First Report of Root Collar Canker Caused by Neoscytalidium dimidiatum on Jacaranda mimosifolia in China.

IF 4.4 2区 农林科学 Q1 PLANT SCIENCES Plant disease Pub Date : 2024-08-22 DOI:10.1094/PDIS-07-24-1381-PDN
Xiaoli Li, Lingzihang Huang, Bo Tao, Qian Lu, Gaoqing Yuan
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引用次数: 0

Abstract

Jacaranda mimosifolia is widely cultivated as a garden ornamental tree. In July 2023, an unknown root collar canker of J. mimosifolia was discovered in green belts of Qingxiu District, Nanning, China, with a 8% incidence rate. Crowns of affected trees ranged from reddish brown leaves to deciduous or dead. Root collar tissue became necrotic matched by underbark dark brown lesions with irregular margins, and rotted at last. Six diseased plants distributed within 3000 m2 were choosed, and 24 root collar tissues were surface sterilized and placed on potato dextrose agar (PDA) plates to incubate at 28℃ for 3 to 5 days. Same colonies were consistently isolated from 18 tissues, and three isolates (M3-B1-1, M3-B1-2 and M3-B1-3) were purified for morphological and molecular determination. These isolates formed colonies with lush aerial mycelia rapidly, which covered a 90 mm plate in 72h. The colonies were initially white, then grayish-green to black. Arthrospores were colourless to light brown, short columnar, aseptate, truncate base, averaging 12.1±2.5 µm × 3.4±0.7 µm, sometimes formed arthric chains. Chlamydospores were dark brown, round or oval, aseptate, averaging 8.7±1.6 µm × 5.0±0.9 µm. Mature pycnidia and conidia produced for about 50 days on oatmeal agar medium (OMA), and conidia were colorless, oblong, aseptate, averaging 11.2±1.2 µm × 6.0±1.4 µm. These morphological characteristics were consistent with the description of Neoscytalidium dimidiatum (Penz.) Crous & Slippers (Crous et al. 2006). Genomic DNA was extracted from three isolates. The partial ITS region, TUB2 and TEF1-α genes were amplified (White et al., 1990; Glass and Donaldson 1995; Carbone and Kohn 1999). The sequences were deposited in GenBank (ITS: PP939650-PP939652; TUB2: PP942728-PP942730; TEF1-α: PP942731-PP942733). Blastn analysis revealed that ITS sequences of three isolates showed 99.8%, 100%, 100% identity (506 bp out of 507 bp, 507 bp out of 507 bp, 507 bp out of 507 bp) to N. dimidiatum C21 (KX447539), the TUB2 sequences showed 100% identity (436 bp out of 436 bp, 437 bp out of 437 bp, 437 bp out of 437 bp) to N.dimidiatum LNeo (ON099066), and the TEF1-α sequences showed 99.64% identity (276 bp out of 277 bp) to N.dimidiatum ARM230 (MK495384), respectively. Phylogenetic analysis based on concatenated ITS, TUB2 and TEF1-α sequences showed that three isolates were clustered into the same clade as N. dimidiatum. To fulfill Koch's postulates, pathogenicity of these isolates was tested on healthy two-year-old J. mimosifolia trees. Stem and root collar were wounded and placed mycelial plugs (8mm), and the inoculation sites were wrapped with parafilm or covered with nursery substrate to maintain the humidity. Four plants were inoculated with each isolate. As a control, four plants were inoculated with noncolonized PDA plugs. All treated plants were kept in a greenhouse at 28 ± 3°C and 70% relative humidity. Foliar blight and necrotic lesions around inoculation points were observed about 65 days after inoculation, and 50% of inoculated trees exhibited symptoms, whereas the control trees remained symptomless. Neoscytalidium dimidiatum was successfully reisolated from symptomatic tissue via morphological analysis. To our knowledge, this is the first report of root collar canker caused by N. dimidiatum on J. mimosifolia. Neoscytalidium dimidiatum has a wide range of hosts, including pitaya, pine, mulberry, pear, grape, locust tree (Luo et al. 2024). This finding will help in controlling of the disease epidemic.

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在中国首次报告由 Neoscytalidium dimidiatum 在含笑树上引起的根领腐烂病。
含笑树是一种广泛栽培的园林观赏树种。2023 年 7 月,在中国南宁市青秀区的绿化带中发现了一种未知的细叶女贞根领腐烂病,发病率为 8%。受害树木的树冠从红褐色叶片到落叶或枯死不等。根领组织坏死,树皮下出现边缘不规则的黑褐色病斑,最后腐烂。选取分布在 3000 平方米范围内的 6 株病株,对 24 个根领组织进行表面消毒,并将其置于马铃薯葡萄糖琼脂(PDA)平板上,在 28℃下培养 3 至 5 天。从 18 个组织中持续分离出相同的菌落,并纯化了 3 个分离株(M3-B1-1、M3-B1-2 和 M3-B1-3)进行形态和分子测定。这些分离物迅速形成菌落,气生菌丝茂盛,在 72 小时内覆盖了 90 毫米的平板。菌落最初为白色,然后变为灰绿色至黑色。节孢子无色至浅棕色,短柱状,无节,基部截形,平均长 12.1±2.5 µm × 3.4±0.7 µm,有时形成节链。衣孢子暗褐色,圆形或椭圆形,无节,平均 8.7±1.6 µm × 5.0±0.9 µm。成熟的分生孢子和分生孢子在燕麦琼脂培养基(OMA)上生长约 50 天,分生孢子无色,长圆形,无节,平均 11.2±1.2 µm × 6.0±1.4 µm。这些形态特征与 Neoscytalidium dimidiatum (Penz.) Crous & Slippers 的描述一致(Crous 等,2006 年)。从三个分离株中提取了基因组 DNA。扩增了部分 ITS 区域、TUB2 和 TEF1-α 基因(White 等人,1990 年;Glass 和 Donaldson,1995 年;Carbone 和 Kohn,1999 年)。序列已存入 GenBank(ITS:PP939650-PP939652;TUB2:PP942728-PP942730;TEF1-α:PP942731-PP942733)。Blastn 分析表明,三个分离株的 ITS 序列与 N. dimidiatum C21(K.N. Dimidiatum)的 ITS 序列(507 bp 中的 506 bp、507 bp 中的 507 bp、507 bp 中的 507 bp)分别显示出 99.8%、100%、100% 的一致性。TUB2序列与N.dimidiatum LNeo(ON099066)显示出100%的同一性(436 bp中的436 bp、437 bp中的437 bp、437 bp中的437 bp),TEF1-α序列与N.dimidiatum ARM230(MK495384)显示出99.64%的同一性(277 bp中的276 bp)。基于ITS、TUB2和TEF1-α序列的系统进化分析表明,三个分离物与N.dimidiatum聚为同一支系。为了验证科赫假设,在健康的两年树龄的 J. mimosifolia 树上测试了这些分离物的致病性。在茎和根的颈部伤口处放置菌丝体插条(8 毫米),接种部位用保鲜膜包裹或覆盖苗圃基质以保持湿度。每种分离物接种四株植物。作为对照,四株植物接种了未移栽的 PDA 插条。所有处理过的植物都放在 28 ± 3°C 和 70% 相对湿度的温室中。接种后约 65 天,观察到接种点周围出现叶枯病和坏死病变,50% 的接种树出现症状,而对照树仍无症状。通过形态分析,我们成功地从有症状的组织中重新分离出了 Neoscytalidium dimidiatum。据我们所知,这是首次报道 N. dimidiatum 在 J. mimosifolia 上引起的根领腐烂病。Neoscytalidium dimidiatum 的寄主范围很广,包括番木瓜、松树、桑树、梨树、葡萄、槐树等(Luo 等,2024 年)。这一发现将有助于控制该疾病的流行。
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来源期刊
Plant disease
Plant disease 农林科学-植物科学
CiteScore
5.10
自引率
13.30%
发文量
1993
审稿时长
2 months
期刊介绍: Plant Disease is the leading international journal for rapid reporting of research on new, emerging, and established plant diseases. The journal publishes papers that describe basic and applied research focusing on practical aspects of disease diagnosis, development, and management.
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