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小麦病原菌镰刀菌中微型反向重复转座元件 mimp1 的转位。

Transposition of the miniature inverted-repeat transposable element mimp1 in the wheat pathogen Fusarium culmorum.

机构信息

Dipartimento di Agraria - Sezione di Patologia Vegetale ed Entomologia and Centro interdisciplinare per lo sviluppo della ricerca biotecnologica e per lo studio della biodiversità della Sardegna e dell'area Mediterranea, Università degli Studi di Sassari, Via E. De Nicola 9, I-07100 Sassari, Italy.

出版信息

Mol Plant Pathol. 2012 Dec;13(9):1149-55. doi: 10.1111/j.1364-3703.2012.00823.x. Epub 2012 Aug 16.

Abstract

High-throughput methods are needed for functional genomics analysis in Fusarium culmorum, the cause of crown and foot rot on wheat and a type B trichothecene producer. Our aim was to develop and test the efficacy of a double-component system based on the ability of the impala transposase to transactivate the miniature inverted-repeat transposable element mimp1 of Fusarium oxysporum. We report, for the first time, the application of a tagging system based on a heterologous transposon and of splinkerette-polymerase chain reaction to identify mimp1 flanking regions in the filamentous fungus F. culmorum. Similar to previous observations in Fusarium graminearum, mimp1 transposes in F. culmorum by a cut-and-paste mechanism into TA dinucleotides, which are duplicated on insertion. mimp1 was reinserted in open reading frames in 16.4% (i.e. 10 of 61) of the strains analysed, probably spanning throughout the entire genome of F. culmorum. The effectiveness of the mimp1/impala double-component system for gene tagging in F. culmorum was confirmed phenotypically for a putative aurofusarin gene. This system also allowed the identification of two genes putatively involved in oxidative stress-coping capabilities in F. culmorum, as well as a sequence specific to this fungus, thus suggesting the valuable exploratory role of this tool.

摘要

高通量方法对于研究引起小麦冠腐病和根腐病的尖孢镰刀菌的功能基因组学分析是必要的,该菌也是 B 型单端孢霉烯族毒素的生产者。我们的目的是开发和测试基于 impala 转座酶激活尖孢镰刀菌微小反向重复转座元件 mimp1 的双成分系统的功效。我们首次报道了一种基于异源转座子和 splinkerette-聚合酶链反应的标记系统,用于鉴定丝状真菌尖孢镰刀菌中 mimp1 的侧翼区域。与在禾谷镰刀菌中的先前观察结果相似,mimp1 在尖孢镰刀菌中通过“切接”机制转座到 TA 二核苷酸,在插入时会重复。mimp1 在分析的 61 株菌株中的 16.4%(即 10 株)中重新插入开放阅读框,可能跨越尖孢镰刀菌整个基因组。mimp1/impala 双成分系统用于尖孢镰刀菌基因标记的有效性在一个假定的金毒素基因上得到了表型证实。该系统还允许鉴定出两个在尖孢镰刀菌中可能参与氧化应激应对能力的基因,以及一个特定于该真菌的序列,因此表明该工具具有宝贵的探索作用。

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