A polyketide synthase is required for fungal virulence and production of the polyketide T-toxin.

Yang, Ge; Rose, Mark S.; Turgeon, B. Gillian; Yoder, O. C.

doi:10.1105/tpc.8.11.2139

Cited by 178 publications

(113 citation statements)

References 40 publications

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“…Tox1B includes two genes, DEC1 (similar to acetoacetate decarboxylaseencoding genes) and RED1 (similar to genes encoding members of the medium-chain dehydrogenase/ reductase superfamily) (Rose et al 2002). DEC1 and RED1 map within 1.5 kb of each other on the Tox1B chromosome 6;12 ( Figure 2B) and are unique to the genome of race T, an observation consistent with the hypothesis that these genes were acquired by C. heterostrophus via a horizontal transfer event (Yang et al 1996). Targeted disruption of DEC1 drastically reduced both T-toxin production and virulence of race T to T-cytoplasm maize, whereas specific inactivation of RED1 had no apparent effect on T-toxin production or virulence (Rose et al 2002).…”

supporting

confidence: 75%

Cochliobolus heterostrophus T-toxin gene expression modulation via G protein and MAPK pathways

Degani

2015

Plant Prot. Sci.

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Degani O. (2015): Cochliobolus heterostrophus T-toxin gene expression modulation via G protein and MAPK pathways. Plant Protect Sci., 51: 53-60.The role of G-protein and mitogen-activated protein kinase (MAPK) in filamentous fungi has been studied for over a decade, but downstream elements are less known. Here, we used microarray and Northern blot analysis to examine the involvement of these signalling pathways in controlling the known Cochliobolus heterostrophus T-toxin biosynthetic gene, DEC1, whose control is important in epidemic prevention. Comparison of the expression profile in wild-type strains and in G-protein and MAPK signalling deficient mutants revealed a unique, environmental-dependent control mechanism for the DEC1 gene. The results suggest, for the first time, a possible role in pathogenicity for the G-protein α2 subunit in this organism, and hint to a common role of G-protein α1 and β1 subunits and MAPK in maintaining accurate levels of this toxin during pathogenesis.

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confidence: 75%

Cochliobolus heterostrophus T-toxin gene expression modulation via G protein and MAPK pathways

Degani

2015

Plant Prot. Sci.

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“…To further confirm transformants, genomic DNA was extracted as previously described by Raeder and Broda [37], and Southern blot analysis was performed according to the method of Yang et al [18]. DNA samples, digested with enzymes as indicated in the figure, were resolved on 0.8% agarose gels, and transferred onto Magmaprobe Nylon Transfer Membrane-N + (Osmonics, Minnetonka, MN, USA).…”

Section: Southern Blot Analysismentioning

confidence: 99%

“…Molecular studies have also been performed to determine the biosynthetic principle of important bioactive polyketides, such as aflatoxin [17][18][19][20][21][22]. Regulatory networks governing secondary metabolism have been gradually uncovered in several fungal species, for example, the central roles of the G protein-cAMP-PKA pathway and the LaeA and VeA protein complex have been determined [19,[23][24][25].…”

mentioning

confidence: 99%

A PKS gene, pks-1, is involved in chaetoglobosin biosynthesis, pigmentation and sporulation in Chaetomium globosum

Hao

Lou

et al. 2012

Sci. China Life Sci.

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Chaetomium globosum is one of the most common fungi in nature. It is best known for producing chaetoglobosins; however, the molecular basis of chaetoglobosin biosynthesis is poorly understood in this fungus. In this study, we utilized RNA interference (RNAi) to characterize a polyketide synthase gene, pks-1, in C. globosum that is involved in the production of chaetoglobosin A. When pks-1 was knocked down by RNAi, the production of chaetoglobosin A dramatically decreased. Knock-down mutants also displayed a pigment-deficient phenotype. These results suggest that the two polyketides, melanin and chaetoglobosin, are likely to share common biosynthetic steps. Most importantly, we found that pks-1 also plays a critical role in sporulation. The silenced mutants of pks-1 lost the ability to produce spores. We propose that polyketides may modulate cellular development via an unidentified action. We also suggest that C. globosum pks-1 is unique because of its triple role in melanin formation, chaetoglobosin biosynthesis and sporulation. This work may shed light on chaetoglobosin biosynthesis and indicates a relationship between secondary metabolism and fungal morphogenesis.

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“…1) [21]. This organization is almost identical to several other PKSs for the biosynthesis of reduced polyketides, such as LDKS and LNKS for lovastatin in A. terreus [15] and PKS1 for T-toxins in Cochliobolus heterostrophus [32], although the polyketide chain-length of fumonisins, lovastatin, and T-toxins is substantially different from each other. The objectives of this study were to test whether a heterologous PKS is functionally interchangeable with FUM1 in F. verticillioides and whether such a swapping would result in polyketide products with an altered chain-length.…”

Section: Introductionmentioning

confidence: 73%

“…In experiments using PCR to quickly screen putative mutants, genomic DNA was mini-prepared from the mutants by using UltraClean TM Microbial DNA Isolation Kit (Mo Bio, Fig. 3d, f) was amplifi ed by PCR using primers tKS-F/tKS-R (Table 1) with C. heterostrophus clone pF5P1 [32] as template. The probe t1 (703 bp) and t2 (681 bp) in Fig.…”

Section: Preparation and Analysis Of Nucleic Acidsmentioning

confidence: 99%

Functional replacement of the ketosynthase domain of FUM1 for the biosynthesis of fumonisins, a group of fungal reduced polyketides

Zhu

Bojja

et al. 2006

J IND MICROBIOL BIOTECHNOL

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Functional replacement of the ketosynthase domain of FUM1 for the biosynthesis of fumonisins, a group of fungal reduced polyketides" (2006). Liangcheng Du Publications. 5. http://digitalcommons.unl.edu/chemistrydu/5Abstract: The genetic manipulation of the biosynthesis of fungal reduced polyketides has been challenging due to the lack of knowledge on the biosynthetic mechanism, the diffi culties in the detection of the acyclic, non-aromatic metabolites, and the complexity in genetically manipulating fi lamentous fungi. Fumonisins are a group of economically important mycotoxins that contaminate maize-based food and feed products worldwide. Fumonisins contain a linear dimethylated C 18 chain that is synthesized by Fum1p, which is a single module polyketide synthase (PKS). Using a genetic system that allows the specifi c manipulation of PKS domains in fi lamentous fungus Fusarium verticillioides, we replaced the KS domain of fumonisin FUM1 with the KS domain of T-toxin PKS1 from Cochliobolus heterostrophus. Although PKS1 synthesizes different polyketides, the F. verticillioides strain carrying the chimeric PKS produced fumonisins. This represents the fi rst successful domain swapping in PKSs for fungal reduced polyketides and suggests that KS domain alone may not be suffi cient to control the product's structure. To further test if the whole fumonisin PKS could be functionally replaced by a PKS that has a similar domain architecture, we replaced entire FUM1 with PKS1. This strain did not produce any fumonisin or new metabolites, suggesting that the intrinsic interactions between the intact PKS and downstream enzymes in the biosynthetic pathway may play a role in the control of fungal reduced polyketides.

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A polyketide synthase is required for fungal virulence and production of the polyketide T-toxin.

Cited by 178 publications

References 40 publications

Cochliobolus heterostrophus T-toxin gene expression modulation via G protein and MAPK pathways

Cochliobolus heterostrophus T-toxin gene expression modulation via G protein and MAPK pathways

A PKS gene, pks-1, is involved in chaetoglobosin biosynthesis, pigmentation and sporulation in Chaetomium globosum

Functional replacement of the ketosynthase domain of FUM1 for the biosynthesis of fumonisins, a group of fungal reduced polyketides

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