广东番茄曲叶病毒G3分离物基因组DNA-A的分子特征

 从采集于广东花都的番茄曲叶病病株上分离到病毒分离物ToLCGDV-[G3],序列分析结果表明,其DNA-A为单链环状,全长2744 nt,共有6个ORFs,其中病毒链上编码AV1(CP)、AV2,互补链上编码AC1、AC2、AC3和AC4。BLAST结果显示,与ToLCGDV-[G3]基因组有同源关系的均属双生病毒科菜豆金色花叶病毒属。进一步比较结果表明,ToLCGDV-[G3]与有同源性的菜豆金色花叶病毒属病毒的DNA-A全序列同源率最高为87.9%。其中IR的同源率为59.0%~85.3%,而AV1、AV2、AC1、AC2、AC3和AC4这6个ORFs同源率分别为73.6%~95.2%、64.0%~95.4%、71.7%~87.7%、69.6%~93.9%、67.7%~95.1%和64.1%~94.2%,它们各自编码的氨基酸序列同源率分别为76.3%~99.2%、52.6%~95.7%、69.7%~88.1%、51.9%~88.9%、63.4%~92.5%和33.0%~90.7%。系统进化关系分析结果显示,ToLCGDV-[G3]与ToLCGDV-[G2]亲缘关系最近,二者组成一个独立的分支,与其它40种菜豆金色花叶病毒属病毒的亲缘关系均较远。因此,ToLCGDV-[G3]可能是一个先前未报道的双生病毒科菜豆金色花叶病毒属新种。     

复合侵染水茄的两种菜豆金色花叶病毒属病毒基因组结构特征分析

为明确水茄Solanum torvum植株叶片邹缩、褪绿是否由菜豆金色花叶病毒属病毒侵染引起,从云南省西双版纳傣族自治州田间采集具有疑似感染症状的水茄植株叶片样品,应用菜豆金色花叶病毒属病毒简并引物和特异性引物进行PCR扩增、克隆和测序,通过生物信息软件分析比较其核苷酸序列特征,并对其进行系统发育分析。结果显示,从采集的疑似病叶中共克隆获得了5条菜豆金色花叶病毒属病毒DNA-A全序列和3条DNA-B全序列,经全序列分析发现,侵染水茄的2种菜豆金色花叶病毒属病毒分离物分别属于中国南瓜曲叶病毒(squash leaf curl China virus,SLCCNV)和野茼蒿黄脉病毒(Crassocephalum yellow vein virus,CraYVV)。SLCCNV水茄分离物的基因组具有典型的菜豆金色花叶病毒属病毒双组分结构特征,与来自泰国的SLCCNV分离物(AB330078)亲缘关系最近,相似性最高达到99.0%;CraYVV水茄分离物的基因组具有典型的菜豆金色花叶病毒属病毒单组分结构特征,与来自云南省景洪市的CraYVV分离物(EF165536)亲缘关系最近,相似性最高达到97.6%。表明水茄是这2种菜豆金色花叶病毒属病毒的新寄主,并首次发现双组分和单组分菜豆金色花叶病毒属病毒可复合侵染水茄。     

番茄黄化曲叶病毒在湖北首次报道

2014年春季,在湖北省武汉市发现种植的番茄表现植株矮缩,叶片上卷,叶缘黄化等症状。PCR检测结果显示,所有采集的病样中均存在菜豆金色花叶病毒属病毒。进一步通过滚环扩增方法获得了该病毒的湖北分离物HB01的全基因组。基因克隆及序列分析结果表明,该病毒基因组全长为2 781nt,与已报道的番茄黄化曲叶病毒(TYLCV)各分离物同源性在89.0%以上,而与来自中国不同地区的TYLCV分离物的同源率均在97.0%以上。因此,HB01属于TYLCV的一个分离物。     

侵染青蒿的烟草曲茎病毒的分子鉴定及基因组结构特征分析

菜豆金色花叶病毒属病毒是一类在全球热带及亚热带地区造成严重经济损失的植物病毒,田间杂草是这类病毒重要的中间寄主。 本研究从云南省玉溪市采集了表现黄脉的青蒿植株,通过PCR扩增、克隆及测序从样品中获得两条菜豆金色花叶病毒属病毒DNA-A全基因组序列,分别为YN6393-23和YN6393-27,其全长均为2 739 bp,相似性为100%。序列分析发现,YN6393-23和YN6393-27的核苷酸序列与烟草曲茎病毒Tobacco curly shoot virus(TbCSV）的分离物YN4584的核苷酸序列相似性最高,为99.45%。根据国际病毒分类委员会对菜豆金色花叶病毒属病毒种的分类标准,全基因组序列相似性大于91%则为同种病毒,表明此病毒分离物为烟草曲茎病毒的一个分离物。这是菜豆金色花叶病毒属病毒侵染青蒿植株的首次报道。     

侵染垂花悬铃花的木尔坦棉花曲叶病毒分子特征研究

 垂花悬铃花曲叶病是近期在广东发现的一种新病害,病株表现为叶片向上卷曲,叶脉肿大,叶脉变深绿色等症状。PCR检测结果显示, 该病样中均存在菜豆金色花叶病毒属病毒。基因克隆及序列分析结果表明,该病毒分离物（GD11）DNA-A全长为2 737 nt,具有菜豆金色花叶病毒属病毒基因组典型特征,为闭合环状单链DNA,编码6个ORFs;该序列与木尔坦棉花曲叶病毒(CLCuMV)各分离物序列的相似性均大于89.0%,其中与G6、Okra06及GX1等分离物序列的相似性大于99.0%。该病毒分离物也伴有卫星DNA β分子,其全长为1 348 nt,与CLCuMV各分离物的DNA β序列相似性大于85.0%,其中与G6、Okra06及GX1等DNA β的序列相似性均大于99.0%。因此,侵染广东垂花悬铃花的病毒分离物属于CLCuMV,且与入侵我国的朱槿分离物G6、黄秋葵分离物Okra06及棉花分离物GX1亲缘关系很近。本文首次报道了CLCuMV及其卫星β复合侵染垂花悬铃花。     

侵染木薯的两种单组分菜豆金色花叶病毒属病毒及卫星分子基因组结构特征分析

 为明确木薯(Manihot esculenta Crantz)植株叶片皱缩、畸形是否由菜豆金色花叶病毒属病毒侵染引起,从云南省红河州田间采集具有疑似感染症状的木薯植株叶片样品,应用菜豆金色花叶病毒属病毒简并引物、种专化性引物及卫星分子引物进行PCR扩增、克隆,通过测序分析其核苷酸序列特征并对其进行系统进化分析。结果显示,从采集疑似病叶中共克隆获得4条菜豆金色花叶病毒属病毒DNA-A全序列和6条beta卫星分子全序列,经全序列分析发现侵染木薯的2种菜豆金色花叶病毒属病毒分离物分别属于烟草曲茎病毒(tobacco curly shoot virus,TbCSV)和中国胜红蓟黄脉病毒(ageratum yellow vein China virus,AYVCNV)。TbCSV木薯分离物全基因组核苷酸序列与分离自云南的TbCSV-YN2247(KX290925)分离物亲缘关系最近,相似性最高达到96.67%;AYVCNV木薯分离物全基因组核苷酸序列与分离自云南的AYVCNV-YN4326(KU601622)分离物亲缘关系最近,相似性最高达到95.80%;侵染木薯的beta卫星分子分别为赛葵黄脉病毒beta卫星(malvastrum yellow vein betasatellite,MaYVB)和中国胜红蓟黄脉病毒beta卫星(ageratum yellow vein China virus betasatellite,AYVCNB),MaYVB-YN6332-12全基因组核苷酸序列与分离自云南的MaYVB-Y216(KX290925)分离物亲缘关系最近,相似性最高达到96.4%;AYVCNB-YN6338-17全基因组核苷酸序列与分离自海南的AYVCNB-Hn9(KU601622)分离物亲缘关系最近,相似性最高达到90.4%,表明木薯是这两种菜豆金色花叶病毒属病毒的新寄主。单组分菜豆金色花叶病毒属病毒及其伴随beta卫星分子可以复合侵染木薯植株为首次发现。     

一种侵染鳢肠的双生病毒基因组特征

菜豆金色花叶病毒属病毒是热带及亚热带地区经济作物的重要病原病毒,该类病毒在田间的杂草寄主范围较为广泛。本研究从云南红河流域采集到叶脉黄化的鳢肠植株,经克隆获得了菜豆金色花叶病毒属病毒分离物YN3306,该分离物核苷酸序列全长2749 nt,具有典型的双生病毒基因组结构特征。进一步分析发现,分离物属于金腰剑曲叶病毒(Synedrella leaf curl virus,SyLCV),RDP软件分析表明,该分离物是由烟草曲茎病毒(Tobacco curly shoot virus,Tb CSV)、云南烟草曲叶病毒(Tobacco leaf curl Yunnan virus,TbLCYnV)和金腰剑曲叶病毒重组产生的病毒。本研究首次报道了GenBank中在印度注册的SyLCV可以侵染鳢肠植株。     

海南红麻曲叶病的病原检测与鉴定

 红麻曲叶病是2012年在海南省海口市发现的一种新病害,病株表现为叶片向上卷曲、叶脉肿大、叶脉变深绿色等症状。PCR检测结果显示,该病样中均存在菜豆金色花叶病毒属病毒。基因克隆及序列分析结果表明,该病毒分离物(HN08)基因组仅含A组分(DNA-A),其全长为2 738 nt,与木尔坦棉花曲叶病毒(CLCuMuV)各分离物的相似性均大于89.0 %,其中与中国各分离物的相似性均大于99.0 %。该病毒分离物也伴随有β卫星分子,其全长为1 346 nt,与CLCuMuV各分离物伴随的β卫星分子(CLCuMuB)序列相似性大于83.0 %,其中与分离物Fz1的序列相似性最高,为99.7 %。构建了HN08 DNA-A及其β卫星分子侵染性克隆,通过农杆菌注射接种红麻,接种后30 d,HN08 DNA-A及其β卫星分子混合接种的红麻植株新出叶片开始产生曲叶症状;接种后60 d,二者混合接种的植株大部分叶片表现为严重的曲叶症状,且与田间自然病株症状相同,而二者各自单独接种的红麻植株没有产生明显的症状。PCR及Southern blot检测进一步证实这些症状是由HN08 DNA-A及其β卫星分子的共同侵染引起的。因此,海南红麻曲叶病是由CLCuMuV及其伴随的β卫星分子(CLCuMuB)共同侵染引起的。本文首次报道了红麻是CLCuMuV自然新寄主。     

广东黄秋葵黄脉曲叶病样中检测到烟粉虱传双生病毒

黄秋葵是近几年来从日本和我国台湾引进的一种蔬菜作物。近期,广东的黄秋葵上发生了黄脉曲叶病。病株的典型症状表现为叶脉黄化,在叶片正面形成网络状,在叶背面叶脉肿大突起明显,病株幼叶小且向下卷曲,甚至整片幼叶黄化。植株早期被感染表现矮化。在发生黄脉曲叶病的黄秋葵田间,其病株率高达60%以上。用烟粉虱传双生病毒简并引物对随机采集的病样进行PCR检测,从这些病样中均能扩增出1条预期大小为570 bp的特异片段;基因克隆及测序分析结果表明,与该特异片段同源的均属双生病毒科菜豆金色花叶病毒属病毒DNA,其中与木尔坦棉花曲叶病毒（Cotton leaf curl Multan virus, CLCuMV）分离物G6相似性最高,为99%。这些研究结果表明,广东黄秋葵黄脉曲叶病中存在烟粉虱传双生病毒,该病害可能也是由CLCuMV侵染引起的。     

侵染假酸浆的泰国番茄黄化曲叶病毒全基因组结构特征

为明确假酸浆Nicandra physalodes叶片黄化、皱缩症状是否由菜豆金色花叶病毒属病毒侵染引起,本研究利用分子检测方法和生物信息学技术鉴定了假酸浆样品中的病毒种类。从采集的病样中克隆并获得了2条菜豆金色花叶病毒属病毒DNA-A全序列和1条beta卫星全序列,经全序列分析发现,该双生病毒的两条DNA-A全序列与泰国番茄黄化曲叶病毒(tomato yellow leaf curl Thailand virus, TYLCTHV)云南分离物TYLCTHV-YN1732一致性最高,达99.3%,亲缘关系较近;beta卫星的全序列与云南番茄曲叶beta卫星(tomato leaf curl Yunnan betasatellite, TLCYnB)的分离物YN5230一致性最高,达99.3%,亲缘关系较近。重组分析显示,假酸浆上分离的TYLCTHV-YN5735-12是一个重组病毒,有两个重组事件,一个主要发生在AV1的编码区,由中国番茄黄化曲叶病毒(tomato yellow leaf curl China virus, TYLCCNV)和广西大戟曲叶病毒(euphorbia lea...     

First identification of a sweet potato begomovirus (sweepovirus) in Uganda: characterization,detection and distribution

Sweet potato begomoviruses diverge basally from all other begomoviruses and have been named sweepoviruses. In 2009, a sweepovirus was detected for the first time in sweet potato crops in Uganda by using the indicator plant Ipomoea setosa and generic primers in a polymerase chain reaction (PCR). An isolate was cloned and sequenced, the first fully sequenced genome of a sweepovirus from mainland Africa. At the nucleotide level, this isolate differed from other sweepoviruses by at least 13%, discriminating the Ugandan isolate as a new species which has been tentatively named Sweet potato leaf curl Uganda virus (SPLCUV). In infected sweet potato plants, SPLCUV showed an uneven distribution; it was detected more often in samples from the midrib and lamina of middle and lower leaves, and reversion to healthy tissue occurred, especially in shoots of cv. New Kawogo. This appears to be the first report of resistance to a sweepovirus in sweet potato. While it was only detected at relatively low efficiency by PCR, use of I. setosa plants as an indicator of sweepovirus infection in sweet potato plants was as efficient as using real‐time quantitative PCR (qPCR). Storage of dry leaves for 84 days and dried DNA extracts for 21 days did not affect the ability of PCR and qPCR to detect it. Sweepovirus(es) was detected frequently using generic primers in cultivars Ejumula, New Kawogo and 318L in eastern and central Uganda.     

湖南省番茄和牵牛花上双生病毒的分子鉴定

双生病毒是一类在全世界范围内广泛发生的单链环状DNA病毒。本文对从湖南采集到的6例(洋姜、番茄、萝卜、赛葵、甘薯、牵牛花)疑似双生病毒侵染的植物叶片进行了分子鉴定。利用滚环扩增技术(RCA)对样品DNA进行扩增,分别对其RCA产物进行酶切,并将酶切得到的片段测序后进行BLAST比对,结果显示番茄样品中的病毒分离物与番茄黄化曲叶病毒相似性最高(99%),牵牛花样品中的病毒分离物与甘薯卷叶病毒相似性最高(99%),证明这两个分离物是单组分DNA-A双生病毒。这是在湖南省首次发现并报道双生病毒的全核酸序列。     

Seed transmission of Sweet potato leaf curl virus in sweet potato (Ipomoea batatas)

Sweet potato leaf curl virus (SPLCV) infects sweet potato and is a member of the family Geminiviridae (genus Begomovirus). SPLCV transmission occurs from plant to plant mostly via vegetative propagation as well as by the insect vector Bemisia tabaci. When sweet potato seeds were planted and cultivated in a whitefly‐free greenhouse, some sweet potato plants started to show SPLCV‐specific symptoms. SPLCV was detected by PCR from all leaves and floral tissues that showed leaf curl disease symptoms. More than 70% of the seeds harvested from SPLCV‐infected sweet potato plants tested positive for SPLCV. SPLCV was also identified from dissected endosperm and embryos. The transmission level of SPLCV from seeds to seedlings was up to 15%. Southern blot hybridization showed SPLCV‐specific single‐ and double‐stranded DNAs in seedlings germinated from SPLCV‐infected seeds. Taken altogether, the results show that SPLCV in plants of the tested sweet potato cultivars can be transmitted via seeds and SPLCV DNA can replicate in developing seedlings. This is the first seed transmission report of SPLCV in sweet potato plants and also, to the authors' knowledge, the first report of seed transmission for any geminivirus.     

广西部分烟区烟草曲叶病病原的分子鉴定

[目的]明确广西西部地区靖西(JX)、凌云(LY)、德保(DB)和乐业(LeY)等4个县市烟草曲叶病的病原。[方法]2010年5-6月分别从广西靖西、凌云、德保和乐业等县市采集具有典型曲叶症状的烟草叶片,用基于双生病毒DNA保守序列设计简并引物Bego-1和Bego-6对病叶组织总DNA抽提物进行PCR扩增和对PCR产物进行序列测定,用BLAST、Vector NTI、MEGA 4.0和Simplot program 3.2软件等进行病毒序列分析、系统进化树构建和病毒重组分析。[结果]从选取的9个表现典型曲叶症状的样品叶组织总DNA抽提物中均可扩增出约1500bp与预期大小相符的DNA片段。测序和序列比对分析显示,9个样品扩增产物核苷酸序列相似性为73.7%～99.2%,与已报道的双生病毒具较高的相似性。其中,JX-2与中国番茄曲叶病毒广西番茄分离物(G32)的相似性最高,达99.2%;JX-3和JX-5与云南胡椒曲叶病毒云南辣椒分离物(YN323)相似性最高,分别为92.5%和93.4%;LeY-1、LY-1、DB-1、JX-1、JX-4和JX-6则与中国番茄黄化曲叶病毒中国番茄分离物(CHI)和广西烟草分离物(G102)的相似性最高,均高于95.0%。基于PCR扩增产物及已报道的双生病毒属代表种相应核苷酸序列构建的系统进化树分析表明,9个广西烟草分离物分属3个簇群:中国番茄曲叶病毒簇、云南辣椒曲叶病毒簇和中国番茄黄化曲叶病毒簇。重组分析结果表明:JX-3是云南辣椒曲叶病毒和中国番茄曲叶病毒的重组病毒,JX-5是云南辣椒曲叶病毒和中国番茄黄化曲叶病毒的重组病毒。[结论]9个广西烟草分离物分属于4种双生病毒:中国番茄曲叶病毒和中国番茄黄化曲叶病毒,以及分别由上述两种病毒与云南辣椒曲叶病毒重组而来的2种重组病毒。其中,中国番茄曲叶病毒自然侵染烟草、云南辣椒曲叶病毒和中国番茄曲叶病毒及中国番茄黄化曲叶病毒的重组病毒等结果此前均未见报道。     

取食马铃薯块茎和叶片的马铃薯块茎蛾肠道内可培养细菌的多样性

为明确取食马铃薯块茎和叶片的马铃薯块茎蛾Phthorimaea operculella幼虫肠道可培养细菌种类组成的多样性及其差异,分别对取食马铃薯块茎和叶片的马铃薯块茎蛾4龄幼虫的肠道细菌进行分离培养,根据菌落形态和生理生化特征及16S rDNA序列分析对菌株进行分类鉴定。结果表明,从取食马铃薯块茎的马铃薯块茎蛾肠道内共分离获得细菌有4门8科10属15种,其中褪色沙雷氏菌Serratia marcescen和乙酸钙不动杆菌Acinetobacter calcoaceticus为优势种,其相对多度分别为17.20%和16.06%。从取食马铃薯叶片的马铃薯块茎蛾肠道内共分离获得细菌有4门10科10属16种,其中琥珀葡萄球菌Staphylococcus succinus和乙酸钙不动杆菌为优势种,其相对多度分别为11.86%和15.07%。取食马铃薯块茎和叶片的马铃薯块茎蛾肠道内相同的可培养细菌有4属5种,分别为褪色沙雷氏菌、深红沙雷氏菌Serratia rubidaea、阿氏肠杆菌Enterobacter asburiae、乙酸钙不动杆菌和琥珀葡萄球菌。表明取食马铃薯块茎和叶片的马铃薯块茎蛾幼虫的肠道内可培养细菌组成结构不同,且优势种存在差异。     

木尔坦棉花曲叶病毒已对我国棉花生产构成严重威胁

木尔坦棉花曲叶病毒是引起巴基斯坦和印度棉花曲叶病流行的主要病原之一,是由烟粉虱以持久方式传播。近年来,在广东和广西分别发现了严重侵染朱槿和黄秋葵的木尔坦棉花曲叶病毒。虽然广东和广西不种植棉花,但该病毒传播介体烟粉虱在广东、广西及我国棉花产区都有分布。因此该病毒的入侵,对我国棉花生产构成严重威胁。     

Characterization of a New Begomovirus from Egypt Infecting Hollyhock (Althea Rosea)

A viral isolate from Egypt associated with symptoms of enations and leaf curling on hollyhock (Althea rosea) was characterized at the cytopathological and molecular levels. Microscopic observations showed that enations resulted from a reorganization of the vascular tissues, including activation of a cambial activity in the phloem, the development of a palisade parenchyma in place of a spongy one and the differentiation of minor vascular tissues. From this isolate, the full-length DNA-A of a begomovirus (family Geminiviridae) was cloned and sequenced. This genome exhibited a genetic organization similar to that of other old-world begomoviruses like Tomato yellow leaf curl virus from Israel and Ageratum yellow vein virus from Singapore. However, its sequence was significantly distinct (similarity < 69%) from any other geminivirus. This begomovirus was thus considered as representative of a new viral species named Althea rosea enation virus (AREV). AREV was agroinfectious on Nicotiana benthamiana, on which it induced a severe leaf-curling and vein distortion, but could not re-establish infection on A. rosea. To determine if AREV was also associated with a similar disease affecting okra in Upper-Egypt, the partial sequence of the coat protein gene of an isolate was determined. It exhibited 90% nt identity with the hollyhock isolate (97% amino acid), suggesting a genetic heterogeneity in the begomovirus population associated with the enation diseases.     

Geminate Particle Morphology of Sweet Potato Leaf Curl Virus in Partially Purified Preparation and Its Serological Relationship to Two Begomoviruses by Western Blotting

Sweet potato leaf curl virus (SPLCV) is a possible member of the genus Begomovirus; however, the presence of typical geminate particles in sap has not been confirmed. We attempted to observe SPLCV virions by partially purifying the virus using an enzyme-assisted procedure. The observed virions in the partially purified preparations were typical geminate particles with a size of ca. 18×30nm. This virus preparation was subjected to western blot analysis using antisera against Bean golden mosaic virus (BGMV) and Mungbean yellow mosaic virus (MYMV). SPLCV reacted with both antisera. Specific bands appeared to be slightly larger than the 30-kDa marker protein and were considered to be SPLCV coat protein. This western blot analysis revealed for the first time a serelogical relationship between SPLCV and the two well-characterized begomoviruses. Received 28 June 1999/ Accepted in revised form 17 November 1999     

番茄黄化曲叶病毒V 2基因原核表达及多克隆抗体制备

 通过PCR的方法,从番茄黄化曲叶病毒江苏分离物DNA中扩增到V2基因,并克隆到pMD18-T载体,序列测定结果显示其与报道的XH2分离物序列完全一致,核苷酸序列全长351 bp,编码115个氨基酸,推测分子量约13 kD。将该V2基因亚克隆到原核表达载体PET32a中获得重组表达载体PET32a-V2,转化大肠杆菌BL21（DE3）,IPTG可诱导1个分子量约为32 kDa的融合蛋白（含His标签）表达,经Ni⁺ NTA亲和柱纯化,获得纯化的重组蛋白,免疫家兔制备TYLCV-V2蛋白的多克隆抗体Anti-V2,间接ELISA测定Anti-V2的效价达1∶655 360,Western blot及DIBA分析结果表明Anti-V2可与V2蛋白发生特异血清反应,可为进一步研究V2蛋白的功能提供参考。