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西班牙葡萄砧木母株衰退与可可毛色二孢菌相关性的首次报道

First Report of Lasiodiplodia theobromae Associated with Decline of Grapevine Rootstock Mother Plants in Spain.

作者信息

Aroca A, Raposo R, Gramaje D, Armengol J, Martos S, Luque J

机构信息

CIFOR, INIA, Ctra. La Coruña km 7.5, 28040 Madrid, Spain.

Instituto Agroforestal Mediterráneo, Universidad Politécnica de Valencia, Camino de Vera s/n, 46022 Valencia, Spain.

出版信息

Plant Dis. 2008 May;92(5):832. doi: 10.1094/PDIS-92-5-0832B.

DOI:10.1094/PDIS-92-5-0832B
PMID:30769618
Abstract

A field of Richter 110 rootstock mother plants in Valencia Province (eastern Spain) was surveyed during November 2006 to study the mycoflora of declining plants. Two canes with stunted leaves were collected from a plant with a reduced number of shoots. No cankers or vascular lesions were observed in the collected canes. Six wood chips (1 to 2 mm thick) were taken from one basal fragment (3 to 4 cm long) of each cane, surface sterilized in 70% ethanol for 1 min, and plated on malt extract agar supplemented with 0.5 g L of streptomycin sulfate. Petri dishes were incubated for 7 days at 25°C. A fungus was consistently isolated from all samples that showed the following characteristics: colonies grown on potato dextrose agar (PDA) at 25°C developed a white, aerial mycelium that turned gray after 4 to 6 days and produced pycnidia after 1 month on sterile grapevine slivers of twigs placed on the PDA surface; conidia from culture were ellipsoidal, thick walled, initially hyaline, nonseptate, and measuring 20 to 25 (22.5) × 12 to 14 (13) μm; aged conidia were brown, 1-septate with longitudinal striations in the wall; and pseudoparaphyses variable in form and length were interspersed within the fertile tissue. The fungus was identified as Lasiodiplodia theobromae (Pat.) Griffon & Maubl. from the above characteristics (2). Identity was confirmed by analysis of the nucleotide sequences of the internal transcribed spacer (ITS) region from the rRNA repeat and part of the translation elongation factor 1-alpha (EF1-α) and the β-tubulin (B-tub) genes, as done elsewhere (1,3). BLAST searches at GenBank showed a high identity with reference sequences (ITS: 100%, EF1-α: 97%; B-tub: 99%). Representative sequences of the studied DNA regions were deposited at GenBank (Accession Nos.: ITS: EU254718; EF1-α: EU254719; and B-tub: EU254720). A pathogenicity test was conducted on 1-year-old grapevine plants cv. Macabeo grafted onto Richter 110 rootstocks maintained in a greenhouse. A superficial wound was made on the bark of 10 plants with a sterilized scalpel, ≈10 cm above the graft union. A mycelial plug obtained from the margin of an actively growing fungal colony (isolate JL664) was placed in the wound and the wound was wrapped with Parafilm. Ten additional control plants were inoculated with sterile PDA plugs. All control plants grew normally, and the inoculation wound healed 3 months after inoculation. Plants inoculated with L. theobromae showed no foliar symptoms in the same period, but developed cankers variable in size surrounding the inoculation sites. Vascular necroses measuring 8.4 ± 1.5 cm (mean ± standard error) developed in the inoculated plants that were significantly longer than the controls (0.3 ± 0.2 cm). The pathogen was reisolated from all inoculated plants and no fungus was reisolated from the controls. These results confirmed the pathogenicity of L. theobromae to grapevine and points to a possible involvement of L. theobromae in the aetiology of grapevine decline as previously reported (3,4). To our knowledge, this is the first report of L. theobromae isolated from grapevine in Spain. References: (1) J. Luque et al. Mycologia 97:1111, 2005. (2) E. Punithalingam. No. 519 in: Descriptions of Pathogenic Fungi and Bacteria. CMI, Kew, Surrey, UK, 1976. (3) J. R. Úrbez-Torres et al. Plant Dis. 90:1490, 2006. (4) J. M. van Niekerk et al. Phytopathol. Mediterr. 45(suppl.):S43, 2006.

摘要

2006年11月,对西班牙东部巴伦西亚省一片里氏110砧木母本植株种植园进行了调查,以研究生长衰退植株的真菌区系。从一株新梢数量减少的植株上采集了两根叶片发育不良的茎。采集的茎上未观察到溃疡或维管束病变。从每根茎的一个基部片段(3至4厘米长)上取6片木屑(1至2毫米厚),在70%乙醇中表面消毒1分钟,然后接种到添加了0.5克/升硫酸链霉素的麦芽提取物琼脂上。培养皿在25°C下培养7天。从所有样本中始终分离出一种真菌,其具有以下特征:在25°C的马铃薯葡萄糖琼脂(PDA)上生长的菌落形成白色气生菌丝体,4至6天后变为灰色,1个月后在放置于PDA表面的无菌葡萄嫩枝切片上产生分生孢子器;培养产生的分生孢子呈椭圆形,壁厚,最初无色透明,无隔膜,大小为20至25(22.5)×12至14(13)微米;老化的分生孢子为褐色,具1个隔膜,壁上有纵向条纹;假侧丝形态和长度各异,散布于可育组织中。根据上述特征,该真菌被鉴定为可可毛色二孢(Lasiodiplodia theobromae (Pat.) Griffon & Maubl.)(2)。如其他研究一样(1,3),通过分析核糖体RNA重复序列的内部转录间隔区(ITS)区域以及翻译延伸因子1-α(EF1-α)和β-微管蛋白(B-tub)基因的部分核苷酸序列,确认了其身份。在GenBank上进行的BLAST搜索显示与参考序列具有高度同源性(ITS:100%,EF1-α:97%;B-tub:99%)。所研究DNA区域的代表性序列已存入GenBank(登录号:ITS:EU254718;EF1-α:EU254719;B-tub:EU254720)。对温室中嫁接到里氏110砧木上的1年生酿酒葡萄品种马卡贝奥(Macabeo)植株进行了致病性测试。用消毒手术刀在10株植株的树皮上,在嫁接部位上方约10厘米处造成一个浅表伤口。从一个活跃生长的真菌菌落(分离株JL664)边缘获取的菌丝块置于伤口处,并用Parafilm包裹。另外10株对照植株接种无菌PDA块。所有对照植株生长正常,接种3个月后接种伤口愈合。接种可可毛色二孢的植株在此期间未出现叶片症状,但在接种部位周围形成了大小不一的溃疡。接种植株中出现了长度为8.4±1.5厘米(平均值±标准误)的维管束坏死,显著长于对照植株(0.3±0.2厘米)。从所有接种植株中重新分离出了病原菌,对照植株中未重新分离出真菌。这些结果证实了可可毛色二孢对葡萄的致病性,并表明可可毛色二孢可能如先前报道(3,4)那样参与了葡萄衰退的病因。据我们所知,这是西班牙首次从葡萄中分离出可可毛色二孢的报道。参考文献:(1) J. Luque等人,《真菌学》97:1111,2005年。(2) E. Punithalingam,《致病真菌和细菌描述》第519号。英国皇家植物园邱园真菌研究所,萨里郡,英国,1976年。(3) J. R. Úrbez-Torres等人,《植物病害》90:1490,2006年。(4) J. M. van Niekerk等人,《地中海植物病理学》45(增刊):S43,2006年。

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