Adesemoye A O, Eskalen A
Department of Plant Pathology and Microbiology, University of California, Riverside, 92521.
Plant Dis. 2011 Sep;95(9):1187. doi: 10.1094/PDIS-01-11-0047.
Eutypella is one of the few genera in the Diatrypaceae considered plant pathogens (1). In California, E. vitis and other members of the Diatrypaceae cause branch and trunk canker on grapevine (3,4). Eutypella spp. have not previously been documented as pathogens of citrus. In a 2010 survey on citrus branch canker and dieback in six citrus-growing counties of California, four isolates of Eutypella species were detected in Riverside and San Diego counties. Canker symptoms included dieback and bark cracking, and cuts made through symptomatic trees showed that the cankers were expanding through the center of the tree. Branch samples were collected from 10 trees per orchard and 5 to 10 orchards per county (102 trees for two counties). Pieces of symptomatic tissue (1 to 2 mm) were plated onto potato dextrose agar amended with 0.01% tetracycline (PDA-tet) and incubated at 25°C for 4 days. All isolates were identified by morphological and molecular characteristics. PCR of isolates was performed in a thermal cycler using two primer pairs, ITS4/5 and Bt2a/2b for amplifying the internal transcribed spacer (ITS1), 5.8S, and ITS2 region and the β-tubulin gene, respectively (2,3). PCR products were sequenced at the University of California, Riverside Genomics Core and the sequences compared in a BLAST search. Four isolates identified as Eutypella spp. included two (UCR1088 and UCR1101) from San Diego County and two (UCR1148 and UCR1149) from the Riverside County samples. The sequences were deposited in GenBank (HQ880579, JF758610, HQ880581, and HQ880582 and HQ880583, JF758611, HQ880585, and HQ880586 for the ITS regions and β-tubulin gene, respectively. ITS sequences for UCR1088 and UCR1101 had 98 and 100% match, respectively, to Eutypella spp. ITS sequences in GenBank (GQ293959 to GQ293961), while UCR1148 and UCR1149 matched 99% (GQ293956 to GQ293958). On the basis of morphological characteristics, UCR1088 and UCR1101 were similar to Eutypella spp. group 1, while UCR1148 and UCR1149 were similar to Eutypella spp. group 3 (4). Pathogenicity tests were conducted with all four isolates on detached shoots from healthy citrus trees of the same cultivar/rootstock from which each isolate was obtained. One wound per shoot was made on 1-year-old, green, detached shoots using a 3-mm-diameter cork borer and the wounded surfaces were inoculated with 3-mm-diameter mycelial plugs of 5-day-old cultures of each isolate growing on PDA-tet. Inoculated wounds and shoot ends were covered with petroleum jelly and wrapped with Parafilm (3). Control shoots were inoculated with sterile agar plugs. There were 10 inoculated shoots per isolate and noninoculated control treatment. Shoots were incubated at 25°C in moist chambers for 6 weeks. Lesions similar to those on the original infected shoots were observed on all inoculated shoots except the control treatment. Reisolation and identification of fungi from inoculated and control shoots were done using methods described above. Inoculated isolates were recovered from 100% of inoculated shoots but none was recovered from noninoculated shoots, indicating association of Eutypella spp. with citrus branch canker. To our knowledge, this is the first report of Eutypella spp. associated with cankers on citrus in California. References: (1) B. Piskur et al. Plant Dis. 91:1579, 2007. (2) B. Slippers et al. Mycologia 96:83, 2004. (3) F. P. Trouillas and W. D. Gubler. Plant Dis. 94:867, 2010. (4) F. P. Trouillas et al. Mycologia 102:319, 2010.
真座腔菌属是座囊菌科中少数被认为是植物病原体的属之一(1)。在加利福尼亚州,葡萄座腔菌和座囊菌科的其他成员会导致葡萄树的枝干溃疡(3,4)。此前尚未有真座腔菌属作为柑橘病原体的记录。在2010年对加利福尼亚州六个柑橘种植县的柑橘枝干溃疡和枯死病的调查中,在河滨县和圣地亚哥县检测到了四株真座腔菌属分离株。溃疡症状包括枯死和树皮开裂,对有症状的树木进行切割显示溃疡正在向树的中心扩展。每个果园从10棵树上采集枝条样本,每个县采集5至10个果园的样本(两个县共102棵树)。将有症状的组织块(1至2毫米)接种到添加了0.01%四环素的马铃薯葡萄糖琼脂(PDA - tet)上,在25°C下培养4天。所有分离株均通过形态学和分子特征进行鉴定。使用两对引物对分离株进行PCR扩增,ITS4/5和Bt2a/2b分别用于扩增内部转录间隔区(ITS1)、5.8S和ITS2区域以及β - 微管蛋白基因(2,3)。PCR产物在加利福尼亚大学河滨分校基因组学核心实验室进行测序,并在BLAST搜索中比较序列。鉴定为真座腔菌属的四株分离株包括来自圣地亚哥县的两株(UCR1088和UCR1101)以及来自河滨县样本的两株(UCR1148和UCR1149)。序列已存入GenBank(ITS区域和β - 微管蛋白基因分别为HQ880579、JF758610、HQ880581、HQ880582和HQ880583、JF758611、HQ880585、HQ880586)。UCR1088和UCR1101的ITS序列与GenBank中真座腔菌属的ITS序列分别有98%和100%的匹配度(GQ293959至GQ293961),而UCR1148和UCR1149的匹配度为99%(GQ293956至GQ293958)。根据形态学特征,UCR1088和UCR1101与真座腔菌属第1组相似,而UCR1148和UCR1149与真座腔菌属第3组相似(4)。对所有四株分离株在从获得各分离株的相同品种/砧木的健康柑橘树上剪下的离体枝条上进行致病性测试。使用3毫米直径的木塞打孔器在1年生绿色离体枝条上每枝造成一个伤口,并用生长在PDA - tet上的5日龄各分离株培养物的3毫米直径菌丝块接种伤口表面。接种的伤口和枝条末端用凡士林覆盖并用保鲜膜包裹(3)。对照枝条接种无菌琼脂块。每个分离株和未接种对照处理各有10个接种枝条。枝条在25°C的潮湿培养箱中培养6周。除对照处理外,在所有接种枝条上均观察到与原始感染枝条上相似的病斑。使用上述方法对接种和对照枝条上的真菌进行再分离和鉴定。从100%的接种枝条上重新分离到接种的分离株,但未从未接种枝条上分离到,表明真座腔菌属与柑橘枝干溃疡有关。据我们所知,这是加利福尼亚州真座腔菌属与柑橘溃疡病相关的首次报道。参考文献:(1)B. Piskur等人,《植物病害》91:1579,2007。(2)B. Slippers等人,《真菌学》96:83,2004。(3)F. P. Trouillas和W. D. Gubler,《植物病害》94:867,2010。(4)F. P. Trouillas等人,《真菌学》102:319,2010。
