应用逆转录套式PCR检测新城疫病毒核酸

选择DNV融合蛋白保守的编码区域,设计并合成了一对外引物和一对内引物,建立并优化了检测新城疫病毒核酸的逆转录套式PCRI地,通过检测NDV感染的实验客观存在病料和临床病料,结果表明,逆转录套式PCR法最低能鉴别出约0.3pg的NDV RNA,攻毒后第8天还能从非免疫鸡和SPF鸡泄殖腔拭子中检出DNV,第8天非免疫鸡泄殖腔拭子中NDV的最大检出率为5/10,第8天SPF鸡泄殖腔拭子中NDV的最大检出率为6/10,对非免疫鸡和SPF鸡的泄殖腔中NDV最佳检出时间均在攻毒后第5天。逆转录套式PCRY应运地临床样品中DNV的最大检出率为6/7,经核酸杂交验证,该法具有很高的特异性和敏感性,也比较简便快速,为从分子水平探讨NDV的发病机理、临床早期快速诊断提供了新的研究手段。     

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。     

Molecular characterization of Erwinia amylovora strains from different host plants through RFLP analysis and sequencing of hrpN and dspA/E genes

A total of 73 Erwinia amylovora strains obtained from 13 Maloideae host species and from Rubus spp., and isolated from different geographic areas, were assessed using RFLP and DNA sequencing analysis of the 3' hrp N gene and/or of a fragment of 1341 bp of the dsp A/E region. An Erwinia pyrifoliae strain, used as outgroup, was checked in the same way. For the three strains isolated from Rubus spp. and for one strain from Amelanchier sp., RFLP analysis of the hrp N gene using the Rsa I enzyme yielded a PCR product 60 bp smaller than that of all the other strains. Sequence analysis of the gene revealed this was due to the absence of a 60 bp fragment in the noncoding region downstream of the gene. The strain PD 2915, isolated from Amelanchier sp. grown in Canada, showed five same-sense substitutions and one missense substitution at position 868 of the hrp N gene, converting aspartic acid into asparagine. Also, restriction analysis of a fragment of 613 bp of the dsp A/E region with Cfo I revealed an RFLP pattern suitable for differentiating the E. amylovora strains isolated from Rubus spp. and Amelanchier sp. from all the others. In the dsp A/E coding region, the four strains showed 13–14 missense point mutations, in some cases yielding drastic amino acid substitutions. In addition, partial sequencing of the dsp A/E region of PD 2915 from Amelanchier sp. indicated a higher similarity to E. amylovora strains isolated from Rubus spp. than towards strains from other Maloideae hosts. The E. pyrifoliae strain showed 23 single nucleotide substitutions along the hrp N gene and 88% of nucleotide identity with E. amylovora strains in the portion of dsp A/E region. Artificial inoculations on immature pear fruits and young shoots of Maloideae and Ruboideae showed a restricted pathogenicity for the strains from Rubus and Amelanchier , with the latter inciting blight symptoms only on Amelanchier .     

生长抑素基因疫苗质粒pEGS/2SS的构建及表达

将pcS／2SS中的乙肝表面抗原（HBsAg）S基因及插入S基因中的生长抑素（somatostatin，ss）基因亚克隆到pUC19中，构建成pUSS／S质粒；PCR扩增pcS／SS中SS基因，调整阅读框，融合到pUSS／S质柱S基因后，构建成pUS／2SSG质粒；最后将S／2SSG融合基因克隆到pEGFPN1中EGFP基因的5’端，构建S／2SS-EGFP融合表达质粒pEGS／2SS。酶切、测序鉴定后脂质体包裹法将pEGS／2SS转染HeLa细胞，荧光显微镜下检测荧光，ELISA检测表达产物的SS免疫反应原性。酶切和测序鉴定表明，重组质粒pEGS／2SS构建成功。pEGS／2SS转染24h后的HeLa细胞检测到绿色荧光，72h检测到强烈荧光，表明融合基因在HeLa细胞获得高表达；ELISA证实融合蛋白具有SS的抗原抗体反应原性。质粒pEGS／2SS的成功构建及表达为生长抑素基因免疫的机理及安全性研究奠定了基础。     

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.     

JS/1/97/Go株GPMV NP基因的克隆、序列分析

根据GenBank中发表的GPMV SF02株的NP基因的核苷酸序列设计合成一对引物,采用RT-PCR扩增出与预期设计的1470bp大小相符的片断,将此扩增产物克隆入PMD18-T载体,进行序列测定和分析.结果表明:所扩增的NP基因的核苷酸长为1 470bp,共编码490个氨基酸.同源性分析表明:JS/1/97/Go与国内的SF02株的NP基因核苷酸同源性为98.6%,氨基酸同源性为99.6%.由此可见,鹅副粘病毒JS/1/97/Go分离株与SF02株的亲缘关系较近,同属于新城疫Ⅶ型基因.而其与LaSota株的核苷酸同源性为85.2%,氨基酸同源性为90.8%.说明该毒株相对于经典的NDV在NP基因上已发生了较大的变异.     

三株广西狂犬病病毒NS基因和M基因的克隆与序列分析

本研究设计了一对特异性引物NSM1/NSM2,对三株广西狂犬病病毒NS和M基因同时进行了RT_PCR扩增、克隆和测序。同源性分析表明,三株广西野毒NS基因核苷酸同源性为87.2%~98.4%,M基因核苷酸同源性为90.1%~99.7%;与固定毒和狂犬病相关病毒比较,NS基因分别为79.9%~82.8%和69.7%~71.0%;M基因的分别为82.8%~87.8%和75.0%~77.8%。三株野毒NS基因氨基酸同源性为93.3%~98.7%,M基因氨基酸同源性分别为97.5%~100%。表明广西各地毒株之间亲缘关系不同,但最为相近;与狂犬病固定毒株亲缘关系较远;与狂犬病相关病毒亲缘关系最远。     

中国禽(番鸭)呼肠孤病毒YB株S4基因序列分析

应用非免疫番鸭胚增殖中国禽(番鸭)呼肠孤病毒YB分离株,用LSTRIAZOL提取病毒RNA,反转录-聚合酶链反应(RT-PCR)扩增中国禽(番鸭)呼肠孤病毒YB分离株S4基因节段cDNA.将S4cDNA克隆到PMDl8-T载体上,并进行了鉴定和核苷酸序列测定.序列分析结果,克隆的S4cDNA共1 124bp,包括非编码区和完整的阅读框架.分子进化系统分析表明该毒株与禽呼肠孤病毒(鸡呼肠孤病毒)的亲缘关系较远,DRV-YB与DRV-89330同缘率为93.3%.     

Isolation of Olive latent virus 1 from Tulip in Toyama Prefecture

A virus whose coat protein gene had a high sequence homology with the coat protein gene of Olive latent virus 1 was isolated from diseased tulip in Toyama Prefecture. Received 1 June 2001/ Accepted in revised form 1 August 2001     

Characterization of an endopolygalacturonase Gene cppg1 from Phytopathogenic Fungus Chondrostereum purpureum

Chondrostereum purpureum, a phytopathogenic fungus, produces endopolygalacturonase (endoPG) which has been suggested to have a causal role in the silver-leaf symptom of apple trees. In this paper, we detected C. purpureurn-derived endoPG at the infection sites using ELISA with a polyclonal antibody against endoPG I. A gene encoding endoPG I and its homolog were also isolated from the C. purpureum genome. The endoPG I gene was designated as cppg1. The cppg1 gene is the first fungal endoPG gene reported in the Basidiomycetes. Received 31 May 2000/ Accepted in revised form 13 September 2000