烟草蚀纹病毒外壳蛋白基因的克隆、原核表达及抗血清的制备

从山东省感病的烟草上分离获得了一烟草蚀纹病毒(TEV)分离物,命名为TEV-SD1.根据已报道烟草蚀纹病毒外壳蛋白(coat protein CP)基因序列设计并合成2条引物,通过RT-PCR扩增得到长度约800bp的目的片段.将目的片段与质粒pET-22b( )连接,构建了包含TEV CP基因的原核表达载体pETEV-CP,并导入大肠杆菌BL21中.序列分析表明:TEV-SD1的CP基因全长789bp,编码263个氨基酸;与GenBank中已报道的TEV 5个分离物CP基因相比,核苷酸及推导的氨基酸序列同源性为94.1%～98.6%.37℃培养条件下,BL21/pETEV-CP经IPTG诱导表达,SDS-PAGE结果显示,表达的TEV CP融合蛋白的相对分子质量约为33 kDa.以表达的融合蛋白为抗原,免疫家兔,制备的抗血清的效价为1/2048,且具有良好的特异性.     

葡萄卷叶伴随病毒1号和3号宁夏分离物部分基因序列分析

为明确葡萄卷叶伴随病毒(GLRaVs)在宁夏贺兰山东麓酿酒葡萄上的侵染状况,采用RT-PCR技术对40份酿酒葡萄样品中的GLRaV-1~GLRaV-5进行了外壳蛋白(CP)、复制酶(RdRp)和热激蛋白(HSP70)基因序列的克隆和分析。检测结果表明,在所检测的5种病毒中,除GLRaV-2和GLRaV-4未检测到外,GLRaV-1和GLRaV-3的检出率最高,分别为20.0%和32.5%,GLRaV-5的检出率仅为5.0%;有6个样品存在GLRaV-1和GLRaV-3两种病毒复合侵染。序列分析表明,GLRaV-1宁夏分离物的部分CP基因序列长度为232nt,其两种分离物间的核苷酸序列同源率为90%,与已报道的国内外其他分离物CP基因序列相比,其同源率为90%~99%;GLRaV-3宁夏分离物的CP基因序列长度为942nt,其两种分离物间的核苷酸序列同源率为40%,与已报道的国内外其他分离物CP基因序列相比,其同源率为40%~99%;GLRaV-3宁夏分离物的RdRp基因序列长度为683nt,其各分离物间的核苷酸序列同源率为90%以上,与已报道的国内外其他分离物RdRp基因序列相比,其同源率为90%~99%;GLRaV-3宁夏分离物的HSP70基因序列长度为546nt,其两种分离物间的核苷酸序列同源率为96%,与已报道的国内外其他分离物HSP70基因序列相比,其同源率为96%~99%。     

烟草花叶病毒丁香分离物的分离与鉴定

 从表现花叶症状的丁香病株上获得一病毒分离物,其在电镜下为约300 nm×18nm的杆状粒子;电泳分析表明感病组织中ds RNA大约为6.4kbp,而其外壳蛋白分子量约为17.6k Da。以上实验结果初步将该病毒分离物鉴定为烟草花叶病毒属(Tobamovirus)。根据该属病毒复制酶基因序列设计通用引物,进行RT-PCR检测,扩增出约1000 bp的预期特异片段(Gen Bank AY566703)。将PCR产物克隆后测序,序列分析表明,与从蚕豆中分离的TMV-B株系序列(Gen Bank AJ011933.1)同源性为99.90%。根据烟草花叶病毒(Tobacco mosaic virus,TMV)的RNA CP基因序列设计引物,进行RT-PCR,扩增出约800 bp的预期特异片段(Gen Bank AY56672),序列分析表明,与TMV-B株系序列(Gen Bank AJ011933.1)同源性达99%,上述实验结果表明,该病毒分离物为TMV。由于该分离物与TMV-B在指示植物上的症状存在明显差异,所以,作者把该分离物暂命名为TMV-S。     

北京地区百合无症病毒CP基因的克隆与分析

以感染百合无症病毒(LSV)的百合叶片为材料,提取总RNA为模板,通过反转录聚合酶链式反应(RT-PCR)扩增出856bp大小的LSV CP基因片段.经Blast比对发现,该基因片段与Genbank上发表的ISV CP基因序列(DQ294655.1)同源性为97.31%.由该序列推导出的氨基酸序列与其相似度为98.6%,仅存在某些氨基酸的差异.经过聚类分析表明,该CP基因的氨基酸序列与厦门和兰州分离的病毒遗传距离较近,而与海宁和广州分离的病毒遗传距离较远.     

合肥地区发生的西瓜花叶病的病原鉴定

 从合肥市郊区的西瓜病叶上分离出一病毒分离物,该分离物的热钝化温度为60~65℃,稀释终点为10^-4~10^-5,寄主体外存活期为20~23 d,电镜观察病毒粒子约750 nm×13 nm。参考已发表的小西葫芦黄化花叶病毒(Zucchini yellow mosaic virus,ZYMV) CP基因序列设计引物,RT-PCR扩增得到CP基因片段。将该CP片段克隆到pGEM-3Zf (+)中,测序结果表明,该CP基因全长840 nt,共编码279个氨基酸,与国内报道的ZYMV CP基因的核苷酸序列同源性为83.0%~97.3%,氨基酸序列的同源性为91.8%~99.8%,证明该分离物为ZYMV。     

韭葱黄条病毒厦门分离物外壳蛋白基因序列分析及其分组

 本文在测定了侵染厦门古宅大蒜的病毒分离物（LYSV XM）CP基因序列的基础上,进一步从GenBank登录的58个分离物中选取具有代表性的29个分离物建立CP基因核苷酸序列系统进化树。利用该系统进化树明确了LYSV XM与其他分离物间的进化关系,并在前人研究基础上提出一种基于CP基因核苷酸序列的类群分组方法。     

4种柑橘衰退病毒源单蚜传毒分离株CP基因的分子特征

 对4种柑橘衰退病毒源及其31个单蚜传毒分离株的CP基因做了限制性片段长度多态性(RFLP)和单链构象多态性(SSCP)分析,并对其中8个单蚜传毒分离株的CP基因进行了序列分析。实验明确了所研究柑橘衰退病毒(Citrus tristeza virus,CTV)的CPG/Hinf I RFLP组群和CPG/SSCP模式,二者能较好地对应并有效验证了单蚜传毒对CTV毒源的分离纯化作用;CP基因序列分析结果表明,相同CPG/Hinf I RFLP组群的单蚜传毒分离株间具有高度的序列相似性,而不同CPG/Hinf I RFLP组群单蚜传毒分离株间则存在较大差异;通过与已知生物学特性CTV分离株比较,初步建立了上述CP基因分子特征与病毒生物学特性之间的联系。     

北京地区茄子感染番茄褪绿病毒的分子鉴定

为明确北京地区茄子感染番茄褪绿病毒(Tomato chlorosis virus,To CV)的情况,于2015年3—6月收集了10份疑似感染To CV的设施茄子样品,通过PCR分子鉴定法进行检测,并进一步对扩增阳性样品To CV的CP基因采用邻接法进行了系统进化分析。结果表明,10个检测样品中有4个扩增得到约463 bp的特异条带,经测序与Gen Bank中To CV序列相似性达到99.0%以上,表明这4个样品均携带有该病毒,检出率为40%;To CV茄子分离物的CP基因序列大小为774 bp,Gen Bank登录号为KT751008,与To CV北京番茄分离物(KC311375)同源性最高,达到99.9%,确认该序列为To CV片段;系统进化树显示,To CV茄子分离物与To CV日本分离物(AB513443)处于同一分支,具有密切的亲缘关系,表明不同国家To CV分离物之间的亲缘关系与地理距离具有一定的相关性。     

一种侵染滇重楼的Potexvirus病毒分离物分子鉴定及其3′末端序列分析

从云南武定的滇重楼上得到一个病毒分离物Paris-YN,病毒粒体为弯曲线状。利用RT-PCR扩增获得一条1074bp的片段,序列比较分析发现其与马铃薯X病毒属(Potexvirus)病毒3′末端的结构最为相似,且与属内的白三叶草花叶病毒等20个不同分离物3′末端有36.7%～58.9%的同源性;该病毒cp基因长639个核苷酸,编码212个氨基酸(22.8kDa),与20个Potexvirus病毒分离物的CP氨基酸序列比较发现,Paris-YN与白三叶草花叶病毒的CP氨基酸同源性最高(60.1%)。证据表明,该分离物可能为Potexvirus的新成员,暂命名为重楼X病毒(Paris polyphylla virus X)。     

建兰花叶病毒外壳蛋白基因和3′UTR序列测定与分析

采用单链构象多态性分析从建兰花叶病毒(Cymbidium mosaic virus,CyMV)的8个分离物筛选得到5个存在遗传变异的分离物,并测定了外壳蛋白(coat protein,CP)基因和3'非编码区(3'UTR)序列,经序列分析表明5个分离物与其他分离物间的CP核苷酸和氨基酸序列相似性分别为87,1％～99.9％和91.1％～99.6％,属于亚组A成员.CP基因不同片段受到正选择压力的作用不一样,C端受到负选择压力的作用不易发生变异,而N端受到正选择压力的作用容易发生变异.通过RNAsharpes软件分析3 'UTR序列发现各分离物均形成带有Potexvirus属保守核苷酸序列“AC(C/T) TAA”的三叶草茎环结构,这种结构的功能可能与病毒RNA复制有关.     

Biological, serological, and molecular differences among isolates of potato a potyvirus

ABSTRACT Sequences of the coat protein (CP) and 3'-end nontranslated region (3'NTR) of 13 isolates and the helper component proteinase (HC) of nine isolates of potato A potyvirus (PVA) were determined and compared with the eight previously determined PVA CP and 3'NTR sequences and one HC sequence. CP amino acid (aa), 3'NTR nucleotide, and HC aa sequence identities were 92.9, 93.4, and 94.8%, respectively. Sequence data, serological tests, and the necrotic local lesions induced in the leaves of the potato hybrid 'A6' confirmed that tamarillo mosaic virus is a strain of PVA. The aa substitutions A6T and G7S in the CP N-terminus were correlated with loss of aphid transmissibility. Development of necrotic lesions or nonnecrotic symptoms in the systemically infected leaves or lack of systemic spread in potato cv. King Edward were used to place the PVA isolates into four strain groups, but this grouping was not correlated with any differences in CP, HC, or 3'NTR. Recognition of CP by three monoclonal antibodies was used to place the PVA isolates into three groups different from the four groups above. The epitopes of two mono-clonal antibodies were mapped by site-directed mutagenesis to the same lysine residue at the CP aa 34.     

番木瓜环斑病毒南瓜分离物外壳蛋白基因的克隆及序列分析

利用电镜和酶联免疫法在云南省采集到的5份南瓜病样中检测到番木瓜环斑病毒(Papayaring spot virus,PRSV)。为了进一步从分子水平确定云南省南瓜病毒病原种类,并为下一步转基因育种提供抗性基因,采用反转录PCR(RT-PCR)方法扩增了5个分离物的外壳蛋白(coat protein,CP)基因片段,并克隆到pGEM-T载体中。核苷酸序列测定表明,番木瓜环斑病毒石屏分离物(PRSV-SP)和番木瓜环斑病毒蒙自分离物(PRSV-MZ)的CP基因长873nt,编码290个氨基酸,番木瓜环斑病毒峨山分离物(PRSV-ES)、番木瓜环斑病毒版纳分离物(PRSV-BN)和番木瓜环斑病毒宾川分离物(PRSV-BC),3个分离物CP基因长867nt,编码288个氨基酸。PRSV5个分离物核苷酸序列的同源性在94%以上,氨基酸序列的同源性在96%以上。与国内外17个分离物相比,核苷酸序列同源性为89.6%~98.7%,氨基酸序列同源性为86.5%~99.6%。其中PRSV-SP和来自于越南分离物PRSV-V47无论是核苷酸序列,还是氨基酸序列同源性都达到了最高,而5个分离物与来自于巴西(PRSV-BR)、美国(PRSV-USA)、墨西哥(PRSV-Y)核苷酸序列同源性均低于90%。     

一个马铃薯X病毒分离物的外壳蛋白基因序列分析与株系鉴定

对山东省侵染马铃薯的一个马铃薯X病毒(PVX)分离物PVX—SD1的外壳蛋白(CP)基因进行了克隆和序列分析。以提纯的病毒RNA为模板，应用RT-PCR扩增目的基因，通过常规的基因克隆法将扩增的CP基因导入pUC19载体，测序。结果表明，PVX—SD1的CP基因长719bp，可编码248个氨基酸；与Gen—Bank中报道的15个有代表性的株系或分离物相比较，核苷酸同源性在80．1％-99．7％，氨基酸同源性在89．8％-100％；与欧洲株系UK3仅1个核苷酸不同，同源性为99．7％，氨基酸同源性达100％，表明它们可能为同一株系，属于X^3组．     

Sequence analysis within the RNA 3 of seven Spanish tomato isolates of Parietaria mottle virus (PMoV-T) reveals important structural differences with the parietaria isolates (PMoV)

The genomic regions encoding the putative movement protein (MP), coat protein (CP) and intergenic region (IGR) of seven Spanish isolates of the Parietaria mottle virus which infects tomato plants (PMoV-T) were sequenced. Values for the genetic diversity of the PMoV-T isolates were 0.056, 0.047 and 0.013 for the CP, MP genes and IGR, respectively. Nucleotide and amino acid sequence comparison of the seven PMoV-T isolates with those of PMoV revealed significant differences. All of them had a cytosine deletion at position 1366, also confirmed in an Italian tomato isolate, which involves a start codon for the CP gene different from that for the PMoV sequence, resulting in a CP 16 amino acids shorter than the PMoV CP. The certainty of a cytosine deletion only associated to the tomato isolates or the possibility of a mistake in the PMoV published sequence are the two hypotheses that could explain this difference. Structural motifs highly conserved in Ilarviruses were identified in PMoV-T MP and CP. A stable hairpin structure is proposed for IGR, by the initiation site for subgenomic RNA 4 synthesis. Phylogenetic analysis of CP and MP amino acid sequences showed that Spanish PMoV-T isolates form a separate group from PMoV and other members of the Ilarvirus genus. Comparative analysis with different PMoV isolates including tomato isolates from other regions and isolates from different hosts are necessary to confirm this differentiation.     

Characterization of Citrus tristeza virus isolates in northern Iran

The biological and molecular properties of four Citrus tristeza virus (CTV) isolates isolated from infected Satsuma trees imported from Japan, and growing in citrus groves in northern Iran (Mahdasht orchards, Mazandaran Province), were investigated. CTV-infected samples were collected from sweet orange trees and grafted onto Alemow (Citrus macrophylla Wester) seedlings. On indicator plants, these isolates produced various symptoms including vein clearing and stem pitting on Mexican lime, Alemow, and Citrus hystrix, and yellowing and stunting on sour orange and grapefruit seedlings. Citrus samples were also surveyed for CTV using serological tests. The coat protein (CP) gene of these isolates was amplified using specific primers, yielding an amplicon of 672 bp for all isolates. Sequence analysis showed 98%–99% sequence homology of Iranian isolates with the Californian CTV severe stem-pitting isolate SY568 and 97%–98% homology with the Japanese seedling yellows isolate NUagA. The Iranian isolates were compared by restriction fragment length polymorphism (RFLP) analysis of the CP amplicon for further classification.