PS/SBR-g-PS共混物的力学性能和形态结构

采用种子乳液聚合技术在丁苯胶乳上接枝聚合苯乙烯 ,合成了一系列丁苯橡胶接枝聚苯乙烯共聚物 (SBR-g-PS)。将其与聚苯乙烯 (PS)树脂共混后 ,考察了 SBR-g-PS的组成 (SBR/ PS)对共混物的力学性能和形态结构的影响。结果发现 ,当 SBR/ PS为 6 7/ 33-5 0 / 5 0时 ,PS/ SBR-g-PS共混物表现出良好的综合力学性能 ,在 SBR-g-PS中随着接枝 PS的增多 ,像胶粒子在基体中的分散状况获得改善 ,在大橡胶颗粒中含有大量的 PS次级粒子。在外负载的作用下 ,共混物中的大橡胶颗粒引发了大量的银纹 ,吸收了断裂应变能 ,从而提高了材料的冲击韧性。

硅藻土/Bi/g-C_(3)N_(4)复合材料的制备及其可见光催化性能研究

以三聚氰胺和五水合硝酸铋[Bi(NO_(3))3·5H_(2)O]为前驱体,硅藻土为基质,制备了硅藻土/Bi/石墨相氮化碳(g-C_(3)N_(4))复合材料。采用多种表征方法对复合材料的形貌、结构和化学组成等进行分析,在可见光(波长大于400nm)照射下,通过还原液相体系中的甲基橙(MO)考察了复合材料的光催化性能。光催化实验结果表明,质量分数为6%的硅藻土/Bi/g-C_(3)N_(4)复合材料在30min内对MO降解效率可达100%。金属Bi的表面等离子体共振效应引起的内置电场加快了电子和空穴的分离速度,硅藻土作为基质可以有效避免复合材料的团聚,其超大的比表面积有利于催化过程中复合材料活性位点的暴露,同时其复杂的孔隙结构可以促进复合材料对污染物的吸附,提高MO的降解效率。

重图的T-染色

重图的T-染色是图的T-染色的一个较为实用的部分,这是因为在研究频率分配时,干扰可能会在不同的水平上发生。由于一个重图G能够被剖分成K个不同部分,用G(V,G0,G1,……,GK-1)来表示G。重图G(V,G0,G1,…,GK-1)的一个T-染色是指一个函数f,f满足同时是Gi的T(i)染色,即:对i=0,1,……,K-1,{x,y}∈E(Gi)|f(x)-f(y)|T(i)。G的f染色的色数是指值不同的f(x)的个数,记作:XT(f)。其中x∈V(G)。G的f染色的跨度等于m ax|f(x)-f(y)|,记作:spT(f),其中{x,y}∈E(G)。G的T-染色的色数和跨度分别记作XT(G)和spT(G),当f取遍所有G的T-染色时,XT(G)=m inXT(f),spT(G)=m inspT(f)。本文将给出一些关于重图的T-染色的已知结论,同时还将给出一种计算重图的spT的新算法。

G protein b_1λ_2 subunits purification and their interaction with adenylyl cyclase

A preliminary study on the interaction of G protein (guanine triphosphate binding pro- tein) b1g2 subunits and their coupled components in cell signal transduction was conducted in vitro. The insect cell lines, Sf9 (Spodoptera frugiperda) and H5 (Trichoplusia ni ) were used to express the recombinant protein Gb1g2. The cell membrane containing Gb1g2 was isolated through affinity chromatography column with Ni-NTA agarose by FPLC method, and the highly purified protein was obtained. The adenylyl cyclase 2 (AC2) activity assay showed that the purified Gb1g2 could signifi-cantly stimulate AC2 activity. The interaction of b1g2 subunits of G protein with the cytoplasmic tail of various mammalian adenylyl cyclases was monitored by BIAcore technology using NTA sensor chip, which relies on the phenomenon of surface plasmon resonance (SPR). The experiments showed the direct binding of Gb1g2 to the cytoplasmic tail C2 domain of AC2. The specific binding domain of AC2 with Gb1g2 was the same as AC2 activity domain which was stimulated by Gb1g2.