Snyder A L, Kasson M T, Salom S M, Davis D D, Griffin G J, Kok L T
Virginia Tech, Department of Entomology, Blacksburg, VA.
Virginia Tech, Department of Plant Pathology, Physiology, and Weed Science, Blacksburg, VA.
Plant Dis. 2013 Jun;97(6):837. doi: 10.1094/PDIS-05-12-0502-PDN.
Ailanthus altissima (Mill.) Swingle, commonly known as tree-of-heaven, is an invasive tree species that has spread throughout the United States since its introduction in 1784 (2). During a survey in July 2009, approximately 1,100 A. altissima trees were observed at two locations in western Virginia (a roadside in Montgomery Co. and a wooded area adjacent to a railroad in Bedford Co.) exhibiting foliar wilt symptoms, defoliation, yellowish vascular discoloration, or death at an incidence of ~77%. Similar symptoms on A. altissima were reported in Roanoke, VA in the early 1930s and after 2005 in Pennsylvania, attributed to a Verticillium sp. (1,2). To identify the causal agent, discolored xylem tissue samples were excised from 10 symptomatic A. altissima trees at both locations, soaked in 1% NaOCl for 2 min, rinsed with sterilized distilled water for 5 min, and placed onto plum extract agar. Cultures were incubated in the dark at 22°C for 7 to 14 days. The resultant colonies (three to four per location) were subcultured and identified putatively as a Verticillium sp. closely related to Verticillium albo-atrum Reinke and Berthold (3), based on melanized, thick-walled, resting mycelia and phialides arranged in verticillate whorls that amassed round, oval-shaped conidia (5.1 ± 1.2 μm × 2.8 ± 0.4 μm, n = 100). Molecular identification of two fungal isolates (one per location) was determined by amplification of the protein coding genes elongation factor 1-alpha (EF), glyceraldehyde-3-phosphate dehydrogenase (GPD), and tryptophan synthase (TS), using PCR primers developed recently for Verticillium (3). A BLAST search on the edited contigs revealed 100% sequence similarity for all three protein coding genes among the two isolates and reference sequences of isolates PD592 (GenBank Accessions JN188227, JN188163, and JN188035 for EF, GPD, and TS, respectively) and VnAaPA140 (KC307764, KC307766, and KC307768 for EF, GPD, and TS, respectively) of the newly-proposed species, V. nonalfalfae (formerly V. albo-atrum). Aligned sequences from one representative isolate, VnAaVA2 (Bedford Co.), were deposited into GenBank as KC307758 (EF), KC307759 (GPD), and KC307760 (TS). To confirm pathogenicity to A. altissima, the two molecularly characterized isolates (one per location) were inoculated into 18 10-week old A. altissima stems that were grown in an environmental chamber at 24°C, 60% RH, and a 12-h photoperiod from seeds collected in Blacksburg, VA. A conidial suspension of each isolate was injected into each stem (0.1 ml of 1 × 10 CFU/ml/stem). All 36 seedlings inoculated with the proposed V. nonalfalfae isolates developed wilting of leaflets within 2 weeks post-inoculation (WPI), defoliation of leaflets by 6 WPI, and were dead by 9 WPI. Eighteen control seedlings were inoculated similarly with distilled water, and remained asymptomatic. Fungi resembling the proposed species V. nonalfalfae were reisolated from all inoculated stems except the control plants, and the species confirmed morphologically as described above. V. nonalfalfae is a recently proposed species that can infect a variety of plant species (3). To our knowledge, this is the first report of this proposed species on A. altissima in Virginia. New state reports of this pathogen on A. altissima are important for regulatory issues associated with using this pathogen as a potential biological control agent. References: (1) G. F. Gravatt and R. B. Clapper. Plant Dis. Rep. 16:96, 1932. (2) M. J. Schall and D. D. Davis. Plant Dis. 93:747, 2009. (3) P. Inderbitzin et al. PLoS ONE, 6, e28341, 2011.
臭椿(Ailanthus altissima (Mill.) Swingle),俗称天堂树,是一种入侵树种,自1784年引入美国后已遍布全美(2)。在2009年7月的一次调查中,在弗吉尼亚州西部的两个地点(蒙哥马利县的一条路边以及贝德福德县一条铁路旁的林区)观察到约1100棵臭椿树出现叶片枯萎症状、落叶、维管束发黄变色或死亡,发病率约为77%。20世纪30年代初在弗吉尼亚州罗阿诺克以及2005年后在宾夕法尼亚州,也曾报道过臭椿出现类似症状,病因是一种轮枝菌(1,2)。为确定致病因子,从两个地点的10棵有症状的臭椿树上切取变色的木质部组织样本,在1%次氯酸钠中浸泡2分钟,用无菌蒸馏水冲洗5分钟,然后置于李子提取物琼脂上。培养物在22°C黑暗条件下培养7至14天。每个地点得到的菌落(三到四个)进行继代培养,并初步鉴定为与黑白轮枝菌(Verticillium albo-atrum Reinke and Berthold)密切相关的一种轮枝菌(3),依据是黑化、厚壁的休眠菌丝体以及呈轮状排列的瓶梗,这些瓶梗产生圆形、椭圆形分生孢子(5.1 ± 1.2 μm × 2.8 ± 0.4 μm,n = 100)。使用最近为轮枝菌开发的PCR引物(3),通过扩增编码蛋白的基因延伸因子1-α(EF)、甘油醛-3-磷酸脱氢酶(GPD)和色氨酸合成酶(TS),对两个真菌分离株(每个地点一个)进行分子鉴定。对编辑后的重叠群进行BLAST搜索发现,两个分离株的所有三个编码蛋白基因与新提出的物种非苜蓿轮枝菌(V. nonalfalfae,以前称为黑白轮枝菌)的分离株PD592(EF、GPD和TS的GenBank登录号分别为JN188227、JN188163和JN188035)以及VnAaPA140(EF、GPD和TS的KC307764、KC307766和KC307768)的参考序列具有100%的序列相似性。来自一个代表性分离株VnAaVA2(贝德福德县)的比对序列作为KC307758(EF)、KC307759(GPD)和KC307760(TS)存入GenBank。为确认对臭椿的致病性,将两个经分子鉴定的分离株(每个地点一个)接种到18株10周龄的臭椿茎中,这些臭椿是从弗吉尼亚州布莱克斯堡收集的种子在温度24°C、相对湿度60%、光周期12小时的环境室中培育的。将每个分离株的分生孢子悬浮液注入每个茎中(0.1 ml,1 × 10 CFU/ml/茎)。接种了拟南芥非苜蓿轮枝菌分离株的所有36株幼苗在接种后2周内出现小叶枯萎,接种后6周小叶脱落,接种后9周死亡。18株对照幼苗同样接种蒸馏水,未出现症状。除对照植株外,从所有接种的茎中重新分离出类似拟南芥非苜蓿轮枝菌的真菌,且该物种经形态学鉴定与上述描述一致。非苜蓿轮枝菌是最近提出的一个物种,可感染多种植物(3)。据我们所知,这是该拟南芥非苜蓿轮枝菌在弗吉尼亚州臭椿上的首次报道。该病原菌在弗吉尼亚州臭椿上的新报道对于将该病原菌用作潜在生物防治剂的监管问题很重要。参考文献:(1)G. F. Gravatt和R. B. Clapper。植物病害报告16:96,1932年。(2)M. J. Schall和D. D. Davis。植物病害93:747,2009年。(3)P. Inderbitzin等人。公共科学图书馆·综合6,e28341,2011年。
