Gauthier N W, Polashock J, Veetil T T, Martin R R, Beale J
University of Kentucky, Lexington, KY 40546.
USDA-ARS, Chatsworth, NJ 08019.
Plant Dis. 2015 Mar;99(3):421. doi: 10.1094/PDIS-09-14-0946-PDN.
In 2011, a grower in Casey County, Kentucky, observed persistent yellow, green, and red mosaic patterns on leaves of highbush blueberry plants. Twenty-three randomly-scattered cv. Bluecrop plants out of approximately 1,400 5-year-old plants showed symptoms, with coverage on each plant ranging from 5 to 100%. Asymptomatic canes bloomed normally and produced fruit; affected canes were stunted and did not bloom. These symptoms are generally consistent with those described for blueberry mosaic disease (BMD) (1,3), the casual agent of which is Blueberry mosaic associated virus (BlMaV) (4). All plants were purchased from a local nursery, but their origin was unknown. In 2012, leaves from each of five symptomatic plants were tested by reverse transcription-polymerase chain reaction (RT-PCR) for BlMaV. Total nucleic acid was isolated from the symptomatic leaves, and asymptomatic leaves of randomly selected healthy plants served as negative controls. The CTAB method was used as described (2), and RNA was isolated using lithium chloride. cDNA was synthesized using the SuperScript VILO cDNA synthesis kit (Invitrogen, Carlsbad, CA). Two different primer sets were used for detection of BlMaV; BlMaVCP5'-1F (GGTTGATGGATGCTTACGAA) and BlMaVRNA3-1378R (CTTCACTTACCACATTATACATCTC) to amplify a 1,370-bp portion of RNA3 and RNA2-2F (TTCGATCCCAGCCCTCTCCC) and RNA2-2R (AGGCAAAGGGAAAGAAATTCAGGTGTC) to amplify a 1,281-bp portion of RNA2. All symptomatic samples tested by RT-PCR yielded a fragment for each primer set, and the amplicon sizes were as expected. No fragments were amplified from the negative controls. To further confirm diagnosis, the primer sets noted above were used to re-amplify the same two fragments from each of three of the samples. These fragments were cloned and sequenced on the CEQ8000 (Beckman-Coulter, Brea, CA) using the GenomeLab DTCS Quick Start sequencing kit (Beckman-Coulter) and the universal M13 forward and reverse primers as well as internal primers: BlMaV-CP Int 1F (ACAATTAAGAAGTCCTCGTAT), BlMaV-CP Int 2F (ATGTCCGGATGCTAGTCGCT), and BlMaV RNA2 IntR (GGTGGGGACGGAATAATACAGAG). All sequences were consistent with those now published for BlMaV, with 98% identity at the nucleic acid level for both fragments. In 2013, the grower removed plants with more than 50% symptomatic tissue, and no newly symptomatic plants were observed that year. Sixteen remaining symptomatic plants, as well as 36 asymptomatic plants adjacent to those with symptoms, were sampled and tested by RT-PCR. All symptomatic plants were confirmed to be infected with BlMaV, as well as 30 of the 36 asymptomatic plants. It has been suggested that newly infected plants may take a year to express symptoms (5), which may explain the finding of 30 infected but asymptomatic plants. This is the first report of an association of BIMaV with BMD in Kentucky. These results indicate that BMD can establish in Kentucky blueberry fields. References: (1) R. R. Martin et al. Viruses 4:2831-2852, 2012. (2) J. J. Polashock et al. Plant Pathol. 58:1116, 2009. (3) D. C. Ramsdell. In: Compendium of Blueberry and Cranberry Diseases. APS Press, St. Paul, MN, 1995. (4) T. Thekke-Veetil et al. Virus Res. 189:92, 2014. (5) E. H. Varney. Phytopathology 47:307, 1957.
2011年,肯塔基州凯西县的一位种植者发现高丛蓝莓植株的叶片上出现了持续的黄色、绿色和红色花叶图案。在大约1400株5年生植株中,随机分布的23株“蓝丰”品种植株出现了症状,每株植株的症状覆盖范围为5%至100%。无症状的茎正常开花并结果;受影响的茎发育不良且不开花。这些症状通常与蓝莓花叶病(BMD)所描述的症状一致(1,3),其病原为蓝莓花叶相关病毒(BlMaV)(4)。所有植株均从当地苗圃购买,但其来源不明。2012年,对5株有症状植株的叶片进行逆转录聚合酶链反应(RT-PCR)检测,以检测BlMaV。从有症状的叶片中分离总核酸,随机选取的健康植株的无症状叶片作为阴性对照。采用所述的CTAB方法(2),并用氯化锂分离RNA。使用SuperScript VILO cDNA合成试剂盒(Invitrogen,卡尔斯巴德,加利福尼亚州)合成cDNA。使用两组不同的引物检测BlMaV;BlMaVCP5'-1F(GGTTGATGGATGCTTACGAA)和BlMaVRNA3-1378R(CTTCACTTACCACATTATACATCTC)用于扩增RNA3的1370 bp片段,RNA2-2F(TTCGATCCCAGCCCTCTCCC)和RNA2-2R(AGGCAAAGGGAAAGAAATTCAGGTGTC)用于扩增RNA2的1281 bp片段。通过RT-PCR检测的所有有症状样品对每组引物均产生一个片段,扩增子大小符合预期。阴性对照未扩增出片段。为进一步确诊,使用上述引物组从三个样品中的每个样品重新扩增相同的两个片段。这些片段使用GenomeLab DTCS Quick Start测序试剂盒(Beckman-Coulter)和通用M13正向和反向引物以及内部引物:BlMaV-CP Int 1F(ACAATTAAGAAGTCCTCGTAT)、BlMaV-CP Int 2F(ATGTCCGGATGCTAGTCGCT)和BlMaV RNA2 IntR(GGTGGGGACGGAATAATACAGAG)在CEQ8000(Beckman-Coulter,布雷亚,加利福尼亚州)上进行克隆和测序。所有序列均与现已发表的BlMaV序列一致,两个片段在核酸水平上的同一性为98%。2013年,种植者移除了症状组织超过50%的植株,当年未观察到新的有症状植株。对16株剩余的有症状植株以及与有症状植株相邻的36株无症状植株进行采样并通过RT-PCR检测。所有有症状植株均被确认为感染了BlMaV,36株无症状植株中的30株也被感染。有人提出新感染的植株可能需要一年时间才会表现出症状(5),这可能解释了发现30株感染但无症状植株的原因。这是肯塔基州首次报道BIMaV与BMD相关联。这些结果表明BMD可在肯塔基州的蓝莓田中发生。参考文献:(1)R.R.Martin等人,《病毒》4:2831 - 2852,2012年。(2)J.J.Polashock等人,《植物病理学》58:1116,2009年。(3)D.C.Ramsdell,载于《蓝莓和蔓越莓病害汇编》。APS出版社,明尼苏达州圣保罗,1995年。(4)T.Thekke-Veetil等人,《病毒研究》189:92,2014年。(5)E.H.Varney,《植物病理学》47:307,1957年。
