海枣曲霉β—D—岩藻糖苷酶的研究

Although beta-D-fucosidase (beta-D-fucoside fucohydrolase, EC 3.2.1.38) has been isolated from various sources, the identity of this enzyme is still not settled. We have purified a specific beta-D-fucosidase in electrophoretically homogeneous form crude extracts of Aspergillus phoenicis by polyethyleneglycol 6000-phosphate buffer aqueous two-phase separation, and successive chromatography on DEAE-Sephadex A-50, hydroxyapatite and Sephadex G-100 columns. The molecular weight of the enzyme was estimated to be 57000 by SDS-polyacrylamide gel electrophoresis and 50000 to 60000 by gel filtration on Sephadex G-100. The enzyme showed optimum coside were 2.4mmol/L, and 1.28 mumol min-1 the pH range 5.5-6.5 and below 35 degrees C. The Km and the Vmax values for pNP-beta-D-fucoside were 2.4mmol/L, and 1.28 mumol.min-1.mg-1 respectively. The enzyme was strongly inhibited by sulfhydryl group reagents, PCMB-NEM and iodoacetate. It was also inhibited by EDC, DEP and NBS. Thus, -SH, -COOH groups, histidyl and tryptophyl residues were essential for enzyme activity. The purified beta-D-fucosidase showed high specificity toward p-nitrophenyl beta-D-fucoside. The enzyme was inhibited by D-fucose and D-fucono-gamma-lactone, but not by D-galactose, D-galactono-gamma-lactone, D-glucose or D-glucono-gamma-lactone; the latter compounds are specific inhibitors of beta-D-galactosidase and beta-D-glucosidase respectively. Thus, this enzyme is the most strictly specific beta-D-fucosidase when compared with those previously reported.     

华癸中慢生根瘤菌7653R 3个脂质转运蛋白基因的克隆、突变及共生表型北大核心CSCD

【目的】脂类转移家族蛋白基因编码一类参与脂类转运及代谢的蛋白。本研究旨在构建华癸中慢生根瘤菌3个脂质转运家族蛋白基因的突变株,检测及分析突变体与紫云英共生条件下的表型及功能。【方法】利用生物信息学分析与预测转脂蛋白的结构特征及功能,采用荧光定量技术检测目标基因在自生和共生条件下的表达特性,通过插入突变技术构建目标基因突变株,并进行植物盆栽实验考察其共生表型。【结果】MCHK-5577、MCHK-2172和MCHK-2779基因编码蛋白属于START/RHO alpha_C/PITP/Bet_v1/Cox G/Cal C(SRPBCC)超家族,包含脂类转移结构域,参与脂类转运或代谢,与百脉根等中慢生根瘤菌相应基因的序列相似性达95%以上。这3个基因在共生条件下的表达水平都增高。分别构建了MCHK-5577、MCHK-2172和MCHK-2779基因突变菌株,与野生型菌株7653R相比,接种突变株MCHK-2172mut、MCHK-2779mut和MCHK-5577mut后的植株地上部分生物量和根瘤固氮酶活性显著降低。【结论】华癸中慢生根瘤菌脂质转移家族蛋白基因在共生互作过程中发挥重要作用,突变后明显影响共生固氮表型。本文的实验结果为深入研究脂类转移蛋白在共生固氮作用中的功能机制奠定了基础。     

猪眼角膜的生物力学特性

对猪眼角膜进行了有系统的单轴拉伸实验,通过实验来确定其极限强度,断裂能、显著非线性的应力-应变关系和滞后环.在不同的应变水平下进行了应为松弛实验并确定了连续松弛谱的各参数.从极限强度、断裂能和应力松弛来看,角膜的纵向和横向之间无重大的差异,据此,各向同性假定可用于初步的角膜力学模型.     

Steel slag amendment reduces methane emission and increases rice productivity in subtropical paddy fields in China

Paddy field, being a man-made wetland, is recognized as one of the major sources of global methane (CH₄) emission. Since China has the second-largest area of rice cultivation in the world, it is important to develop valid and reliable strategies to reduce CH₄ emission and sustain rice productivity in Chinese paddy fields. In this study, we applied steel slag fertilizer, a by-product of steel industry with a high concentration of active iron (Fe), at rates of 0, 2, 4, and 8 Mg ha^?1 in subtropical rice (Oryza sativa L.) paddy fields in China to assess the effect of steel slag amendment on CH₄ emissions as well as rice growth and yield characteristics. Results showed that the Fe concentrations in paddy soils significantly increased with the application levels of steel slag fertilizer. Steel slag amendment in paddy fields largely reduced the CH₄ production rate, resulting in a decrease in the overall CH₄ emission rate. In response to the applications of steel slag at a rate of 2, 4 and 8 Mg ha^?1, total CH₄ emission during rice cultivation decreased by 26.6, 43.3 and 49.3 %, respectively. Furthermore, steel slag amendment had a significant, positive effect on the rice grain yield and the percentage of ripened grain, most probably due to the increased availability of inorganic nutrients such as silicate and manganese. Our results suggest that steel slag can be an effective soil amendment for reducing CH₄ emissions as well as increasing rice productivity in subtropical paddy fields in China.     

真菌降解木质素研究进展及在好氧堆肥中的研究展望

综述了近十年来真菌降解木质素的研究进展,包括木质素的存在与结构,真菌降解木质素生物学、酶系及作用机理、生理学以及在环境工程中应用方面的研究进展,并对好氧堆肥处理城市垃圾中木质素生物降解的研究作了展望 。     

大气CO2浓度升高对香蕉光合作用及光合碳循环过程中叶氮分配的影响

生长在高CC2浓度(700±56μl     

食用菌灭活原生质体电融合及属间融合产物的鉴定分析

食用菌因其显著的营养、保健、药用及综合利用价值受到世人青睐。原生质体融合技术则为食用菌的育种和遗传学研究提供了一条很好的途径。食用菌的种内、种间乃至属间、目间的原生质体融合均已有过报道,但这些工作大多利用营养缺陷型标记的亲株,采用化学融合法完成。这种融合的效率较低,对亲株的标记繁琐费时,甚至会对菌株性状产生不良影响。最近,一种具有较高融合效率的物理融合法——电融合法以及非遗传性标记法分别被一些研究者所采用。本研究将原生质体电融合法与灭活标记法相结合来获得食用菌的属间融合产物,并采用包括同工酶分析和RAPD(或AP-PCR)方法在内的分子生物学方法,对食用菌属间杂交后代的遗传学特性进行初步探讨。1 材料和方法     

一株高抗汞细菌的分离鉴定及其抗性基因的克隆与表达

摘要：【目的】本研究旨在从重金属汞抗性细菌中分离鉴定汞抗性基因【方法】从北京凉水河河床底泥中分离抗汞细菌,采用16S rRNA基因序列分析结合生理生化特征对菌株进行鉴定。根据GenBank中已发表的多种抗汞细菌的merA基因序列设计引物,以抗性细菌基因组DNA为模板,扩增merA基因,并在大肠杆菌（Escherichia coli）BL21(DE3)表达。同时对表达菌株的重金属汞抗性进行测定。【结果】分离得到一株能在含HgCl2为70 mg/L的平板上生长良好的高抗汞细菌,编号为KHg2。16S rRNA     

Time-resolved fluorescence biosensor for adenosine detection based on home-made europium complexes

In this protocol, the authors report a time-resolved fluorescence biosensor based on home-made europium complexes for highly sensitive detection of small molecules using adenosine as a model analyte. The fluorophore that used is europium complexes. Its signal can be measured in a time-resolved manner that eliminates most of the unspecific fluorescent background. The amino modified aptamer probe, which is designed to specifically recognize adenosine, is combined to the aldehyde-group modified glass slide by covalent bond. Europium complex-labeled a short ssDNA, designed to segment hybridize with aptamer probe is immobilized on the glass slide by hybridization reaction. In the presence of adenosine, the aptamer part is more inclined to bounds with adenosine and triggers structure-switching of the aptamer from aptamer/ssDNA duplex to aptamer/target complex. As a result, europium complexes-labeled ssDNA is forced to dissociate from the sensor interface, resulting in time-resolved fluorescence intensity decrease. The decrement intensity is proportional to the amount of adenosine. Under optimized assay conditions, a linear range (1.0×10(-8)M to 1.0×10(-7)M) is got with low detection limit of 5.61nM. The biosensor exhibits excellent selectivity and can provide a promising potential for aptamer-based adenosine detection.     

转基因白桦中GUS基因表达的定量分析

以转基因白桦（Betula platyphylla）为材料,采用单酶切结合Southern杂交的方法揭示不同转基因植株中GUS基因的整合拷贝数为1—4个。采用组织化学染色法定性分析不同整合方式转基因白桦植株中GUS基因的表达。结果表明,11个转基因植株中有2株出现了GUS基因沉默,其余植株均有不同水平的GUS表达。在此基础上应用分光光度法定量分析不同拷贝数的GUS转基因白桦中β-葡萄糖醛酸酶活性。结果表明,在11个转基因尢性系中除2个株系的GUS基因沉默外,其它9个转基因植株中GUS酶活力差异明显,但这种差异与GUS基因的拷贝数没有必然联系。