昆虫病原真菌球孢白僵菌(子囊菌:下creales)分离物的PCR-RFLP分化

IF 0.3 4区 农林科学 Q4 PLANT SCIENCES
Phytoprotection Pub Date : 2010-06-28 DOI:10.7202/044022AR
Rachid Sabbahi, R. Lavallée, A. Merzouki, C. Guertin
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引用次数: 9

摘要

球孢白僵菌(Beauveria bassiana)是一种很有前途的农业害虫生物防治剂。采用分子方法(PCR、DNA序列分析和PCR- rflp)对不同的球孢白僵菌进行鉴定。我们的工作包括鉴定球孢白孢核糖体DNA的18S、ITS1、5.8S、ITS2和28S区域。扩增区域的DNA序列表明,18S rDNA是最保守的单位,同源性高(99.5%),而28S rDNA 3′端具有很大的变异性,这为区分菌株提供了可能。采用PCR-RFLP方法对球孢白僵菌分离株进行了监测,并与目标害虫线线虫进行了区分。这种方法包括两个主要步骤。首先,利用PCR扩增球孢白僵菌28S基因的一个区域。其次,用限制性内切酶酶切该PCR产物,并用凝胶电泳对产生的片段进行比较。由于PCR-RFLP的高特异性和敏感性,从被感染昆虫的表面刮取孢子作为样本,可以区分球孢白僵菌分离株。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Differentiation of entomopathogenic fungus Beauveria bassiana (Ascomycetes: Hypocreales) isolates by PCR-RFLP
The entomopathogenic fungus Beauveria bassiana is a promising biological control agent of several insect pests in agriculture. Molecular approaches (PCR, DNA sequence analysis and PCR-RFLP) were used in our research as tools for the identification of different B. bassiana isolates. Our work consisted in identifying the 18S, ITS1, 5.8S, ITS2 and 28S regions of B. bassiana ribosomal DNA. The DNA sequences of the amplified regions showed that the 18S rDNA is the most conserved unit, with a high homology (99.5%) between the isolates studied, while the 3’ end of the 28S rDNA has a great variability, which makes it possible to differentiate the isolates. The PCR-RFLP method was used to monitor isolates of B. bassiana and distinguish them in a target pest, Lygus lineolaris. This method involved two main steps. First, PCR was used to amplify a region of the 28S gene of B. bassiana. Second, this PCR product was digested using restriction endonucleases, and the fragments produced were compared using gel electrophoresis. Because of the high specificity and sensitivity of PCR-RFLP, it was possible to discriminate between B. bassiana isolates using spores scraped from the surface of an infected insect as samples.
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Phytoprotection
Phytoprotection 生物-植物科学
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