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中国首次报道茄科劳尔氏菌引起的藿香细菌性萎蔫病

First Report of Bacterial Wilt Caused by Ralstonia solanacearum on Ageratum conyzoides in China.

作者信息

She X-M, He Z-F, Luo F-F, Li H-P

机构信息

College of Natural Resources and Environment, South China Agricultural University, Guangzhou, Guangdong 510642, China and Plant Protection Research Institute, Guangdong Academy of Agricultural Sciences, Guangzhou, Guangdong 510640, China.

Plant Protection Research Institute, Guangdong Academy of Agricultural Sciences, Guangzhou, Guangdong 510640, China and Guangdong Provincial Key Laboratory of High Technology for Plant Protection, Guangzhou, Guangdong 510640, China.

出版信息

Plant Dis. 2013 Mar;97(3):418. doi: 10.1094/PDIS-08-12-0780-PDN.

Abstract

Ageratum conyzoides L. is believed to act as reservoir host for many plant diseases. In June 2011, a 30% incidence of bacterial wilt on A. conyzoides was observed in a field of Rhizoma kaempferiae in Yangchun city of Guangdong province. The initial symptoms were wilting of the apical leaves during the day, which recovered at night. After 4 to 6 days, the leaves became totally necrotic. The basal stems of the diseased plants were blackened and the vascular tissue turned brown. To investigate the disease etiology before understanding the disease link between A. conyzoides and R. kaempferiae, 10 plants with typical wilting symptoms were collected from the field. A total of 10 bacterial isolates were isolated from the vascular tissue of each diseased plant on tripheny tetrazolium chloride (TZC) medium. After incubation at 30°C for 2 days, the plates had large, irregular round, fluidal, white colonies with a pink center. Thirty healthy A. conyzoides plants at the four- to six-leaf growth stage were inoculated by injuring the roots and soaking them in a bacterial suspension (1 × 10 cfu/ml) for 20 min with the 10 bacterial isolates separately, and planted in 10-cm pots with sterile gardening soil in a glasshouse (28 to 35°C). Sterile water was used as a negative control. Five days after inoculation, a few leaves of the inoculated plants began to exhibit wilting. The inoculated plants eventually showed the same symptoms as those in the field. The same bacterium was reisolated from inoculated plants. The 30 negative control plants did not have wilt symptoms. With the same inoculation procedure, the bacterium also caused wilting on tomato (25 of 30), pepper (10 of 30), eggplant (2 of 30), ginger (11 of 15), and R. kaempferiae (8 of 15). Using the universal bacterial 16S rDNA primer set 27f/1541R (3), approximately 1,400 bp-fragments were amplified from the 10 isolates, respectively. The sequences for the 10 fragments (GenBank Accession Nos. JX294065 to JX294074) were identical and had 100% sequence identity with 16S rDNA of R. solanacearum GMI1000 (AL646052). The 10 isolates were able to oxidize disaccharides (lactose, maltose, and cellobiose) and hexose alcohols (mannitol, dulcitol, and sorbitol). According to Hayward's classification, all isolates were biovar 3 (2). Based on the pathogenicity tests, carbohydrate utilization, and near full-length 16S rDNA sequences, the bacterial isolates from the diseased A. conyzoides belonged to race 4 and biovar 3 of R. solanacearum. Furthermore, the specific 280-bp and 140-bp fragments were respectively amplified from all 10 isolates by using the multiplex PCR (1). In addition, specific 165-bp fragments were amplified from all the isolates using the specific primers AKIF/AKIR (3), which indicates the bacterium belongs to R. solanacearum Phylotype I. To our knowledge, this is the first report of a disease caused by R. solanacearum on A. conyzoides in China. References: (1) M. Fegan and P. Prior. Page 449 in: Bacterial Wilt Disease and the Ralstonia solanacearum Species Complex. C. Allen et al., eds. The American Phytopathological Society. St. Paul, MN, 2005. (2) A. C. Hayward. J. Appl. Bacteriol. 27:265, 1964. (3) M. Horita et al. J. Gen. Plant Pathol. 70:278, 2004.

摘要

胜红蓟被认为是多种植物病害的寄主。2011年6月,在广东省阳春市的一片山柰种植田中,观察到胜红蓟的青枯病发病率为30%。最初症状是白天顶端叶片萎蔫,夜间恢复。4至6天后,叶片完全坏死。患病植株的基部茎干变黑,维管束组织变为褐色。为了在了解胜红蓟与山柰之间的病害联系之前调查病因,从田间采集了10株具有典型萎蔫症状的植株。在氯化三苯基四氮唑(TZC)培养基上,从每株患病植株的维管束组织中总共分离出10个细菌分离株。在30°C下培养2天后,平板上出现大的、不规则圆形、流质、白色且中心粉红色的菌落。将30株处于四至六叶生长期的健康胜红蓟植株的根部进行损伤,然后分别用这10个细菌分离株的菌悬液(1×10 cfu/ml)浸泡20分钟,种植于温室(28至35°C)中装有无菌园艺土壤的10厘米花盆中。无菌水用作阴性对照。接种5天后,接种植株的一些叶片开始出现萎蔫。接种植株最终表现出与田间相同的症状。从接种植株中重新分离出相同的细菌。30株阴性对照植株没有萎蔫症状。采用相同的接种程序,该细菌也能使番茄(30株中的25株)、辣椒(30株中的10株)、茄子(30株中的2株)、生姜(15株中的11株)和山柰(15株中的8株)发生萎蔫。使用通用细菌16S rDNA引物对27f/1541R(3),分别从这10个分离株中扩增出约1400 bp的片段。这10个片段的序列(GenBank登录号JX294065至JX294074)相同,与青枯雷尔氏菌GMI1000的16S rDNA具有100%的序列同一性。这10个分离株能够氧化双糖(乳糖、麦芽糖和纤维二糖)和己糖醇(甘露醇、卫矛醇和山梨醇)。根据海沃德的分类,所有分离株均为生物变种3(2)。基于致病性测试、碳水化合物利用情况以及近乎全长的16S rDNA序列,从患病胜红蓟中分离出的细菌分离株属于青枯雷尔氏菌的4号小种和生物变种3。此外,使用多重PCR(1)分别从所有10个分离株中扩增出特异性的280 bp和140 bp片段。另外,使用特异性引物AKIF/AKIR(3)从所有分离株中扩增出特异性的165 bp片段,这表明该细菌属于青枯雷尔氏菌I型。据我们所知,这是中国首次报道青枯雷尔氏菌引起胜红蓟病害的情况。参考文献:(1)M. Fegan和P. Prior。载于:《青枯病与青枯雷尔氏菌物种复合体》第449页。C. Allen等人编著。美国植物病理学会。明尼苏达州圣保罗,2005年。(2)A. C. Hayward。《应用细菌学杂志》27:265,1964年。((3)M. Horita等人。《植物病理学报》70:278,2004年。

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