甘蓝型油菜热激蛋白HSP70基因家族的鉴定和分析

热休克蛋白也称热激蛋白(heat shock protein, HSP),是植物在受到生长环境中不利的生长因子胁迫时产生的一种用于抗逆的防御蛋白,其中在生物体中分布最普遍的一种热激蛋白是热休克蛋白70 (heat shock protein 70, HSP70)。为全面、深入地了解芸薹属HSP70基因家族的信息,本研究对芸薹属的3个物种(白菜,甘蓝和甘蓝型油菜)进行了生物信息学分析,首先在BRAD数据库中对芸薹属的3个物种进行HSP70基因数目的鉴定,分别在白菜和甘蓝中鉴定出了2个HSP70,在甘蓝型油菜中鉴定出了4个HSP70。将鉴定出来的这8个HSP70基因进行生物信息学分析(系统发生关系,基因结构,保守基序,染色体定位和同源性等),结果显示,芸薹属HSP70基因结构相似,在核酸和蛋白水平均具有高度保守性,进化过程中基本种之间以及天然杂交种与基本种之间均保持着极高的同源性,进化树以及其他生物信息学分析结果还表明甘蓝型油菜的HSP70位点与白菜、甘蓝的HSP70位点符合"禹氏三角"理论,但是根据3个物种的HSP70基因数量及对应关系等分析结果可推测白菜、甘蓝、甘蓝型油菜3个物种的HSP70位点与三倍化理论不完全一致,此结果可反映芸薹属的这3个物种在进化过程中其HSP70基因在数量或结构上发生过变化,致使其不满足三倍化学说。     

家蚕耐氟近等基因系SSH文库的构建及部分差异表达基因的分析

为了获取与家蚕耐氟性状相关的基因信息,利用家蚕耐氟品种T6和氟化物敏感品种733新建立耐氟近等基因系,以回交11代的家蚕耐氟近等基因系群体中的耐氟个体和敏感个体的中肠为材料,构建家蚕耐氟近等基因系抑制消减杂交(SSH)cDNA文库。通过对抑制消减杂交cDNA文库中随机挑选的153个阳性克隆测序和聚类拼接,得到19个重叠群(con-tig)、47个已知功能基因(un igene)和28个未知功能基因。获得的表达序列标签(EST)经BLASTx比对和同源性分析,初步发现这些基因参与家蚕体内物质转运、能量代谢、基因转录、蛋白质合成与降解、蛋白质加工、信号转导、机体免疫防御、细胞结构形成等诸多生物学过程。采用实时定量RT-PCR方法,对部分基因在家蚕耐氟近等基因系群体中的耐氟个体和敏感个体的不同组织的表达进行定量分析,发现磷酸根离子转运蛋白基因、三磷酸腺苷(ATP)合成酶基因、液胞型H+-ATP酶基因、脂肪酶基因以及主要过敏原蛋白基因在耐氟个体的中肠、马氏管、脂肪体组织中的表达量有较明显上调。     

Homologies between prolamins of different minor millets

Minor millets, viz. Barnyard millet, Proso millet, Little millet, Foxtail millet and Kodo millet, one variety in each grown in Tamil Nadu Agricultural University (TNAU), Coimbatore, Tamil Nadu were selected for the study. The protein contents of the selected decorticated millets were found to be 11.0, 12.3, 12.9, 10.5 and 10.6% respectively. Fractionation of these proteins revealed that prolamin forms major storage protein in Foxtail millet whereas, glutelin forms major storage protein in all the other millets. The extractability was studied using different solvents, viz. isopropyl alcohol, t-butyl alcohol and ethyl alcohol with varying concentration of 2-mercapto ethanol. Electrophoretic pattern of the extracted prolamins from these millets were compared and found that a protein band at the molecular weight range of 20 kD was found homologous in all except Proso millet. The extractability of the 20kD protein in 90% isopropyl alcohol showed its strong hydrophobic nature.     

鸡卡氏杆菌的分子鉴定及其16S rRNA基因序列分析(英文)

Two strains of Gallibacterium, isolated from one laying hen flock in Zhengzhou City of Henan Province, were identified by the morphological observation, genus-specific PCR, and analysis of 16S rRNA gene, which was used to generate the phylogenetic tree, with the 21 members of the 12 genera belonging to Pasteurellaceae to analyze the homology. Two strains were named Yu-ZZ-HL-I-SLG and Yu-ZZ-HL-II-GZ. The comparative result of the 16S rDNA sequence shows that the 2 isolated strains are identical in sequence; the highest identity (99.9%) was observed between the isolated strain and one of the strains of Gallibacterium anatis (AF228002), the homologies between the isolated strain and 3 strains of gallibacterium accessed in NCBI (AF228016, Gallibacterium genomosp.1, AF228017, Gallibacterium genomosp.2, AF228018, Gallibacterium genomosp.1) were above 97.1%, higher than that of the isolated strain and the other strains of the other 11 genera which were between 90.7%-93.2%. It can be seen from the phylogenetic tree that the 2 isolated strains and the other 4 strain of gallibacterium fell into the same branch, furthermore the 2 isolated strains and the strain of Gallibacterium anatis locate in an internal branch, indicating that the 2 isolated strains belong to Gallibacterium anatis.     

鸡传染性支气管炎病毒SC株N基因序列测定与同源性分析

从我国四川省一疑似鸡传染性支气管炎(Avianinfectious bronchitisvirus,IB)的雏鸡病料中成功分离到一株鸡传染性支气管炎病毒(Infectious Bronchitis Virus,IBV),命名为SC。病毒经鸡胚传代、血凝试验监测和负染电镜检查证实为IBV。自接毒鸡胚尿囊液中提取RNA后应用反转录-聚合酶链反应(RT-PCR)扩增得到了IBVSC株mRNA6 cDNA(编码N蛋白)。应用DNAstar5．06,Clustal1．8分析软件将克隆测序的N蛋白基因与Genbank中11株国内外参考毒株进行序列比较分析和同源性分析,发现IBV SC株变异独特,明显不同于国内外参考毒株。     

禽I型副粘病毒广西分离株F基因序列及毒力的研究

对源于鸡、鹅、鸽的 9株APMV_1广西分离株及我国常用的中发型疫苗毒株I系 (Mukteswar株 )的F基因N_端前段进行了RT_PCR扩增 ,产物进行核苷酸序列测定 ,用基因分析软件DNAStar进行分析并与已发表的其它参考毒株进行比较。结果发现 ,广西分离株在裂解位点的氨基酸组成和排列均符合强毒株的特征 ;根据F基因绘制的系谱树来看 ,广西鸡和鹅分离株都归属于基因型VII,证实近年来广西流行的基因型与国内其他地区的相同 ;并发现中发型疫苗毒株I系 (Mukteswar株 )也属于基因型VII。研究还对分离株进行了常规的毒力和致病性测定试验 ,并与根据F基因序列特征判定的结果相比较 ,结果发现其中一株鸽源和两株鹅源分离株根据常规方法判定的结果与毒株在临床上的致病性不相符 ,而根据F基因序列特征判定的结果与毒株在临床上的致病性相一致     

感染高原鼠兔的皮蝇蛆16SrRNA基因序列研究

利用分子生物学技术对高原鼠兔感染皮蝇蛆16SrRNA基因进行了研究,扩增出长度为551 bp的序列,克隆测序,将其序列与GenBank中的皮蝇科、胃蝇科的序列进行了聚类分析,并构建分子进化树.结果显示,感染高原鼠兔的皮蝇蛆与皮蝇科的皮蝇蛆遗传距离更近,在一个大的进化树分支上,基因片段同源性84.6％～88.4％之间,与胃蝇科的红尾胃蝇基因片段同源性60.1％ ～64.4％之间.几株感染高原鼠兔的皮蝇蛆之间的基因片段同源性94.4％～99.6％之间.     

FMDV OA/58病毒株VP3蛋白结构的模拟与分析

以口蹄疫病毒株OA／58 RNA为模板,反转录并扩增目的cDNA,然后与pMD18-T载体连接并转化JM109菌株,提取的重组质粒用凝胶电泳、PCR和BarnHⅠ、HindⅢ双酶切法鉴定。分析表明,口蹄疫病毒VP1、VP2、VP3和VP4在核苷酸水平上的变异率是无差异的（P〉0．05）;而它们在氨基酸水平上的变异率差异显著（P〈0．05）。该毒株与20株源于GenBank中的VP3氨基酸序列比较发现其保守区主要位于第1～24、26～35、37～43、45～57、61～122、124～173、175～209、211～220位。运用同源模建,OA／58 VP3蛋白三维空间结构可分为A,B,C3个结构区域。保守区氨基酸残基在维持VP3蛋白的空间构象和功能方面具有重要作用。     

马流感病毒(A/equine/Qinghai/1/94)核蛋白基因的序列测定及同源性分析

根据已发表的马流感病毒核蛋白基因序列，设计并合成一对特异性引物，经反转录-聚合酶链反应（RT-PCR）成功扩增出了我国马流感病毒（A/equine/Qinghai/1/94核蛋白基因。将该片段连接到PGEM-T-EASY载体并转化DH5α，提取阳性菌落的质粒径EcRo1酶切的PCR鉴定其大小为1.5kb左右，对其测序并进行分析发现，与A/Equine/Kentucky/2/86,A/Equine/Miami/1/63等关系较近，同源率为93.3%--93.4%，而与我国马流感吉林A/Equine/Jilin/1/89株关系较远，同源率仅为84.6%。     

一株海洋细菌HZBN43的鉴定(英文)

[Objective] The aim of this study is to identify a bacterial strain isolated from ocean water from the Yellow Sea.[Method]Using 16S rRNA technique,a strain from Yellow Sea was preliminarily identified and analyzed.[Result]One 1 521 bp fragment of 16S rRNA was amplified from the strain HZBN43;homology analysis between the yielded sequence and the 16S rRNA sequences accessed in NCBI from other strains showed that HZBN43 belonged to Bacillus,and shared 99.79% homologue with the known species of Bacillus selenatarsenatis.[Conclusion]The sequence of strain HZBN43 was obtained.However,because of the incomplete sequence,the confidence level is just 46,so other corroborations are still required for grouping HZBN43 into an exact species.