Mapuranga N
Kutsaga Research Station, P.O. Box 1909, Harare, Zimbabwe.
Plant Dis. 1998 Dec;82(12):1404. doi: 10.1094/PDIS.1998.82.12.1404A.
Two forms of Pseudomonas syringae pv. tabaci cause wildfire (Tox) and angular leaf spot (Tox) diseases of tobacco in Zimbabwe. Two races of the pathogen (races 0 and 1) occur in Zimbabwe (4). Two groups of cultivars are available: one with resistance to race 0 only, tbe second with resistance to races 0 and 1 (4). P. syringae pv. tabaci was first observed on cultivars with resistance to races 0 and 1 in 1993, and infection on these cultivars is now widespread. The bacteria isolated from the infected plants were gram-negative rods and produced fluorescent pigment on King's medium B. Levan-oxidase-potato rot-arginine dihydrolase-tobacco hypersensitivity (LOPAT) tests indicated that the pathogen was a Group 1a pseudomonad (2). Pathogenicity and race designation for 58 isolates of the pathogen were determined on 8-week-old, greenhouse-raised tobacco plants. Inoculated plants were kept in controlled environment units (13/11 h photoperiod, 30 ± 2°C, relative humidity >75%) for 10 days. Pathogenicity was determined on cv. Kutsaga E1, which has no known resistance to any races of P. syringae pv. tabaci (4), and isolates from typical wildfire and angular leaf spot lesions were used for race designation by inoculating six plants of each indicator tobacco genotype. Genotypes included Nicotiana tabacum cv. Kutsaga E1 (susceptible to races 0, 1, and 2), which was used as the indicator genotype for race 0, N. longiflora (race 0 resistance) (1), N. tabacum cv. Kutsaga Mammoth 10 (resistance to race 0 derived from N. longiflora), N. rustica var. brasilea (resistance to races 0 and 1) (3,4), a breeding line, WZ 3-2-1-1, and cv. Kutsaga 35 (both resistant to races 0 and 1 with resistance derived from N. rustica var. brasilea). Six spots, three on either side of the midrib, were inoculated with an artist's airbrush (Aero-pro 251) operated at 250 kPa. The inoculum, (approximately 1 × 10 CFU/ml) suspended in a quarter-strength Ringer's solution was applied to one side of the midrib and Ringer's solution only to the other side, which served as control. Thirty-eight Tox isolates and 20 Tox isolates were tested in a series of experiments in randomized complete blocks with four replications per treatment. Resistance to wildfire was characterized by localized chlorosis or whitish-tan hypersensitive lesions and susceptibility by necrotic lesions (>2 mm) surrounded by large chlorotic halos. Resistance to angular leaf spot was characterized by hypersensitive lesions or absence of symptoms and susceptibility by presence of symptoms (4). Sixty-six percent of the Tox isolates and 70% of the Tox isolates successfully infected cultivars with known resistance to races 0 and 1, and were therefore designated race 2 (1). All other isolates were race 1. This is the first report of P. syringae pv. tabaci Tox and Tox race 2 in Zimbabwe. References: (1) K. K. Knoche et al. Phytopathology 77:1364, 1987. (2). R. A. Lelliott and D. E. Stead. Methods in Plant Pathology. Vol. 2. 1987. (3). J. R. Stavely and H. A. Skoog. Proc. Am. Phytopathol. Soc. 3:231 (Abstr.), 1976. (4). J. J. Woodend and E. Mudzengerere. Euphytica 64:149, 1992.
丁香假单胞菌烟草致病变种的两种形式在津巴布韦引发烟草野火病(Tox)和角斑病(Tox)。该病原菌的两个小种(小种0和1)在津巴布韦存在(4)。有两类品种:一类仅对小种0有抗性,另一类对小种0和1都有抗性(4)。丁香假单胞菌烟草致病变种于1993年首次在对小种0和1有抗性的品种上被观察到,如今这些品种上的感染已很普遍。从受感染植株分离出的细菌为革兰氏阴性杆菌,在King氏培养基B上产生荧光色素。左旋酶 - 马铃薯腐烂 - 精氨酸双水解酶 - 烟草过敏反应(LOPAT)试验表明该病原菌是1a组假单胞菌(2)。在温室培育的8周龄烟草植株上测定了该病原菌58个分离株的致病性和小种鉴定。接种后的植株置于可控环境单元(光周期13/11小时,30±2°C,相对湿度>75%)中10天。在对丁香假单胞菌烟草致病变种的任何小种都无已知抗性的库察加E1品种(4)上测定致病性,从典型野火病和角斑病病斑分离的菌株通过接种每种指示烟草基因型的6株植株来进行小种鉴定。基因型包括烟草品种库察加E1(对小种0、1和2敏感),用作小种0的指示基因型,长花烟草(抗小种0)(1),烟草品种库察加猛犸10(从长花烟草衍生而来的抗小种0),黄花烟草变种巴西烟草(抗小种0和1)(3,4),一个育种系WZ 3 - 2 - 1 - 1,以及品种库察加35(均抗小种0和1,抗性源自黄花烟草变种巴西烟草)。用压力为250 kPa的喷枪(Aero - pro 251)在中脉两侧各接种6个点。将悬浮于四分之一强度林格氏溶液中的接种物(约1×10 CFU/ml)施用于中脉一侧,另一侧仅施用林格氏溶液作为对照。在一系列实验中,以随机完全区组设计对38个Tox分离株和20个Tox分离株进行测试,每个处理重复4次。对野火病的抗性表现为局部黄化或浅棕白色过敏病斑,感病表现为坏死病斑(>2 mm)且周围有大的黄化晕圈。对角斑病的抗性表现为过敏病斑或无症状,感病表现为有症状(4)。66%的Tox分离株和70%的Tox分离株成功感染了对小种0和1有已知抗性的品种,因此被鉴定为小种2(1)。所有其他分离株为小种1。这是津巴布韦关于丁香假单胞菌烟草致病变种Tox和小种2的首次报道。参考文献:(1)K. K. Knoche等人,《植物病理学》77:1364,1987。(2)R. A. Lelliott和D. E. Stead,《植物病理学方法》第2卷,1987。(3)J. R. Stavely和H. A. Skoog,《美国植物病理学会会报》3:231(摘要),1976。(4)J. J. Woodend和E. Mudzengerere,《欧洲植物病理学报》64:149,1992。
