Structure of the cutinase gene and detection of promoter activity in the 5'-flanking region by fungal transformation

Soliday, Charles L.; Dickman, Martin B.; Kolattukudy, Pappachan E.

doi:10.1128/jb.171.4.1942-1951.1989

Cited by 68 publications

(35 citation statements)

References 47 publications

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“…Comparison of Promoters of Cutinase Genes-The 5Ј-flanking region that is known to contain the promoter of cut1 (5,17) showed a high degree of identity with the corresponding segment of cut2 and cut3 (Fig. 2).…”

Section: Multiple Cutinase Genes and Identification Of Proteins Encodmentioning

confidence: 99%

“…1 filter and washed twice with 0.6 M MgCl 2 . Protoplast preparation and transformation were done as described (17). The transformed protoplasts were plated on mineral medium containing 2% glucose, 1.2 M sorbitol, and 2% agar.…”

Section: Test For Induction Of Gus Gene Fused To the Promoters Of Cutmentioning

confidence: 99%

“…An overlay of 1% agar containing hygromycin B (300 g/ml) (Calbiochem) was added after 24 h of incubation. Stable transformants were selected as before (17) and verified by PCR using primers designed to amplify the hygromycin gene portion or the gus gene:cut promoter junction portion of the construct. The primers used are as follows: hyg forward, 5Ј-GAA GAA TCT CGT GCT TTC AG-3Ј; hyg reverse, 5Ј-TAC TTC TAC ACA GCC ATC GG-3Ј; cut1 forward, 5Ј-GGG GGA TTC TCT TTC ATG TTT GCG G-3Ј; cut2 forward, 5Ј-GGG GGA TCC TCT TTC TTA TTG GGG G-3Ј; cut3 forward, 5Ј-GGG GGA TCC TCT TTC TTA TTT GCG G-3Ј; and gus reverse, 5Ј-GAT TTC ACG GGT TGG GGT TTC T-3Ј.…”

Section: Test For Induction Of Gus Gene Fused To the Promoters Of Cutmentioning

confidence: 99%

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Regulation of Constitutively Expressed and Induced Cutinase Genes by Different Zinc Finger Transcription Factors inFusarium solani f. sp. pisi(Nectria haematococca)

Sirakova

Rogers

et al. 2002

Journal of Biological Chemistry

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Cutin monomers, generated by the low levels of constitutively expressed cutinase, induce high levels of cutinase that can help pathogenic fungi to penetrate into the host through the cuticle whose major structural polymer is cutin. We cloned three highly homologous cutinase genes, cut1, cut2, and cut3, from Fusarium solani f. pisi (Nectria haematococca). Amino acid sequence deduced from the nucleotide sequence of cut1 and cut2/3 matched with that of the peptides from cutinase 1 and cutinase 2, respectively, isolated from F. solani pisi grown on cutin as the sole carbon source. Induction of ␤-glucuronidase gene fused to the promoters of the cutinases integrated into F. solani pisi genome indicates that cut2 is constitutively expressed and induced under starvation, whereas cut1 is highly induced by cutin monomers. A palindrome binding protein (PBP) previously cloned binds only to palindrome 1 of cut1 promoter but not palindrome 1 of cut2/3 which contains two base substitutions. PBP is thought to interfere with the binding of CTF1␣, the transcription factor involved in induction, to cut1 promoter and thus keep cut1 gene repressed until induced by cutin monomers. Because PBP cannot bind palindrome 1 of cut2, this gene is not repressed. CTF1␣ does not transactivate cut2 promoter. A new Cys 6 Zn 2 motif-containing transcription factor, CTF1␤, that binds palindrome 2 was cloned and sequenced. In yeast, CTF1␤ transactivates cut2 promoter but not cut1 promoter unless its palindrome 1 is mutated, unlike CTF1␣ which transactivates cut1. Thus, CTF1␤ is involved in the constitutive expression of cut2 that causes production of low levels of cutin monomers that strongly induce cut1 using CTF1␣ as the transcription factor.Fungal infection of plants can be assisted by extracellular cutinases that help the pathogen penetrate through the outermost cuticular barrier of the host (1, 2). Conidia of highly virulent pathogens, which can directly penetrate through the cuticle, have low levels of cutinase that release small amounts of cutin monomers when the conidia contact the host surface (3). These monomers transcriptionally activate the expression of an inducible cutinase gene that is responsible for the production of high levels of cutinase that assist the infection peg to gain entry into the host through the cuticle (4). A cis element essential for the inducible expression of cutinase gene was found to be located at Ϫ159 bp in the promoter of this gene (5) in Fusarium solani f. pisi (Nectria haematococca). In this region, two overlapping palindromes were found. Palindrome 2 was found to be necessary for the inducible cutinase gene expression (5). A protein that binds the palindromic region, called palindrome binding protein (PBP), 1 (6) and a cutinase transcription factor 1␣ (CTF1␣), which selectively binds palindrome 2 and transactivates the cutinase promoter (7), have been cloned. CTF1␣, a 101-kDa protein, contains a Cys 6 Zn 2 binuclear cluster motif, sharing homology to the Cys 6 Zn 2 binuclear cluster DNA-binding domains of tr...

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Section: Multiple Cutinase Genes and Identification Of Proteins Encodmentioning

confidence: 99%

Section: Test For Induction Of Gus Gene Fused To the Promoters Of Cutmentioning

confidence: 99%

Section: Test For Induction Of Gus Gene Fused To the Promoters Of Cutmentioning

confidence: 99%

See 1 more Smart Citation

Regulation of Constitutively Expressed and Induced Cutinase Genes by Different Zinc Finger Transcription Factors inFusarium solani f. sp. pisi(Nectria haematococca)

Sirakova

Rogers

et al. 2002

Journal of Biological Chemistry

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“…Protoplast preparation and transformation were performed as before (22). For the double disruptant, the pelA disruptant was transformed with the pelD disruption construct pPELD::zeo.…”

Section: Methodsmentioning

confidence: 99%

Requirement for either a host- or pectin-induced pectate lyase for infection of Pisum sativum by Nectria hematococca

Rogers

Kim

Guo

et al. 2000

Proc. Natl. Acad. Sci. U.S.A.

126

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Fungal pathogens usually have multiple genes that encode extracellular hydrolytic enzymes that may degrade the physical barriers in their hosts during the invasion process. Nectria hematococca, a plant pathogen, has two inducible pectate lyase (PL) genes (pel) encoding PL that can help degrade the carbohydrate barrier in the host. pelA is induced by pectin, whereas pelD is induced only in planta. We show that the disruption of either the pelA or pelD genes alone causes no detectable decrease in virulence. Disruption of both pelA and pelD drastically reduces virulence. Complementation of the double disruptant with pelD gene, or supplementation of the infection droplets of the double disruptant with either purified enzyme, PLA, or PLD, caused a recovery in virulence. These results show that PL is a virulence factor. Thus, we demonstrate that disruption of all functionally redundant genes is required to demonstrate the role of host barrier-degrading enzymes in pathogenesis and that dismissal of the role of such enzymes based on the effects of single-gene disruption may be premature.

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“…With fungal pathogens, only the genes for cutinase production (Dickman et al, 1989;Soliday et al, 1989) and pisatin demethylating ability (Weltring et al, 1988;Schafer et al, 1989) of Nectria haematococca MP VI and the b locus of Ustilago maydis (Kronstad and Leong, 1989;Schulz et al, 1990) have been isolated and characterized as putative pathogenesis determinants. The direct involvement of the b locus in the pathogenic development of U. maydis was unequivocally demonstrated by gene replacement (Kronstad and Leong, 1990).…”

Section: Introductionmentioning

confidence: 99%

Cutinase is not required for fungal pathogenicity on pea.

1992

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Cutinase, a fungal extracellular esterase, has been proposed to be crucial in the early events of plant infection by many pathogenic fungi. To test the long-standing hypothesis that cutinase of Nectria haematococca (Fusarium solani f sp piso is essential to pathogenicity, we constructed cutinase-deficient mutants by transformation-mediated gene disruption of the single cutinase gene of a highly virulent N. haematococca strain. Four independent mutants were obtained lacking a functional cutinase gene, as confirmed by gel blot analyses and enzyme assays. Bioassays of the cutinasedeficient strains showed no difference in pathogenicity and virulence on pea compared to the wild type and a control transformant. We conclude that the cutinase of N. haematococca is not essential for the infection of pea.

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Structure of the cutinase gene and detection of promoter activity in the 5'-flanking region by fungal transformation

Cited by 68 publications

References 47 publications

Regulation of Constitutively Expressed and Induced Cutinase Genes by Different Zinc Finger Transcription Factors inFusarium solani f. sp. pisi(Nectria haematococca)

Regulation of Constitutively Expressed and Induced Cutinase Genes by Different Zinc Finger Transcription Factors inFusarium solani f. sp. pisi(Nectria haematococca)

Requirement for either a host- or pectin-induced pectate lyase for infection of Pisum sativum by Nectria hematococca

Cutinase is not required for fungal pathogenicity on pea.

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