山药粗多糖的提取工艺

对鲜山药中水溶性粗多糖的提取工艺进行了研究,通过单因素试验和L9（34）正交试验,研究了料液比、提取温度、时间和乙醇体积分数对粗多糖得率的影响,极差分析及方差分析结果表明提取温度和料液比是影响山药粗多糖提取的主要因素,较优的工艺为料液比1 g：9 mL,温度50 ℃,时间2.5 h,乙醇体积分数75%,在此工艺条件下,鲜山药粗多糖得率为0.2449%（以鲜山药质量计）.     

枳椇子总黄酮提取工艺及其解酒作用

分别用水和乙醇作为溶剂加热提取枳椇子中的总黄酮,用比色法测定黄酮的含量,分别以提取时间、加热温度、料液比、提取次数等因素进行正交试验.对两种提取方法进行比较,确定各因素对提取效果的影响并对其解酒作用进行研究.水提取法的最优条件是：100 ℃,料液比1 g：8 mL,加热0.5 h,回流提取3次;醇提取法的最佳条件：80 ℃,料液比1 g：6 mL,加热1.5 h,以体积分数50%的乙醇回流提取3次.实验结果显示,醇提取法比水提取法效果更好,枳椇子提取液具有一定的解酒作用.     

RP—HPLC用于紫苏油及其习用品白苏油,野苏油的鉴别

本文采用RP－HPLC方法对紫苏油及其习用品白苏油、野苏油甘油酯进行了定性定量分析。利用HPLC分析油脂也为中药材真伪鉴别提供了一条有效途径。     

Septal innervation of mossy cells in the hilus of the rat dentate gyrus: an anterograde tracing and intracellular labeling study

 Mossy cells in the hilus of the rat dentate gyrus are the main cells of origin of the dentate commissural and associational projections. They project along the septotemporal axis of the dentate gyrus and may thus influence the hippocampal signal flow in a longitudinal direction. To analyze the septal innervation of these hilar neurons, anterograde tracing with Phaseolus vulgaris leucoagglutinin (PHAL) was used in combination with intracellular labeling of mossy cells (Lucifer yellow). Anterogradely labeled septal fibers impinge on proximal and distal dendrites of hilar mossy cells but spare the cell body. In contrast, numerous aspiny hilar neurons, presumably GABAergic interneurons, receive a septal innervation on their somata and proximal primary dendrites. These data demonstrate that septal fibers show a specificity for the dendritic segments of hilar mossy cells. Since mossy cells project predominantly to adjacent hippocampal lamellae, the activity of adjacent portions of the dentate gyrus may be influenced by the septal input onto these neurons. Received: 22 July 1996 / Accepted: 24 October 1996     

鱼腥草的研究进展

综述了鱼腥草在分布,栽培,化学成分,药理作用,临床应用及产品开发等方面的研究进展,并对鱼腥草今后研究和方向进行了展望。     

2-异丁基苹果酸葡萄糖氧基苄酯类对照提取物在白及质量控制中的应用研究

目的 建立以2-异丁基苹果酸葡萄糖氧基苄酯类对照提取物为对照的白及质量控制方法。方法 采用ZORBAX Eclipse Plus C₁₈(100 mm×2.1 mm,1.8μm)色谱柱,流动相为0.05%磷酸水溶液(A)-乙腈(B),梯度洗脱,柱温35℃,体积流量0.15 mL/min,进样体积为2μL,检测波长为220 nm。分别采用对照品法和对照提取物法测定17批白及饮片中1,4-二[4-(葡萄糖氧)苄基]-2-异丁基苹果酸酯-2-葡萄糖苷(2-O-葡萄糖基白及苷)、1-[4-(葡萄糖氧)苄基]-2-异丁基苹果酸酯(手参苷Ⅰ)、1,4-二[4-(葡萄糖氧)苄基]-2-异丁基苹果酸-2-(6-O-乙酰基)葡萄糖苷(手参苷Ⅲ)、1,4-二[4-(葡萄糖氧)苄基]-2-异丁基苹果酸酯(白及苷)4个成分的含量,并进行比较。结果 2-异丁基苹果酸葡萄糖氧基苄酯类对照提取物中2-O-葡萄糖基白及苷、手参苷Ⅰ、手参苷Ⅲ、白及苷线性关系良好(r≥0.999 9),进样精密度RSD值在0.001%～0.58%,重复性RSD值在0.27%～0.53%,4种成分的加样回收率在98....     

参与连翘苯丙烷合成途径的WRKY转录因子的筛选与鉴定

目的 筛选出参与连翘Forsythia suspensa苯丙烷合成途径的WRKY转录因子并进行生物信息学分析。方法 通过对从连翘转录组数据中筛选出的62条连翘WRKY基因序列进行鉴定;通过采用蛋白理化性质和基序分析、蛋白结构分析、系统进化分析、功能注释、蛋白互作分析、外源激素处理后实时荧光定量分析等方式进行相关分析。结果 最终筛选出52条具有WRKY结构域的连翘WRKY转录因子。WRKY转录因子编码蛋白的氨基酸数目在105～728,相对分子质量在12277.95～80 321.99。蛋白基序分析显示其均有WRKY结构域,与拟南芥WRKY转录因子构建系统进化树将连翘52个WRKY转录因子进一步分为3大类;筛选出5个可能参与连翘苯丙烷合成途径的连翘WRKY转录因子,并推测其可能以被MAPK级联反应所调控的方式介导连翘中苯丙烷合成途径。结论 通过分析转录组测序结果,从52个连翘WRKY转录因子中筛选出5个可能参与连翘苯丙烷合成途径的转录因子,其表现出组织特异性表达,且对不同浓度茉莉酸甲脂表现出不同的响应,为进一步研究其作用机制提供研究方向。     

山药对糖尿病小鼠组织丙二醛含量的影响

目的：观察山药对糖尿病小鼠组织丙二醛（ ＭＤＡ） 含量的影响。方法：采用四氧嘧啶制作糖尿病小鼠模型,并以优降糖作阳性对照,连续２１ 天用不同剂量山药灌胃治疗,比较各组心脏、肝脏、肾脏和胰脏过氧化脂质的终末代谢产物ＭＤＡ 含量。结果：①对照组四器官ＭＤＡ显著高于正常组（Ｐ＜ ０ ．０１ 或Ｐ＜ ０ ．００１） ;②剂量在６ ．００ｇ／ｋｇ·ｄ－ １ 以上山药各治疗组四器官ＭＤＡ显著低于对照组（Ｐ＜ ０ ．０５ 或Ｐ＜ ０．００１） ;③与优降糖组比,除肝脏ＭＤＡ 较高外（Ｐ＜ ０．００１） ,中、大剂量山药组心、胰、肾组织ＭＤＡ 较低（Ｐ＜ ０ ．０５ 或Ｐ＜ ０ ．００１） 。结论：山药能明显降低糖尿病小鼠组织内过氧化脂质含量,尤其对心组织作用最强,其次为胰、肾和肝组织,而优降糖对胰组织过氧化脂质无明显影响。     

The chondroitin sulphate proteoglycan brevican is upregulated by astrocytes after entorhinal cortex lesions in adult rats

The chondroitin sulphate proteoglycan brevican is one of the most abundant extracellular matrix molecules in the adult rat brain. It is primarily synthesized by astrocytes and is believed to influence astroglial motility during development and under certain pathological conditions. In order to study a potential role of brevican in the glial reaction after brain injury, its expression was analysed following entorhinal cortex lesion in rats (12 h, 1, 2, 4, 10, 14 and 28 days and 6 months post lesion). In situ hybridization and immunohistochemistry were employed to study brevican mRNA and protein, respectively, in the denervated outer molecular layer of the fascia dentata and at the lesion site. In both regions brevican mRNA was upregulated between 1 and 4 days post lesion. The combination of in situ hybridization with immunohistochemistry for glial fibrillary acidic protein demonstrated that many brevican mRNA-expressing cells are astrocytes. In the denervated zone of the fascia dentata, immunostaining for brevican was increased by 4 days, reached a maximum by 4 weeks and remained detectable up to 6 months post lesion. Electron microscopic immunocytochemistry showed that brevican is a component of the extracellular matrix compartment. At the lesion site a similar time course of brevican upregulation was observed. These data demonstrate that brevican is upregulated in areas of brain damage as well as in areas denervated by a lesion. They suggest a role of brevican in reactive gliosis and are compatible with the hypothesis that brevican is involved in the synaptic reorganization of denervated brain areas.