产小檗碱诱变菌株培养条件的优化

S-NU-3-2菌株是对源自药用植物黄檗的内生真菌S6进行诱变获得的小檗碱产量比出发菌株有明显提高的突变株,本研究对其培养条件进行了优化,以期进一步提高其产量,为开发利用真菌发酵生产植物活性成分的新途径奠定基础。以菌丝生长和小檗碱产量为指标,筛选出了适宜该菌株发酵的基本培养基、碳源、氮源、光照和培养温度,并经进一步的正交试验优化,得出该高产菌株的最佳培养条件为豆芽汁基本培养基含蔗糖3%,酵母膏0.2%,pH7.0,温度26℃,全光照培养。与初始培养条件相比,在优化后的条件下,该菌株的小檗碱得率提高了47.2%,菌体生物量提高了24%。     

Evidence for a Hyperexcitability State of Staggerer Mutant Mice Macrophages

We recently reported an abnormal production of interleukin-1 (IL-1) in peripheral macrophages of several neurological mutant mice that exhibit patterns of neuronal degeneration, especially in the cerebellum. After in vitro activation by lipopolysaccharide acid (LPS), these macrophages hyperexpress IL-1 beta mRNA and hyperproduce IL-1 protein in comparison with +/+ controls. In the present study, focused on the staggerer mutant mice, we investigate if this genetic dysregulation is specific for IL-1 beta or if it reflects a generalized hyperexcitability of these macrophages. The hyperexpression of IL-1 beta mRNA in sg/sg macrophages is present whatever the duration of LPS stimulation, even for periods as short as 15 min, although it reaches a maximum after 4 h of stimulation. The hyperinducibility of sg/sg macrophages is observed even when very low doses of LPS are used (0.01 microgram/ml) and reaches its maximum for 5 micrograms/ml LPS. Synthetic molecules (muramyl dipeptides), such as N-acetylmuramyl-L-alanyl-D-isoglutamine or murabutide, known as macrophage activators, are also efficient in revealing the cytokine hyperexpression in sg/sg macrophages. In addition, hyperexpression of two other cytokines, i.e., tumor necrosis factor-alpha and IL-1 alpha mRNAs, is also detected in LPS-stimulated macrophages of mutant mice. Finally, the effect of an inhibitor of protein synthesis, cycloheximide, is similar in +/+ and sg/sg macrophages. As a whole, these data lead us to conclude that the sg/sg macrophages are in a state of general hyperexcitability when compared with +/+ ones.     

Some Characteristics of Pseudomonas 0–3 which Utilizes Polyvinyl Alcohol

Pseudomonas 0–3 strain which was isolated from soil can grow on polyvinyl alcohol (PVA) as a sole carbon source. When 0.5 per cent of PVA (500, 1500 or 2000) was employed as the carbon source in the culture medium, PVA was almost completely lost from the culture fluid after a week and the concentration of total organic carbon measured by a TOC analyzer decreased from the initial value of about 2700 ppm to 250~300 ppm after 7~10 days culture. This bacterium was found to produce and secrete an inducible enzyme which degrade PVA. The way by which this enzyme degrades PVA was examined and the results were obtained which suggested that PVA was broken down oxidatively in a way of endowise splitting. However, the mechanism of PVA degradation has not been clarified yet. The optimum pH and temperature for enzyme activity were examined and they were 7.5~8.5 and 35~45°C, respectively. Morphological and biological characteristics of this bacterium were examined and it was similar to a strain of Pseudomonas boreopolis.     

固氮酶铬铁蛋白的晶体生长

在合适的结晶条件下 ,从含Cr无氨培养基中生长的固氮菌 (AzotobactervinelandiiLipmann)突变种UW3 中纯化出的CrFe蛋白可从溶液中析出深棕色斜四棱柱晶体 ,晶体最大的两条对角线长度分别可达 0 .2 5mm和 0 .12mm。PEG 80 0 0、MgCl2 、NaCl、Tris和Hepes缓冲液的浓度及结晶方法等对该蛋白的出晶率、晶核数目、晶体大小和质量都有明显影响。CrFe蛋白结晶所需的上述化合物的最适浓度与在Mn中生长的固氮菌突变种UW3 的MnFe蛋白和缺失nifZ固氮菌突变种的ΔnifZMoFe蛋白结晶所需的最适浓度有所不同。结果表明 ,该蛋白晶体可能为CrFe蛋白的晶体     

2-Deoxyglucose Incorporation in the Cerebellum of Weaver and Nervous Mutant Mice

Abstract: The 2-deoxyglucose autoradiographic method has been used to study activity in cerebellum of the weaver and nervous mutant mice. Patterns of 2-deoxyglucose incorporation into the cerebral hemispheres from weaver and nervous strains did not differ significantly from those of the controls. In the normal cerebellum, 2-deoxyglucose incorporation was maximal in the granular layer, where mossy fibers form synapses with the dendrites of granule cells. In the cerebellum of nervous mice, which lacks Purkinje cells, the incorporation of the 2-deoxyglucose was maximal in the granular layer, but the incorporation into the molecular layer appeared less than in the control. The incorporation into the cerebellum from weaver, which lacks granule cells, was much higher than that of the control, the maximal incorporation being found in the Purkinje cell layer and in cell masses located in the white matter. These data suggest that the heterologous synapses that mossy fibers or climbing fibers form with the cells in the Purkinje cell layer and the cells in the white matter in the weaver cerebellum are functional.     

低氮下拟南芥叶酰聚谷氨酸合成酶突变体atdfb根发育研究

利用叶酰聚谷氨酸合成酶功能缺失突变体atdfb解析叶酸在拟南芥根发育过程中的生物学功能。纯合T-DNA插入功能缺失突变体atdfb 在土壤培养条件下生长3周,与野生型表型无明显差异。在氮源充足的1/2MS培养基上,atdfb的主根显著短于野生型,互补植株的主根长度恢复到野生型水平,说明主根缩短的表型是由AtDFB基因功能缺失造成的。在1/2MS培养基生长11 d的突变体主根长度只有野生型的23%。在低氮条件下,突变体的生长发育几乎停滞,培养11 d的突变体主根长度只有野生型的4%;5-甲酰四氢叶酸(5-F-THF)可以恢复低氮条件下atdfb-3的表型,其主根长度、根毛长度及静止中心的细胞排列均得到恢复。进一步分析发现,低氮条件下培养少于3 d的atdfb-3补充充足的5-F-THF,3 d后能像野生型一样适应低氮环境。由此说明叶酸对拟南芥根部发育及对低氮环境的适应是必需的。     

kpsE和kpsD双基因缺失显著降低肠道外致病性大肠杆菌的毒力

【目的】探究荚膜对肠道外致病性大肠杆菌致病作用的影响。【方法】选取负责荚膜多糖转运的基因kpsE和kpsD,利用λRed重组系统构建APEC E058和UPEC U17荚膜缺失株E058ΔkpsED和U17ΔkpsED,并通过一系列的体内及体外试验对其生物学特性及致病性进行研究。【结果】双基因缺失株的生长速度较野生株没有明显差异,但缺失株抗血清补体杀菌能力和抗鸡巨噬细胞HD-11细胞吞噬能力显著下降。1日龄雏鸡LD50致病性试验结果显示,缺失株E058ΔkpsED和U17ΔkpsED对鸡失去致病力,而回复株毒力恢复至野生株水平;35日龄SPF鸡体内动态分布和竞争试验显示ΔkpsED缺失株在鸡体内定殖能力和竞争性生长能力显著下降,表明kpsED双基因的缺失能显著降低APEC E058和UPEC U17的致病力。【结论】荚膜与肠道外致病性大肠杆菌的致病性相关,是其重要的毒力因子。     

拟南芥DTX31基因表达研究

以模式植物拟南芥为材料,通过PCR和RT-PCR在DNA和RNA水平上筛选鉴定了DTX31基因对应的T-DNA插入突变体,对其表型变化进行了观察.通过半定量RT-PCR分析检测了DTX31基因在拟南芥不同器官及环境胁迫响应中的表达情况,结果发现:DTX31基因在根中表达最高,而在茎、叶、叶柄、花中的表达则较弱;盐和赤霉素使DTX31基因的表达迅速升高,盐胁迫2 h后的表达量达到最高峰,GA处理1 h时就达到最高峰,热激使DTX31基因的表达变化不明显.因此,推测该基因可能是盐和GA信号传导通路中的一个重要调控因子.     

重组人可溶性B淋巴细胞刺激因子及其突变体的克隆、表达及活性测定

采用RT PCR方法从人外周血白细胞总RNA中钓取人可溶性B淋巴细胞刺激因子 (humansolubleBlym phocytestimulator,hsBLyS)的cDNA片段 ,再运用基因重组手段 ,利用通用型质粒pBV2 2 0构建表达载体pBV2 2 0 /hsBLyS。经测序鉴定后 ,以之为模板使用重叠PCR法扩增得到hsBLyS的两个点突变体hsBY A(Cys14 6→Ala14 6)和hsBY V (Cys14 6→Val14 6)的基因片段 ,构建表达载体 pBV2 2 0 /hsBY A及 pBV2 2 0 /hsBY V。经测序无误后 ,将上述 3种载体分别转化大肠杆菌DH5α并诱导重组蛋白质表达 ,薄层扫描结果显示 3种蛋白质在DH5α中表达量都在 2 0 %～ 30 %之间。再分别运用变性、凝胶过滤层析及复性等手段纯化目的蛋白质 ,最后通过B淋巴细胞增殖实验检测纯化产物促人B细胞增殖的活性。实验结果表明 ,3种重组蛋白质都能明显刺激人B细胞增殖 ;统计学检验显示 ,突变体rhsBY V较野生型rhsBLyS的促人B淋巴细胞增殖活性显著增强。