Pintos Varela C, Redondo Fernández V, Mansilla Vázquez J P, Aguín Casal O
Estación Fitopatolóxica Do Areeiro, Deputación Pontevedra, Subida a la Robleda s/n. 36153 Pontevedra, Spain.
Plant Dis. 2011 Feb;95(2):221. doi: 10.1094/PDIS-10-10-0723.
During the conducting of Phytophthora ramorum surveys at Galician public parks (northwestern Spain) in 2010, established Rhododendron spp. plants were observed to be exhibiting leaf spots and necrosis, shoot blight, and cankers and dieback of shoots and branches. Branches and leaves of affected rhododendrons contained pseudothecia with bitunicate asci and hyaline pseudoparaphyses, and pycnidia were observed within the same stromatic masses. Symptomatic samples were disinfested in 0.5% sodium hypochlorite for 3 min. Tissues were cut from the margin of lesions, placed onto malt extract agar amended with streptomycin (25 μg ml), and incubated at 25°C in the dark. Cultures displaying morphological characteristics associated with Botryosphaeriaceae species were subcultured on 2% water agar with sterilized Pinus pinaster needles as a substrate and incubated at 25°C under near-UV light to encourage pycnidial production (1). Single conidial cultures gave rise to two distinct colonies on potato dextrose agar (PDA) at 25°C. In type 1, isolates produced a sparse, aerial mycelium and a characteristic yellow pigment that was more intense after 3 days, thereafter becoming violaceous and gradually turning dark gray. Growth occurred in the range of 4 to 38°C with an optimum at 29°C. Conidia were hyaline, fusiform, aseptate, thin walled, and averaged 21.1 (14.3 to 25.0) × 5.7 (4.3 to 6.8) μm with a length/width (L/W) ratio of 3.7 ± 0.4 (n = 100). On the basis of these characteristics, isolates were identified as Neofusicoccum luteum (1,3). Colonies of type 2 produced a dense, white-to-yellowish mycelium that rapidly became gray followed by marked diurnal zonation. Mycelial growth occurred in the range of 6 to 38°C with an optimum at 29 to 30°C. Conidia were hyaline, elliptical or fusiform, aseptate, thin walled, and averaging 18.3 (14.1 to 20.7) × 5.8 (4.6 to 7.0) μm with a L/W ratio of 3.2 ± 0.4 (n = 100). These isolates were identified as N. parvum (1,2). Identity was confirmed by DNA sequences analysis of internal transcribed spacer (ITS) regions. Comparison of the sequences of type 1 and 2 showed 100% homology with N. luteum and N. parvum (GenBank Accession Nos. EU673311 and GU251146, respectively). Representative sequences were deposited at GenBank (Accession Nos. HQ197352 and HQ197351). Pathogenicity of each isolate of N. luteum and N. parvum was confirmed by inoculating four 3-year-old Rhododendron spp. seedlings grown in pots. Shallow cuts were made in three branches of each plant. A colonized 6-mm agar plug, removed from the margin of an actively growing colony, was inserted beneath the flap and sealed with Parafilm. Four control seedlings received only sterile PDA agar plugs. Plants were maintained at 26°C and 70% humidity for 21 days. Inoculated plants began showing symptoms after 3 days. Necrosis progressed quickly and bidirectionally from the wound, resulting in death of leaves and wilting of shoots. N. luteum and N. parvum were reisolated from all inoculated plants but not from the controls. To our knowledge, this is the first report of N. luteum and N. parvum on Rhododendron spp. in Spain. References: (1) P. W. Crous et al. Stud. Mycol. 55:235, 2006. (2) S. R. Pennycook et al. Mycotaxon 24:445, 1985. (3) A .J. L. Phillips et al. Sydowia 54:59, 2002.
2010年在西班牙西北部加利西亚的公共公园进行樟疫霉调查时,发现已定植的杜鹃花属植物出现叶斑和坏死、枝枯以及嫩枝和枝条的溃疡和枯死。受影响杜鹃花的枝叶含有具双层壁子囊和透明假侧丝的子囊壳,并且在相同的子座团块中观察到分生孢子器。有症状的样本在0.5%次氯酸钠中消毒3分钟。从病斑边缘切取组织,置于添加链霉素(25 μg/ml)的麦芽提取物琼脂上,在25°C黑暗条件下培养。表现出与葡萄座腔菌科物种相关形态特征的培养物转接至以灭菌的海岸松针叶为底物的2%水琼脂上,并在25°C近紫外光下培养以促进分生孢子器产生(1)。单孢培养物在25°C的马铃薯葡萄糖琼脂(PDA)上产生了两个不同的菌落。在第1种类型中,分离株产生稀疏的气生菌丝体和一种特征性黄色色素,3天后颜色加深,此后变为紫色并逐渐变为深灰色。生长温度范围为4至38°C,最适温度为29°C。分生孢子透明,梭形,无隔膜,薄壁,平均大小为21.1(14.3至25.0)×5.7(4.3至6.8)μm,长宽比为3.7±0.4(n = 100)。基于这些特征,分离株被鉴定为黄色新壳梭孢(1,3)。第2种类型的菌落产生密集的白色至淡黄色菌丝体,迅速变为灰色,随后出现明显的昼夜分区。菌丝生长温度范围为6至38°C,最适温度为29至30°C。分生孢子透明,椭圆形或梭形,无隔膜,薄壁,平均大小为18.3(14.1至20.7)×5.8(4.6至7.0)μm,长宽比为3.2±0.4(n = 100)。这些分离株被鉴定为微小新壳梭孢(1,2)。通过对内部转录间隔区(ITS)区域的DNA序列分析确认了其身份。第1种和第2种类型序列的比较显示与黄色新壳梭孢和微小新壳梭孢(分别为GenBank登录号EU673311和GU251146)具有100%的同源性。代表性序列保藏于GenBank(登录号HQ197352和HQ197351)。通过接种四株盆栽3年生杜鹃花属幼苗,证实了黄色新壳梭孢和微小新壳梭孢每个分离株的致病性。在每株植物的三个枝条上进行浅切口。从活跃生长菌落边缘切下一个6毫米的定殖琼脂块,插入皮瓣下方并用Parafilm密封。四株对照幼苗仅接种无菌PDA琼脂块。将植物保持在26°C和70%湿度下21天。接种后3天植物开始出现症状。坏死从伤口迅速双向发展,导致叶片死亡和嫩枝枯萎。从所有接种植物中重新分离出黄色新壳梭孢和微小新壳梭孢,但对照植物中未分离到。据我们所知,这是西班牙关于杜鹃花属植物上黄色新壳梭孢和微小新壳梭孢的首次报道。参考文献:(1)P. W. Crous等人,《Stud. Mycol.》55:235,2006年。(2)S. R. Pennycook等人,《Mycotaxon》24:445,1985年。(3)A. J. L. Phillips等人,《Sydowia》54:59,2002年。
