Control of membrane morphogenesis in bacteriophage PM2

The regulation of membrane formation in bacteriophage PM2 serves as a simple model for changes in membrane structure in eukaryotic cells. Prior to Pseudomonas host lysis, wild-type virions mature to an icosahedral morphology at the inner face of the cytoplasmic membrane. The proliminary charcterization of two temperature-sensitive mutants of PM2 is described. In cells infected at the restrictive temperature with ts 1, an abundance of “empty” virus-size membrane vesicles are seen. Synthesis of DNA is also reduced in ts 1 infected cells. The preponderance of vesicles is not sen in cells infected with wil-type virus or with ts 1 at the permissive temperature. The “empty” appearance of the viral membranes suggests that viral DNA is not encapsulated. The major viral capsid protein (MW 26,000) is located just out side the viral membrane and normallyl sediments with host and virus membranes; insted, large amounts of capsid protein can be precipitated from the supernatant with TCA. Compared to cells infected with wild type virus, cells infected with is 5 at th restrictive temperature produce inside the cell an aboundance of virus-soze membrane vesicles. Taken Together, These results with viral mutants suggest that formation of a viral membrane of the proper size does not require a DNA core around which to form, or an outer scaffolding of coat protein against which to form a spherical bilayer.     

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。     

黑曲霉突变株葡萄糖淀粉酶的化学组成及其光谱学性质

黑曲霉突变株葡萄糖淀粉酶中一型GAI舍糖量为17.6%。氨基酸分析表明,天门冬氨酸和谷氨酸(包括酰胺)占20.3%,苏氨酸和丝氨酸占25.1%,三种碱性氨基酸占6%。紫外光谱在278nm和250nm处分别有最大和最小吸收;其荧光光谱的最大激发波长和发射波长分别为284nm与342nm;远紫外CD谱表现为一双负峰;在溶液中的构象是α-螺旋10.6%,β折叠16.3%和无规卷曲73.1%。     

含硫多肽类抗生素那西肽的菌种诱变及产量提高

那西肽（Ｎｏｓｉｈｅｐｔｉｄｅ）产生菌Ｓｔｒｅｐｔｏｍｙｃｅｓ ａｃｔｕｏｓｕｓ Ｚ１１,经ＮＴＧ处理和对Ｃｕ＾２＋,Ｍｎ＾２＋耐受选育,获得突变株Ｚ１５,其可耐受Ｃｕ＾２＋为３００μｇ／ｍｌ,耐Ｍｎ＾２＋１０００μｇ／ｍｌ,产生那西肽可达１５００μｇ／ｍｌ是Ｚ１１活力的１．６倍。     

理性设计盐桥构建伯克霍尔德菌脂肪酶热稳定突变体

【目的】借助蛋白质工程技术提高伯克霍尔德菌ZYB002脂肪酶LipA的热稳定性,以期更好地将其应用于工业生产中。【方法】利用YASARA、Fold X、Rosetta、Gromacs等生物信息学软件,构建1个脂肪酶Lip A的热稳定性提高的微型突变体电子文库;通过对突变体的结构信息和自由能变化进行评估,筛选出潜在的有价值的突变体。继而利用基因定点突变技术,构建上述候选突变体的突变基因文库,通过实验筛选出热稳定性提高的脂肪酶LipA突变体。【结果】利用上述方法,从构建的20个脂肪酶LipA突变体中,筛选到热稳定性有显著提高的3个突变体LipA-Asn~(125)Asp、LipA-Asn~(125)Glu和LipA-Gln~(262)Glu。经55°C处理12 min后,上述3个突变体的T1250值较野生型分别提高4.0°C、5.5°C和4.4°C;在55°C下的半衰期较野生型分别提高了2.2倍、3.8倍和2.6倍。【结论】利用生物信息学软件,构建脂肪酶LipA突变体电子文库,结合蛋白质的结构信息,可以快速筛选到热稳定性提高的脂肪酶LipA突变体。     

逆境下拟南芥野生型和突变体sex1游离态水杨酸含量及根形态差异

以拟南芥野生型(WT)和突变体sex1为材料,采用HPLC、显微观察等方法,研究了WT在10个不同生长期时游离态水杨酸(SA)含量的变化,比较了在丁香假单胞菌番茄致病变种(Pst.DC3000)、H2O2、甲基紫精(MV)和SA处理环境下WT和sex1中游离态SA含量及幼苗根形态的差异.结果表明:在花序继续开放期(6.30、6.50)以及长角果出现期(8.0),WT中游离态SA含量处在更低水平;2 mmol·L-1 SA处理能够极显著提高WT和突变体sex1中游离态SA的积累,且突变体sex1中游离态SA水平增加更明显,是其他处理游离态SA水平的10倍左右;在MV和H2O2处理下,WT和sex1主根生长受抑制的程度没有明显差异,而突变体sex1幼苗的根毛在低浓度MV环境中比WT更长但密度差异不明显,且WT和sex1根毛在低浓度H2O2环境中差异情况与对照组相似,但外源SA处理使WT和突变体sex1的主根生长均受到明显的抑制,两者的根毛密度随SA增加逐渐降低甚至消失,且突变体sex1比WT受到的抑制作用更明显.研究发现:拟南芥的开花和结果过程与SA依赖途径有一定关系;外源添加SA比Pst.DC3000、H2O2和MV处理更能直接促使拟南芥突变体sex1产生更多的游离态SA;突变体sex1根的生长发育比WT更易受到生长环境条件的影响,且sex1根形态的生长存在一定的SA浓度依赖模式.     

Reversible unfolding of the severe acute respiratory syndrome coronavirus main protease in guanidinium chloride

Chemical denaturant sensitivity of the dimeric main protease from severe acute respiratory syndrome (SARS) coronavirus to guanidinium chloride was examined in terms of fluorescence spectroscopy, circular dichroism, analytical ultracentrifuge, and enzyme activity change. The dimeric enzyme dissociated at guanidinium chloride concentration of <0.4 M, at which the enzymatic activity loss showed close correlation with the subunit dissociation. Further increase in guanidinium chloride induced a reversible biphasic unfolding of the enzyme. The unfolding of the C-terminal domain-truncated enzyme, on the other hand, followed a monophasic unfolding curve. Different mutants of the full-length protease (W31 and W207/W218), with tryptophanyl residue(s) mutated to phenylalanine at the C-terminal or N-terminal domain, respectively, were constructed. Unfolding curves of these mutants were monophasic but corresponded to the first and second phases of the protease, respectively. The unfolding intermediate of the protease thus represented a folded C-terminal domain but an unfolded N-terminal domain, which is enzymatically inactive due to loss of regulatory properties. The various enzyme forms were characterized in terms of hydrophobicity and size-and-shape distributions. We provide direct evidence for the functional role of C-terminal domain in stabilization of the catalytic N-terminal domain of SARS coronavirus main protease.     

Production and Accumulation of Xylooligosaccharides with Long Chains by Growing Culture and Xylanase of a Mutant Strain of Bacillus pumilus X-6-19

Bacillus pumilus X-6-9 isolated from soil and subsequently identified, produced xylooligosacchatides with long chainsfrom xylan and accumulated them in the culture. By improving the culture conditions and mutating the bacterium, a 3.2-fold increasein the production of the xylooligosaccharides was established, when compared to the original culture conditions of B. pumilus X-6-19.The addition of D-glucose to the culture of the mutant swain U-3 of B. pumilus X-6-9 repressed the synthesis of β-xylosidase, but notxylanase. Thus, it was revealed that strain U-3 was a good organism for the production and accumulation of xylooligosaccharideswith long chains from xylan by a microbial culture. Xylanase produced by strain U-3 was purified to homogeneity and characterized.The hydrolyzates generated by the purified xylanase contained xylobiose, xylotrinse, xylotewaose, and xylopentaose, but not xylose.