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松针红斑病病原的检测与鉴定

Detection and Identification of the Causal Agents of Dothistroma Needle Blight.

作者信息

Oskay Funda, Lehtijärvi Asko, Lehtijärvi Hatice Tuğba Doğmuş

机构信息

Faculty of Forestry, Çankırı Karatekin University, Çankırı, Turkey.

Isparta University of Applied Sciences, Sütçüler Prof. Dr. Hasan Gürbüz Vocational School, Isparta, Turkey.

出版信息

Methods Mol Biol. 2022;2536:155-166. doi: 10.1007/978-1-0716-2517-0_10.

Abstract

Dothistroma needle blight (DNB) is one of the most damaging foliage diseases of pine in plantations and natural forests worldwide and is caused by two closely related fungi: Dothistroma septosporum and D. pini, which are virtually impossible to differentiate from each other based on morphology. Although diagnosis of DNB based on symptoms is relatively reliable in the later stages of the disease when fruit bodies (conidiomata) are formed, for diagnosis in the early stages, as well as identification of the causal agent at species level, molecular methods are required. In addition, reliable and sensitive diagnostics before sporulation is a prerequisite for early detection to minimize accidental introductions of disease through movement of infected plant materials, especially seedlings. While amplification and sequencing of the ITS region of the rDNA alone is not reliable to differentiate the two species, conventional PCR (cPCR) using species-specific primers or mating type-specific primers and quantitative PCR (qPCR) are widely used and accepted molecular methods to identify and differentiate the DNB pathogens, either from cultures or directly from needles.

摘要

散斑壳针孢叶枯病(DNB)是全球人工林和天然林中对松树危害最大的叶部病害之一,由两种亲缘关系密切的真菌引起: septosporum散斑壳针孢和松针散斑壳针孢,基于形态学几乎无法将它们彼此区分开来。虽然在病害后期形成子实体(分生孢子盘)时,基于症状对DNB进行诊断相对可靠,但在早期阶段进行诊断以及在物种水平上鉴定病原菌时,则需要分子方法。此外,在孢子形成前进行可靠且灵敏的诊断是早期检测的前提条件,以便尽量减少通过感染植物材料(尤其是幼苗)的移动而意外引入病害的情况。虽然单独对rDNA的ITS区域进行扩增和测序并不能可靠地区分这两个物种,但使用物种特异性引物或交配型特异性引物的常规PCR(cPCR)和定量PCR(qPCR)是广泛使用且被认可的分子方法,可用于从培养物或直接从针叶中鉴定和区分DNB病原菌。

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