崇明东滩夏冬季表层沉积物细菌多样性研究

以长江口崇明东滩高、中、低潮滩夏、冬两季表层沉积物中基因组DNA为模板,PCR扩增样品中细菌16S rRNA基因V3区片段,通过克隆、测序,构建相应基因文库.系统发育分析结果表明,崇明东滩高、中、低潮滩表层沉积物共包含12个主要门类的细菌:变形菌门(Proteobacteria)(α-、β-、γ-、δ-和ε-亚群)、拟杆菌门(Bacteroidetes)、放线菌门(Actinobacteria)、酸杆菌门(Acidobacteria)、绿弯菌门(Chloroflexi)、厚壁菌门(Firmicutes)、螺旋体门(Spirochaetes)、疣微菌门(Verrucomicrobia)、浮霉菌门(Planctomycetes)、绿菌门(Chlorobi)、网团菌门(Dictyoglomi)、硝化螺旋菌门(Nitrospirae),此外还存在大量未被认知的序列.中潮滩和低潮滩的优势菌为变形菌,高潮滩的优势菌为拟杆菌.DOTUR多样性分析结果表明,崇明中潮滩细菌多样性最高,低潮滩次之,高潮滩最低;夏季细菌多样性高于冬季.夏、冬两季细菌群落差异高潮滩最大,低潮滩次之,中潮滩最小.     

稀有鮈鲫神经发育相关基因的克隆、同源性分析及组织分布

作为重要的本土模式鱼类,稀有鮈鲫神经发育相关的生物学背景几乎空白,导致其在神经毒性评价方面的应用受到限制。本文从稀有鮈鲫脑部克隆得到了神经发育相关的神经生长因子(nerve growth factor;ngf)、脑源性神经营养因子(brain-derived neurotrophic factor;bdnf)、胶质纤维酸性蛋白(glial fibrillary acidic protein;gfap)、髓鞘相关糖蛋白(myelin-associated glycoprotein;mag)、P0蛋白(myelin protein zero;mpz)、微管蛋白α1(α1-tubulin)和Y染色体性别决定基因10(SRY-box containing gene 10;sox10)等基因的片段,并对其进化树及表达谱进行了分析。序列分析表明,bdnf的核苷酸序列与鲫鱼、鲤鱼的同源性最高,均为98%;gfap、ngf、mag和α1-tubulin与斑马鱼的同源性最高,分别为95%、92%、92%和96%;mpz与黑头软口鲦的同源性最高,为94%;sox10与鳙鱼同源性最高,达97%。表达谱分析结果表明,ngf、bdnf、mag、mpz、α1-tubulin和sox10基因均在脑组织中表达量最高,gfap在脊髓中表达量最高,上述结果为这一模式鱼类在神经发育学和神经毒性效应评价方面的应用奠定了基础。     

Abundance and distribution of ammonia-oxidizing archaea in Tibetan and Yunnan plateau agricultural soils of China

As low oxygen and high ultraviolet （UV） exposure might significantly affect the microbial existence in plateau, it could lead to a specialized microbial community. To determine the abundance and distribution of ammonia-oxidizing archaea （AOA） in agricultural soil of plateau, seven soil samples were collected respectively from farmlands in Tibet and Yunnan cultivating the wheat, highland-barley, and colza, which are located at altitudes of 3200-3800 m above sea level. Quantitative PCR （q-PCR） and clone library targeting on amoA gene were used to quantify the abundances of AOA and ammonia-oxidizing bacteria （AOB）, and characterize the community structures of AOA in the samples. The number of AOA cells （9.34 × 10^7-2.32× 10^8 g^-1 soil） was 3.86-21.84 times greater than that of AOB cells （6.91 × 10^6-1.24 × 10^8 g^-1 soil） in most of the samples, except a soil sample cultivating highland- barley with an AOA/AOB ratio of 0.90. Based Kendall＇s correlation coefficient, no remarkable correlation between AOA abundance and the environmental factor was observed. Additionally, the diversities of AOA community were affected by total nitrogen and organic matter concentration in soils, suggesting that AOA was probably sensitive to several environmental factors, and could adjust its community structure to adapt to the environmental variation while maintaining its abundance.     

Effects of cotton straw amendment on soil fertility and microbial communities

Maintaining soil fertility, while controlling pollution from excessive chemical fertilizer application is important for keeping soil productivity of sustainable agriculture. Variety of straws have been used and proven to be good soil amendments for increasing soil organic matter (OM) and a range of additional soil nutrients. However, little is known about the utilization of cotton straw for soil amendment. To better understand the mechanism behind cotton straw soil amendments, investigations were performed upon cucumber seedlings, where changes to soil nutrients and microbial communities were investigated. The results revealed that the cotton straw application promoted the cucumber seedling growth by significantly increasing the soil OM, available nitrogen, available phosphorus, and available potassium. The concentration of cotton straw was positively correlated to both the number of the culturable microorganisms and also the total microbial biomass within soil. Furthermore, assessment of cotton straw application using Biolog metabolic profiling and phospholipid fatty acid analysis revealed that such application increased the microbial community metabolic activity, and markedly changed the structure of microbial community. 16S rRNA gene clone library construction and phylogenetic analysis of soil bacteria revealed γ- Proteobacteria sequences dominated the cotton straw amendment soil, comprising 27.8% of the total number of analyzed sequences, while they were less represented in control soil (13.4%). On the contrary, the Sphingobacteria (7.8%) and Verrucomicrobia (2.4%) in the cotton straw amendment soil decreased after application when compared to the control soil 15.2% and 15.2%.     

同步硝化反硝化系统中反硝化细菌多样性研究

采用聚合酶链式反应(PCR)和分子克隆构建nirS克隆文库对同步硝化反硝化系统好氧池中反硝化细菌多样性进行了研究.从克隆文库中随机挑选75个克隆子进行序列测定,对测序结果进行了BLAST比对.结果表明,有74个克隆子分属于3个不同的细菌类群,包括β-Proteobacteria、γ-Proteobacteria和Uncultured bacterium. β-Proteobacteria纲为好氧池内优势菌群,占文库比例的54.41%;其次是γ-Proteobacteria纲,占文库比例的25%.对测序得到的12个OTU用MEGA软件进行系统发育分析,结果显示Thauera属为该系统中最主要的脱氮菌属.     

黄河三角洲湿地土壤微生物群落结构分析

采用末端限制性片段长度多态性分析(T-RFLP)技术和16S rDNA克隆文库的方法,分析了黄河三角洲滨海湿地土壤不同深度细菌和古菌的群落结构.研究表明,随着深度的增加,细菌群落的多样性下降,而古菌群落多样性则有上升的趋势,且土壤的细菌和古菌群落结构都呈现出规律的层状分布.该土壤包括各种硫酸盐还原菌、产甲烷古菌、光合细菌等丰富的细菌和古菌资源.图5参27     

Soil fungistasis and its relations to soil microbial composition and diversity: A case study of a series of soils with di erent fungistasis

Fungistasis is one of the important approaches to control soil-borne plant pathogens.Some hypotheses about the mechanisms for soil fungistasis had been established,which mainly focused on the soil bacterial community composition,structure,diversity as well as function.In this study,the bacterial community composition and diversity of a series of soils treated by autoclaving,which coming from the same original soil sample and showing gradient fungistasis to the target soil-borne pathogen fungi Fusarium gr...     

水中轮状病毒实时定量PCR外标准品的构建

采用细胞培养和T-A克隆技术,在轮状病毒主要结构蛋白VP7基因序列上设计合成引物,经PCR扩增后将特异性产物连接入pGEM-T-easy载体中,经过酶切鉴定和测序分析获得轮状病毒cDNA标准品.利用常规PCR和实时定量PCR方法对所获得的cDNA标准品进行特异性、稳定性和重复性指标的检验.结果表明,利用此标准品制备的标准曲线具有较高的扩增效率和良好的线性关系(斜率为-3.353,R2=0.995);实时定量PCR熔解曲线分析表明,温度在81℃±0.5℃的PCR产物是轮状病毒VP7序列上的特异性产物,表明此标准品是轮状病毒特异性的;同时,所制备的标准品在实时定量PCR检测中具有较大的线性范围(9×100～9×1011 copies/μL,每个反应最低可以检测到9个拷贝数的轮状病毒cDNA,表明利用该标准品进行实时定量PCR分析时具有较高的检测灵敏性;此外,该标准品具有较高的稳定性和重复性(3次独立实验CV值在0.2%～0.9%之间),可长期稳定保存.构建的标准品可用作检测水环境中轮状病毒的实时荧光定量PCR的外标准品.     

高氨氮废水处理系统中功能微生物的检测

利用16S rDNA分子检测技术对高氨氮废水处理系统中的氨氧化细菌、亚硝酸盐氧化细菌等难分离培养微生物进行了分析检测.从实验室处理高氨氮废水的生物流化床硝化系统生物膜中提取细菌总DNA,以其为模板,利用氨氧化细菌(AOB)和亚硝酸盐氧化细菌(NOB)的16S rDNA特异性引物进行多聚酶链式反应(PCR)扩增,获得AOB和NOB的特异片段.将特异片段与pGEM-T载体连接并转化到E.coli DH5α中获得重组子,对阳性重组子进行酶切分型,AOB可分为8种不同类型.选取AOB的8种类型代表以及随即选取8个NOB克隆进行测序.经GenBank搜索以及同源性分析,发现所获得的8个AOB类型来自不同的菌株,处理系统中以Nitrosomonas sp.和Nitrosococcus sp.为氨氧化细菌的优势菌属;8株NOB重组子中有7株来自不同的菌株,系统中Nitrobacter sp.和Afipia sp.为亚硝酸盐氧化细菌的优势菌属.图6表1参14     

纳豆激酶原核表达载体的构建及其活性鉴定

利用引物搭桥的方法,经PCR扩增,获得了纳豆激酶成熟肽基因(NK),从而构建了大肠杆菌表达质粒NK/pTWIN1,NK/PET32a及NK/PML-c2x,经分别转化宿主菌ER2566,BL21和ER2566,获得了转纳豆激酶基因重组菌.结果表明,NK/pTWIN1-ER2566和NK/PET32a-BL21的纳豆激酶蛋白表达量较高.本研究选用NK/pTWIN1-ER2566作为表达菌株,对其进行发酵表达.SDS-PAGE显示,目的蛋白约占菌体总蛋白的36%,该蛋白是以包涵体形式存在的.包涵体经收集、蛋白变性及复性,并经过SP Sepharose分离纯化,得到了纯化的纳豆激酶蛋白,琼脂糖-纤维蛋白平板法测出1mg纳豆激酶干粉的溶栓活性相当于600u尿激酶.本文从基因工程角度研究纳豆激酶基因的克隆、表达及纯化,为利用基因工程菌生产纳豆激酶奠定了基础.图5表1参11