Lin C-H, Chuang M-H, Wang J-F
AVRDC-The World Vegetable Center, Shanhua, Tainan 74199, Taiwan.
Plant Dis. 2015 Feb;99(2):282. doi: 10.1094/PDIS-07-14-0715-PDN.
Chard (Beta vulgaris var. cicla L.) is a biennial herbaceous plant in the Chenopodiaceae family. It is rich in vitamins and minerals and is one of the most popular traditional vegetables in Taiwan. Chard accessions VI048530 and VI050121 growing in fields at Shanhua, Tainan, showed wilting symptoms in March and April 2013. The initial symptoms of wilt were observed on young green leaves. These symptoms progressed over time to chlorosis, interveinal necrosis, and finally blight. Finally, the plants collapsed and died. Vascular and pith tissues were discolored, especially at the stem base. A whitish mass oozed from the cut end of diseased stems. A total of eight bacterial strains were isolated from stems and roots of wilted chard plants. On tetrazolium chloride (TZC) medium (4), colonies were round to oval, fluidal, and white with a pink or red center after incubation at 30°C for 48 h. A typical hypersensitive reaction was induced within 24 h when the strains were infiltrated into tobacco leaves. Koch's postulates on chard plants were confirmed using the eight strains within a greenhouse, under natural light, with temperature and humidity ranges from 25 to 34°C and 56 to 98%, respectively. Fifteen chard (VI048530) plants at the four- to six-leaf stage were inoculated by soil drenching with 30 ml of a ~10 CFU/ml bacterial suspension. Sterile water was used as negative control. After 4 to 6 days, the first symptoms of wilt were observed on the young chard leaves. The progression of symptom development was identical to that observed in the field. The colony morphology on TZC medium of isolates from the inoculated plants was identical to that previously described from field samples. Pathogenicity of the strains was also tested on tomato (VI005790), eggplant (VI046095), and pepper (PBC1367) plants using the previously described inoculation procedure. The mean disease incidences on tomato, eggplant, and pepper plants were 100% (120/120), 100% (120/120), and 79.2% (95/120) respectively. Latent infection was found in asymptomatic pepper plants (16/120) by a printing method. Polymerase chain reaction (PCR) amplification of total DNA from each strain using the Ralstonia solanacearum-specific primer pair AU759f and AU760r (5) produced the expected 282-bp amplicon. All the isolated strains were identified as biovar 3 based on their capacity to utilize three hexose alcohols (mannitol, sorbitol, and dulcitol) and three disaccharides (lactose, maltose, and cellobiose) (2) to produce acid. Based on the phylotype-specific multiplex PCR assay and the partial egl gene sequence (GenBank accession numbers KM100442 to KM100449) (1), all chard isolates were identified as R. solanacearum phylotype I, sequevar 34. Bacterial wilt symptoms have also been observed on beet (Beta vulgaris L.), a close relative of chard, but beet has not been confirmed as a host plant (3). To our knowledge, this is the first report of chard as a host of R. solanacearum worldwide. References: (1) M. Fegan and P. Prior. Page 449 in: Bacterial Wilt Disease and the Ralstonia solanacearum Species Complex. C. Allen et al., eds. APS Press, St. Paul, MN, 2005. (2) A. C. Hayward. J. Appl. Bacteriol. 27:265, 1964. (3) A. Kelman. The Bacterial Wilt caused by Pseudomonas solanacearum. Tech. Bull. No. 99. N.C. Agric. Exp. Stn., 1953. (4) A. Kelman. Phytopathology 44:693, 1954. (5) N. Opina et al. Asia Pac. J. Mol. Biol. Biotechnol. 5:19, 1997.
叶用甜菜(Beta vulgaris var. cicla L.)是藜科的一种二年生草本植物。它富含维生素和矿物质,是台湾最受欢迎的传统蔬菜之一。2013年3月和4月,种植在台南市善化田间的叶用甜菜品种VI048530和VI050121出现了萎蔫症状。萎蔫的最初症状出现在幼嫩的绿叶上。随着时间的推移,这些症状发展为黄化、脉间坏死,最终枯萎。最后,植株倒伏死亡。维管束和髓组织变色,尤其是茎基部。从患病茎的切口处渗出白色物质。从萎蔫的叶用甜菜植株的茎和根中总共分离出8个细菌菌株。在氯化三苯基四氮唑(TZC)培养基上(4),菌落圆形至椭圆形,呈流质状,在30°C下培养48小时后为白色,中心为粉红色或红色。当将这些菌株渗入烟草叶片时,在24小时内诱导出典型的过敏反应。在温室中,在自然光下,温度和湿度范围分别为25至34°C和56至98%的条件下,使用这8个菌株在叶用甜菜植株上证实了柯赫氏法则。对15株处于四至六叶期的叶用甜菜(VI048530)植株进行土壤浇灌接种,接种30 ml约10 CFU/ml的细菌悬浮液。无菌水用作阴性对照。4至6天后,在幼嫩的叶用甜菜叶片上观察到萎蔫的最初症状。症状发展过程与在田间观察到的相同。接种植株分离物在TZC培养基上的菌落形态与之前从田间样本中描述的相同。还使用之前描述的接种程序在番茄(VI005790)、茄子(VI046095)和辣椒(PBC1367)植株上测试了这些菌株的致病性。番茄、茄子和辣椒植株上的平均发病率分别为100%(120/120)、100%(120/120)和79.2%(95/120)。通过印片法在无症状的辣椒植株(16/120)中发现了潜伏感染。使用青枯雷尔氏菌特异性引物对AU759f和AU760r(5)对每个菌株总DNA进行聚合酶链反应(PCR)扩增,产生了预期的282 bp扩增子。根据它们利用三种己糖醇(甘露醇、山梨醇和卫矛醇)和三种二糖(乳糖、麦芽糖和纤维二糖)(2)产酸的能力,所有分离菌株均被鉴定为生物变种3。根据系统型特异性多重PCR分析和部分egl基因序列(GenBank登录号KM100442至KM100449)(1),所有叶用甜菜分离物均被鉴定为青枯雷尔氏菌系统型I,序列变种34。在叶用甜菜的近缘种甜菜(Beta vulgaris L.)上也观察到了青枯病症状,但甜菜尚未被确认为寄主植物(3)。据我们所知,这是全世界关于叶用甜菜作为青枯雷尔氏菌寄主的首次报道。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》。C. Allen等人编。美国植物病理学会出版社,明尼苏达州圣保罗,2005年,第449页。(2)A. C. Hayward。《应用细菌学杂志》27:265,1964年。(3)A. Kelman。由青枯假单胞菌引起的青枯病。技术通报第99号。北卡罗来纳州农业试验站,1953年。(4)A. Kelman。《植物病理学》44:693,1954年。(5)N. Opina等人。《亚太分子生物学与生物技术杂志》5:19,1997年。
