Intracellular siderophore but not extracellular siderophore is required for full virulence in Metarhizium robertsii
•M. robertsii core biosynthetic genes for metachelin A and ferricrocin were deleted.•Null mutants for the transcriptional repressor mrsreA were also produced.•Metachelins were found to be dispensable for virulence while ferricrocin was not.•M. robertsii mrsreA mutants were unaltered in virulence. Ef...
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Veröffentlicht in: | Fungal genetics and biology 2015-09, Vol.82, p.56-68 |
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Sprache: | eng |
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Zusammenfassung: | •M. robertsii core biosynthetic genes for metachelin A and ferricrocin were deleted.•Null mutants for the transcriptional repressor mrsreA were also produced.•Metachelins were found to be dispensable for virulence while ferricrocin was not.•M. robertsii mrsreA mutants were unaltered in virulence.
Efficient iron acquisition mechanisms are fundamental for microbial survival in the environment and for pathogen virulence within their hosts. M. robertsii produces two known iron-binding natural products: metachelins, which are used to scavenge extracellular iron, and ferricrocin, which is strictly intracellular. To study the contribution of siderophore-mediated iron uptake and storage to M. robertsii fitness, we generated null mutants for each siderophore synthase gene (mrsidD and mrsidC, respectively), as well as for the iron uptake transcriptional repressor mrsreA. All of these mutants showed impaired germination speed, differential sensitivity to hydrogen peroxide, and differential ability to overcome iron chelation on growth-limiting iron concentrations. RT-qPCR data supported regulation of mrsreA, mrsidC, and mrsidD by supplied iron in vitro and during growth within the insect host, Spodoptera exigua. We also observed strong upregulation of the insect iron-binding proteins, transferrins, during infection. Insect bioassays revealed that ferricrocin is required for full virulence against S. exigua; neither the loss of metachelin production nor the deletion of the transcription factor mrsreA significantly affected M. robertsii virulence. |
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ISSN: | 1087-1845 1096-0937 |
DOI: | 10.1016/j.fgb.2015.06.008 |