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Growth inhibition of the cereal root pathogens<i>Rhizoctonia solani</i>AG8,<i>R. oryzae</i>and<i>Gaeumannomyces graminis</i>var.<i>tritici</i>by a recombinant 42-kDa endochitinase from<i>Trichoderma harzianum</i>
12
Citations
60
References
2006
Year
Cereal RootEngineeringPlant PathologyThen42 GeneBiosynthesisGrowth InhibitionMicrobial EcologyPlant Pathogen EffectorInhibitory ActivityRhizosphereBiochemistryPlant-microbe InteractionFungal PhysiologyFungal PathogenBiomolecular EngineeringIntermediate Inhibitory ActivityCrop ProtectionBiotechnologyGenetic EngineeringRecombinant 42-Kda EndochitinaseMicrobiologyMedicine
Abstract The objective of this study was to determine the effectiveness of a 42-kDa endochitinase coded by the ThEn42 gene from Trichoderma harzianum as a potential source of transgenic resistance to Rhizoctonia root rot of barley caused by Rhizoctonia solani AG8 and/or R. oryzae. The gene cThEn42 was codon optimized (GC content increased from 53.3 to 65.1%) and then synthesized to produce the modified cThEn42GC in Pichia pastoris for in vitro tests. Two expression vectors were constructed: one with the fungal signal peptide and the fungal activation peptide [FSP-FAP-cThEn(GC)] and the other with barley chitinase 26 signal peptide followed by the fungal signal and activation peptides [SP(HVChi26)-FSP-FAP-cThEn(GC)]. N-terminal sequencing showed that, of two proteins secreted into liquid medium, FSP was cleaved off faithfully in one protein and both FSP and FAP were cleaved from the other protein. Purified endochitinase provided strong in vitro inhibition of both R. solani AG8 and R. oryzae. The enzyme had an intermediate inhibitory activity against Gaeumannomyces graminis var. tritici, and no inhibitory activity against Fusarium graminearum, F. pseudograminearum, and F. culmorum.
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