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丁香疫霉在土耳其黎巴嫩雪松上的首次报道。

First Report of Phytophthora syringae on Cedrus libani in Turkey.

作者信息

Doğmuş-Lehtijärvi T, Kaya A G Aday, Lehtijärvi A, Jung T

机构信息

Süleyman Demirel University, Faculty of Forestry, 32260 Isparta, Turkey.

Süleyman Demirel University, Yenişarbademli Vocational School, 32000 Isparta, Turkey.

出版信息

Plant Dis. 2014 Jun;98(6):846. doi: 10.1094/PDIS-09-13-0962-PDN.

DOI:10.1094/PDIS-09-13-0962-PDN
PMID:30708685
Abstract

Cedrus libani, commonly known as Lebanon cedar, is one of the most important coniferous tree species in Turkey. Its main distribution is in the Taurus Mountains in the Mediterranean Region. The total area of pure Taurus cedar forest covers 109,440 ha in Turkey, all located in the southwestern regions of the country. Due to its drought resistance, Taurus cedar has been commonly used for afforestations in these semi-arid areas (1). In September 2011, during surveys for Phytophthora spp. in forest nurseries in Adapazari and İzmir in eastern Turkey, initial symptoms such as death of fine roots, yellowing, and wilting of Taurus cedar seedlings were observed. Soil samples were collected from 10 symptomatic C. libani seedlings and isolation tests for Phytophthora species were carried out using leaflets from young Quercus suber, Azalea sp., and Rhodendron sp. saplings as baits floated over flooded soil. Necrotic baits were blotted dry, cut into small pieces, and placed on selective PARPNH carrot agar. Out growing colonies were subcultured on carrot agar and kept at 12°C for morphological and molecular identifications (2). In total, six Pythiaceous isolates were obtained from the C. libani soil samples. The isolates were investigated using a light microscope and grouped according to their morphological characteristics (3). DNA was extracted from two representative isolates using Qiagen DNeasy Plant Mini Kit following the manufacturer's instructions. PCR amplifications and sequencing of the internal transcribed spacer (ITS) region of rDNA and the β-tubulin gene were performed using ITS1 and ITS4 and Tub1 and Tub2 primer sets (4). Sequencing of the PCR products in both directions was conducted by IonTek Inc. (Istanbul, Turkey) in an ABI PRISM automated sequencer. The obtained sequences were compared with those in the GenBank and Phytophthora database using BLAST search. On the basis of morphological features and molecular analyses, the two isolates were identified as Phytophthora syringae. Morphological characteristics on carrot agar were identical with the description of P. syringae (2). At 20°C, colonies reached 7 cm in diameter after 1 week. Sporangia were semipapillate to non-papillate, ovoid, with average length of 59 μm (SD ± 2.8) (range 58 to 70 μm). Oogonia were 38 μm (SD ± 5.4) in diameter (range 30 to 47 μm) with paragynous antheridia. The morphological identification was confirmed by sequence comparison at GenBank with 99% homology for both ITS and β-tubulin. The ITS sequences of the two isolates were deposited in GenBank with the accession nos. KF430614 and KF944377. Under-bark inoculation tests with mycelia plugs were conducted with both isolates of P. syringae at 18°C in a growth chamber on a total of six 1-year-old shoots cut from two C. libani trees. Lesions with an average length of 19 mm (SD ± 6) developed after 10 days. P. syringae was consistently re-isolated from the margins of necrotic tissues. Control shoots remained symptomless. To our knowledge, this is the first report of damage caused by P. syringae on C. libani seedlings in forest nursery in Turkey. References: (1) T. Çalışkan. Pages 109-130 in: Proceedings of Workshop "Hızlı gelişen türlerle ilgili rapor," Ankara, Turkey, 1998. (2) T. Jung et al. Eur. J. For. Pathol. 26:253, 1996. (3) T. Jung et al. Mycol. Res. 107:772, 2003. (4) L. P. N. M. Kroon et al. Fung. Genet. Biol. 41:766, 2004.

摘要

黎巴嫩雪松(Cedrus libani),通常被称为黎巴嫩杉,是土耳其最重要的针叶树种之一。其主要分布在地中海地区的托罗斯山脉。土耳其纯托罗斯雪松林的总面积为109,440公顷,全部位于该国西南部地区。由于其耐旱性,托罗斯雪松常用于这些半干旱地区的造林(1)。2011年9月,在土耳其东部阿达帕扎里和伊兹密尔的森林苗圃中对疫霉属(Phytophthora spp.)进行调查期间,观察到托罗斯雪松幼苗出现细根死亡、发黄和枯萎等初始症状。从10株有症状的黎巴嫩雪松幼苗上采集土壤样本,并使用来自嫩栓皮栎(Quercus suber)、杜鹃花属(Azalea sp.)和杜鹃属(Rhodendron sp.)幼树苗的叶片作为诱饵漂浮在淹水土壤上,对疫霉属物种进行分离试验。将坏死的诱饵吸干,切成小块,置于选择性PARPNH胡萝卜琼脂上。长出的菌落转接至胡萝卜琼脂上,并保存在12°C下进行形态学和分子鉴定(2)。总共从黎巴嫩雪松土壤样本中获得了6个腐霉科分离株。使用光学显微镜对这些分离株进行研究,并根据其形态特征进行分组(3)。按照制造商的说明,使用Qiagen DNeasy植物微量提取试剂盒从两个代表性分离株中提取DNA。使用ITS1和ITS4以及Tub1和Tub2引物对rDNA的内部转录间隔区(ITS)和β-微管蛋白基因进行PCR扩增和测序(4)。PCR产物的双向测序由土耳其伊斯坦布尔的IonTek公司在ABI PRISM自动测序仪上进行。使用BLAST搜索将获得的序列与GenBank和疫霉属数据库中的序列进行比较。基于形态特征和分子分析,这两个分离株被鉴定为丁香疫霉(Phytophthora syringae)。在胡萝卜琼脂上的形态特征与丁香疫霉的描述一致(2)。在20°C下,菌落1周后直径达到7厘米。孢子囊半乳头状至非乳头状,卵形,平均长度为59μm(标准差±2.8)(范围58至70μm)。藏卵器直径为38μm(标准差±5.4)(范围30至47μm),雄器侧生。通过在GenBank上进行序列比较,ITS和β-微管蛋白的同源性均为99%,从而确认了形态学鉴定。这两个分离株的ITS序列已存入GenBank,登录号分别为KF430614和KF944377。在生长室中于18°C下,对总共从两棵黎巴嫩雪松树上剪下的6个1年生嫩枝进行了丁香疫霉两个分离株的菌丝块皮下接种试验。10天后出现平均长度为19mm(标准差±6)的病斑。始终能从坏死组织边缘重新分离出丁香疫霉。对照嫩枝无症状。据我们所知,这是土耳其森林苗圃中丁香疫霉对黎巴嫩雪松幼苗造成损害的首次报道。参考文献:(1)T. Çalışkan。载于:“快速生长树种相关报告”研讨会论文集,土耳其安卡拉,1998年,第109 - 130页。(2)T. Jung等人。《欧洲森林病理学杂志》26:253,1996年。((3)T. Jung等人。《真菌学研究》107:772,2003年。(4)L. P. N. M. Kroon等人。《真菌遗传学与生物学》41:766,2004年。

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