Woodward J E, Nui C, Wright R J, Batla M A, Baughman T A
Department of Plant and Soil Science, Texas Tech University, Lubbock 79403.
Department of Soil and Crop Sciences, Texas AgriLife Extension Service, Vernon, 76384.
Plant Dis. 2008 Oct;92(10):1468. doi: 10.1094/PDIS-92-10-1468B.
Peanut (Arachis hypogaea L.) is grown extensively in several counties in West Texas. Sclerotinia blight, caused by the soilborne fungus Sclerotinia minor Jagger, is an increasingly important disease throughout this region. In September of 2007, diseased peanut plants (cv. Tamrun OL02) exhibiting symptoms of Sclerotinia blight (2,4) were collected from a commercial farm in Gaines County during a regional survey. Infected stem sections were surface disinfested in 0.5% sodium hypochlorite for 1 min, air dried, and placed in petri dishes containing water agar. Hyphae were subsequently transferred to petri dishes containing potato dextrose agar (PDA) after 3 days of incubation at room temperature. Pure cultures formed abundant, aerial, white mycelia, which later became darkly pigmented. Black, spherical to elongated sclerotia, 3.8 ± 0.8 mm, formed on the outer edge of petri dishes after 1 week. These characteristics are consistent with S. sclerotiorum (Lib.) de Bary (1,2). Pathogenicity tests were conducted by inoculating stems of greenhouse-grown peanut plants (cvs. Tamrun OL02, n = 4 and Flavorrunner 458, n = 4) with PDA plugs containing S. sclerotiorum. Mounting pins were used to create a shallow wound and affix inoculum plugs to stems. Control plants (n = 4) were inoculated with noncolonized PDA plugs. Plants were placed in a dew chamber at 20°C and 95% relative humidity in a randomized complete block design. The experiment was conducted two times. Symptoms identical to those observed on the original plant specimens were observed after 3 days on all inoculated plants; the controls remained healthy. Darkly pigmented cultures of S. sclerotiorum were consistently reisolated from all symptomatic stem sections. Fungal DNA was extracted from mycelia and sclerotia with a Qiagen DNeasy Plant Mini kit (Valencia, CA) and amplified by PCR using three S. sclerotiorum-specific primer pairs (3). PCR products for three replicates (two from mycelia and one from sclerotia) were sequenced and subjected to a NCBI BLAST search of highly similar sequences (megablast). The BLAST search revealed that our sequences are highly similar only with reported sequences of S. sclerotiorum. Sequences generated from three primer pairs in this study were 99, 95, and 95% homologous to S. sclerotiorum Accessions Nos. AF377925.1, AF377919.1, and AF377904.1 over 373, 376, and 300 bp of aligned sequence, respectively. Results from the pathogenicity tests and molecular study confirm that the S. sclerotiorum isolate obtained in this study is capable of inciting Sclerotinia blight of peanut. While S. minor is the primary causal agent of the disease, recent reports indicate that S. sclerotiorum is becoming more prevalent throughout the peanut-producing regions of the United States (2,4), and must therefore be considered in disease diagnosis. References: (1) L. M. Kohn. Phytopathology 69:881, 1979. (2) S. Sanogo and N. Puppala. Plant Dis. 91:1077, 2007. (3) C. Sirjusingh and L. M. Kohn. Mol. Ecol. Notes 1:267, 2001. (4) J. E. Woodward et al. Plant Dis. 90:111, 2006.
花生(Arachis hypogaea L.)在得克萨斯州西部的几个县广泛种植。由土壤传播的真菌小核盘菌(Sclerotinia minor Jagger)引起的菌核病,在整个该地区正成为一种日益重要的病害。2007年9月,在一次区域调查期间,从盖恩斯县的一个商业农场采集了表现出菌核病症状(2,4)的患病花生植株(品种Tamrun OL02)。将受感染的茎段在0.5%次氯酸钠中进行表面消毒1分钟,风干后,置于含有水琼脂的培养皿中。在室温下培养3天后,将菌丝体转移到含有马铃薯葡萄糖琼脂(PDA)的培养皿中。纯培养物形成了丰富的气生白色菌丝体,随后颜色变深。1周后,在培养皿的外缘形成了黑色、球形至细长形的菌核,直径为3.8±0.8毫米。这些特征与核盘菌(Sclerotinia sclerotiorum (Lib.) de Bary)一致(1,2)。通过用含有核盘菌的PDA菌块接种温室种植的花生植株(品种Tamrun OL02,n = 4和Flavorrunner 458,n = 4)的茎来进行致病性测试。使用固定针造成一个浅伤口,并将接种菌块固定在茎上。对照植株(n = 4)接种未被定殖的PDA菌块。将植株以随机完全区组设计放置在温度为20°C、相对湿度为95%的保湿箱中。该实验进行了两次。在所有接种植株上3天后观察到与原始植物标本上观察到的相同症状;对照植株保持健康。始终从所有有症状的茎段重新分离出颜色变深的核盘菌培养物。用Qiagen DNeasy植物微量提取试剂盒(加利福尼亚州瓦伦西亚)从菌丝体和菌核中提取真菌DNA,并使用三对核盘菌特异性引物对通过PCR进行扩增(3)。对三个重复样本(两个来自菌丝体,一个来自菌核)的PCR产物进行测序,并在NCBI上对高度相似的序列进行BLAST搜索(megablast)。BLAST搜索显示,我们的序列仅与已报道的核盘菌序列高度相似。本研究中由三对引物对产生的序列在373、376和300 bp的比对序列上分别与核盘菌登录号AF377925.1、AF377919.1和AF377904.1的同源性为99%、95%和95%。致病性测试和分子研究的结果证实,本研究中获得的核盘菌分离物能够引发花生菌核病。虽然小核盘菌是该病的主要病原体,但最近的报告表明,核盘菌在美国花生种植区正变得更加普遍(2,4),因此在疾病诊断中必须予以考虑。参考文献:(1)L. M. Kohn. Phytopathology 69:881, 1979.(2)S. Sanogo和N. Puppala. Plant Dis. 91:1077, 2007.(3)C. Sirjusingh和L. M. Kohn. Mol. Ecol. Notes 1:267, 2001.(4)J. E. Woodward等人. Plant Dis. 90:111, 2006.
