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首页> 外文期刊>European Journal of Plant Pathology >Selection, characterization and genetic analysis of laboratory mutants of Botryotinia fuckeliana (Botrytis cinerea) resistant to the fungicide boscalid
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Selection, characterization and genetic analysis of laboratory mutants of Botryotinia fuckeliana (Botrytis cinerea) resistant to the fungicide boscalid

机译:对杀真菌剂鳞片孢菌的Botryotinia fuckeliana(Botrytis cinerea)实验室突变体的选择,表征和遗传分析

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Resistance to the fungicide boscalid in laboratory mutants of Botryotinia fuckeliana (Botrytis cinerea) was investigated. The baseline sensitivity to boscalid was evaluated in terms of colony growth (EC=0.3-3 peg mlp#; MIC=10-30 peg mlp#) and conidial germination (EC=0.03-0.1 peg mlp#; MIC=1-3 peg mlp#) tests. Mutants were selected in vitro from wild-type strains of the fungus on a fungicide-amended medium containing acetate as a carbon source. Mutants showed two different levels of resistance to boscalid, distinguishable through the conidial germination tests: low (ECo0.3 peg mlp#, ranging from 0.03 to 1 peg mlp#; MIC>100 peg mlp#) and high (EC>100 peg mlp#) resistance. Analysis of meiotic progeny from crosses between resistant mutants and sensitive reference strains showed that resistant phenotypes were due to mutations in single major gene(s) inherited in a Mendelian fashion, and linked with both the Daf1 and Mbc1 genes, responsible for resistance to dicarboximide and benzimidazole fungicides, respectively. Gene sequence analysis of the four sub-units of the boscalid-target protein, the succinate dehydrogenase enzyme, revealed that single or double point mutations in the highly conserved regions of the iron-sulphur protein (Ip) gene were associated with resistance. Mutations resulted in proline to leucine or phenylalanine replacements at position 225 (P225L or P225F) in high resistant mutants, and in a histidine to tyrosine replacement at position 272 (H272Y) in low resistant mutants. Sequences of the flavoprotein and the two transmembrane sub-units of succinate dehydrogenase were never affected.
机译:研究了Botryotinia fuckeliana(灰葡萄孢)的实验室突变体对杀菌剂boscalid的抗性。根据菌落生长(EC = 0.3-3 peg mlp#; MIC = 10-30 peg mlp#)和分生孢子萌发(EC = 0.03-0.1 peg mlp#; MIC = 1-3 peg)评估对Boscalid的基线敏感性mlp#)测试。在含有乙酸盐作为碳源的经杀菌剂改性的培养基上,从真菌的野生型菌株中体外选择突变体。突变体显示出两种不同的抗鳞茎鳞茎抗性,可通过分生孢子萌发测试区分:低(ECo0.3 peg mlp#,范围从0.03至1 peg mlp#; MIC> 100 peg mlp#)和高(EC> 100 peg mlp#) #) 抵抗性。从抗性突变体和敏感参考菌株之间杂交获得的减数分裂后代的分析表明,抗性表型是由于孟德尔遗传的一个主要基因突变所致,并与Daf1和Mbc1基因相关,对双羧酰亚胺和苯并咪唑分别为杀菌剂。基因的序列分析的靶标蛋白的四个亚基,琥珀酸脱氢酶,揭示了高硫区域的铁硫蛋白(Ip)基因中的单点或双点突变与抗性相关。在高抗性突变体中,突变导致脯氨酸被替换为在225位的亮氨酸或苯丙氨酸(P225L或P225F),而在低抗性突变体中导致了在272位(H272Y)被组氨酸替换为酪氨酸。黄素蛋白和琥珀酸脱氢酶的两个跨膜亚单位的序列从未受到影响。

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