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台湾番茄和辣椒中胡椒脉斑驳病毒的首次报道

First Report of Pepper veinal mottle virus in Tomato and Pepper in Taiwan.

作者信息

Cheng Y H, Wang R Y, Chen C C, Chang C A, Jan F-J

机构信息

Division of Plant Pathology, Agricultural Research Institute, Wufeng, Taichung 413, Taiwan.

Department of Plant Pathology, National Chung Hsing University, Taichung 402, Taiwan.

出版信息

Plant Dis. 2009 Jan;93(1):107. doi: 10.1094/PDIS-93-1-0107A.

DOI:10.1094/PDIS-93-1-0107A
PMID:30764280
Abstract

In May of 2006, samples from tomato plants (Solanum lycopersicum cv. Known-you 301) exhibiting necrotic symptoms on stems, petioles, and leaves were collected from Chiayi County, Taiwan. Double-antibody sandwich-ELISAs were performed using Cucumber mosaic virus, Tomato mosaic virus, Potato virus Y, Watermelon silver mottle virus, and Chilli veinal mottle virus (ChiVMV) polyclonal antibodies. Three of eight samples reacted with antibodies against ChiVMV but not with the others. Using the potyvirus degenerate primers (Hrp 5/Pot 1) (2), an expected 1.5-kb DNA fragment including the 3'-end of the NIb gene, the complete coat protein (CP) gene, and the 3'-nontranslatable region of the virus was amplified from total RNA isolated from these three samples by reverse transcription (RT)-PCR. A homology search in GenBank indicated that the new tomato-infecting virus in Taiwan belongs to Pepper veinal mottle virus (PVMV) since they shared >90% amino acid identity in the CP gene. A virus culture (Tom1) isolated from one of the diseased tomatoes was then established in Chenopodium quinoa and Nicotiana benthamiana and the CP gene was amplified and sequenced (GenBank Accession No. EU719647). Comparisons of the 807-nt CP gene with those of five PVMV isolates available in GenBank showed 81.5 to 93.1% nucleotide and 90.0 to 97.8% amino acid identity. Tom1 induced irregular necrotic lesions on stems, petioles, and leaves of tomato while inducing only mild mottle symptoms on pepper. Serological cross reaction between ChiVMV and PVMV has been observed previously (1,3) and also found in this study. To differentiate these two potyviruses by RT-PCR, primer pair CPVMVup/dw (5'-TATTC(T/C)TCAGTGTGG(A/T/C)T(T/C)CCACCAT and 5'-(T/C)C(A/T)C(A/T)(A/T/G)(A/T)AA(A/G)CCATAA(A/C)(A/C)ATA(A/G)T(T/C)T) was designed on the basis of the comparison of the CP gene and the 3'-nontranslatable region of the PVMV and ChiVMV. DNA fragments of 171 and 259 bp are expected to be amplified from ChiVMV and PVMV, respectively, by RT-PCR with primers CPVMVup/dw. In a field survey done in 2006, samples from diseased peppers (Capsicum annuum) that reacted with the polyclonal antibodies against ChiVMV were further identified by RT-PCR with primers CPVMVup/dw, indicating that both ChiVMV and PVMV infected pepper crops (Capsicum spp.) in Taiwan. A pepper isolate (Pep1) of PVMV was obtained from Nantou County through three times of single lesion passages on C. quinoa and then propagated on N. benthamiana. The CP gene of Pep1 was amplified and sequenced (GenBank Accession No. EU719646) and found to share 99.1% nucleotide and 100% amino acid identity with that of Tom1. Pep1 caused mild mottle symptoms on leaves of both tomato and pepper. To our knowledge, this is the first report of the presence of PVMV in Taiwan as well as in East Asia. References: (1) B. Moury et al. Phytopathology 95:227, 2005. (2) S. S. Pappu et al. Plant Dis. 82:1121, 1998. (3) W. S. Tsai et al. Plant Pathol. 58:408, 2008.

摘要

2006年5月,从台湾嘉义县采集了番茄植株(番茄品种“农友301”)样本,这些植株的茎、叶柄和叶片出现坏死症状。使用黄瓜花叶病毒、番茄花叶病毒、马铃薯Y病毒、西瓜银斑驳病毒和辣椒脉斑驳病毒(ChiVMV)的多克隆抗体进行双抗体夹心ELISA检测。8个样本中有3个与抗ChiVMV抗体发生反应,与其他抗体无反应。使用马铃薯Y病毒简并引物(Hrp 5/Pot 1)(2),通过逆转录(RT)-PCR从这3个样本分离的总RNA中扩增出一个预期的1.5 kb DNA片段,该片段包括病毒NIb基因的3'端、完整的外壳蛋白(CP)基因和3'非翻译区。在GenBank中进行同源性搜索表明,台湾这种新的感染番茄的病毒属于辣椒脉斑驳病毒(PVMV),因为它们在CP基因中的氨基酸同一性>90%。然后从一株患病番茄中分离出病毒培养物(Tom1),在藜麦和本氏烟草中进行培养,并对CP基因进行扩增和测序(GenBank登录号EU719647)。将807 nt的CP基因与GenBank中5个PVMV分离株的CP基因进行比较,核苷酸同一性为81.5%至93.1%,氨基酸同一性为90.0%至97.8%。Tom1在番茄的茎、叶柄和叶片上诱导出不规则坏死斑,而在辣椒上仅诱导出轻微斑驳症状。之前已观察到ChiVMV和PVMV之间的血清学交叉反应(1,3),本研究中也发现了这种现象。为通过RT-PCR区分这两种马铃薯Y病毒,根据PVMV和ChiVMV的CP基因及3'非翻译区的比较设计了引物对CPVMVup/dw(5'-TATTC(T/C)TCAGTGTGG(A/T/C)T(T/C)CCACCAT和5'-(T/C)C(A/T)C(A/T)(A/T/G)(A/T)AA(A/G)CCATAA(A/C)(A/C)ATA(A/G)T(T/C)T)。预计用引物CPVMVup/dw通过RT-PCR分别从ChiVMV和PVMV中扩增出171 bp和259 bp的DNA片段。在2006年进行的田间调查中,对与抗ChiVMV多克隆抗体发生反应的患病辣椒(辣椒品种)样本,用引物CPVMVup/dw通过RT-PCR进一步鉴定,表明ChiVMV和PVMV均感染了台湾的辣椒作物(辣椒属)。通过在藜麦上进行三次单斑分离,从南投县获得了PVMV的一个辣椒分离株(Pep1),然后在本氏烟草上繁殖。对Pep1的CP基因进行扩增和测序(GenBank登录号EU719646),发现其与Tom1的CP基因核苷酸同一性为99.1%,氨基酸同一性为100%。Pep1在番茄和辣椒叶片上均引起轻微斑驳症状。据我们所知,这是PVMV在台湾以及东亚存在的首次报道。参考文献:(1)B. Moury等人,《植物病理学》95:227,2005年。(2)S. S. Pappu等人,《植物病害》82:1121,1998年。(3)W. S. Tsai等人,《植物病理学》58:408,2008年。

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