对橡树和东方山毛榉衰退病原菌 Brenneria goodwinii 进行可靠、特异的检测和鉴定

IF 2.7 3区 农林科学 Q2 ECOLOGY
Mohammad-Hossein Araeinejhad, N. F. Charkhabi, C. Brady, Heshmat Rahimian
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引用次数: 0

摘要

栗叶栎(Quercus castaneifolia)和东方山毛榉(Fagus orientalis)是希尔卡尼亚森林中的主要树种。在不同国家,Brenneria goodwinii 被确定为受影响橡树上坏死病变和茎出血的病原体。在伊朗北部的一些森林地点观察到橡树和东方山毛榉树出现出血症状。本研究的目的是确定栎树和东方榉树树皮腐烂病病原体的特征,并开发一套引物,利用聚合酶链式反应(PCR)对 Brenneria goodwinii 菌株进行特异性检测。2020-2021 年,研究人员在伊朗北部戈勒斯坦森林和马赞达兰森林分别采集了 31 份和 20 份栎树和东方榉树样本,这些样本都出现了茎干出血和树皮腐烂症状。从有症状的橡树样本(105 株)和东方榉树样本(32 株)中分离出了在 EMB-agar 培养基上显示绿色金属光泽的细菌菌株,从健康的橡树和东方榉树样本中也分别分离出了 31 株和 20 株细菌。致病性测试表明,分别从橡树和榉树中分离出的 51 株和 25 株菌株能够在接种 15 天后诱导橡树橡子出现坏死区。此外,分别接种在橡树和榉树树枝上的 4 株和 2 株代表性菌株在接种 1 个月后诱导所有接种的绿色树枝坏死。从橡树和东方榉树上分离并被证明具有致病性的代表性菌株的 16S rRNA 和 gyrB 基因序列与 B. goodwinii LMG 26270T 的相似度分别为 100%和 99%以上,这表明这些菌株属于 B. goodwinii 种。针对 hrpN 基因设计的引物对 BgF3/R2 被证明对检测 B. goodwinii 菌株具有特异性。该引物对仅能从 Goodwinii 菌株中扩增出 618-bp 的 DNA 片段,而不能从 Rahnella、Gibbsiella、Lonsdalea 和其他 Brenneria 菌株中扩增出 DNA 片段。使用该引物对从健康树木或幼苗中提取的 DNA 进行 PCR 时,没有扩增出任何片段。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Reliable and specific detection and identification of Brenneria goodwinii, the causal agent of oak and oriental beech decline
Chestnut-leaved oak (Quercus castaneifolia) and oriental beech (Fagus orientalis) are among the major tree species in the Hyrcanian forests. Brenneria goodwinii was identified as the causal agent of necrotic lesions and stem bleeding on affected oak trees in different countries. Oak and oriental beech trees with bleeding symptoms were observed in a few forest sites in northern Iran. The objectives of the present study were to identify and characterize the causal agents of bark canker in oak and oriental beech trees and develop a primer set for specific detection, using polymerase chain reaction (PCR), of Brenneria goodwinii strains. A total of 31 and 20 samples from oak and oriental beech trees, respectively, with stem bleeding and bark canker symptoms were collected from Golestan and Mazandaran forests in northern Iran in 2020–2021. Bacterial strains displaying a green metallic sheen on EMB-agar medium were isolated from symptomatic oak (105 strains) and oriental beech samples (32 strains), while 31 and 20 strains were also isolated from healthy oak and oriental beech, respectively. Pathogenicity tests indicated that 51 and 25 strains isolated from oak and oriental beech, respectively were able to induce a necrotic area on oak acorns 15 days following inoculation. Moreover, four and two representative strains inoculated on oak and oriental beech twigs, respectively induced necrosis on all inoculated green twigs 1 month after inoculation. The sequences of the 16S rRNA and gyrB genes of representative strains isolated from and proved pathogenic on oak and oriental beech trees were 100% and over 99% similar to B. goodwinii LMG 26270T, respectively, which revealed the strains belong to B. goodwinii species. The primer pair BgF3/R2, which was designed to target the hrpN gene, was proven to be specific in the detection of B. goodwinii strains. The primer pair amplified a 618-bp DNA fragment from strains of B. goodwinii only and not from strains belonging to Rahnella, Gibbsiella, Lonsdalea, and the other Brenneria species among several other pathogenic bacteria tested. No fragment was amplified from DNA extracted from healthy trees or seedlings in PCR using this primer pair.
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来源期刊
CiteScore
4.50
自引率
6.20%
发文量
256
审稿时长
12 weeks
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