1 Institute of Biology, Leiden University, Clusius Laboratory, Fungal Genetics Research Group, Wassenaarseweg 64, 2333 AL, Leiden, The Netherlands
2 TNO-Nutrition, Applied Microbiology and Genetechnology, Utrechtseweg 48, 3500 AJ, Zeist, The Netherlands
3 Swammerdam Institute for Life Sciences-Microbiology, University of Amsterdam, Nieuwe Achtergracht 166, 1018 WV, Amsterdam, The Netherlands
Correspondence
Arthur F.J. Ram
ram{at}rulbim.leidenuniv.nl
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ABSTRACT |
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The GenBank/EMBL/DDBJ accession numbers for the sequences reported in this paper are AY594332 (AbGfaA), AY594333 (FoGfaA) and AY594334 (PcGfaA). Nucleotide sequence data reported are available in the Third Party Annotation Section (TPA) of the GenBank/EMBL/DDBJ database under accession numbers BK005223 (AnGfaA) and BK005224 (GzGfaA).
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INTRODUCTION |
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Chitin synthesis has also been shown to be essential in the compensatory response to cell wall stress in S. cerevisiae. Cell wall damage caused by mutations in cell wall-related genes results in hyperaccumulation of chitin (Ram et al., 1994, 1998
; Kapteyn et al., 1997
; Popolo et al., 1997
; Dallies et al., 1998
; Osmond et al., 1999
; Lagorce et al., 2002
). The hyperaccumulation of chitin in response to cell wall stress is not limited to S. cerevisiae and is also found in other yeasts such as Kluyveromyces lactis (Uccelletti et al., 2000
) and Candida albicans (Kapteyn et al., 2000
). Inability of the cells to respond to cell wall damage by increasing chitin levels, either by disrupting the major chitin synthase-encoding gene (ScChs3p) or by adding the chitin synthase inhibitor nikkomycin Z, results in cell lysis, indicating the importance of the chitin response to prevent cell death (Douglas et al., 1994
; el-Sherbeini & Clemas, 1995
; Popolo et al., 1997
).
The sugar donor for the synthesis of chitin is UDP-N-acetylglucosamine. The metabolic pathway leading to the formation of UDP-N-acetylglucosamine from fructose 6-phosphate consists of five steps. The first and also rate-limiting step in this pathway is the formation of glucosamine 6-phosphate from glutamine and fructose 6-phosphate. This step is catalysed by the enzyme glutamine-fructose-6-phosphate amidotransferase (Gfa1p). The hexosamine biosynthetic pathway from fructose 6-phosphate to UDP-N-acetylglucosamine is conserved in lower and higher eukaryotes, as well as in bacteria.
The glucosamine : fructose-6-phosphate amidotransferase-encoding gene has been cloned from bacteria, yeasts and higher eukaryotes. Expression analysis of GFA1 in S. cerevisiae has shown that its expression is strongly enhanced in response to cell wall stress-inducing conditions, both by using cell wall mutants (Lagorce et al., 2002; Terashima et al., 2000
) and in response to the cell wall-perturbing compounds Calcofluor White (CFW) and Zymolyase (Boorsma et al., 2004
; Garcia et al., 2004
), which indicates that increased chitin synthesis requires activation of the hexosamine biosynthetic pathway by increased expression of the rate-limiting step in the pathway.
In this paper, we describe the cloning of the complete gfaA-encoding gene from Aspergillus niger and of gfaA fragments from Penicillium chrysogenum and Fusarium oxysporum. Using these genes as probes, we have shown that these filamentous fungi respond to various cell wall-perturbing conditions by increasing the expression level of gfaA mRNA. We also show that higher gfaA mRNA levels in A. niger are accompanied by increased chitin levels in the cell wall after CFW-induced cell wall stress, presenting further evidence that activation of the chitin biosynthetic pathway is a general response to cell wall stress.
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METHODS |
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Cell wall stress-inducing conditions.
Freshly isolated conidia from A. niger were inoculated into 100 ml CM at a spore density of 1x107 conidia ml1 and grown for 5 h at 37 °C. After 5 h, CFW was added (200 µg ml1) from a freshly prepared stock solution (20 mg ml1). SDS was added from a 100 mg ml1 stock solution to a final concentration of 50 µg ml1. Caspofungin (Merck) was added from a 10 mg ml1 stock solution to a final concentration of 62·5 µg ml1. Freshly isolated P. chrysogenum conidia were used to inoculate 50 ml CM at a spore density of 1x107 conidia ml1 and grown for 6·5 h at 30 °C before adding CFW. F. oxysporum conidia were inoculated at a spore density of 1x106 spores ml1 and grown for 7 h at 30 °C before the addition of CFW. At specific time points after the addition of the antifungal compound, germlings were isolated using a gauze with a 20 µm aperture (Endecotts), frozen with liquid nitrogen and stored at 80 °C prior to isolation of cell walls or RNA. For microscopical studies, freshly harvested conidia were grown on coverslips in MM with Casamino acids at 37 °C with or without 10 mg glucosamine ml1. At specific time points, a coverslip with adherent conidia or germlings was fixed in 3·7 % (v/v) formaldehyde for 2030 min. The coverslip was removed from the fixation buffer and placed in 7 µl mounting solution [50 % (v/v) glycerol in PBS] on a microscope slide. After sealing the coverslip with nail polish, the morphology of the germlings was analysed by viewing at least 400 conidia or germlings. Microscopic images were taken on an Axioplan 2 (Zeiss) equipped with a DKC-5000 (Sony) digital photo camera using differential interference contrast settings.
Determination of chitin content in isolated cell walls.
Cell walls were isolated by grinding frozen mycelium using a pestle and mortar and rinsed three times with 1 M NaCl and three times with water. Cell walls were boiled in the presence of SDS, EDTA and -mercaptoethanol to extract non-covalently linked cell wall components and to remove cytosolic contaminants as described by Montijn et al. (1994)
. Chitin levels were determined as described by Tracey (1956)
. In brief, approximately 200 mg wet weight cell walls was freeze-dried and the dry weight was determined. Cell walls (approx. 15 mg dry wt) were subsequently hydrolysed in 6 M HCl at 100 °C for 4 h. The HCl was removed by evaporation using an air stream at 50 °C. Dried samples were resuspended in 1 ml water and centrifuged to remove insoluble material. To 0·1 ml sample, 0·1 ml solution A [1·5 N Na2CO3 in 4 % (w/v) acetylacetone] was added and the mixture was incubated at 100 °C for 20 min. After cooling to room temperature, 0·7 ml 96 % ethanol and 0·1 ml solution B (1·6 g p-dimethylaminobenzaldehyde in 30 ml concn HCl and 30 ml 96 % ethanol) was added and incubated for 1 h at room temperature. The absorbance at 520 nm was measured and compared to absorbance values from a standard curve of 0100 µg glucosamine taken through the same reactions (Tracey, 1956
; Popolo et al., 1997
).
DNA and RNA manipulations.
Fungal chromosomal DNA was isolated as described by Kolar et al. (1988). Southern blot analyses were done as described by Sambrook et al. (1989)
. [
-32P]dCTP-labelled probes were synthesized using the Rediprime II DNA labelling System (Amersham Pharmacia Biotech) according to the instructions of the manufacturer. RNA was extracted from mycelium, that had been flash-frozen in liquid nitrogen, using TRIzol reagent (InVitrogen). Total RNA (10 µg) was incubated with 3·3 µl 6 M glyoxal, 10 µl DMSO and 2 µl 0·1 M sodium phosphate buffer, pH 7·0, in a total volume of 20 µl for 1 h at 50 °C to denature the RNA. RNA glyoxal electrophoresis was performed in a SEA-2000 (Elchrom Scientific) at 10 °C.
PCR amplification of fungal gfaA fragments.
Sequence alignment of Gfa1p homologues from yeasts and several higher eukaryotic species, including human, mouse and Drosophila, revealed several conserved stretches of amino acids. These conserved sequences were used to design two pairs of degenerated primers, to amplify fragments of gfaA-encoding genes from P. chrysogenum, F. oxysporum and A. niger. Primer set 1, PgfaP1 for (5'-cgggatcccGARTAYMGNGGNTAYGA-3') and PgfaP2rev (5'-cggaattccgTGNGTNGCCAANCKNGT-3') (convenient restriction sites are underlined) was used for the isolation of gfa fragments from P. chrysogenum and F. oxysporum. An expected PCR fragment of about 180 bp was amplified from genomic DNA from both fungi, which was cloned in pGEM-T Easy and sequenced. Primer set 2, PgfaP3for (5'-cgggatcccCAYATHAAYGCNGGNCC-3') and PgfaP4rev (5'-cggaattccgCCYTGNARRCARTCNAC-3') was used to isolate the A. niger gfaA homologue from an A. niger cDNA library. An expected 550 bp PCR fragment was cloned in pGEM-T Easy and sequenced.
Cloning of the full-length A. niger gfaA gene.
To obtain the complete sequence of the A. niger gfaA gene and its promoter sequence, a cosmid library containing genomic inserts of A. niger DNA (kindly provided by Dr F. Schuren and Dr P Punt, TNO Nutrition, The Netherlands) was ordered into 384-well microtitre plates and colonies were spotted on LB plates. After transfer of the colonies to Hybond N+ filters, they were lysed using standard protocols (Sambrook et al., 1989). Out of approximately 5000 colonies screened, six hybridized with the gfaA PCR fragment. Two cosmid clones were isolated and analysed by subcloning, Southern blot analysis and sequence analysis. Only cosmid clone gfaA#5 contained the complete gfaA sequence. Two partially overlapping subclones, pPST-GFA#5 (an 8 kb PstI fragment cloned in pBluescript SK) and pBAMHI-GFA#5 (a 9 kb BamHI fragment cloned in pBluescript SK), were made and these were used to obtain the full-length A. niger gfaA sequence. Sequencing was carried out on a Perkin Elmer ABI PRISM 310 sequencer using the ABI PRISM Big Dye Terminator Cycle Sequencing Ready Reaction kit from Applied Biosystems. All primers used in this study were obtained from Isogen.
Disruption of the A. niger gfaA gene and complementation of the gfaA strain.
To construct the gfaA gene deletion plasmid, pBAMHI-GFA#5 was digested with NotI and XhoI. A 5·9 kb fragment, containing the last 800 nt of the gfaA-encoding sequence, the 3' terminator region (2·4 kb) and the pBluescript vector (2·7 kb), was isolated and used in a three-way ligation. The second fragment was obtained by digestion of pBAMHI-GFA#5 with NotI and BglII, and a 5·0 kb fragment containing the 5' promoter region of gfaA and the first 500 nt of the gfaA-encoding region was isolated. The NotI site is present in the polylinker of pBluescript. A 3·0 kb BamHISalI fragment containing the A. oryzae pyrG gene was obtained from pAO4-13 (de Ruiter-Jacobs et al., 1989). Ligation of the three fragments resulted in the disruption plasmid, p
gfaA. This plasmid was linearized with NotI and used to disrupt the gfaA gene.
Disruption of the gfaA gene in A. niger was confirmed by Southern blot analysis. Genomic DNA of putative gfaA strains and a wild-type strain was isolated and digested with PstI. DNA was separated on a 0·8 % agarose gel, blotted on Hybond N+ and hybridized with a gfaA probe. A 1·2 kb ClaIBglII fragment from pBAMHI-GFA#5 was used as a probe. Plasmid pBAMHI-GFA#5 was used for complementation studies.
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RESULTS |
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We further asked the question whether the induction of gfaA in response to CFW was limited to A. niger. Therefore, P. chrysogenum and F. oxysporum germlings were treated with CFW and RNA was isolated 1 h after CFW addition. Using the gfaA fragments of both P. chrysogenum (PcgfaA) and F. oxysporum (FogfaA), we observed that the levels of gfaA mRNA in these fungi were also increased upon CFW-induced cell wall stress (Fig. 4d and e). This indicates that the induction of gfaA and probably also an increased synthesis of chitin are a general compensatory mechanism to ensure cell wall integrity under cell wall stress conditions.
gfaA is essential for viability
To investigate the consequences of a loss of function of the gfaA gene in A. niger, a gene disruption vector (pgfaA) was constructed in which an internal part (1038 bp) of the gfaA coding region is replaced by the pyrG gene from A. oryzae (Fig. 5
a). An A. niger pyrG strain (AB4.1), was transformed with the
11 kb linear fragment of the disruption cassette. Transformants were selected on MM supplemented with 5 mg glucosamine ml1. In S. cerevisiae, GFA1 is an essential gene and mutants can be rescued by the addition of glucosamine to the medium (Watzele & Tanner, 1989
). From various transformation plates, 40 transformants were randomly picked and subjected to two rounds of purification. Next, the growth of the transformants was examined on plates with or without glucosamine to identify putative
gfaA strains, since these transformants were expected not to grow on plates without glucosamine (Fig. 5c
). Glucosamine-requiring transformants were identified and these were analysed further by Southern blot analysis, which proved that the expected deletion of the gfaA gene had occurred (Fig. 5b
). Whereas supplementation with 5 mg glucosamine ml1 restored growth (Fig. 5b
), supplementation with 1 mg glucosamine ml1 did not result in the formation of colonies (data not shown). We also observed that conidia from a
gfaA strain (obtained from a spore plate containing 10 mg glucosamine ml1) were as viable and able to germinate on a glucosamine-containing plate as the wild-type strain (data not shown). Next, we asked the question whether the addition of glucosamine could fully supplement the
gfaA strain. To determine this, a fixed number of conidia from a wild-type strain and the
gfaA strains were spotted in the centre of an agar plate containing different concentrations of glucosamine (5, 10 and 50 mg ml1) and the size of the colony was determined after a period of 7 days. At all glucosamine concentrations tested, the growth of a
gfaA strain was somewhat slower than the wild-type, resulting in a smaller colony size [5 mg ml1, 3·5±0·1 cm (
gfaA) vs 3·7±0·1 (wild-type); 10 mg ml1, 3·6±0·1 vs 4·0±0·1; 50 mg ml1, 4·7±0·1 vs 5·4±0·1 cm (mean±SD, n=2)] after 7 days of growth at 30 °C. We also observed that the
gfaA strain conidiates poorly on a plate containing 10 mg glucosamine ml1 (Fig. 5d
). This was most pronounced at the outer rim of the colony where hardly any conidiophores were formed. Most likely, the glucosamine in the plate is depleted after vegetative growth and the lack of glucosamine inhibits conidiation. Addition of more glucosamine to the plate (50 mg ml1) resulted in a less pronounced effect on conidiation (data not shown), indicating that lack of glucosamine was indeed causing this effect.
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Addition of high concentrations (50 mg ml1) glucosamine also did not restore wild-type morphology. However, the swelling of the gfaA deletion strain in presence of 50 mg glucosamine ml1 was less pronounced than at 10 mg glucosamine ml1 (data not shown). We also observed that in the presence of 10 mg glucosamine ml1, germination of swollen conidia started after 11 h of incubation whereas the presence of 50 mg glucosamine ml1 resulted in faster germination, already observed after 8 h of growth.
gfaA as a selection marker
The inability of the gfaA strain to grow on medium without glucosamine prompted us to investigate whether the
gfaA strain, in combination with the gfaA gene, could be used as a selection marker for fungal transformation. Therefore, subclone pBAMHI-GFA#5, which contains the complete gfaA ORF, including promoter and terminator regions, was transformed into the
gfaA strain. Protoplasts were obtained from the
gfaA strain which was pregrown in the presence of various concentrations of glucosamine (1, 2·5, 5, 10 and 50 mg ml1). All cultures gave similar amounts of biomass ranging from 2·7 to 3·5 g fresh weight per 250 ml CM, but the number of protoplasts decreased at the higher glucosamine concentrations, indicating that it is more difficult to produce protoplasts from
gfaA cultures after growing them at high concentrations of glucosamine. After transformation, the protoplasts were plated out on MM plates. Analysis of the transformation plates revealed some background growth on the negative control plates (no DNA added). However, no colonies were formed that were able to produce conidiophores. On the transformation plates on which protoplasts had been plated out that were transformed with the gfaA-containing plasmid, sporulating colonies were readily obtained after 5 days of growth against a background of non-sporulating mycelia. Further purification showed that the sporulating colonies had become glucosamine-prototrophic. Southern blot analysis of 16 randomly chosen transformants from different transformation plates revealed that the sporulating colonies contained the disrupted allele of the gfaA gene and a wild-type copy of the gfaA gene in their genome (data not shown).
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DISCUSSION |
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We have extended the finding in the yeast S. cerevisiae that cell wall weakening or cell wall stress activates a compensatory mechanism that includes the increased deposition of chitin in the cell wall to ensure cell wall integrity. We have shown that the addition of the cell wall-disturbing compound CFW to germlings of the filamentous fungus A. niger results in an increased level of cell wall chitin. Increased chitin synthesis also demands a higher flux through the hexosamine metabolic pathway to generate UDP-N-acetylglucosamine, the sugar donor for chitin biosynthesis. In S. cerevisiae, the higher flux is at least partially achieved by an increased expression of GFA1, encoding the glutamine : fructose-6-phosphate amidotransferase activity, which is the rate-limiting step in the pathway (Lagorce et al., 2002). In this paper, we show that in A. niger an increased chitin level in the cell wall in response to cell wall stress is also accompanied by increased transcription levels of gfaA, further indicating that both yeasts and filamentous fungi respond to cell wall stress by activating the chitin biosynthetic pathway. We have used the induction of gfaA to obtain evidence that this response is a general fungal mechanism to cope with cell wall stress, since a similar induction was observed in P. chrysogenum and F. oxysporum. Furthermore, we have shown that the induction of gfaA is activated not only by the addition of CFW, but also after adding SDS or caspofungin, a 1,3-
-glucan synthase inhibitor (Kartsonis et al., 2003
). Mutations that result in cell wall weakening in S. cerevisiae (e.g.
fks1,
knr4,
gas1,
kre6,
mmn9 and
och1) all display increased chitin levels in their cell wall, which is accompanied by higher GFA1 transcript levels and higher GFA activities (Lagorce et al., 2002
; Bulik et al., 2003
). This relationship between an increased level of chitin in the cell wall and a mutant in which cell wall biosynthesis is affected (RhoA) has recently also been found for A. nidulans (Guest et al., 2004
).
In S. cerevisiae, it is well established that increased chitin synthesis is carried out by only one of the three chitin synthase genes, namely CHS3. Deletion of CHS3 in combination with a mutation that affects cell wall biosynthesis results in a synthetic lethal phenotype (Popolo et al., 1997; Osmond et al., 1999
). It will be of interest to identify the chitin synthase gene in A. niger (and in other filamentous fungi) that is responsible for the increased chitin level. Chitin synthase genes have not yet been described in A. niger, but chitin synthesis has been studied in detail in both A. fumigatus and A. nidulans. The chitin synthase family in A. fumigatus consists of at least seven different CHS genes (AfChsAAfChsG) and six CHS genes have been identified in A. nidulans (AnChsA, B, C, E and AnCsmA/ChsD) (Mellado et al., 2003
and references therein). Disruption of AnCsmA resulted in a strain that is highly sensitive to CFW (Fujiwara et al., 1997
; Horiuchi et al., 1999
), which may suggest that this gene is involved in the induction of chitin synthesis in response to cell wall stress. CsmAp is a unique chitin synthase in which the chitin synthase domain is fused with a myosin tail and both domains are required for its function (Horiuchi et al., 1999
). Possibly, the function of the myosin domain in CsmAp is used to rapidly translocate the protein, using the actin cytoskeleton, to places that require additional chitin deposition in response to cell wall stress.
Although chitin levels in S. cerevisiae can increase dramatically under some cell wall stress-inducing conditions, transcription levels of CHS3 increase to a lesser extent (Lagorce et al., 2003). Chs3 protein levels have not been shown to vary significantly (Popolo et al., 1997
; Valdivieso et al., 2000
; Garcia-Rodriquez et al., 2000
), indicating that post-translational events are responsible for increasing Chs3 activity in response to cell wall stress. Indeed, such a mechanism to recruit Chs3p from internal stores (chitosomes) to the plasma membrane has recently been identified (Valdivia & Schekman, 2003
).
UDP-N-acetylglucosamine is incorporated into chitin, but the nucleotide sugar donor also serves as a donor for the biosynthesis of two essential modifications of secretory proteins: N-linked glycosylation and glycosylphosphatidylinositol anchor attachment. The lethality of gfaA is therefore not simply due to the inability to synthesize chitin, although it is generally assumed that also in filamentous fungi chitin biosynthesis is essential for viability. The majority of conidia (70 %) of the
gfaA strain do not swell in the absence of glucosamine. This indicates that most conidia contain only a relative small pool of UDP-N-acetylglucosamine or its precursors in the cell. The addition of glucosamine to the medium allows spore germination, indicating that glucosamine can be taken up by the cell and be converted, probably into glucosamine 6-phosphate, thereby circumventing the need for GfaAp. The finding that higher concentrations of glucosamine (50 mg ml1) accelerated spore germination compared to a lower concentration (10 mg ml1) suggests that the uptake of glucosamine is limiting at low glucosamine concentrations. It further suggests that the glucosamine is taken up by the fungus with a low affinity transport mechanism, but the mechanism by which glucosamine is taken up is not known.
Although most gfaA conidia do not swell in the absence of glucosamine, some conidia do swell and form large cells. The phenotype of those cells resembles the phenotype of A. niger conidia that germinate in the presence of tunicamycin (Katoh et al., 1976
). Tunicamycin inhibits the transfer of N-acetylglucosamine 1-phosphate from UDP-N-acetylglucosamine to dolicholmonophosphate (Tkacz & Lampen, 1975
; Takatsuki et al., 1975
) and thereby blocks N-linked protein glycosylation. Because of the similar phenotype of the
gfaA conidia and tunicamycin-treated conidia, one might suggest that the inability to form N-chains is the primary effect of the absence of UPD-N-acetylglucosamine in the
gfaA strain. Alternatively, tunicamycin is also known as an inducer of the Unfolded Protein Response (UPR) in A. niger (Mulder et al., 2004
). The presence of tunicamycin might therefore result in accumulation of cell wall-synthesizing enzymes in the ER which are normally transported to the cell surface via the secretory pathway, and thereby causing defects in cell wall biosynthesis.
Finally, we have shown that the A. niger gfaA gene, in combination with the A. niger gfaA strain, can be used as a selection marker and a similar approach seems feasible for other filamentous fungi.
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ACKNOWLEDGEMENTS |
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Received 16 April 2004;
revised 27 May 2004;
accepted 3 June 2004.
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