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在尼日利亚引起番茄青枯病的青枯雷尔氏菌生物变种

Biovar of Ralstonia solanacearum Causing Bacterial Wilt of Tomato in Nigeria.

作者信息

Adebayo O S, Ekpo E J A

机构信息

Crop Protection Division, National Horticultural Research Institute, PMB 5432, Idi-Ishin, Ibadan, Nigeria.

Department of Crop Protection and Environmental Biology, University of Ibadan, Ibadan, Nigeria.

出版信息

Plant Dis. 2005 Oct;89(10):1129. doi: 10.1094/PD-89-1129C.

Abstract

A survey of southwestern Nigeria showed an outbreak of wilt disease caused by Ralstonia solanacearum in 80% of tomato (Lycopersicon lycopersicum) fields in the production area of Ogun State (7°15'N, 3°25'E) in June 1996. Subsequent surveys conducted in Edo (6°45'N, 5°30'E), Delta (5°15'N, 5°45'E), Lagos (6°30'N, 3°40'E), Oyo (8°40'N, 3°30'E), and Osun (7°50'N, 4°E) states between May and November 1998 identified 60 to 80% infected fields per state. Observations made at the experimental plots of the National Horticultural Research Institute (NIHORT) at Ibadan (7°23'N, 2°50'E) also showed similar infections. Affected plants exhibited initial wilting of terminal leaves followed (within 2 days) by sudden and permanent wilt. For further identification of the causal organism, 10 tomato plants showing wilt symptoms were collected from each of five fields in the vegetable blocks of the NIHORT at Ibadan and 20 farmers' fields in Ogun State. The 10 plants per field were thereafter bulked as one composite sample. Creamy bacterial sap from these samples was plated on tetrazolium chloride media, and plates were incubated at 30°C for 48 h (2). Colonies that were fluidal and white with pink centers were used for biovar determination. Basal media was prepared to include one of three disaccharides (cellobiose, lactose, or maltose) or three hexose alcohols (dulcitol, mannitol, or sorbitol). A loopful of bacterial cells of all 25 isolates was inoculated individually to each of the six media. Cultures were incubated at 30°C for 28 days and monitored daily for color changes. The pathogenicity of the 25 isolates was tested using 10 4-week-old seedlings each of eggplant cv. black beauty, tomato cv. Ibadan local, sweet pepper cv. California wonder, and potato cv. Kufri. Each inoculum was prepared by adjusting the concentration to 10 CFU/ml with a colorimeter at a wavelength of 600 nm (optical density of approximately 0.3). Plants were inoculated by pouring 10 ml of inoculum around the base of each plant. Ten uninoculated seedlings of each cultivar served as the control. Plants were assessed for wilt severity 30 days after inoculation. All isolates utilized the three disaccharides and three hexose alcohols, and according to Hayward's classification, all isolates were biovar 3 (1). Furthermore, the isolates caused rapid wilting of all four test plants. R. solanacearum was easily reisolated from the vascular bundles of the test plants. To our knowledge, this is the first report of this biovar of R. solanacearum affecting tomato crops in Nigeria. References: (1) A. C. Hayward. J. Appl. Bacteriol, 27:265, 1964 (2) A. Kelman. Phytopathology 44:693, 1954.

摘要

1996年6月对尼日利亚西南部的一项调查显示,在奥贡州(北纬7°15′,东经3°25′)产区80%的番茄(番茄属番茄)田中爆发了由青枯雷尔氏菌引起的枯萎病。1998年5月至11月期间,在江户州(北纬6°45′,东经5°30′)、三角州州(北纬5°15′,东经5°45′)、拉各斯州(北纬6°30′,东经3°40′)、奥约州(北纬8°40′,东经3°30′)和奥孙州(北纬7°50′,东经4°)进行的后续调查发现,每个州有60%至80%的田地受到感染。在伊巴丹(北纬7°23′,东经2°50′)的国家园艺研究所(NIHORT)试验田进行的观察也显示了类似的感染情况。受影响的植株最初表现为顶叶萎蔫,随后(2天内)突然永久萎蔫。为了进一步鉴定致病生物,从伊巴丹NIHORT蔬菜区的5块田地和奥贡州的20块农民田地中,每块田地采集了10株表现出萎蔫症状的番茄植株。此后,将每块田地的10株植株合并为一个复合样本。将这些样本中乳状的细菌汁液接种到氯化三苯基四氮唑培养基上,平板在30°C下培养48小时(2)。将呈流体状、白色且中心为粉红色的菌落用于生物型鉴定。基础培养基中包含三种二糖(纤维二糖、乳糖或麦芽糖)或三种己糖醇(卫矛醇、甘露醇或山梨醇)中的一种。将所有25个分离株的一满环细菌细胞分别接种到六种培养基中的每一种上。培养物在30°C下培养28天,并每天监测颜色变化。使用10株4周龄的茄子品种“黑美人”、番茄品种“伊巴丹本地种”、甜椒品种“加利福尼亚奇迹”和马铃薯品种“库夫里”的幼苗对25个分离株的致病性进行测试。每个接种物通过用比色计在600nm波长下将浓度调整为10CFU/ml(光密度约为0.3)来制备。通过在每株植物基部浇灌10ml接种物对植物进行接种。每个品种的10株未接种幼苗用作对照。接种30天后对植物的萎蔫严重程度进行评估。所有分离株都利用了三种二糖和三种己糖醇,根据海沃德的分类,所有分离株均为生物型3(1)。此外,这些分离株导致所有四种试验植物迅速萎蔫。青枯雷尔氏菌很容易从试验植物的维管束中重新分离出来。据我们所知,这是青枯雷尔氏菌的这种生物型影响尼日利亚番茄作物的首次报道。参考文献:(1)A.C.海沃德。《应用细菌学杂志》,27:265,1964年 (2)A.凯尔曼。《植物病理学》,44:693,1954年。

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