蛋清蛋白辅助水热法制备CeO_2纳米棒及其发光性能

本文以氯化铈和氢氧化钠为反应原料,以新鲜蛋清为络合剂,探索在水热体系中制备CeO2纳米棒。通过XRD、FESEM等测试手段对其进行了结构和形貌分析;应用荧光光谱法对样品的发光性能进行了测试。XRD结果表明,实验所得产物为立方萤石结构CeO2。FESEM分析可知,所得CeO2纳米棒为规则六方柱结构,其长度约为200 nm、直径约为几十纳米。荧光光谱分析可知其在紫蓝色发光区具有较强的发光性能。     

Differential Expression of Molecular Chaperones in PC12 Cells Treated with PSI

<正>Parkinson's disease(PD) is a common neurodegenerative disorder whose primary pathology features are the degeneration of dopaminergic neurons in the substantia nigra pars compacta(SNc) and the presence of eosinophilic inclusions called Lewy body in the cytoplasm of the remained neurons.Growing evidence suggests that dysfunction of the ubiquitin-proteasome system(UPS) is involved in the etiopathogenesis of PD.In order to investigate the pathogenetic mechanism of ubiquitin-proteasome dysfunction in PD,2D-differential gel electrophoresis (2D-DIGE) and MALDI-TOF Pro MS were used to determine the proteins,which were differentially expressed,in PC12 cells that had undergone a synthetic proteasomal inhibitor PSI(10μmol/L) treatment for 24 h.Forty-six protein spots were differentially expressed in response to PSI administration,of which 34 were increased and 12 decreased. Six of these were identified as molecular charperones:endoplasmin precursor(GRP94),heat shock protein 105(HSP105),HSC-70-psl,glucose ruglated protein 75(GRP75),glucose ruglated protein 58(GRP58) and heat shock 27000 protein 1(HSP27).The results suggest that the molecular chaperones play an important role in the PD model induced by proteasomal inhibitor.     

铕(III)对伴清蛋白溶液构象的影响

用TNS疏水探针研究了脱铁伴清蛋白(apoOTf)和不同形式的铕伴清蛋白(Eu_N-OTf, Eu₂-OTf)的表面疏水暴露程度, 依次为apoOTf＞Eu_N-OTf＞Eu₂-OTf, 表明Eu^3＋与脱铁伴清蛋白N端结合引起蛋白构象变化大, 与C端结合引起蛋白构象变化小. 此外, 由盐酸胍对3种蛋白变性实验, 发现Eu^3＋与脱铁伴清蛋白的结合稳定了蛋白的结构, 稳定性依次为apoOTf＜Eu_N-OTf＜Eu₂-OTf. 离子强度效应也充分表明3种蛋白内部疏水基团相互作用依apoOTf＜Eu_N-OTf＜Eu₂-OTf顺序增大, 稳定性也依次增大. 本研究对进一步探讨Eu^3＋的生物效应提供理论依据.     

基于抗肿瘤活性化合物MED烟酸类衍生物的设计及作用靶点

通过变性荧光素酶的再复性实验发现真菌环氧二烯(Mycoepoxydiene,MED)对热休克蛋白(Heat shock protein 90,Hsp90)具有抑制作用.Western Blot实验结果表明,MED影响人宫颈癌细胞株HeLa中Hsp70及Hsp90的客户蛋白质(Akt,Raf-1)的表达,表明MED是Hsp90的抑制剂.通过靶向对接技术预测了MED与人Hsp90 N端ATP结合位点的结合情况,并在此基础上发现,MED的烟酸类衍生物4-NDM与Hsp90的结合具有比MED与Hsp90更强的亲和作用.体外实验结果证明,MED的烟酸类衍生物4-NDM及3-NDM对HeLa细胞表现出比MED更强的细胞毒活性;可通过上调Hsp70,并下调Akt和Raf-1而影响HeLa细胞中Hsp90相关蛋白质的表达.由此推测,MED及其烟酸类衍生物可以通过抑制Hsp90,而使其客户蛋白Akt或Raf-1发生降解,发挥其抗肿瘤作用.     

聚丙烯酰胺凝胶电泳前活性染料与蛋白质共价染色的条件探索

采用聚丙烯酰胺凝胶电泳前染色法,考察了多种类型活性染料与牛血清白蛋白共价染色的条件.实验发现,活性蓝KN-R型标记效果最佳,其优化标记条件为: pH 10.0, 60 ℃, 50 min,蛋白检出限达200 ng,重复性和测试范围内的定量性较好,可在电泳时直接实时观测,作为蛋白标示剂有一定的应用前景.     

水通道蛋白启发下的人工水通道研究进展

受水通道蛋白(AQP)结构与功能启发,含有生物水通道或人工水通道(AWC)的仿生膜近年来取得了显著进展.借鉴AQP的传输特性,所制备的AWC获得了高度的选择性及水快速运输能力.通过对AQP的结构原型进行分析,对标AWC中H2O分子选择性和渗透特性,尝试提出了"门控效应"、"润湿效应"和"排队效应"3种效应,并对现有嵌入...     

莲子蛋白组分二级结构的研究

对莲子蛋白质进行了Osborne蛋白质分类。采用傅里叶变换红外光谱(FTIR)对清蛋白、球蛋白、醇溶蛋白和谷蛋白进行二级结构分析。应用去卷积和曲线拟合方法对四种蛋白组分的酰胺Ⅰ和Ⅲ带进行分析,清蛋白和球蛋白之间以及醇溶蛋白和谷蛋白之间各相应子峰峰位和二级结构峰面积百分比差异较小,但前两者各相应子峰峰位与后两者略有差异;而前两者各相应二级结构峰面积百分比与后两者有较大差异,特别是前两者的各相应有序结构(α-螺旋+β-折叠)峰面积的百分比明显大于后两者。用0.1 mol.L-1NaCl溶液提取的球蛋白和清蛋白有序结构含量均在55%左右,而醇或碱提的醇溶蛋白和谷蛋白的有序结构含量仅为40%左右,盐提的蛋白质二级结构有序性和稳定性更高。     

乳清分离蛋白-葡聚糖接枝物性质的荧光光谱法分析

乳清分离蛋白与葡聚糖的混合物在干热处理条件下,发生了以褐变为特征的美拉德反应。当葡聚糖分子量由67kD增至150kD时,游离氨基含量分别下降了35.77%和30.53%,糖链越长,其接入到蛋白质肽链的难度越大。采用荧光光谱对乳清分离蛋白-葡聚糖接枝物的性质进行分析。内源荧光光谱图显示,接枝产物在405nm的最大荧光强度显著提高,且350～500nm范围内的荧光强度顺序为:G67>G150,这说明接枝物中有Maillard反应体系所特有的荧光物质生成;由外援荧光光谱图得出,接枝产物在470nm的最大荧光强度均有明显降低,各溶液体系中荧光强度高低顺序依次为:WPI>G150>G67。疏水性指数的测定进一步说明两种不同分子量的葡聚糖接入到蛋白质肽链中,对乳清分离蛋白的疏水性均有一定的屏蔽作用。     

Expression and Emmprin Regulated Function of Aquaporinl in SMMC7221 Cells

<正>Herein lie the crosstalk and regulation between AQP1 and Emmprin in SMMC7221 cells by means of siRNA technology and deglycosylation method.Firstly,HAQP1,rather than hAQP3,was selectively upregulated in SMMC7221 cells by FBS,flollowed by the upregulated expression of Emmprin.Emmprin gene silencing caused a remarkable change in the expression of AQP1 gene,just like its downstream gene,MMP9,meanwhile the water permeability and cell migration were also descended prominently.Furthermore,when treated with tunicamycin, Emmprin was deglycosylated,which made the expression of AQP1 significantly declined,followed by remarkably decreased cell membrane water permeability and cell migration.Taken together,all the data indicates the expression level and the modification of Emmprin by glycosylation are the key factors in regulating the expression of AQP1.     

藻蓝蛋白(C-Pc)的三阶光学非线性和激发态弛豫

藻蓝蛋白（Ｃ－Ｐｃ）的三阶光学非线性和激发态弛豫＊刘志斌彭俊彪ａ）李文连（中国科学院长春物理研究所，长春１３００２１）ａ）（中国科学院激发态物理开放研究实验室，长春１３００２１）邓湘君（吉林省生物研究所，长春１３００１２）关键词藻蓝蛋白，χ（３）值，...