盐生杜氏藻(Dunaliella salina)cDNA文库构建及功能基因筛选

采用Qiagen公司的植物总RNA提取技术、Clontech公司的CreatorTM技术平台以及SMARTTM技术进行cDNA文库构建.从杜氏藻中提取出了高质量的总RNA,通过PowerScript反转录酶反转录杜氏藻的总RNA,采用LD-PCR、酶处理等方法对cDNA进行等比例扩增、纯化,同时使用CHROMA SPIN-400柱子将cDNA分段化,最后将长片段连入pDNR-LIB质粒,1.5 kV,25 μ F电转化大肠杆菌JM109,得到含1.5×106个克隆子的原始文库,滴度为1.5×106cfu ml-1.结合酶切和PCR,对该文库的质量进行了鉴定和统计,文库的平均片段插入长度为1.5kb.采用烯醇酶和UDP葡萄糖脱氢酶的EST作为同源探针,对文库中的功能基因进行筛选,并采用放射性原位杂交法,对扩增文库进行了初筛和复筛,得到了含这两条基因全编码序列的cDNA,烯醇酶为1.8kb,UDP葡萄糖脱氢酶为1.9kb,为今后对该种进行大规模功能基因组学研究奠定基础.     

杜氏盐藻(Dunalielle salina)盐适应相关蛋白

观察不同盐浓度培养液中生长的杜氏盐藻可溶性蛋白SDS-PAG图谱,发现高盐与低盐相比,其51kD和63kD蛋白含量高,而23kD的蛋白含量则低。高渗骤变后,51kD蛋白的含量减少,而23kD蛋白的含量增加两倍或两倍以上,骤变23h后含量增加已非常明显;低渗骤变后24h,51kD和23kD蛋白的含量变化不明显。另外,有一分子量约为26kD的蛋白在高盐下易降解。分析了这些蛋白与社氏盐藻渗透调节的可能关系。     

杜氏盐藻（Dunaliella salina）基因工程的研究现状及应用前景

杜氏盐藻（简称盐藻）作为新型的生物反应器,成为藻类基因工程的研究热点之一。利用基因工程手段对盐藻进行遗传改造以生产外源物质是目前研究的重要领域。本文从盐藻相关基因的克隆、cDNA文库的建立、基因组文库的构建、筛选标记的确立和外源基因的表达等五个方面全面概述了国内外盐藻基因工程的研究进展,特别是对最新的研究结果进行了综述,并对基因工程技术在盐藻深入研究中的应用做了前景展望。     

人canstatin基因转化新型生物反应器－杜氏盐藻(Dunaliella salina)的初步研究

本文采用RT-PCR技术从人的胎盘组织中克隆canstatin基因,定向连接到表达载体pUΩ上,然后与筛选标记bar盒连接得到真核表达载体pUΩ-Can-Bar。采用玻璃珠转化法将该表达载体转化杜氏盐藻（以下简称盐藻）,通过草丁膦固体平板筛选得到转化株,进而对转化株进行阳性鉴定。PCR结果显示,在盐藻转化株中均能够扩增出约700 bp特异的条带,而在阴性对照中没有扩增出该条带。Southern blot结果进一步证明人canstatin基因已经整合到盐藻细胞的基因组中。此外,本文对盐藻转化株的遗传稳定行进行了分析,结果表明canstatin基因能够在转化藻株中稳定遗传。人canstatin转基因盐藻株的成功制备为利用盐藻反应器大规模生产人canstatin蛋白提供了实验依据,为及早实现canstatin蛋白在治疗肿瘤上的临床应用提供了前期工作基础。     

盐生杜氏藻和青岛大扁藻的超低温保存

采用两步法冷冻技术超低浊保存盐生杜氏藻（Ｄｕｎａｌｉｅｌｌａ ｓａｌｉｎｕ（Ｄｕｎａｌ）Ｔｅｏｄ．）和青岛大扁藻（Ｐｌａｔｙｍｏｎａｓ ｈｅｌｇｏｌａｎｄｉｃａ Ｋｙｌｉｎ ｖａｒ．ｔｓｉｇｔａｏｅｎｓｉｓ）。当二甲基亚砚（ＤＭＳＯ）浓度分别为５％和２０％,平衡时间均为ｍｉｎ,预冻温度及保持时间分别为－４０℃,６０ｍｉｎ和－３０℃,３０ｍｉｎ;化冻后分别在０℃和到温下采用慢速稀释法去除ＤＭＳＯ时,     

盐生杜氏藻对盐度改变的生理响应

以盐生杜氏藻为实验材料,采用f/2培养基,设置了8个盐度(15、20、25、30、50、70、90、110)处理,分盐度改变前(A)和盐度改变后(B)两个实验阶段,研究了盐生杜氏藻在不同盐度处理下的生长情况,测定了藻液的OD值、叶绿素a、β-胡萝卜素、可溶性蛋白质和可溶性糖含量等指标。结果表明,A阶段,几个较低盐度(15、20、25和30)处理生长状况较好,其中又以盐度20的处理最好;余下的处理,盐度越高,其生长所受的影响越大。B阶段,盐生杜氏藻的生长进入平台期后,50、70、90、110几个盐度较高处理的细胞密度、叶绿素a、β-胡萝卜素含量均显著超过了作为对照的盐度20的处理。且B阶段末期,先前盐度15的处理蛋白质、糖的积累量,与A阶段末期相比都有了不同程度的增加,而其余盐度处理组的蛋白质、糖含量则分别产生了不同程度的下降。     

盐生杜氏藻细胞光合特性的研究

研究了盐生杜氏藻细胞的光合特性获知：⑴在７００－３００ｎｍ波长范围,出现三个吸收峰,分别位于６８０．４８５和４００ｎｍ处;⑵测定了该藻细胞内ＡＴＰ／ＡＤＰ比值,钒酸钠处理可以提高ＡＴＰ／ＡＤＰ比值;⑶以培养液为反应介质,测出该藻细胞的光合放氧,钒酸钠抑制放氧速率;⑷用调制式荧光计测出该藻细胞的Ｆｏ,Ｆｍ以及经间隔饱和光脉冲引起的Ｆｍ,表明盐生杜氏藻具有正常的光系统结构;⑸该藻细胞可诱导可逆的光状态     

通过cDNARDA法分离和识别盐藻(Dunaliella salina)盐胁迫相关基因

采用cDNA代表性差异分析 (RDA)技术 ,对盐藻在盐胁迫时差异表达的基因进行了分离鉴定 .在分离到的 10个基因中 ,有 5个与已知基因同源 (包括叶绿素a b结合蛋白基因、蛋白磷酸酶I催化亚基基因和 3个核糖体蛋白基因 ) ,还有 5个未知功能基因则是首次在盐藻中被分离 .值得注意的是 ,所有这 5个已知基因的功能都与细胞分裂或盐胁迫有关 .结果表明 :取样时盐藻细胞仍处于恢复阶段 ,所分离到的基因对于盐藻耐盐可能具有重要意义 ;蛋白磷酸酶I的下调表达可能是盐藻调节离子平衡的一个重要过程和细胞分裂受阻的原因所在 ;盐藻减缓细胞分裂速度可能是为了减少能量消耗 ,以留出足够的能量来应对盐胁迫 ;其它 5个未知基因可能也与盐藻适应盐胁迫机制有关 .     

盐生杜氏藻质膜ATPase及其对高渗震动的反应

用水溶性多聚物 ( dextran T5 0 0 PEG 335 0 )两相法制备盐生杜氏藻细胞质膜 ,经检测质膜纯度较高 ,原位膜约占 78%。质膜 ATPase的动力学常数 Km 和 Vmax分别为0 5 8mmol L和 4 3 5 9μmol Pi ( mg protein· h) ;最适 p H值是 7 5。质膜 ATPase的活性随Mg Cl2 和 Ca Cl2 浓度的升高而增加 ,但较高浓度的 Mg Cl2 和 Ca Cl2 有轻微的抑制作用 ;KCl促进质膜 ATPase的活性 ,在 1 0 0 mmol L时达到最大 ,高于 1 0 0 mmol L时抑制效应显著。钒酸钠、DES、DCCD和 NEM明显地抑制质膜 ATPase的活性 ;而 Na N3、Na NO3、Na Mo O4和KCN对质膜 ATPase的活性影响不大。高渗震动刺激了质膜 ATPase的活性。     

盐生杜氏藻生长及β-胡萝卜素累积的动力学过程

国内外学者多注重研究环境因子对盐生杜氏藻生长和β-胡萝卜素累积的影响,为此,作者从温度和盐浓度对盐生杜氏藻生长的动力学及盐度与β-胡萝卜素累积的关系作了初步探讨。       

Capillary Zone Electrophoresis Separation of Recombinant Human Interleukin-3 and Related Proteins

ABSTRACT

Zone electrophoresis separations of human recombinant interleukin-3 (rh IL-3) and related proteins in untreated fused silica capillaries are presented. Results using pH 9 CHES buffer show that rh IL-3 is easily separated from a common carrier, human serum albumin, in a commercial preparation.     

毛细管电泳在细菌分离分析中的应用

介绍了近年来毛细管电泳技术在细菌分离分析方面的研究进展。毛细管电泳以细菌表面的特征信息为分离的基础,可以快速鉴定相应的菌株,可以对微生物进行快速定量,可以反映细菌特殊时期的生理特征,也可以研究微生物与分子之间的相互作用。同时应用该技术可分离分析自然界不能纯培养的微生物。因而毛细管电泳分离与检测细菌方法的建立及其应用在分离科学和微生物学方面都有很大的实际意义。     

电泳亲和色谱技术分离蛋白质

亲和色谱利用亲和配体与目标组分间的特异性结合作用实现对目标组分的纯化,该分离方法分辨率高,在生物物质的分析和分离领域得到日益广泛的应用［１］。亲和色谱在分离过程每一步操作中,液相主体中的溶质分子必须经过一系列扩散过程才能进入到固定相颗粒孔内完成吸附或...     

Electrophoretic Separation of Proteins

Electrophoresis is used to separate complex mixtures of proteins (e.g., from cells, subcellular fractions, column fractions, or immunoprecipitates), to investigate subunit compositions, and to verify homogeneity of protein samples. It can also serve to purify proteins for use in further applications. In polyacrylamide gel electrophoresis, proteins migrate in response to an electrical field through pores in a polyacrylamide gel matrix; pore size decreases with increasing acrylamide concentration. The combination of pore size and protein charge, size, and shape determines the migration rate of the protein. In this unit, the standard Laemmli method is described for discontinuous gel electrophoresis under denaturing conditions, i.e., in the presence of sodium dodecyl sulfate (SDS). Download video file.^{(49M, mov)}     

Micellar Electrokinetic Capillary Chromatography of Proteins

Separations of model proteins obtained under denaturing conditions in the presence of micellar concentrations of ionic surfactants displayed high resolution and efficiency using either bare silica or C18-derivatized silica capillaries. Superior migration time reproducibility was achieved through the use of the C18-derivatized capillaries (run-to-run migration time % RSD = 0.2), relative to that obtained in bare silica capillaries (run-to-run migration time % RSD = 2.2), in the absence of buffer replenishment. The effects of surfactant concentration and pH upon the separation of a mixture of five model proteins of varying ionic and hydrophobic character were investigated, and the application of this technique to the analysis of a recombinant DNA-derived protein in fermentation broth was demonstrated.     

Tonoplast and Soluble Vacuolar Proteins Are Targeted by Different Mechanisms

The delivery of proteins to the vacuole and its limiting membrane (the tonoplast) by the secretory system is thought to be a dissociative process in which vesicles bud from one compartment and fuse with another. We studied the transport kinetics of phytohemagglutinin (PHA) and tonoplast intrinsic protein (TIP) in mesophyll protoplasts obtained from transgenic tobacco plants transformed with genes encoding these two proteins. In pulse-chase experiments, arrival of PHA in the vacuole was found to be slower (completed 24 hr after synthesis) than the arrival of TIP in the tonoplast (completed 6 hr after synthesis). Brefeldin A and monensin block protein transport by interfering in specific vesicle transport steps. Brefeldin A prevents anterograde vesicle transport between the endoplasmic reticulum and the Golgi, whereas monensin inhibits correct sorting in the trans-Golgi network by disrupting the proton gradient across the membrane. Both inhibitors blocked the transport of PHA to the vacuole and altered the rate at which its complex glycan is processed by Golgi enzymes. Neither drug stopped the arrival of TIP in the tonoplast, suggesting that the flow of vesicles continues in the presence of these inhibitors. We suggest that soluble proteins like PHA and membrane proteins like TIP reach their vacuolar destinations by different paths.     

高效毛细管电泳分离多种植物激素的方法研究

建立了高效毛细管电泳法分离测定茶叶中赤霉素(GA)、吲哚-3-乙酸(IAA)、脱落酸(ABA)、吲哚-3-丁酸(IBA)、细胞分裂素(CTK)等5种植物激素的分析方法。采用正交试验设计对高效毛细管电泳方法中的运行电压、缓冲液pH值和添加剂SDS浓度等分离条件进行优化,结果发现在30 mmol/L H3BO4-KH2PO4、40 mmol/LSDS组成的pH9.0缓冲液中,选择18 kV电压,25℃柱温和200 nm波长,可在11 min以内实现茶叶中5种激素的分离检测。本方法具有较高的灵敏度,5种激素的相关系数r=0.9907～0.9974,加标回收率为78.06%-95.5%,变异系数≤1.8%。利用本方法测定了茶叶不同部位的5种植物激素的含量变化。     

Fatty Acid Acylated Proteins of the Halotolerant Alga Dunaliella salina

The unicellular, wall-less alga Dunaliella salina has been shown to contain an array of proteins modified by the covalent attachment of fatty acids. Myristic acid (14:0) comprised approximately 80% by weight of the protein-linked acyl groups in samples derived from cells cultured in medium containing 1.7 molar NaCl and 93% in samples from cells grown in medium containing 3.0 molar NaCl. Palmitic and stearic acids accounted for most of the remaining protein-bound acyl chains. Approximately 0.2% of the incorporated radioactivity was estimated to be in linkage with protein. The bulk of acyl chains (about 99%) were resistant to cleavage by alkali, indicating a preponderance of amide bonding. The sodium dodecyl sulfate-polyacrylamide electrophoresis labeling pattern of proteins from [³H]myristic-labeled cells was significantly different from that of proteins from cells exposed to [³H]palmitate. The appearance of radioactivity in certain proteins was also influenced by the salinity of the culture medium. Thus growth in moderate (1.7 molar) salt favored the acylation of a 48-kilodalton polypeptide whereas in high (3.0 molar) salt, a 17-kilodalton polypeptide was more heavily labeled.     

亚硒酸钠诱导的晶状体蛋白质聚合作用

不仅在体内,而且在体外亚硒酸钠可引起晶状体蛋白质聚合。将亚硒酸钠加到pH7.4的晶状体蛋白质溶液中,在37℃保温30min后观察到蛋白质溶液变混浊,随时间的延长混浊程度加重并有沉淀形成。经SDS聚丙烯酰胺凝胶电泳发现,加硒保温后形成的不溶性蛋白质中有大量的高分子聚合物。当加入二硫苏糖醇后混浊的蛋白质溶液变清,其中的高分子聚合物也基本消失,我们还发现;在亚硒酸钠使晶状体蛋白质变混浊的同时,蛋白质巯基减少,而蛋白质结合的硒量增加,且二者之间有较固定的比例关系,即蛋白质上每增加一个硒原子,蛋白质巯基就减少4.26个。当用二硫苏糖醇还原后,68％的硒从蛋白质中释放出来。这些结果表明,亚硒酸钠可引起大鼠晶状体水溶性蛋白质聚合,其可能方式如下:4PSH+SeO_3~-→PSSP+PS-Se-SP+H_2O+2OH~-这可能是亚硒酸钠诱发白内障的主要原因。     

Enhancing Production and Cytotoxic Activity of Polymeric Soluble FasL-Based Chimeric Proteins by Concomitant Expression of Soluble FasL

Membrane FasL is the natural trigger of Fas-mediated apoptosis. A soluble homotrimeric counterpart (sFasL) also exists which is very weakly active, and needs oligomerization beyond its trimeric state to induce apoptosis. We recently generated a soluble FasL chimera by fusing the immunoglobulin-like domain of the leukemia inhibitory factor receptor gp190 to the extracellular region of human FasL, which enabled spontaneous dodecameric homotypic polymerization of FasL. This polymeric soluble human FasL (pFasL) displayed anti-tumoral activity in vitro and in vivo without systemic cytotoxicity in mouse. In the present work, we focused on the improvement of pFasL, with two complementary objectives. First, we developed more complex pFasL-based chimeras that contained a cell-targeting module. Secondly, we attempted to improve the production and/or the specific activity of pFasL and of the cell-targeting chimeras. We designed two chimeras by fusing to pFasL the extracellular portions of the HLA-A2 molecule or of a human gamma-delta TCR, and analyzed the consequences of co-expressing these molecules or pFasL together with sFasL on their heterotopic cell production. This strategy significantly enhanced the production of pFasL and of the two chimeras, as well as the cytotoxic activity of the two chimeras but not of pFasL. These results provide the proof of concept for an optimization of FasL-based chimeric proteins for a therapeutic use.