湿地生态系统健康评价指标体系Ⅰ.理论

湿地生态系统健康是一个新的研究领域。主要从湿地生态系统指标的概念出发,阐述了选择生态系统指标的基本理论,分析了湿地生态特征指标体系,湿地功能整合性指标体系和湿地社会政治环境指标体系所包含的基本内涵,特别强调了生态系统结构和内在功能是生态特征的主要表现。功能整合性是湿地生态系统健康的外在表现,同时,社会政治环境因素中,政策法规,总体规划,政策保障,公众参与程度,代际周期的社会公平性,个人接受能力,团体接受能力等是影响湿地生态系统健康的重要因素。     

代谢工程酵母菌合成紫杉烯的研究

紫杉烯是紫杉醇生物合成的重要中间体,为在酿酒酵母(Saccharomyces cerevisiae)中建立一个生物合成紫杉烯的代谢途径,克隆了酵母的羟甲基戊二酰CoA(3-hydroxy-3-methylglutarylcoenzyme A,HMG-CoA)还原酶基因和=牛儿基=牛儿基二磷酸(geranylgeranyl diphosphate,GGDP)合酶基因,并构建了其融合表达载体pGBT9/HG;同时构建了包含紫杉烯合酶基因的表达载体pADH/TS;将这两个表达载体共转化酵母细胞,通过GC-MS分析检测工程酵母的代谢产物,结果表明获得的工程酵母能够合成紫杉烯,即在酵母细胞中建立了一个合成紫杉烯的代谢途径。     

RNA 沉默的病毒抑制子

RNA 沉默是一种在真核生物体内普遍保守的、通过核酸序列特异性的相互作用来抑制基因表达的调控机制 . RNA 沉默的一种重要生物学效应是防御病毒的侵染,而针对寄主的这种防御机制,许多植物病毒已演化通过编码 RNA 沉默的抑制子来克服这种防御反应 . 目前,已从植物、动物和人类病毒中鉴定了 20 多种 RNA 沉默的抑制子,围绕抑制子的鉴定和作用机理研究已成为病毒学研究的一个热点 . 对 RNA 沉默抑制子的发现、鉴定方法、作用机理及与病毒病症状形成的关系、动物病毒的沉默抑制子等方面的最新进展做了综述,并对沉默抑制子的应用和存在的问题进行了讨论 .     

Dynamic osmotic loading of chondrocytes using a novel microfluidic device

Many cells exhibit disparate responses to a mechanical stimulus depending on whether it is applied dynamically or statically. In this context, few studies have examined how cells respond to dynamic changes of the extracellular osmolality. In this study, we hypothesized that the cell size change response of cultured articular chondrocytes would be dependent on the frequency of applied osmotic loading. To test this hypothesis, we developed a novel microfluidic device, to apply hydrostatic pressure-driven dynamic osmotic loading by applying composition modulated flow, adapted from Tang and co-workers. This microfluidic device was used to study osmotic loads of +/-180 mOsm at a frequency up to 0.1 Hz with a constant minimal fluid-shear stress, and permit real-time monitoring of cell responses. Bovine articular chondrocytes were observed to exhibit increasing changes in cell volume with decreasing osmotic loading frequency. When the cell volume response was modeled by an exponential function, chondrocytes exhibited significantly different volume change responses to dynamic osmotic loading at 0.0125 Hz and static osmotic loading applied for a period of four minutes (Delta = +/-180 mOsm relative to the isotonic 360 mOsm). The intracellular calcium response at 0.0125 Hz was also monitored and compared with the response to static loading. Coupled with phenomenological or constitutive models, this novel approach could yield new information regarding cell material properties in response to dynamic loading that may contribute new insights into mechanisms of cellular homeostasis and mechanotransduction.     

蜂毒素分子的改造及其基因在毕赤酵母中的表达

为获得保留有抗菌活性而降低溶血作用的蜂毒素,对蜂毒素的分子结构进行了改造。将第5位的Val变为Arg,第15位Ala变为Arg,删除了第16位的Leu。用PCR技术获得了改造后的蜂毒素基因,将其克隆入酵母表达载体pPICZa-A,获得重组表达质粒pPICZa-A-MEA。该质粒转化毕赤酵母菌GS115,甲醇诱导下表达,发酵上清液经抑菌活性、溶血活性测定及亲和层析纯化,结果表明,蜂毒素基因成功地在毕赤酵母中表达,经改造后表达的蜂毒素保留了抗菌活性且溶血活性显著降低,经纯化后用Bradford法测定表达蜂毒素的含量约为0.29mg／ml。     

Kinetic difference of berberine between hippocampus and plasma in rat after intravenous administration of Coptidis rhizoma extract

In order to investigate the pharmacokinetics of berberine in Coptidis rhizoma extract in rat hippocampus and plasma, a simple and accurate high-performance liquid chromatography method was employed in this study. Berberine was determined using a Hypersil C(18) column with an isocratic mobile phase of acetonitrile-0.05 M potassium dihydrogen phosphate (containing 0.5% triethylamine, pH 3.0) and with UV detection at 236 nm. The lower limit of quantification for berberine in both hippocampus and plasma was 24 ng/ml, and the lowest concentrations of berberine determined in rat hippocampus and plasma samples were 30.7 ng/ml at 48 h and 38.5 ng/ml at 4 h, respectively. The calibration curve for berberine was linear over the concentration range 24--6000 ng/ml. At this concentration range, the overall recoveries (90.6--94.2%) for berberine were determined and the accuracy of intra- and inter-day assays from rat samples were less than 7% RSD. Following intravenous administration of C. rhizoma extract at a dose of 10.2 mg/kg containing 3 mg/kg berberine, berberine in the plasma eliminated rapidly (t(1/2 beta)=1.13 h). However, berberine in the hippocampus increased rapidly (t(1/2 alpha)=0.215 h), peaked at 3.67 h with a concentration of 272 ng/g, and had a slow elimination rate (t(1/2 beta)=12.0 h), which suggests that berberine could have a direct action on neuron and accumulate in the hippocampus. This study first showed the pharmacokinetic characteristics of berberine in rat hippocampus and the kinetic characteristics of berberine are dissimilar in the hippocampus and plasma.     

槲皮素诱导Hep G2自噬与胞内游离Ca2+浓度的变化相关

槲皮素具有诱导细胞自噬、抑制肿瘤细胞增殖等抗癌功能,但其诱导细胞自噬的分子机制还不太清楚. 本文通过激光共聚焦显微镜观察槲皮素对Hep G2细胞自噬的影响; Fluo-3 AM和Cyto-IDTM Green Detection Reagent染色标记, 流式细胞术测定了槲皮素对Hep G2细胞内游离钙离子浓度［Ca2+］_i 及Ca2＋螯合剂BAPTA-AM对自噬水平的影响. 探讨了槲皮素诱导人肝癌细胞 Hep G2自噬过程中［Ca2+］i的变化. 结果表明, 在槲皮素较低浓度范围内(0 ～ 50 μg/mL), 可明显抑制Hep G2细胞增殖, 并以剂量依赖方式诱导细胞自噬. 同时发现,槲皮素刺激Hep G2细胞可使［Ca2+］i明显增加, 进而促进自噬. 而当胞内Ca2＋螯合剂 BAPTA-AM存在时, 细胞的自噬水平受到一定的抑制. 这些结果表明,细胞内［Ca2+］i的升高可促进自噬, ［Ca2+］_i 的降低可能会抑制自噬. Hep G2细胞自噬与细胞内游离钙离子浓度的变化有关系.     

典型气候条件下东北地区生态系统水源涵养功能特征

东北地区是我国重要的生态功能区,其包含的典型生态系统具有独特的水源涵养功能,在防洪减灾,保障生态安全和人居安全中发挥着关键作用。以往有关水源涵养功能的研究主要是依托不同水文模型方法,从单一年份或多个年份的角度进行研究,较少考虑不同气候条件下水源涵养功能的空间分异特征。采用标准化降水蒸散发指数(Standardized Precipitation Evapotranspiration Index,SPEI)划分研究区的典型气候年份(干旱、正常和湿润);基于水量平衡法,结合SCS-CN模型以及Penman-Monteith方程对东北地区典型气候条件下生长季内的水源涵养功能进行研究。结果表明:(1)研究区水源涵养功能在不同气候条件下差异明显,三个典型气候年份生长季内的水源涵养总量分别为:干旱年(SPEI=-1.26)为2214.64亿m~3、正常年(SPEI=-0.22)为3231.49亿m~3和湿润年(SPEI=1.05)为3969.33亿m~3。(2)水源涵养功能空间变异突出,但在三种典型气候条件下呈现出一致变化,均表现为长白山地区水源涵养量最大,大小兴安岭地区次之,水源涵养量最低的地方主要出现在呼伦贝尔以西的草原地区,在东北平原的部分地区也有低值的出现,如白城、通辽、鸡西等地区,水源涵养量较一般的地方出现在东北平原大部分以农田为主的地区。(3)水源涵养功能除受气候因素的影响外,还取决于土地利用类型的变化,对于整个东北地区来讲,水源涵养总量表现为林地农田草地湿地,单位面积水源涵养量在干旱年和正常年表现为林地农田湿地草地,在湿润年份表现为林地湿地农田草地。研究结果揭示了东北地区三种典型气候条件下重要生态系统的水源涵养功能大小、空间分布特征及其主要驱动因素,可为区域生态空间规划和生态系统管理提供科学指导。     

平滑肌肌球蛋白轻链激酶N端删除载体的构建

目的:构建重组平滑肌肌球蛋白轻链激酶(myosin light chain kinase,MLCK)N端删除栽体,为研究平滑肌MLCK的分子机制提供研究模型.方法:以重组质粒pCoid/155为模板,根据其待删除序列(N端1-41个氨基酸)设计上下游引物,行PCR扩增.将扩增片段以NdeI/EeoRl双酶切,产物行琼脂糖凝胶电泳回收得到目的基因.将目的基因与栽体连接,转化至大肠杆菌.筛选阳性克隆,并对阳性克隆进行测序.结果:用NdeI和EcoRI双酶切重组质粒pCold/155,琼脂糖凝胶电泳显示得到约4.4kb栽体和约3.4kb的MLCK片段.阳性克隆经测序证实MLCK的N端41个氨基酸序列已被成功删除.结论:成功构建了重组MLCK N端删除栽体 pCold/155/D41.