项回归方程求解得知,在上述自变量分别为葡萄糖8．13g／L、NH4NO36．14g／L、谷氨酸4．2g／L、CaCl23．98mg／L、MnSO44．87mg／L时,新型抗菌肽的产量从1304．2μg／mL提高到了1487．58μg／mL。     

磷酸肌醇磷脂酶C在DREB2表达调控中的作用

环境胁迫对植物的生长不利。转录因子DREB2对干旱、高温、低温等非生物胁迫应答基因的表达具有重要的调控作用。磷酸肌醇磷脂酶C对 DREB2 基因有双向调节机制。深入了解 DREB2 和磷酸肌醇磷脂酶C的研究进展及其在生物工程上的应用,以及磷酸肌醇磷脂酶C对 DREB2 基因的表达调控机理,可以为磷酸肌醇磷脂酶C和 DREB2 基因在提高植物胁迫耐受性中的利用提供基础。     

胶质芽孢杆菌突变株021120的培养条件及发酵工艺优化

对离子束诱变所获得的突变菌株021120进行了培养条件和发酵工艺研究。单因子及正交试验结果表明,碳源对生物量和芽孢形成的影响最大,其次是氮源,磷和钾的影响较小;添加CaCO3和增加氧通量显著促进芽孢的形成。发酵培养基的理想配方为：2%淀粉、0.4% 酵母、0.1% K2HPO4、0.1％ MgSO4·7H20、0.5 ％CaCO3,pH 7.5。种子菌经二级扩大培养后,按6％的接种量接入70 L发酵罐,在32℃进行发酵,氧通量2.0-2.5 vvm,培养周期38-42 h,芽孢量达到9.80×108 cfu ml-1。通过以上培养基和发酵条件的优化,有效控制了多糖荚膜的产生,并促进了芽孢的形成,获得合格产品。     

鞘氨醇单胞菌TP-3合成新型生物聚合物Ss的发酵条件优化

鞘氨醇单胞菌(Sphingomonas sp.)TP-3能合成一种具有增稠性、假塑性、成凝胶特性和乳化性能的新型生物聚合物Ss。运用单因素实验和均匀设计法对菌株TP-3合成聚合物Ss的发酵条件进行优化, 实验结果表明, 培养基组成为葡萄糖41.2 g/L, 豆饼粉2.0 g/L, NaCl 0.85 g/L, K2HPO4 1.46 g/L, MgSO4 0.12 g/L, MnCl2 0.0075 g/L, FeSO4 0.002 g/L, 初始pH为7.0, 在27°C, 180 r/min的条件下摇床培养60 h, 聚合物Ss的产量达到21.5 g/L。该聚合物生产成本低, 在油田开发中极具应用前景。     

Solubilization of the Membrane-Bound Sialidase from Pig Brain by Treatment with Bacterial Phosphatidylinositol Phospholipase C

The total pellet from pig forebrain (from which the cytosolic sialidase was completely washed out) was treated with phosphatidylinositol phospholipase C (PIPLC) and centrifuged at high speed. The supernatant contained sialidase and 5'-nucleotidase activities. The greatest liberation of sialidase was obtained after incubation for 20 min with PIPLC at 37 degrees C using pH 6.0 and a ratio between PIPLC (as units) and protein of 1.6. Under these conditions, the release of sialidase, 5'-nucleotidase, and protein was 22, 50, and 18.5%, respectively. On treatment with PIPLC, a purified preparation of pig brain neuronal (synaptosomal) membranes released 28% of its sialidase whereas a purified preparation of pig brain lysosomes did not liberate any sialidase activity. The pH optimum of sialidase present in the supernatant obtained after PIPLC treatment of the total pellet was 4.2, the same as that of the enzyme embedded in the membrane. When this supernatant was subjected to ammonium sulfate fractionation, 88% of its sialidase, having a pH optimum of 4.2, was recovered in the fraction precipitated between 20 and 45% of salt saturation and subsequently dialyzed. Ammonium sulfate treatment caused the appearance of a second sialidase activity, having a pH optimum of 6.6 and behaving on fractionation similarly to the pH 4.2 sialidase. The Km and Vmax values of pH 4.2 and pH 6.6 sialidase were similar (1.48 x 10(-4) and 0.98 x 10(-4) M for Km and 1.6 and 1.4 mU/mg of protein for Vmax, respectively), whereas the stability on standing at 4 degrees C or exposure to freezing and thawing cycles was greater for pH 4.2 sialidase.(ABSTRACT TRUNCATED AT 250 WORDS)