概念图及其在教与学中的应用

1 关于概念图的概述概念 图是一种关于概念知识、思维过程或思维结果、系统结构、计划流程等的图形化表征方式，它由节点、链接（节点间的连线）和节点间的关联词组成。康奈尔大学的Joseph D．Novak博士根据奥苏贝尔（David P．Ausubel）学习理论于1960年始研究概念图技术，并使之成为一种教学工具。学生利用概念图进行知识的自主建构，教师利用概念图引导和考察学生组织知识、理解知识的过程，都与建构主义学习观是一致的。     

绣球菌多糖表征及其抗氧化和免疫活性

提取纯化绣球菌多糖(Sparassis latifolia polysaccharides,SCPs),研究其表征和功能活性,探索绣球菌多糖表征与其抗氧化及免疫活性之间的关系。以绣球菌子实体为原料,采用聚能超声波辅助水提醇沉法提取绣球菌多糖,经DEAE-52、SephadexG-100纯化,用高效凝胶渗透色谱法、离子色谱法、傅里叶红外色谱法、扫描电镜、原子力显微镜对绣球菌多糖进行初步表征,检测绣球菌多糖清除DPPH、·OH、O2^-·自由基能力以及总还原力,用MTT法检测绣球菌多糖对巨噬细胞RAW264.7增殖的影响。结果表明,SCPs分子量范围为215Da–393kDa,由葡萄糖、甘露糖、半乳糖、木糖、果糖构成,摩尔比13:4:1:2:3,其表观形貌为簇状堆积,交织,结构规律性不强,表面光滑,呈一定的网络状结构,分子呈现链状构象,具有高度的分支结构,链间形成小环且伴随一定的球形颗粒。SCPs具有一定的还原能力和清除DPPH、·OH、O2^-·自由基的能力,且能够促进巨噬细胞RAW264.7的增殖。绣球菌多糖的抗氧化及免疫活性可能与其分子量、单糖组成、糖链分支及分子构象有关。     

Ag/TiO2纳米材料对烟曲霉的抑制作用及机制

目的合成Ag/TiO_2纳米材料,对其进行表征测定,并探讨其对烟曲霉的抑制作用及具体机制。方法采用光催化还原法制备Ag/TiO_2纳米材料,紫外可见分析和扫描电镜对其进行表征测定;微量液基稀释法检测对烟曲霉的最低抑菌浓度(MIC),以及生物量的抑制作用;ELISA试剂盒检测对真菌谷胱甘肽还原酶、总谷胱甘肽、线粒体膜电位的影响,荧光显微镜检测活性氧的产生。结果成功制备Ag/TiO_2纳米材料,分布均匀;对烟曲霉的MIC值为0.5μg/mL,能完全抑制烟曲霉生物量,与单独纳米银相比,具有更好的抗菌活性。机制研究发现其主要通过降低烟曲霉体内谷胱甘肽及其还原酶的含量,诱导过量活性氧的产生,最终导致线粒体膜电位降低,使真菌细胞发生凋亡。结论 Ag/TiO2纳米材料可有效阻断烟曲霉等真菌在空气中的传播,具有广泛的应用前景。     

苹果多酚氧化酶的纯化与表征

运用丙酮浸漬干燥、磷酸盐缓冲液提取、低温离心、硫酸铵沉淀、DEAE-Sephadex(A-50)、Sephadex(G-75) 和DEAE-celluse(DE-52)层析等方法从苹果中分离获得一种新的含铜酶蛋白,该酶被命名为多酚氧化酶Ⅱ(polyphenol oxidase Ⅱ, PPOⅡ),纯化倍数是215,纯化收率是23%.PAGE、SDS-PAGE和MALDI-TOF 等技术用于测定所获的酶的纯度和分子量.在PAGE和SDS-PAGE 均显示一条带,表明PPOⅡ只由一个亚基组成,且已达到单一组分(MALDI-TOF的结果更证实了这一点).SDS-PAGE 和 MALDI-TOF 的结果都表明PPO的分子量为 38204 Da.pH值对酶活性和稳定性研究的结果显示,从pH值4.0～7.0随着pH值的增加,酶活性也不断增加;从pH值 7.0～11.0, 酶活性不断降低.PPOⅡ的最适pH值为6.6最适温度为30℃.     

耐高盐枯草芽孢杆菌XP合成球形纳米硒及其抑制草莓病原真菌生物活性

生物方法合成纳米材料具有低能耗、高安全性以及环境友好等优良特点,因而备受人们关注。利用细菌将硒酸盐或亚硒酸盐还原为单质硒,不仅可以降低硒毒性,而且还能获得价值更高的生物纳米材料。文中选用可耐受高盐环境胁迫的枯草芽孢杆菌亚种Bacillus subtilis subspecies stercoris strain XP构建生物模型,分别以LB液体培养基和亚硒酸钠为介质和底物 (电子受体),解析菌株XP合成纳米硒的基本规律。通过扫描电镜 (Scanning electron microscope,SEM) 观察、X射线能谱分析 (X-ray energy dispersive spectral analysis,EDAX)、X射线衍射 (X-ray diffraction,XRD) 分析、傅里叶红外变换光谱 (Fourier transform infrared spectroscopy,FTIR) 技术对合成的纳米硒进行物理化学表征分析,同时选用草莓枯萎、红叶、紫斑病病原真菌对其抗菌活性进行分析。结果表明,菌株XP介导合成的单质硒为球形纳米颗粒 (Selenium nanoparticles,SeNPs),其生成量与反应时间呈正相关 (0–48 h),且细胞形态未发生褶皱或破损等变化 (耐受力强);SeNPs为非晶态,粒径范围在135–165 nm,表面元素组成以Se为主,同时存在C、O、N、S等有机元素;颗粒表面包裹生物大分子物质,-OH、C=O、N-H、C-H等官能团与SeNPs稳定性和生物活性密切相关;高浓度纳米硒对枯萎、红叶、紫斑病病原真菌均有显著抑制活性 (P<0.05),其中对草莓红叶病与枯萎病病原真菌的抑制活性明显优于对紫斑病病原真菌的抑制活性。总而言之,菌株XP不仅耐受高盐胁迫能力强,同时还可介导合成生物SeNPs,其合成的纳米硒颗粒具有良好的稳定性和生物活性,在草莓病害防治以及绿色富硒草莓种植等领域具有潜在的应用价值。     

Towards Characterization of the Chloroplast NAD（P）H Dehydrogenase Complex

The NAD（P）H dehydrogenase （NDH） complex in chloroplast thylakoid membranes functions in cyclic electron transfer, and in chlororespiration. NDH is composed of at least 15 subunits, including both chloroplast- and nuclear-encoded proteins. During the past few years, extensive proteomic and genetic research on the higher plant NDH complex has been carried out, resulting in identification of several novel nuclear-encoded subunits. In addition, a number of auxiliary proteins, which mainly regulate the expression of chloroplast-encoded ndh genes as well as the assembly and stabilization of the NDH complex, have been discovered and characterized. In the absence of detailed crystallographic data, the structure of the NDH complex has remained obscure, and therefore the role of several NDH-associated nuclear-encoded proteins either as auxiliary proteins or structural subunits remains uncertain. In this review, we summarize the current knowledge on the subunit composition and assembly process of the chloroplast NDH complex. In addition, a novel oligomeric structure of NDH, the PSI/NDH supercomplex, is discussed.     

Expression,purification and characterization of recombinant protein tyrosine phosphatase from Thermus thermophilus HB27

The low-molecular-weight protein tyrosine phospha- tases （PTPase） exist ubiquitously in prokaryotes and eukaryotes and play important roles in the regulation of physiological activities. We report here the expression, purification and characterization of an active and soluble PTPase from Thermus thermophilus HB27 in Escherichia coli. This PTPase has an optimum pH range of 2.8-4.8 when using p-nitrophenyl phosphate as the substrate. The thermal inactivation results indicate a high thermal stability of this enzyme, with the optimum temperature of 75℃ for activity. It can be activated by Mn^2＋, Mg^2＋, Ca^2＋, Ba^2＋, and Ni^2＋, but inhibited by Zn^2＋, Cu^2＋, Cl^-, and SO^2-. These results suggest that this heat-resistant PTPase may play important roles in vivo in the adaptation of the microorganism to extreme temperatures and specific nutritional conditions.     

Characterization of the putative tryptophan synthase β-subunit from Mycobacterium tuberculosis

The increasing emergence of drug-resistant tuberculosis （TB） poses a serious threat to the control of this disease. It is in urgent need to develop new TB drugs. Tryptophan biosynthetic pathway plays an important role in the growth and replication of Mycobacterium tuberculosis （Mtb）. The β-subunit of tryptophan synthase （TrpB） catalyzes the last step of the tryptophan biosynthetic pathway, and it might be a potential target for TB drug design. In this study, we overexpressed, purified, and characterized the putative TrpB-encoding gene Rv1612 in Mtb H37Rv. Results showed that Mtb His-TrpB optimal enzymatic activity is at pH 7.8 with 0.15 M Na^＋ or 0.18 M Mg^2＋ at 37℃. Structure analysis indicated that Mtb TrpB exhibited a typical β/α barrel structure. The amino acid residues believed to interact with the enzyme cofactor pyridoxal-5＇-phosphate were predicted by homology modeling and structure alignment. The role of these residues in catalytic activity of the Mtb His-TrpB was confirmed by site-directed mutagenesis. These results provided reassuring structural information for drug design based on TrpB.     

Immunoaffinity purification and characterization of glyceraldehyde-3-phosphate dehydrogenase from human erythrocytes

A new procedure utilizing immunoaffinity column chromatography has been used for the purification of glyceraldehyde-3-phosphate dehydrogenase （GAPDH, EC 1.2.1.12） from human erythrocytes. The comparison between this rapid method （one step） and the tra- ditional procedure including ammonium sulfate fractionation followed by Blue Sepharose CL-6B chromatography shows that the new method gives a highest specific activity with a highest yield in a short time. The characterization of the purified GAPDH reveals that the native enzyme is a homotetramer of -150 kDa with an absolute specificity for the oxidized form of nicotinamide adenine dinucleotide （NAD＋）. Western blot analysis using purified monospecific polyclonal antibodies raised against the purified GAPDH showed a single 36 kDa band corresponding to the enzyme subunit. Studies on the effect of temperature and pH on enzyme activity revealed optimal values of about 43℃ and 8.5, respectively. The kinetic parameters were also calculated： the Vmax was 4.3 U/mg and the Km values against G3P and NAD＋ were 20.7 and 17.8 μM, respectively. The new protocol described represents a simple, economic, and reproducible tool for the purification of GAPDH and can be used for other proteins.     

亲淋巴磁共振造影剂的合成、表征和性能研究

目的:探讨合成亲淋巴造影剂的方法并对其体内外性能进行研究.方法:采用二氨基乙基乙二醇醚(EOEA)-二乙三胺五乙酸(DTPA)线性共聚合物(poly-DTPA-EOEA)为配体,与钆(Gd)的三价盐配位构建T1类线性大分子造影剂,检测二氨基乙基乙二醇-DTPA酰胺共聚物钆配合物(Gd-poly-DTPA-EOEA)的表征和性能.结果:Gd-poly-DTPA-EOEA分子量为20kDa,其中钆的含量为14%(w/w).T1值为6.45L mM-1s-1.Gd-poly-DTPA-EOEA在血液中的存留时间明显长于小分子造影剂Gd-DTPA,并可进入淋巴结巨噬细胞内.结论:Gd-poly-DTPA-EOEA是一种具有高驰豫率、循环时间长和亲淋巴特性的T1类大分子造影剂.