弹齿滚筒式捡拾装置弹齿的静力学分析

针对弹齿滚筒式捡拾装置在工作过程中弹齿变形现象,对弹齿滚筒式捡拾装置弹齿进行静力学分析,以寻求解决的途径。通过对捡拾装置弹齿在3个工作阶段上的载荷进行分析后,获得各工作阶段弹齿的受力简图,通过比较判断出在捡拾升运阶段弹齿受力比较复杂。以9KJ-1.4A型压捆机捡拾装置为实例,经过计算在有随机载荷和无随机载荷时弹齿齿臂末端的应力情况,得出结论:在没有随机载荷的情况下,齿根处应力远小于其许用应力,弹齿产生弹性变形,有足够的强度;当有随机载荷时,对弹齿产生冲击,若随机载荷过大,垂直于弹齿轴向的分力大于24N,则弹齿会产生塑性变形。对捡拾装置进行静力分析,可为捡拾装置整体结构优化设计供理论依据。     

Expression and homology modelling of sterol 14α‐demethylase of Magnaporthe grisea and its interaction with azoles

BACKGROUND: Magnaporthe grisea (Hebert) ME Barr infection is one of the most serious diseases for cultivated rice in the world. Sterol 14α‐demethylase (CYP51) is an important drug target for microbial pathogenic infections. To exploit specific and effective fungicides for M. grisea better, the authors have analysed the characteristics of interaction between sterol 14α‐demethylase from M. grisea (MGCYP51) and azoles. MGCYP51 with truncation of N‐terminal residues was cloned and expressed in E. coli, difference binding spectra of MGCYP51 induced by addition of four commercial azoles were determined and molecular modelling of MGCYP51 based on the crystal structure of Mycobacterium tuberculosis Lehmann & Newman and docking with the azoles were performed. RESULTS: The affinity of the azoles for MGCYP51 was positively correlated with their hydrophobicity. Amino acid residues Tyr112, Phe120, Phe220, His308 and Phe497 of MGCYP51, forming a large hydrophobic cavity, are the key residues interacting with azole fungicides. Furthermore, Phe220 and Phe497 are fungus and species specific respectively. CONCLUSION: The results suggest that the more potent azole fungicides for MGCYP51 should possess more hydrophobic groups interacting with residues Phe220 and Phe497. Copyright © 2009 Society of Chemical Industry     

斜纹夜蛾化学感受蛋白SlitCSP2的表达模式定位及配体结合特性分析

研究斜纹夜蛾Spodoptera litura化学感受蛋白Slit CSP2的表达模式、组织定位及与配体结合特性,为揭示SlitCSP2在化学通讯中的功能提供理论依据。利用RT-qPCR检测了SlitCSP2在蛹及雌、雄成虫各组织的基因表达水平;Westernblot方法检测了SlitCSP2在幼虫期和雄成虫头部、触角和足部的蛋白表达水平;利用免疫组织化学技术对Slit CSP2在幼虫各龄期的分布情况进行定位分析;利用荧光竞争结合试验检测Slit CSP2与13种非挥发性化合物的结合特性。RT-qPCR结果表明,SlitCSP2在3龄幼虫表达量最高,3～6龄表达量逐渐降低;成虫阶段雄成虫足部及胸部和雌成虫头部及翅的表达量最高,且雄成虫头部、足部和胸部的表达量显著高于雌成虫。Western blot结果显示,SlitCSP2在3龄幼虫头部（去触角）的蛋白表达水平较高。免疫组化结果表明,Slit CSP2在幼虫阶段主要分布于头部、口器和胸足;在雄成虫中,Slit CSP2主要分布于足部前跗节和足部外骨骼内侧。荧光竞争结合试验表明,Slit CSP2与单宁（Ki=1.77）、花青素（Ki=2...     

东亚飞蝗FK506结合蛋白基因克隆及其免疫功能分析

为明确东亚飞蝗Locusta migratoria manilensis免疫相关FK506结合蛋白(FK506 binding protein,FKBP)的功能,了解FKBP对金龟子绿僵菌Metarhizium anisopliae侵染东亚飞蝗的影响,分离克隆获得FKBP46基因及其纯化蛋白,采用荧光定量PCR方法测定...     

微波处理条件对蛋清结构和IgG结合能力的影响

为探究降低蛋清致敏性的新方法,在不同的微波条件下处理蛋清蛋白,通过SDS-PAGE(十二烷基磺酸钠-聚丙烯酰氨凝胶电泳)分析分子量变化、圆二色光谱分析二级结构变化、紫外光谱分析三级结构变化、外源性荧光光谱分析疏水性变化、间接ELISA(酶联免疫吸附试验)分析IgG(免疫球蛋白G)结合能力的变化,研究微波对蛋清的影响。研究证实,微波处理降低蛋清蛋白的潜在致敏性,其中400 W/30 s处理后的蛋白显示出最低的IgG结合能力,所有条件下处理后的蛋清蛋白的二、三级结构均发生显著改变。80 W的微波功率下,蛋白质的结构先折叠,该条件下处理30 s后,蛋白结构又展开;当微波功率达到640 W时,处理时间较长的蛋白分子产生堆叠。蛋白质分子的结构变化导致了其抗原性的变化。     

opaque-2玉米近等基因系的构建与赖氨酸含量快速检测

我国高赖氨酸玉米种质资源狭窄,opaque-2(o2)突变基因能大幅提高玉米赖氨酸含量,通过分子标记辅助选择构建o2玉米近等基因系并检测其赖氨酸含量具有重要意义。其中,要解决的两个关键问题是如何准确地将不同供体的o2突变基因导入受体系和如何快速地检测导入系的赖氨酸含量。本研究利用O2基因内紧密连锁的SSR共显性标记引物phi057检测玉米供体和受体自交系的多态性,利用其特异性和共显性构建o2近等基因系;参考已有研究,改进染料结合(DBL)法,测定18组构建成功的o2近等基因系的赖氨酸含量。结果表明,不仅在不同供体(CA339和山东2548)之间存在多态性,而且在不同受体系间也存在多态性,利用phi057能够成功地将不同供体的o2突变基因导入受体系,构建o2近等基因系;改进的DBL法分析表明,不同受体系赖氨酸含量变化较大,不同背景的受体系导入o2突变基因后赖氨酸含量增加的幅度差异也较大;普通玉米自交系间赖氨酸含量为0.223%~0.368%,构建成功的不同o2近等基因系间,赖氨酸含量为0.373%~0.527%,与受体亲本相比,赖氨酸增加幅度最低为13%,最高为74%。分析表明,phi057能准确筛选导入o2突变基因的受体系,结合改进的DBL法能快速地选择赖氨酸含量高的玉米。     

瓦氏黄颡鱼脂肪酸结合蛋白基因cDNA片段的克隆及分析

采用简并引物扩增得到瓦氏黄颡鱼肝型和心型脂肪酸结合蛋白cDNA片段,长度分别为335、425 bp;获得的111、114个氨基酸残基与鲤鱼(Cyprinus carpio)肝型、斜齿鳊(Rutilus rutilus)心型脂肪酸结合蛋白的氨基酸序列同源性分别达到81%和85%,表明克隆所得序列均为瓦氏黄颡鱼脂肪酸结合蛋白.定量PCR分析表明,肝脏和腹腔脂肪组织均是肝型和心型脂肪酸结合蛋白表达的主要场所.     

Purification and characterization of a β–glucan binding protein from the haemolymph of freshwater prawn Macrobrachium rosenbergii

β‐glucan binding protein (βGBP), a pattern recognition protein was purified from the haemolymph of freshwater prawn Macrobrachium rosenbergii by heparin affinity chromatography that showed a single band in native gradient PAGE. The β‐glucan binding property of the purified protein was confirmed in a phenoloxidase (PO) assay, where addition of βGBP along with β‐glucan increased the specific PO activity compared with that of β‐glucan alone. The molecular weight of the βGBP was found to be ~316 kDa on gel filtration chromatography. In SDS‐PAGE, βGBP molecule was reduced to one polypeptide chain of molecular weight ~113 kDa. Thus the βGBP in M. rosenbergii is possibly a homotrimeric molecule. The purified sample run on unreduced condition in SDS‐PAGE also revealed a similar size band (~113 kDa) and hence, the polypeptide chains of βGBP are held by non‐covalent interactions. The purified βGBP samples run in native PAGE was stained positively with alcian blue for carbohydrates and Sudan black for lipids indicating the βGBP to be a glycolipoprotein. With rabbit polyclonal anti‐βGBP serum developed, an indirect ELISA was standardized and the normal βGBP concentration in adult M. rosenbergii serum was quantified to be ~2 mg mL^?1. Furthermore, the applicability of the developed ELISA is discussed.     

Binding and bioactivity of insulin in primary cultures of carp (Cyprinus carpio) hepatocytes

Isolated carp hepatocytes cultured in serum-free, chemically defined medium were used to investigate within the same cell preparation characteristics of the binding of insulin as well as effects of insulin on cellular metabolism. The binding of human [¹²⁵I]-insulin to carp hepatocytes was studied in kinetic, saturation and displacement experiments. A dependency of insulin binding on the collagenase used for cell isolation was demonstrated. Insulin binding decreased during the first 12h of culture but remained constant during the following 12h. The kinetic experiments revealed that [¹²⁵I]-insulin binding reached a steady state within 20–30 min of incubation. The mathematical analysis of the saturation experiments demonstrated the existence of two populations of binding sites, one with high affinity (K_d1 = 5.5 pM) and low capacity (B_max1 = 0.14 fmol/mg protein or 77 binding sites/cell) and one with low affinity (K_d2 = 2.4 nM) and high capacity (B_max2 = 17.6 fmol/mg protein or 9623 binding sites/cell). In competition experiments, 312 pM [¹²⁵I]-insulin was displaced by cold insulin, IGF-I and IGF-II with IC₅₀ values of 2.2, 7.9 and 20.3 nM, respectively. Glucagon was without effect. Binding of insulin to carp hepatocytes resulted in a significant reduction of glucose release and a significant increase of protein synthesis as of de novo fatty acid synthesis. dedicated to Prof. Dr. W. Hanke on the occasion of his 65^th birthday.     

植物抗冻蛋白及其高级结构研究进展

抗冻蛋白是一类能控制冰晶生长和抑制冰晶之间发生重结晶的蛋白质．并具有两种明显不同的活性——热滞活性和重结晶抑制活性．植物抗冻蛋白的抗冻特性是低热滞活性和高重结晶抑制活性．植物抗冻蛋白虽然在DNA和氨基酸水平上具有较大的差异-几乎没有同源性，但却拥有相似的高级结构．冰晶结合位点也有一定的相似性．而且都可以通过“表面互补”模型较好地解释它们与冰晶之间的相互作用．全面介绍了植物抗冻蛋白的种类及特性，以及它们的高级结构和冰晶结合位点．