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佛罗里达州葫芦科作物上黄瓜黄化矮化失调病毒的首次报道

First Report of Cucurbit yellow stunting disorder virus in Cucurbits in Florida.

作者信息

Polston J E, Hladky L L, Akad F, Wintermantel W M

机构信息

Department of Plant Pathology, University of Florida, Gainesville.

USDA-ARS, Salinas, CA.

出版信息

Plant Dis. 2008 Aug;92(8):1251. doi: 10.1094/PDIS-92-8-1251B.

DOI:10.1094/PDIS-92-8-1251B
PMID:30769460
Abstract

In August and September 2007, watermelon plants (Citrullus lanatus L.) in commercial fields in Manatee and Hillsborough counties in Florida exhibited stunting, deformation, interveinal chlorosis, and leaf mottling. Adult and immature whiteflies (Bemisia tabaci biotype B) were observed. Leaf samples were collected from seven watermelon and two squash plants showing different combinations of symptoms. Total RNA was extracted using RNeasy Plant Mini Kit (Qiagen, Valencia, CA) and subjected to reverse transcription (RT)-PCR for the presence of criniviruses using primers specific to regions of the Cucurbit yellow stunting disorder virus (CYSDV) genome encoding the coat protein (CysCP5206F 5' TTTGGAAAAGAACCTGACGAG 3'; CysCP5600R 5' TTCATCAACAGATTGGCTGC 3') and HSP70h genes (2). Total nucleic acids were extracted using Gentra Puregene Kit (Qiagen) and subjected to PCR for the presence of begomoviruses using the degenerate primer pairs AC1048 and AV494, designed to amplify a region of the begomovirus coat protein gene (4), and PBL1v2040 and PCRc154, designed to amplify a region of the hypervariable region of the begomovirus B component (3). RT-PCR amplified the expected 394-bp fragment of the coat protein gene from three symptomatic plants (one squash, two watermelon) and from CYSDV-infected control plants but not from healthy controls. Similarly, the 175-bp HSP70h fragment was amplified from the same samples and from CYSDV-infected control plants but not from healthy controls. The coat protein amplicon was sequenced from one of the Manatee County isolates (GenBank Accession No. EU596528) and the 344 nt sequenced portion of the amplicon was found to be 100% identical to sequences of CYSDV from Texas, California, Jordan, and France (GenBank Accession Nos. AF312823, EU596529, DQ903107, and AY204220, respectively) and shared 99% identity with an isolate from Spain (GenBank Accession No. NC_004810), but only 91% with an isolate from Iran (GenBank Accession No. AY730779). The begomovirus primer pair pBL1v2040 and PCRc154 produced a 678-bp amplicon that is consistent with the presence of a bipartite begomovirus in all nine samples. Sequence analysis of four of the 678-bp amplicons revealed that all had greater than 97% sequence identity to isolates of Cucurbit leaf crumple virus (CuLCrV) from Arizona (GenBank Accession No. AF327559) and California (GenBank Accession No. AF224761). These results are similar to those reported in the first detection of CuLCrV in Florida in 2006 (1). In October 2007, CYSDV was detected in squash plants (Cucurbita pepo L.) in two additional fields in Manatee and Hillsborough counties, and additional fields with CYSDV-like symptoms have been observed with increasing frequency throughout the region. The appearance of CYSDV in Florida follows the recent emergence of CYSDV in California and Arizona and Sonora, Mexico in 2006 where the CYSDV infection of fall melons resulted in severe economic losses (2). The emergence of CYSDV in Florida, where the vector B. tabaci biotype B is well established, warrants concern for all cucurbit production in the southern United States. Disease monitoring efforts are in progress to determine the extent, severity, and impact of CYSDV on Florida cucurbit production. References: (1) F. Akad et al. Plant Dis.92:648, 2008. (2) Y.-W. Kuo et al. Plant Dis. 91:330, 2007. (3) M. R. Rojas et al. Plant Dis. 77:340, 1993. (4) S. D. Wyatt and J. K. Brown. Phytopathology 86:1288, 1996.

摘要

2007年8月和9月,佛罗里达州马纳蒂县和希尔斯伯勒县商业种植地的西瓜植株(西瓜属)出现发育迟缓、变形、脉间失绿和叶片斑驳症状。观察到有成年和未成熟的烟粉虱(B型烟粉虱)。从7株西瓜和2株南瓜植株上采集了表现出不同症状组合的叶片样本。使用RNeasy植物微型试剂盒(Qiagen公司,加利福尼亚州瓦伦西亚)提取总RNA,并使用针对葫芦科黄化矮缩病毒(CYSDV)基因组编码外壳蛋白区域的引物(CysCP5206F 5' TTTGGAAAAGAACCTGACGAG 3';CysCP5600R 5' TTCATCAACAGATTGGCTGC 3')和HSP70h基因进行逆转录(RT)-PCR,检测是否存在褪绿病毒(2)。使用Gentra Puregene试剂盒(Qiagen公司)提取总核酸,并使用简并引物对AC1048和AV494进行PCR检测是否存在双生病毒,这对引物设计用于扩增双生病毒外壳蛋白基因的一个区域(4),以及PBL1v2040和PCRc154,用于扩增双生病毒B组分高变区的一个区域(3)。RT-PCR从3株有症状的植株(1株南瓜、2株西瓜)以及CYSDV感染的对照植株中扩增出预期的394 bp外壳蛋白基因片段,但未从健康对照植株中扩增出。同样,从相同样本以及CYSDV感染的对照植株中扩增出175 bp的HSP70h片段,但未从健康对照植株中扩增出。对马纳蒂县的一个分离株的外壳蛋白扩增子进行了测序(GenBank登录号EU596528),发现扩增子的344 nt测序部分与来自德克萨斯州、加利福尼亚州、约旦和法国的CYSDV序列100%相同(GenBank登录号分别为AF312823、EU596529、DQ903107和AY20422),与来自西班牙的一个分离株有99%的同一性(GenBank登录号NC_004810),但与来自伊朗的一个分离株只有91%的同一性(GenBank登录号AY730779)。双生病毒引物对pBL1v2040和PCRc154产生了一个678 bp的扩增子,这与所有9个样本中存在双分体双生病毒一致。对678 bp扩增子中的4个进行序列分析发现,所有扩增子与来自亚利桑那州(GenBank登录号AF327559)和加利福尼亚州(GenBank登录号AF224761)的葫芦科叶片皱缩病毒(CuLCrV)分离株的序列同一性均大于97%。这些结果与2006年佛罗里达州首次检测到CuLCrV时报道的结果相似(1)。2007年10月在马纳蒂县和希尔斯伯勒县的另外两块田地的南瓜植株(西葫芦)中检测到CYSDV,并且在整个地区观察到有越来越多的田地出现类似CYSDV症状。CYSDV在佛罗里达州的出现是继2006年加利福尼亚州、亚利桑那州以及墨西哥索诺拉州最近出现CYSDV之后,在这些地方秋季甜瓜感染CYSDV导致了严重的经济损失(2)。在烟粉虱B型生物型已广泛存在的佛罗里达州出现CYSDV,值得美国南部所有葫芦科作物生产关注。目前正在进行病害监测工作,以确定CYSDV对佛罗里达州葫芦科作物生产的范围、严重程度和影响。参考文献:(1)F. Akad等人,《植物病害》92:第648页,2008年。(2)Y.-W. Kuo等人,《植物病害》91:第330页,2007年。(3)M. R. Rojas等人,《植物病害》77:第340页,1993年。(4)S. D. Wyatt和J. K. Brown,《植物病理学》86:第1288页,1996年。

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