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Previous Article | Next Article 
Applied and Environmental Microbiology, January 2001, p. 75-81, Vol. 67, No. 1
Department of Plant Pathology, University of
Nebraska, Lincoln, Nebraska 68583
Received 11 February 2000/Accepted 4 October 2000
Sclerotinia sclerotiorum acidifies its ambient
environment by producing oxalic acid. This production of oxalic acid
during plant infection has been implicated as a primary determinant of pathogenicity in this and other phytopathogenic fungi. We found that
ambient pH conditions affect multiple processes in S. sclerotiorum. Exposure to increasing alkaline ambient pH
increased the oxalic acid accumulation independent of carbon source,
sclerotial development was favored by acidic ambient pH conditions but
inhibited by neutral ambient pH, and transcripts encoding the
endopolygalacturonase gene pg1 accumulated maximally under
acidic culture conditions. We cloned a putative transcription
factor-encoding gene, pac1, that may participate in a
molecular signaling pathway for regulating gene expression in response
to ambient pH. The three zinc finger domains of the predicted Pac1
protein are similar in sequence and organization to the zinc finger
domains of the A. nidulans pH-responsive transcription
factor PacC. The promoter of pac1 contains eight PacC
consensus binding sites, suggesting that this gene, like its homologs,
is autoregulated. Consistent with this suggestion, the accumulation of
pac1 transcripts paralleled increases in ambient pH. Pac1
was determined to be a functional homolog of PacC by complementation of
an A. nidulans pacC-null strain with pac1. Our
results suggest that ambient pH is a regulatory cue for processes
linked to pathogenicity, development, and virulence and that these
processes may be under the molecular regulation of a conserved
pH-dependent signaling pathway analogous to that in the nonpathogenic
fungus A. nidulans.
Sclerotinia sclerotiorum
is a filamentous ascomycete phytopathogen that produces oxalic acid
during growth in vitro and in planta. Mutants deficient in the ability
to produce oxalic acid are nonpathogenic and fail to produce sclerotia
(14). Multiple synergistic roles have been proposed for
oxalic acid during pathogenesis (29, 32). During plant
infection, the secretion of oxalic acid creates an acidic pH
environment necessary for the activities of many hydrolytic enzymes
(3), including polygalacturonases (24).
Polygalacturonase enzymes have been implicated as colonization and
virulence factors in other plant-infecting fungi (44, 49). Furthermore, oxalic acid chelates calcium, resulting in a
destabilization of pectate polymers allowing increased access and
sensitivity to pathogen-produced pectolytic enzymes (32).
Oxalic acid also suppresses the plant oxidative burst (5)
and inhibits the activities of plant-produced polyphenol oxidase
(27, 29), suggesting that oxalic acid plays more subtle
roles in pathogenesis as well.
Secretion of oxalic acid by S. sclerotiorum results in the
acidification of the growth environment. The pH of in vitro-grown liquid cultures and infected host tissues can be as low as 2 and 4, respectively (29, 32). Numerous carbon sources, including components of plant cell walls, can support oxalic acid accumulation when provided as the sole carbon source (30, 32, 51).
Culture pH also is a strong regulator of oxalic acid biosynthesis
(32, 51). Oxalic acid production increases with the
ambient pH of the growth medium, as does oxaloacetase activity, the
enzyme proposed to catalyze oxalic acid production by hydrolysis of
oxaloacetate (31). Since S. sclerotiorum
acidifies the extracellular environment and yet cytosolic pH is assumed
to remain relatively stable, any effects of external pH change on
intracellular enzyme activities should be transient. These findings
suggest that a signaling pathway responsive to external pH conditions
regulates the expression of a gene(s) for oxalic acid biosynthesis.
In Aspergillus nidulans, an ambient pH-sensing signal
transduction pathway affects expression of genes encoding several
secreted and outer membrane bound proteins, as well as enzymes that
synthesize metabolites destined for export (4, 8, 9, 26, 43, 50). The gene product of pacC is the terminal
component of the pH signaling pathway and the regulator of pH-dependent
gene expression (4). This protein has a zinc finger
DNA-binding domain with a core DNA consensus binding site of
5'-GCCARG-3' (50). pacCc
mutations result in constitutive activation of the pH-responsive gene
expression pathway and mimic gene expression patterns observed in the
wild type under alkaline growth conditions (4).
pacC-null mutations result in severe defects in growth and
conidiation, and gene expression is similar to that observed in the
wild type at acidic pH (50).
Our objectives in this study were (i) to determine if ambient pH was a
major regulator of oxalic acid biosynthesis and sclerotial development.
(ii) to identify ambient pH-responsive gene expression, and (iii) to
determine if a homolog of the ambient pH transcriptional regulator
pacC was present in S. sclerotiorum. We
hypothesize that ambient pH is a signal for the transcriptional
regulation of genes necessary for the disease process and developmental
life cycle of this organism. We found that diverse processes in
S. sclerotiorum are influenced by ambient pH and that
pac1 is a functional homolog of the pacC
pH-responsive transcription factor. Our results suggest that
pH-responsive gene regulation plays a role in S. sclerotiorum pathogenicity and development.
S. sclerotiorum growth conditions.
We utilized
wild-type S. sclerotiorum isolate 1980 obtained from J. R. Steadman at the University of Nebraska-Lincoln. This isolate was
originally obtained from dry bean culls in western Nebraska
(14) and was routinely cultured on potato dextrose agar
(PDA; Difco, Detroit, Mich.). To analyze the effects of ambient pH and
carbon source on oxalic acid accumulation, we inoculated 500 ml of YPSu
medium (containing, per liter, 4 g of yeast extract [Difco],
15 g of sucrose, 1 g of K2HPO4, and
0.5 g of MgSO4) in a 1-liter flask with 20 ~5-mm3 agar-mycelium plugs of S. sclerotiorum
obtained from the advancing margin of a PDA culture. This liquid
culture was incubated at room temperature, with shaking at 150 rpm, for
5 days and then blended in a Waring blender and incubated for an
additional 24 h. The entire culture was harvested by vacuum
filtration onto filter paper and washed three times by resuspension in
600 ml of distilled water. Then, 10-ml aliquots of the washed mycelia (average mycelial wet weight, 200 mg) were harvested by vacuum filtration and resuspended in 50 ml of fresh medium containing, per
liter, 4 g of yeast extract, 1 g of
K2HPO4, 0.5 g of MgSO4, 0.5 M
3-(N-morpholino)propanesulfonic acid (MOPS) buffer, and either one of four carbon sources
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.1.75-81.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
pH Signaling in Sclerotinia
sclerotiorum: Identification of a pacC/RIM1 Homolog
and
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
sucrose (7.5 g), glucose (15 g),
mannitol (15 g), or soluble starch (15 g)or no carbon. Preliminary results indicated that the need for greatest control of pH would be at
pH 7; therefore, although MOPS provides little buffering capacity below
pH 7, it was used for all pH treatments to control for buffer effects.
Nine flasks were inoculated for each carbon source, three each with
initial pH values of 3.0, 5.0, or 7.0. These cultures were incubated
for an additional 24 h. These secondary cultures were harvested by
vacuum filtration, and supernatants were saved for oxalic acid quantification.
Oxalic acid quantification. Supernatants from cultures grown on different carbon sources and at various pH levels were analyzed for oxalic acid content with an enzymatic assay kit (Sigma, St. Louis, Mo.) according to the manufacturer's instructions. The oxalic acid concentration was calculated by extrapolation from a standard curve and adjusted for the dilution factors. Values represent the mean and standard deviation of three replications and are adjusted by subtraction of background obtained by incubating in buffer alone at the three different pH values.
Library construction and pac1 cloning. A 145-bp sequence from the A. nidulans pacC gene was obtained by PCR amplification of A. nidulans genomic DNA with forward primer 5'-AACCTCAACCTGAACTTGTCAATGGG-3' and reverse primer 5'-AAATCCTGGGGACGCTT GAA-3' followed TOPO TA Cloning into pCRII (Invitrogen, Carlsbad, Calif.) to generate pCRPacC. Total genomic DNA was isolated from the mycelia of S. sclerotiorum using the protocol of Panaccione et al. (35). Southern hybridization of S. sclerotiorum DNA digested with PstI and fractionated on a 0.8% agarose gel was carried out by standard protocols (2) using a 32P-labeled probe prepared by PCR labeling (33) of the pCRPacC insert. Low-stringency hybridization was performed in 1% bovine serum albumin (BSA), 1 mM EDTA, 0.5 M NaHPO4, and 7% sodium dodecyl sulfate (SDS) at 55°C, followed by two room temperature washes and two 55°C washes in 0.5% BSA, 1 mM EDTA, 40 mM NaHPO4, and 5% SDS.
We constructed a library from total genomic DNA of S. sclerotiorum isolate 1980 by ligating partially Sau3AI-digested, size-selected- (14 to 23-kb) DNA fragments into the BamHI site of the
replacement vector EMBL3
(Promega, Madison, Wis.). This library was plated and screened using
standard protocols (2) under the same conditions and with
the same 32P-labeled pacC probe as those
described above for the Southern hybridization. Positive plaques were
identified by autoradiography and purified by three successive rounds
of screening. Sequences hybridizing to the pacC probe were
localized to a 9.5-kb PstI fragment on clone PacS7.2 and
to a 6.7-kb XbaI fragment on clone PacS4.2. These
fragments were cloned into the pBluescript II KS(
) vector
(Stratagene, La Jolla, Calif.) and were designated pBSPacS7.2 and
pBSPacS4.2, respectively. The pacC-related sequence was
further localized to a 543-bp HindIII-Sau3AI
fragment on pBSPacS7.2, and a subclone, pBSPacS7.2HS, containing this
fragment was made.
We prepared a cDNA library in the ZipLox vector (Gibco-BRL,
Rockville, Md.) with a SuperScript cloning System (Gibco-BRL) from
poly (A)+ RNA obtained from developing sclerotia of
S. sclerotiorum isolate 1980. S. sclerotiorum was
cultured on PDA medium in 9-cm-diameter petri plates by inoculating a
single mycelium-agar plug onto the center of each plate. After 4 days
of growth at room temperature, nonmelanized, developing sclerotia with
liquid exudate on the surface were harvested with forceps, frozen in
liquid nitrogen, and stored at 80°C. These immature sclerotia were
frozen in liquid nitrogen and ground to a fine powder with a mortar and
pestle. Total RNA was isolated with Trizol reagent (Gibco-BRL)
according to the manufacturer's instructions. Poly(A)+ RNA
was purified with a Dynabead mRNA detection kit (Dynal, Oslo, Norway)
according to the manufacturer's instructions. This
poly(A)+ RNA was used to construct a unidirectional cDNA
library. This library was screened with the pacC-hybridizing
HindIII-Sau3AI fragment from pBSPacS7.2HS
according to standard protocols (2).
Hybridization was done in 1% BSA, 1 mM EDTA, 0.5 M NaHPO4,
and 7% SDS at 65°C, followed by a 10-min room temperature wash in
0.5% BSA, 1 mM EDTA, 40 mM NaHPO4, and 5% SDS and then
three 10-min washes, the first at room temperature and the last two at
65°C, in 1 mM EDTA, 40 mM NaHPO4, and 1% SDS. cDNA
clones were recovered as autonomously replicating pZL plasmids by using
the in vivo excision protocol supplied with the cloning kit
(Gibco-BRL). One of these clones with a 2.4-kb insert, designated
pZLPacS1, was chosen for further analysis.
pac1 sequence analysis. Plasmids pBSPacS4.2 and pZLPacS1, containing the genomic and cDNA sequences of pac1, respectively, were used as DNA sequencing templates. Both strands of each insert were sequenced using universal, reverse, and custom-made oligonucleotide primers (DNA Sequencing Core Research Facility, University of Nebraska-Lincoln). Sequence contigs were assembled and analyzed with DNASIS (Hitachi Software Engineering Co., Yokohama, Japan). Homology searches were conducted with the BLAST algorithm (1). Multiple amino acid sequence alignment with S. sclerotiorum Pac1 (accession no. AY005467), A. niger PacC (accession no. X98417), A. nidulans PacC (accession no. Z47081), Penicillium chrysogenum PacC (accession no. U44726), Yarrowia lipolytica YIRIM101 (accession no. X99616), Candida albicans HRM101 (accession no. AF173841), and Saccharomyces cerevisiae RIM1 (accession no. X72960) were conducted with the Wisconsin Sequence Analysis Program 9.1 (Genetics Computer Group, Madison, Wis.). Shading of conserved residues on the multiple amino acid sequence analysis output was conducted with MacBoxShade v2.01 (http://ulrec3.unil.ch/software/BOX_form.html).
Northern analysis. Primary cultures were grown and harvested as described above for experiments to determine the effect of ambient pH on sclerotial development. For ambient pH series experiments, harvested cultures were transferred to fresh YPSu medium buffered with citric acid-sodium phosphate buffer to achieve initial pH values between 3.0 and 7.0; the actual initial pH value for each culture was determined after autoclaving. These secondary cultures were incubated for 6 h, harvested by vacuum filtration, and quick frozen in liquid nitrogen. For expression kinetics experiments, primary cultures were incubated for 0, 10, and 30 min and for 1, 2, 3, 4, 5, and 6 h in YPSu medium buffered with citric acid-sodium phosphate buffer at pH 7.9. Total RNA was prepared with Trizol reagent as described above. For Northern blot analysis, 15 µg of RNA and RNA size standards was electrophoresed in a 0.8% agarose-0.66 M formaldehyde gel and transferred to MagnaGraph nylon membranes (Micron Separations, Inc., Westborough, Mass.) according to standard protocols (2). Hybridization probes were generated by 32P-random primer labeling (11). The sequences used as hybridization probes were the pac1 cDNA sequence from pZLPacS1; the endopolygalacturonase-encoding pg1 coding sequence (39), obtained by PCR amplification of S. sclerotiorum DNA with primers derived from the published sequence (39) and subsequent TOPO TA cloning into the pCRII vector (Invitrogen); and the rDNA repeat sequence from Neurospora crassa from pMF2 (13). Hybridization and washing conditions were the same as for cDNA library screening. The washed blots were autoradiographed and exposed to a phosphor screen that was scanned by a PhosphorImager (Molecular Dynamics, Sunnyvale, Calif.). Hybridization signals were quantified using ImageQuant software (Molecular Dynamics), and the reported relative level of signal in each lane was corrected based on the hybridization signal from the rDNA probe. All pH-transfer experiments and Northern blots were conducted a minimum of three times.
A. nidulans strains and transformation. A. nidulans strain RDP2 (pabaA1 argB2 pacC veA1) (37) carrying the null pacC allele (50) was provided by Nancy Keller. This strain was transformed with the argB-containing plasmid pPK1 (53) and pPKPacS, created by ligating a 5.9-kb XbaI-XhoI fragment from pBSPacS4.2 containing the pac1 coding sequence plus 3.3 kb of the upstream sequence and 666 bp of the downstream sequence into pPK1. To obtain RDP2 protoplasts, the strain was cultured on solid pH 4-buffered minimal medium (7) supplemented with 200 mg of L-arginine hydrochloride, 85 µg of p-aminobenzoate (PABA), and 5 g of yeast extract (Difco) per liter. Conidia were collected from the surface of plates by scraping into sterile water. Conidia and hyphae collected from all 10 plates were inoculated into 400 ml of liquid, pH 4-buffered minimal medium (7), supplemented as necessary, and incubated at 37°C and at 150 rpm for 16 h. Protoplasts were prepared and transformed essentially as described by Yelton et al. (55). Transformants were selected on solid, pH 4-buffered minimal medium containing 1.2 M sorbitol and 85 µg of PABA per liter. Transformants were evaluated for rate of growth, conidiation, and morphology on pH 4- and pH 8-buffered minimal medium supplemented with PABA. Photomicrographs of conidiophores were taken on a Zeiss (Jena, Germany) Axioskop compound light microscope with differential interference contrast optics. Comparisons were made between strains RKS1 (pabaA1 yA2 veA1), containing the wild-type pacC allele, and the recipient strain RDP2, RDP2 transformed with pPK1, and RDP2 transformed with pPKPacS.
Nucleotide sequence number. The pac1 genomic sequence has been deposited in the GenBank, EMBL, and DDBJ DNA data banks under accession no. AY005467.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Ambient pH and carbon source regulation of oxalic acid
accumulation.
Total oxalic acid accumulation in media buffered at
an initial pH of 7.0 ranged from an average of 1,500 mg of oxalic acid per liter of culture supernatant with glucose, sucrose, and starch as
the carbon source to 150 mg of oxalic acid per liter of culture supernatant in media with mannitol as the carbon source (Table 1). When oxalic acid levels in media were
compared at three different initial pH values, pH 3, 5, and 7, the
highest levels of oxalic acid were observed at pH 7, with lower levels
at pH 5 and the lowest levels at pH 3 (Table 1). If the initial culture
pH was 5 or 3, then no difference in oxalic acid accumulation between mannitol media and media prepared from other carbon sources was observed.
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Ambient pH and sclerotial development.
Sclerotia do not
develop from mycelia in liquid submerged culture but do develop
synchronously when mycelia are transferred to aerial conditions. After
transfer to conditions conducive for sclerotial development at pH 5, sclerotial initials were evident by 24 h, melanized sclerotia were
evident by 48 h, and nearly mature sclerotia were evident by 4 days (Fig. 1). In contrast, sclerotial
initiation and development were almost completely inhibited under the
same conditions when the pH was held constant at pH 7 for 4 days (Fig.
1). This pH effect on sclerotial development was independent of
nutrient requirements since sclerotia developed normally and with the
same kinetics when YPSu medium buffered at pH 5 was used and since
development was inhibited in buffered YPSu medium at pH 7 (data not
shown). In these same YPSu cultures 24 h after transfer to
sclerotium-inducing conditions, nearly five times as much oxalic acid
(1,600 ± 30 mg/liter) accumulates at pH 7 relative to pH 5 (330 ± 45 mg/liter).
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pg1 expression.
The influence of ambient culture
pH on the accumulation of transcripts encoding the
endopolygalacturonase enzyme PG1 was examined by Northern blot
analysis. Mycelia were transferred from primary cultures with an
average pH of 3.2 to fresh cultures with a series of pH values from 3.0 to 7.4. pg1 expression decreases as ambient pH increases
(Fig. 2A). Transcript levels of
pg1 were highest between pH 3.0 and 3.8 and decreased
dramatically at pH 4.2 and above (Fig. 2A).
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Isolation and characterization of a pacC homolog.
We probed a Southern blot of restriction enzyme-digested S. sclerotiorum genomic DNA at low stringency with a fragment of the
pacC gene and observed a single, weakly hybridizing band. From the S. sclerotiorum genomic library in EMBL3, we
identified six hybridizing clones. We localized the
pacC-related sequences to an approximately 6.7-kb
XbaI fragment from clone PacS4.2. This fragment was
subcloned into pBluescript II KS() to create pBSPacS4.2.
ZipLox
library that we had constructed from S. sclerotiorum cDNA. The largest insert size, 2.4 kb, was present in three of these clones.
We sequenced one of these cDNA clones designated pZLPacS1. We
identified a single open reading frame of 1,878 bp, predicted to encode
a 626-amino-acid, 68-kDa protein (GenBank accession no. AY005467). This
predicted protein shares high sequence similarity with the PacC/RIM1
family of transcription factors which have been identified from
A. nidulans (50), A. niger
(25), P. chrysogenum (47),
S. cerevisae (46), Y. lipolytica
(20), and C. albicans (38). Over
its entire sequence, the predicted peptide shares greatest identity
(44%) and similarity (51%) to the A. nidulans and A. niger PacC peptides. We refer to this gene as pac1 and
the encoded peptide as Pac1.
Several of the sequence features described for the A. nidulans PacC peptide (50) are conserved in Pac1.
These include a tyrosine-rich region and two proline-glycine-rich
regions downstream of the zinc finger. Additionally, the
carboxy-terminal half of Pac1 is serine- and threonine-rich, and the
S/TPXX motif that is frequently found in transcription factors
(48), including PacC (50), occurs 13 times in
Pac1. Two putative nuclear localization signals (NLS) were identified
in the Pac1 sequence using PSORT II (34). The first,
KRNFDNLNDFFAGAAKRR, begins at residue 236 and fits the
pattern of a bipartite NLS (40). These Pac1 residues align
with a putative bipartite NLS in the PacC homologs (data not shown). A
second potential NLS of the SV40 large T antigen type (16)
was identified, PRRR, beginning at residue 475.
The amino terminus of Pac1, comprising 44 residues upstream of the zinc
finger domain, is glutamine-rich (11 of 44 residues), including a
stretch of six contiguous glutamine residues, serine-rich (10 of 44 residues), and threonine-rich (6 of 44 residues) but, in contrast to
the N termini of the aspergilli and Penicillium PacC
homologs, is not particularly alanine-rich (4 of 44 residues in Pac1).
The most highly conserved sequence feature among the PacC/RIM1 homologs
is the zinc finger region. Pac1 contains three
Cys2His2 zinc finger domains designated Zf1,
Zf2, and Zf3 (Fig. 3). The Cys-Cys and
His-His spacing (Zf1: C4C, H4H; Zf2: C4C, H3H; and Zf3: C2C, H3H)
present in the other homologs is conserved in Pac1. The greatest
sequence conservation is observed in Zf3, in which Pac1 Zf3 contains
one conservative substitution, Glu (E) for Asp (D) at position c2
(following the conventional notation established by Jacobs
[17]), relative to Zf3, c2 residues in aspergilli, and
Penicillium PacC homologs. Compared to Zf2 of the aspergilli PacC peptides, Pac1 Zf2 contains two nonconservative amino acid substitutions: Gly (G) for Gln (Q) at position c2 and Asn (N) for Gly
(G) at position c4. The amino acid substitutions observed in Zf2 and
Zf3 of Pac1 relative to PacC are in the predicted b2 strand and not in
residues of the alpha helix involved with specific DNA base recognition
by PacC (10). Among the zinc fingers of all the PacC/RIM1
homologs, the weakest sequence conservation is within Zf1. In the Pac1
Zf1, there are four conservative and six nonconservative substitutions
relative to the Zf1 of A. nidulans PacC. However, a pair of
Trp (W) residues that are thought to be necessary for Zf1-Zf2
interaction are conserved at the c3 position within the Cys knuckles of
Zf1 and Zf2.
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339 and 599 bases
upstream of the ATG start codon. Seven of the eight copies were found
in the plus orientation, and all conformed to the more strictly defined
consensus of 5'-GCCAAG-3'.
Effect of ambient pH on pac1 expression. Primary mycelial cultures, average pH 3.2, were transferred to fresh medium buffered with citrate phosphate buffer to maintain a pH between 3.0 and 7.4. After a 6-h incubation, cultures were harvested and examined by Northern analysis (Fig. 2A). The pac1 gene hybridizes with a single mRNA transcript of approximately 2.4 kb. The steady-state levels of pac1 are influenced by and increase with ambient pH. The difference between pac1 transcript accumulations at pH 3.0 and at pH 7.4 is approximately 300-fold. pac1 transcripts accumulate following transfer from acidic (pH 3.0) to alkaline (pH 7.9) growth conditions. pac1 transcripts are barely detectable in total RNA from primary cultures (Fig 2B, time zero), but after 10 min at pH 7.9 the pac1 transcripts are easily detected (Fig. 2B). The steady-state level of pac1 transcripts increases under alkaline conditions, peaking at between 2 and 3 h after transfer with levels 12- to 13-fold higher than those found at the 10-min time point (Fig. 2B). By 6 h at alkaline pH, pac1 levels had dropped to approximately one-half of their maximal levels.
Complementation of a null pacC A. nidulans strain with
pac1.
We used vectors pPKPacS and pPK1 to
independently transform a null pacC argB A. nidulans strain (RDP2). Transformants were selected on pH4 minimal
medium, and argB+ prototrophs were retained for
further analysis. Several hundred pPKPacS and pPK1 transformants were
collected. All pPK1 transformants were arginine prototrophs but
otherwise retained RDP2 growth and conidiation phenotypes (Fig.
4). Single-spore strains of pPKPacS transformants all had the same phenotypes: arginine prototrophy and
wild-type growth and conidiation at both alkaline and acidic ambient pH
levels (Fig. 4).
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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S. sclerotiorum is a broad-host-range phytopathogenic fungus that produces oxalic acid in high concentrations, thus creating an acidic environment in which it grows and causes disease. The carbon source and the pH of the growth medium influence the accumulation of oxalic acid in culture. Previous studies on the effect of pH on oxalic acid production in Sclerotinia spp. have focused on single carbon sources (32, 51), and most studies of carbon source effects on oxalic acid accumulation do not examine a range of pH values (30, 36, 51). We grew S. sclerotiorum on various carbon sources that support different levels of oxalic acid accumulation at a neutral ambient pH and compared these levels with the levels of oxalic acid accumulation at lower pH. Carbon source plays a substantial role in the ability to synthesize oxalic acid, but an alkaline environment increases oxalic acid biosynthesis independent of carbon source. Determining the hierarchial positioning of carbon and ambient pH regulation of oxalic acid biosynthesis awaits the identification of molecular components of this pathway.
The synthesis of oxalic acid in S. sclerotiorum is proposed to be catalyzed by oxaloacetate acetylhydrolase. This enzyme activity increases as the pH of the ambient environment increases, paralleling oxalic acid accumulation (19, 21, 31, 42). A second enzymatic activity, oxalate decarboxylase, catalyzes the breakdown of oxalic acid. This enzyme activity is higher in mycelial extracts from cultures grown under acidic growth conditions (28). In Aspergillus spp., genes encoding enzymes in the penicillin, sterigmatocystin, and aflatoxin biosynthetic pathways are regulated by ambient pH (6, 18, 43). Based on these findings, a differential pH expression strategy would appear to be a plausible approach for cloning genes involved in oxalic acid biosynthesis and degradation from S. sclerotiorum.
Oxalic acid synthesis and degradation may be tightly regulated to provide an optimal pH environment for lytic enzyme activities. Numerous pectinolytic, proteolytic, cellulytic, and other hydrolytic enzymes from S. sclerotiorum with acidic pH optima have been described (15, 22, 23, 24). Our Northern analysis with the endopolygalacturonase-encoding gene pg1 demonstrate that ambient pH can also regulate enzyme levels through gene transcription. pg1 is a member of a multigene family whose members share a high degree (97 to 98%) of sequence identity (12). At least one member of this family displayed acidic pH-specific expression. Specifically determining which member(s) of this family was regulated by ambient pH was not possible with the probe we used. Whether genes encoding other lytic enzymes also are pH regulated has yet to be determined. In Colletotrichum gloeosporioides, endopolygalacturonase gene expression and pectate lyase gene transcription and enzyme secretion were recently demonstrated to be regulated by ambient pH (54). Transcriptional regulation of host-degrading enzymes by ambient pH also has been demonstrated in the entomopathogenic fungus Metarhizium anisopliae (45). In this fungus, the kinetics of extracellular protease and chitinase transcript accumulation is pH dependent, with expression patterns closely paralleling the pH optima of enzyme activities. Thus, a dynamic system of gene regulation based on ambient pH sensing and modification of the ambient pH environment may have a central role in determining the pathogenic success of fungal pathogens such as C. gloeosporioides, M. anisopliae, S. sclerotiorum, and possibly other phytopathogenic fungi.
In addition to its role in pathogenesis, environmental pH may regulate sclerotial development in S. sclerotiorum (51). Sclerotia are compact, melanized, multihyphal structures that can survive long periods of time under adverse environmental conditions and carpogenically germinate to produce apothecia and ascospores. These properties of sclerotia make them essential for the long-term survival and dissemination of Sclerotinia spp. In the present study we found that ambient pH affects sclerotial development. At a neutral or alkaline ambient pH, sclerotial development is inhibited. If ambient conditions are maintained at a neutral pH by buffering, this inhibition of sclerotial development occurs despite the accumulation of high concentrations of oxalic acid. Thus, under normal developmental conditions, it is the lowering of ambient pH due to oxalic acid accumulation, rather than oxalic acid accumulation per se, that appears to be the important regulator of sclerotial development.
The relationship between oxalic acid production and sclerotial development is likely more complex than that of pH alone. Sclerotial development in mutants that can neither synthesize oxalic acid nor develop sclerotia (14) is not restored by simply lowering ambient pH (unpublished observations). Furthermore, cyclic AMP (cAMP)-dependent signaling is known to regulate sclerotial development and oxalic acid biosynthesis in S. sclerotiorum (41), and the effects of high exogenous cAMP levels parallel the effects of elevated ambient pH reported here, i.e., increased oxalic acid production and inhibition of sclerotial development. We are interested in determining whether cAMP-dependent and pH-dependent signaling pathways are components of a common signaling circuit or whether they operate through independent pathways but regulate common components.
The finding that ambient pH plays a major regulatory role in oxalic acid biosynthesis, sclerotial development, and pg1 expression suggests that an ambient pH signal transduction pathway exists in S. sclerotiorum. Such a pathway has been characterized in A. nidulans, and several components of this pathway, including the pH-dependent transcriptional regulator pacC, have been cloned and characterized (50). pacC homologs also have been identified in closely related filamentous fungi (25, 47) and in yeasts (20, 38, 46, 52). The conservation of the zinc finger region among the various fungal homologs and the central role that PacC plays in mediating pH-dependent signaling made the pacC gene the first choice for determining if homologs of a pH-dependent signaling pathway existed in S. sclerotiorum. Pac1 shares the greatest amino acid sequence similarity (51%) with the aspergillus PacC proteins. The most convincing sequence characteristic suggesting that pac1 is a structural homolog of pacC is the existence of the three zinc finger domains that are 85 to 86% identical to the aspergillus PacC zinc finger domains. Furthermore, the spacing, number, and organization of these domains are conserved, and the sequences are 100% homologous for residues proposed to be involved in base specific contacts with the PacC consensus recognition sequences (10). Like pacC, pac1 displays pH-regulated expression with steady-state levels increasing as the pH of the growth medium is increased. Additionally, pacC consensus binding sites found 5' upstream of the pac1 coding sequence suggest that pac1 also is autogenously regulated. The eight perfect 5'-GCCAAG-3' hexamer sequence matches 340 to 600 bp upstream of the putative translational start site represent the largest number of consensus sequences upstream of any pacC homolog.
We showed that the pac1 gene product can serve as a functional homolog of the A. nidulans PacC protein by heterologous complementation of an A. nidulans pacC-null strain. Although sequence-specific DNA binding and regulation by proteolytic processing have not been demonstrated for Pac1, the ability to complement a pacC-null mutant demonstrates that pac1 and pacC are functional homologs and suggests that the pH-responsive pathway regulating pacC and pac1 in both A. nidulans and S. sclerotiorum will contain additional structurally and functionally homologous components.
Our results demonstrate that ambient pH is a major regulator of a pathogenicity determinant, oxalic acid; a possible virulence factor, pg1; and a process necessary for long-term survival, sclerotial development. At least one component of a conserved regulatory pathway mediating pH-regulated gene expression, Pac1, exists in this fungus. These findings suggest that S. sclerotiorum uses the ambient pH environment as a regulatory cue for disease and morphological development. Oxalic acid appears to play a central role in pH responsiveness. Its production is a pH-regulated process and, in turn, its accumulation, by virtue of environment acidification, may serve as a regulator of acid pH-regulated processes such as pg1 expression and sclerotial development. Interfering with ambient pH sensing and gene regulation may be viable strategies for blocking disease development in this broad-host-range plant pathogen.
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ACKNOWLEDGMENTS |
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This work was supported by in part by USDA/NRICGP grant 9802312 and by grant BARD 2473-94 from the United States-Israel Binational Agricultural Research and Development Fund.
We thank Young-Sil Ha for providing technical assistance and Nancy Keller, Robert Butchko, and David Piñero for providing A. nidulans strains, techniques, and helpful discussion during the course of this work.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Plant Pathology, 406 Plant Sciences Hall, University of Nebraska, Lincoln, NE 68583-0722. Phone: (402) 472-2849. Fax: (402) 472-2853. E-mail: mdickman{at}unlnotes.unl.edu.
Present address: Department of Plant Pathology, University of
Florida, Gainesville, FL 32611-0680.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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