‘鸭梨’钙调素基因的克隆与表达分析

以‘鸭梨’为材料,用RT-PCR及RACE技术克隆CaM,并借助实时定量PCR技术分析‘鸭梨’花、叶及果实不同发育时期的表达模式,获得了2个长度为764和801bp的CaM cDNA序列,分别命名为PbCaM1和PbCaM2,二者均含有450bp完整开放阅读框,编码149个氨基酸,且氨基酸序列相同。‘鸭梨’CaM在系统进化上具有高度保守性,与苹果相比,两者氨基酸序列为100%一致性。PbCaM1和PbCaM2具有时空表达特异性,它们在成叶、盛花期花瓣和幼果期表达量较高。本研究表明CaM具有高度保守性,PbCaM1和PbCaM2在‘鸭梨’果实早期生长发育过程中起着非常重要的作用。     

犬瘟热病毒F蛋白分子生物学研究进展

犬瘟热病毒融合蛋白是囊膜糖蛋白,是产生中和抗体的主要保护性抗原,结构相对保守。融合蛋白介导病毒囊膜和细胞膜融合,决定病毒在宿主体内扩散的能力,在病毒的致病性及免疫原性上具有重要作用。因此,对犬瘟热融合蛋白基因及其蛋白的结构和功能进行研究具有重要的意义。本文从蛋白结构、蛋白功能、核酸序列比对等多方面对融合蛋白进行了阐述。     

The first survey and molecular identification of Entamoeba spp. in farm animals on Qinghai-Tibetan Plateau of China

Protozoans of Entamoeba spp. are globally distributed zoonotic parasites that infect diverse animal hosts and humans. Prevalence and species/genotypes distribution of Entamoeba spp. in domestic animals are not fully investigated on Qinghai-Tibetan Plateau (QTP), an animal husbandry and agriculture region of China. In a survey, 528 fecal samples were collected from 7 species of domestic animals on multiple locations across QTP region and analyzed by PCR and sequencing analysis. The overall prevalence of Entamoeba spp. infection in all examined animals was 97.9 %. Four Entamoeba species, E. bovis, E. moshkovskii, E. ecuadoriensis and E. histolytica were found, and majority (94.2 %) of Entamoeba-infected animals harbored E. bovis. Six Entamoeba genotypes, Entamoeba ribosomal lineages (RL) 1, 2, 3, 4, 8 and 9 were identified by sequencing analysis. Two zoonotic species, E. moshkovskii and E. histolytica, were present in horses, while E. ecuadoriensis and E. bovis were found in horses and all species of seven farm animals, respectively. It was also observed that six Entamoeba genotypes were distributed in animals in specific pattern. The results revealed high prevalence of Entamoeba spp. infection in livestock, broad range of hosts as well as diversity and species/genotype distribution of Entamoeba spp. in farm animals inhabiting on the high altitude QTP region.     

日本大耳白兔TLR3部分cDNA克隆及mRNA在组织中的分布

采用RT—PCR技术从日本大耳白兔的脾脏组织克隆出兔的Toll样受体基因3（命名为。TLR3），并对其mRNA在兔的17种组织中的分布情况进行了检测。结果显示，RTLR3核苷酸序列与GenBank中登载的穴兔（Oryctolagus cuniculus）TLR3序列（登录号：NM_001082219）相似性为100％；兔的胸腺、脾脏、睾丸等14种组织中检测出TLR3 mRNA的转录产物，而在骨骼、胃和皮肤中未能发现。推导的氨基酸序列同源性比对表明，兔TLR3与人、野猪、牛、猫、褐鼠等动物的同源性最高，为80％-85％；与原鸡同源性次之，为61％；与草鱼、绿河豚等同源性在45％～48％之间；系统进化树分析表明，兔TLR3与马的亲缘关系最接近，与猪、人／绵羊、牛、猩猩／猫的亲缘关系依次渐远，与鼠的亲缘关系最远。可见，TLR3在不同种属动物及不同组织中所起的作用具有生物多样性。     

Cloning and analysis of cross-intron genomic gene encoding ACO in Paeonia suffruticosa Andr.

The last step of ethylene biosynthesis in higher plants is to convert 1-aminocyclopropane-1-carboxylic acid (ACC) to ethylene by ACC oxidase (ACO). In our investigation, a cross-introns genomic DNA gene encoding ACC oxidase, PsgACO, was isolated from Paeonia suffruticosa. It revealed that PsgACO (FJ855434) has 1281 bases, containing four exons and three introns, encoding 312 amino acids. The four exons stretched from 1 to 105, 217 to 434, 592 to 925 and 1000 to 1281 bases. A splicing junction sequence of all the exon-introns conformed to the GT-AG rule in the cross-intron genomic DNA sequence of the ACO gene. PsgACO showed high homology to many characterized ACC oxidases both at the nucleic acid and amino acid levels. As well, twelve amino acid residues were conserved among many ACOs from other species. A phylogenetic tree analysis indicated that the amino acid of ACOs is quite conserved among the different eudicots. The phylogenetic tree showed that both the tree peony and herbaceous peony are quite isolated taxa. Bioinformatic analysis showed that the molecular weight of ACO is 35.29 kD, with a theoretical pI of 5.25. It is a non-secrete, stable hydrophilic protein, located in the cytoplasm.     

鸡CD4蛋白基因的克隆及其mRNA在淋巴器官中的表达

从鸡胸腺、脾脏、哈德氏腺、外周血液和法氏囊等免疫器官中分离淋巴细胞,应用RT-PCR对这些免疫器官中鸡CD4分子mRNA的表达进行了研究。同时,用RT-PCR对鸡脾淋巴细胞CD4分子cDNA进行了克隆和序列测定。结果表明,在上述器官中,法氏囊淋巴细胞不表达鸡CD4分子mRNA,其他器官中均有表达。通过序列分析表明,本试验扩增得到的基因为编码鸡CD4分子的基因。     

O型口蹄疫病毒VP1嵌合基因的构建及原核表达

首先合成我国O型口蹄疫病毒2个疫苗毒株VP1基因的3个抗原袁位，与另外扩增的流行毒株VP1基因末端273bp片段相连,构建出O型VP1嵌合基因片段（VP1O）。然后，将VPIO基因连接到原核表达载体pET28a上，构建了重组表达质粒pET28a-VP1O，转化大肠杆菌BL21（DE3）进行诱导表达。SDS-PAGE电泳表明。VP1O基因在大肠杆菌中获得表达。Western blotting检测证实表达的VP1O蛋白具有良好的生物学活性。对表达蛋白通过包涵体洗涤的方法进行初步纯化，获得了较高纯度的VP1O蛋白。     

一株禽流感病毒全基因的序列分析

通过反转录-聚合酶链式反应(RT-PCR)技术对禽流感病毒A/Turkey/Wisconsin/1/66(H9N2)的8个基因片段即PA、PB1、PB2、NS、NP、M、HA、NA分别进行扩增,然后将其克隆到PMD18-T载体后进行序列测定和拼接;并将克隆到的8个基因片段与以下毒株各个基因的相应序列进行比较分析:Duck/HongKong/Y280/97(DHKY280/97)、Duck/HongKong/YT439/97(DHKY439/97)、Quail/HongKong/G1/97(QHKG1/97)、A/Chicken/Beijing/1/94(CBJ1/94)、Chicken/HongKong/G9/97(CHKG9/97)、A/Turkey/California1/66(TC/1/66).结果表明:我们克隆到的TW1/66株的8个基因片段均含有相应病毒基因的完整开放阅读框架:TW1/66的各基因与TC/1/66株相应各基因同源性最高(NS基因除外,同源性只有(67.4%).与其它各毒株各基因同源性均较低,但与DHKY439/97各基因同源性高于与DHKY280/97、QHKG1/97、CBJ1/94、CHKG9/97各基因同源性.     

牛分枝杆菌MPB70基因的克隆及其在大肠杆菌中的表达

本研究以牛分枝杆菌Vallee111染色体DNA为模板,以MPB70成熟蛋白基因特异性引物进行PCR扩增,获得约500bp的DNA片段.通过T-A克隆技术,将PCR产物克隆至pGEM-T Vector中,成功地构建出克隆载体pGEM-T-70.以BamH Ⅰ和EcoR Ⅰ双酶切pGEM-T-70和pET28a( ),并将纯化的MPB70基因亚克隆至pET28a( )中,构建出原核表达载体pET28a-70.将pET28a-70转化至感受态E.coli BL21(DE3)中,经IPTG诱导和SDS-PAGE分析,可见约25Ku外源蛋白带.Western blot分析发现,该蛋白具有牛分枝杆菌抗原性,从而为进一步研究MPB70的亚单位疫苗及DNA疫苗奠定基础.