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田纳西州柳枝稷上由索氏离蠕孢引起的叶斑病和普通根腐病的首次报道

First Report of Spot Blotch and Common Root Rot Caused by Bipolaris sorokiniana on Switchgrass in Tennessee.

作者信息

Vu A L, Dee M M, Gwinn K D, Ownley B H

机构信息

Department of Entomology and Plant Pathology, The University of Tennessee, Knoxville 37996.

出版信息

Plant Dis. 2011 Sep;95(9):1195. doi: 10.1094/PDIS-12-10-0880.

Abstract

Light-to-dark brown, irregular-shaped leaf spots, chlorosis, necrotic roots, and severe stunting were observed on 'Alamo' switchgrass (Panicum virgatum L.) grown on the campus of the University of Tennessee in December 2007. Symptomatic leaf and root samples were surface sterilized, air dried on sterile filter paper, and plated on 2% water agar amended with 10 mg/liter of rifampicin (Sigma-Aldrich, St. Louis, MO) and 10 μl/liter of 2,4 EC Danitol miticide (Valent Chemical, Walnut Creek, CA). Plates were incubated at 25°C in darkness for 4 days. A sporulating, dematiaceous mitosporic fungus was noted and transferred to potato dextrose agar (PDA). Conidia were ovate, oblong, mostly straight, and olive to brown with three to nine septa. Conidial dimensions were 12.5 × 27.5 (17.5) to 20 × 77.5 (57) μm. Conidia were produced on single, light brown, multiseptate conidiophores that were polytretic, geniculate, and sympodial. Morphological features were as described for Bipolaris sorokiniana (Sacc.) Shoemaker (teleomorph = Cochliobolus sativus) (2,3). Disease assays were conducted with 5-week-old 'Alamo' switchgrass grown from surface-sterilized seed. Ten 9 × 9-cm with ~20 switchgrass seedlings were sprayed with 2.4 × 10 spores/ml of sterile water. Plants were subjected to high humidity created by enclosure in a plastic bag for 45 h. The bag was removed and plants were incubated at 25/20°C with 50 to 60% relative humidity. During the incubation, plants were maintained in growth chamber with a 12-h photoperiod of fluorescent and incandescent lighting. Foliar leaf spot symptoms appeared 6 to 10 days postinoculation for plants in all 10 replicates and necrotic lesions were observed on roots. Foliar lesions and diseased roots were surface sterilized, plated on water agar, and resultant fungal colonies were identified as B. sorokiniana. The internal transcribed spacer (ITS) and mitochondrial small subunit (SSU) regions of ribosomal DNA from the original isolate, and the isolate recovered from plants in the pathogenicity assay, were amplified with PCR, with primer pairs ITS4 and ITS5 and NMS1 and NMS2. PCR amplicons of ~551 and 571 bp were obtained with the two primer pairs, respectively. Both amplicons were obtained from both isolates and sequenced. Amplicon sequences from the original isolate and re-isolate were identical and the sequences were submitted to GenBank (Accession Nos. HQ611957 and HQ611958). The ITS sequences had 98% homology to 23 B. sorokiniana isolates, including B. sorokiniana strain DSM 62608 (GenBank Accession No. EF187908); SSU sequences had 99% homology to Cochliobolus sativus isolate AFTOL-ID 271 (GenBank Accession No. FJ190589). Spot blotch caused by B. sorokiniana has been reported on switchgrass in Iowa, Nebraska, Pennsylvania, and Virginia (1). To our knowledge, this is the first report of B. sorokiniana causing spot blotch or common root rot of switchgrass in Tennessee, which extends the current known distribution of these diseases. More recently, we isolated B. sorokiniana from switchgrass seed received from commercial sources in the United States, indicating a seedborne transmission. References: (1) D. F. Farr and A. Y. Rossman. Fungal Databases. Systematic Mycology and Microbiology Laboratory, ARS, USDA. Retrieved from http://nt.ars-grin.gov/fungaldatabases/ , 15 November 2010. (2) R. F. Nyvall and J. A. Percich. Plant Dis. 83:936, 1999. (3) A. Sivanesan and P. Holliday. CMI Descr. Pathog. Fungi bact. 71:701, 1981.

摘要

2007年12月,在田纳西大学校园种植的‘阿拉莫’柳枝稷(Panicum virgatum L.)上观察到浅至深褐色、形状不规则的叶斑、褪绿、坏死根以及严重矮化现象。对有症状的叶和根样本进行表面消毒,在无菌滤纸上风干,然后接种到添加了10毫克/升利福平(Sigma - Aldrich公司,密苏里州圣路易斯)和10微升/升2,4 - EC达尼托尔杀螨剂(Valent Chemical公司,加利福尼亚州核桃溪)的2%水琼脂平板上。平板在25°C黑暗条件下培养4天。发现一种产孢的、暗色有丝孢真菌,并将其转移到马铃薯葡萄糖琼脂(PDA)上。分生孢子卵形、长圆形,大多直,橄榄色至褐色,有三至九个隔膜。分生孢子大小为12.5×27.5(17.5)至20×77.5(57)微米。分生孢子产生于单一的、浅褐色、多隔膜的分生孢子梗上,这些分生孢子梗是多分枝的、膝曲状的和合轴式的。形态特征与索氏平脐蠕孢(Bipolaris sorokiniana (Sacc.) Shoemaker)(有性型 = 禾旋孢腔菌(Cochliobolus sativus))描述的一致(2,3)。用从表面消毒种子培育的5周龄‘阿拉莫’柳枝稷进行病害测定。将10个9×9厘米、约有20株柳枝稷幼苗的培养皿用2.4×10个孢子/毫升的无菌水喷雾处理。将植株置于塑料袋中营造高湿度环境45小时。移除塑料袋后,将植株在25/20°C、相对湿度50%至60%的条件下培养。在培养期间,植株置于生长室中,光照周期为12小时荧光和白炽灯照明。接种后6至10天,所有10个重复中的植株均出现叶斑症状,且在根上观察到坏死病斑。对叶部病斑和染病根进行表面消毒,接种到水琼脂上,产生的真菌菌落被鉴定为索氏平脐蠕孢。用引物对ITS4和ITS5以及NMS1和NMS2通过PCR扩增原始分离株以及从致病性测定中植株上分离得到的分离株的核糖体DNA的内部转录间隔区(ITS)和线粒体小亚基(SSU)区域。分别用这两对引物获得了约551和571碱基对的PCR扩增产物。两个分离株均获得了这两个扩增产物并进行了测序。原始分离株和再分离株的扩增产物序列相同,并将序列提交至GenBank(登录号分别为HQ611957和HQ611958)。ITS序列与23个索氏平脐蠕孢分离株有98%的同源性,包括索氏平脐蠕孢菌株DSM

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