葫芦茶地上部分化学成分的研究

运用多种色谱法进行分离纯化,并通过理化性质和波谱数据对化合物进行结构鉴定,研究葫芦茶地上部分的化学成分。结果表明:从葫芦茶地上部分分离并鉴定了13个化合物,分别为山柰酚(1)、山柰酚-3-O-α-L-鼠李糖苷(2)、山柰酚-3-O-β-D-葡萄糖苷(3)、山柰酚-3-O-β-D-芸香糖苷(4)、槲皮素-3-O-α-L-鼠李糖苷(5)、山柰酚-3-O-α-L-鼠李糖(1→6)-β-D-半乳糖苷(6)、槲皮素-3-O-β-D-葡萄糖苷(7)、槲皮素-3-O-α-L-鼠李糖(1→6)-β-D-半乳糖苷(8)、芦丁(9)、间苯三酚-O-β-D-葡萄糖苷(10)、对羟基桂皮酸(11)、RoseosideⅡ(12)、儿茶素(13)。其中化合物2、4、5、6、8、9、10、12为首次从该植物中分离得到。     

响应面法优化超声辅助提取太子参多糖工艺研究

本文探讨超声波作用下太子参多糖提取的最佳工艺条件。在单因素试验基础上,采用响应面法对太子参多糖提取工艺参数进行优化研究。响应面试验表明提取温度、提取时间和水料比对响应值多糖提取得率均有显著影响,优化得到太子参多糖超声提取最佳工艺条件为:提取温度为74℃;提取时间为65 min;水料比为26 mL/g;超声波功率100 W。在此条件下太子参多糖的提取得率为2.48%,与模型预测值非常接近。     

硫酸酯化银耳多糖的制备及抗氧化性活性研究

采用氯磺酸-吡啶法化学合成硫酸酯化银耳多糖,对硫酸酯化反应的吡啶与氯磺酸的体积比进行优化,氯化钡-明胶比浊法测定硫酸酯化银耳多糖的取代度,并对不同取代度的硫酸酯化银耳多糖进行体外抗氧化实验。结果表明:硫酸酯化银耳多糖取代度随吡啶与氯磺酸体积比的提高而增加;当吡啶与氯磺酸体积比为4∶1,反应温度60℃,反应时间3 h时,产物的取代度为1.32,在0.8～2.0 mg/mL浓度范围内对Fenton反应产生的羟基自由基体外清除率相对于银耳多糖具有明显优势。     

Structure-based design and synthesis of a bivalent iminobiotin analog showing strong affinity toward a low immunogenic streptavidin mutant

The streptavidin/biotin interaction has been widely used as a useful tool in research fields. For application to a pre-targeting system, we previously developed a streptavidin mutant that binds to an iminobiotin analog while abolishing affinity for natural biocytin. Here, we design a bivalent iminobiotin analog that shows 1000-fold higher affinity than before, and determine its crystal structure complexed with the mutant protein.     

Extraction of crude polysaccharides from Duchesnea indica (Andrews) Focke: optimization by response surface methodology

A full set of optimization procedure was applied to the extraction of anti-viral polysaccharides from Duchesnea indica (Andrews) Focke. By Plackett–Burman factorial design, three parameters (extraction time, extraction temperature, and ratio of water to raw material) were identified as significant to the extraction yield. However, no significant parameters had been identified for antiviral activity. A three-level-three-factor Box–Behnken factorial design was then employed to further optimize the extraction condition. The experimental data were fitted to a second-order polynomial equation using multiple regression analysis and also examined using appropriate statistical methods. This led to the construction of a response surface indicating the optimal values for each parameter and response studied. Concerning the extraction yield, an extraction at 98.51?ºC for 6.16 h with a ratio of water to raw material of 30.94 mL/g was found to be optimal. Under the optimized conditions, the experimental yield was 6.430 ± 0.078%, which was well matched with the predicted yield of 6.509%.     

Production of Ethanol from Maltose by Zymobacter palmae Fermentation

The production of ethanol from maltose by Zymobacter palmae T109 in monoculture fermentations, and in co-culture fermentations together with Zymomonas mobilis B69 was studies. Zymobacter palmae T109, produced 5.5% (w/v) of ethanol when co-cultured with Zymomonas mobilis B69, but Zymobacter palmae T109 produced only 4.9% (w/v) ethanol from 15% (w/v) maltose medium in monoculture fermentation.     

Rapid expression screening of eukaryotic membrane proteins in Pichia pastoris

The overexpression of milligram quantities of protein remains a key bottleneck in membrane protein structural biology. A challenge of particular difficulty has been the overproduction of eukaryotic membrane proteins. In order to cope with the frequently poor expression levels associated with these challenging proteins, it is often necessary to screen a large number of homologues to find a well expressing clone. To facilitate this process using the heterologous, eukaryotic expression host Pichia pastoris, we have developed a simple fluorescent induction plate‐screening assay that allows for the rapid detection of well expressing clones of eukaryotic membrane proteins that have been fused to GFP. Using a eukaryotic membrane protein known to express well in P. pastoris (human aquaporin 4) and homologues of the ER associated membrane protein phosphatidylethanolamine N‐methyltransferase (PEMT), we demonstrate that when a large number of clones are screened, a small number of highly expressing “jackpot” clones can be isolated. A jackpot PEMT clone resulted in 5 mg/L yield after purification. The method allows for the facile simultaneous screening of hundreds of clones providing an alternate to in‐culture screening and will greatly accelerate the search for overexpressing eukaryotic membrane proteins.     

金黄色葡萄球菌组分疫苗研究进展

临床上,耐药性的金黄色葡萄球菌日益增多,极其耐药的菌株甚至获得了超级耐药细菌的称谓,难以找到有效的抗菌素控制其感染,因而研制有效的疫苗来防治金黄色葡萄球菌感染显得更加重要。对研制开发的金黄色葡萄球菌荚膜多糖疫苗、纤维粘连结合蛋白疫苗、RNAⅢ激活蛋白疫苗以及核酸疫苗等进行了综述。