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Journal of Bacteriology, June 2001, p. 3268-3275, Vol. 183, No. 11
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.11.3268-3275.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Structural and Functional Analysis of the Phosphonoacetate
Hydrolase (phnA) Gene Region in Pseudomonas
fluorescens 23F
Anna N.
Kulakova,1,*
Leonid A.
Kulakov,1
Natalya V.
Akulenko,2
Vladimir N.
Ksenzenko,3
John T. G.
Hamilton,4 and
John P.
Quinn1
The Questor Centre, David Keir Building, The
Queen's University of Belfast, Belfast BT9 5AG, and School of Biology
and Biochemistry, Medical Biology Centre, The Queen's University of
Belfast, Belfast BT9 7BL, Northern Ireland1;
Skryabin Institute of Biochemistry and Physiology of
Microorganisms,2 and Institute of
Protein Research,3 Russian Academy of Sciences,
Pushchino, Moscow Region 142290, Russia; and Food Science
Division, Department of Agriculture for Northern Ireland, Newforge
Lane, Belfast BT9 5PX, Northern Ireland4
Received 11 December 2000/Accepted 7 March 2001
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ABSTRACT |
The Pseudomonas fluorescens 23F phosphonoacetate
hydrolase gene (phnA) encodes a novel carbon-phosphorus
bond cleavage enzyme whose expression is independent of the phosphate
status of the cell. Analysis of the regions adjacent to the
phosphonoacetate hydrolase structural gene (phnA)
indicated the presence of five open reading frames (ORFs). These
include one (phnR) whose putative product shows high
levels of homology to the LysR family of positive transcriptional
regulators. Its presence was shown to be necessary for induction of the
hydrolase activity. 2-Phosphonopropionate was found to be an inducer
(and poor substrate) for phosphonoacetate hydrolase. Unlike
phosphonoacetate, which is also an inducer of phosphonoacetate
hydrolase, entry of 2-phosphonopropionate into cells appeared to be
dependent on the presence of a gene (phnB) that lies
immediately downstream of phnA and whose putative
product shows homology to the glycerol-3-phosphate transporter. RNA
analysis revealed transcripts for the phnAB and
phnR operons, which are transcribed divergently;
the resulting mRNAs overlapped by 29 nucleotide bases at their 5' ends.
Transcripts of phnAB were detected only in cells grown
in the presence of phosphonoacetate, whereas transcripts of
phnR were observed in cells grown under both induced and
uninduced conditions. The expression of three additional genes found in
the phnA region did not appear necessary for the
degradation of phosphonoacetate and 2-phosphonopropionate by either
Pseudomonas putida or Escherichia coli cells.
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INTRODUCTION |
Organophosphonates are a group of
compounds of biogenic and xenobiotic origins that are characterized by
possession of a direct carbon-phosphorus bond. Two different routes of
C-P bond cleavage, each inducible only under conditions of phosphorus
limitation, have been demonstrated when such molecules serve as the
sole phosphorus source for microbial growth. "C-P lyase" is the
trivial name given to an enzyme complex which catalyzes the
cleavage of the C-P bond of both substituted and unsubstituted
phosphonates by a mechanism which may involve redox or radical
chemistry (27). By contrast, phosphonoacetaldehyde
hydrolase ("phosphonatase" [EC 3.11.1.1]) is active in
vitro and hydrolytically cleaves only the substituted C-P bond of
phosphonoacetaldehyde to yield acetaldehyde and
Pi (10). Since bacterial cleavage of
the C-P bond by both C-P lyase(s) and phosphonatase is under control of
the pho regulon (10) and hence occurs only
under conditions of Pi limitation,
organophosphonates generally fail to serve as sources of carbon for
microbial growth because the excess of Pi
released during the catabolism of their carbon skeletons serves to
repress and/or inhibit their further mineralization. Genetic analysis
of C-P bond cleavage by the C-P lyase and phosphonatase pathways has
been reported (10, 18, 26), and the phosphonatase gene of
Pseudomonas aeruginosa has been characterized
(5).
We have recently reported the purification (15) and
molecular cloning (14) of phosphonoacetate (PA) hydrolase
(EC 3.11.1.2), a novel C-P cleavage enzyme from Pseudomonas
fluorescens 23F which is able to mineralize PA with essentially
quantitative Pi release. Expression of the enzyme
is inducible in the presence of its apparently xenobiotic substrate PA
and is independent of the Pi status of the cell.
No mode of regulation had previously been described in which a
phosphorus-containing compound is needed for induction of a gene
required for its own utilization (27). To obtain a better
understanding of this unique biodegradation system we now report the
structural and functional analysis of those regions of the genome of
P. fluorescens 23F adjacent to the phnA gene and
address the function and regulation of the genes comprising the
phn operon.
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MATERIALS AND METHODS |
Bacterial strains and plasmids.
The PA-degrading strain
P. fluorescens 23F has been described (17).
Escherichia coli DH5
and Pseudomonas putida
AC577 trp leu (from A. M. Chakrabarty, University of
Illinois-Chicago, Chicago) were used for the analysis of cloned PA
degradation genes. Preliminary experiments showed that PA and
2-phosphonopropionate could serve as only poor sources of phosphorus
for P. putida AC577 without Pi
release. E. coli DH5 could use PA but not
2-phosphonopropionate as a source of phosphorus, also without
Pi release. Plasmid pRK2013 (7) was
used as a helper plasmid. Cosmid pLAFR5 (12) was used for
analysis of the expression of phn genes in E. coli and P. putida, and plasmid vectors pUC129
(12) and pUC18 were used for the analysis of the same
genes in E. coli only. Promoter probe vector pKK232-8
(Pharmacia) was used for the analysis of phnA gene expression.
Media and growth conditions.
Pseudomonas and
E. coli strains were propagated in a rich (2YT) medium
(19) solidified when required by addition of Difco agar
(1.8% [wt/vol]). For the growth and detection of recombinant plasmids, ampicillin (100 µg ml
1) or
tetracycline (15 µg ml1), IPTG
(isopropyl-
-D-thiogalactopyranoside) (50 µg
ml1), and X-Gal
(5-bromo-4-chloro-3-indolyl--D-galactopyranoside) (50 µg ml1) were used. Mineral salts medium
was free of phosphorus and contained (per liter): KCl, 0.24 g;
MgSO4 · 7H2O,
0.2 g; NH4Cl, 1.0 g;
CaCl2 · 2H2O, 1.0 mg; ferric ammonium citrate, 1.0 mg; HEPES buffer, 25 mM (pH 7.2); and
1 ml of trace element solution (13). Purified agar (1%)
(Oxoid, Basingstoke, United Kingdom) was added when appropriate. As a
source of carbon, sodium gluconate (2.0 g l1)
or sodium pyruvate (2.0 g l1) was used. As a
source of phosphorus, PA (2 mM), 2-phosphonopropionate (2PP) (2 mM), or
Pi (2 mM) was used. A number of phosphonates (2 mM) were also screened for their ability to serve as sources of
phosphorus. Medium for auxotrophic strains was supplemented with
appropriate amino acids (50 mg l1) and vitamins
(5 mg l1). Pseudomonas strains were
routinely grown at 29°C, and E. coli was grown at 37°C.
Bacterial crosses.
Recombinant plasmids constructed using
pLAFR5 were transferred into the P. putida AC577 recipient
strain using a three-factor mating procedure (4) with
pRK2013 as a helper plasmid.
Analysis of PA hydrolase activity.
C-P bond cleavage
activity in cell extracts and resting cells was assayed at 30°C by
measuring the amount of phosphate liberated from phosphonates supplied
as substrates (17). In both cases cultures were grown in a
mineral salts medium with Pi (2 mM) as phosphorus
source to an optical density at 600 nm (OD600) of
1.0. Cells were then harvested, washed with NaCl (0.85%), and
transferred into fresh mineral salts medium without a carbon and
phosphorus source; at this point various phosphonates (2 mM) were added
as potential inducers, and incubation was carried out for another 8 to
10 h. For assay of resting cells, this culture (adjusted to an
OD600 of 0.5) was washed and divided into
aliquots, and each potential substrate phosphonate (5 mM) was added.
After 16 h of incubation at 30°C with aeration, phosphate
release into culture supernatants was measured by the method of Fiske
and Subbarow (8). Cell extracts were prepared as described
earlier (17). As a control, cells incubated in medium
lacking phosphonate supplementation were used. Lack of
Pi release in phosphonate-containing sterile growth medium was confirmed. PA hydrolase activity was expressed as
nanomoles of Pi liberated per minute per
milligram of protein. Protein concentration was determined by the
method of Bradford (2).
In all cases PA hydrolase activity was measured using cell extracts.
However, to investigate the role of PhnB protein as a possible
transporter, activities for both cell extracts and resting cells
induced with PA were measured.
DNA techniques.
Recombinant DNA manipulations were carried
out using standard protocols as described by Sambrook et al.
(23). Restriction analysis of recombinant plasmids was
performed using enzymes obtained from Pharmacia, according to the
manufacturer's instructions. A Sephaglas BandPrep kit (Pharmacia) was
used for the recovery of restriction fragments from agarose gels.
Construction of clones.
Several recombinant plasmids (pLA82,
pLA45, pUA45, pCA452, and pCA455) containing the phn genes
were described earlier (14) and are further characterized
in this paper. Plasmids pUA6, pKK2-26, and pKK6-4 were constructed in
this work. To clone the defined phn region sequences, the
following oligonucleotide primers were used: JQ92,
5'-CTGAAGCTTGTGGCGCTACGATC-3' (a reverse primer;
position in the sequence 6688 to 6671 nt); JQ93,
5'-CATAAGCTTCGAACCGGTAAAACTG-3' (2911 to 2929 nt); and JQ96, 5'-CGGAAGCTTCAAAAATGCGCAGCGC-3'
(3863 to 3881 nt). PCRs were performed on P. fluorescens 23F genomic DNA using two pairs of primers: JQ92-JQ93
and JQ92-JQ96. PfuI polymerase was used to minimize the
number of possible mistakes introduced during amplification. Reactions
were carried out in volumes of 50 µl with concentrations of
deoxynucleoside triphosphates at 200 µM and primers at 0.15 µM
each. The following temperature profile was used: denaturing at 95°C
for 3 min and then 95°C for 30 s, 60°C for 30 s, and
72°C for 7 min, for 30 cycles. The HindIII sites
introduced into all above listed primers (underlined) were used for the
cloning of the resulting PCR fragments into pKK232-8. Primers JQ63
(5'-ACTGGCGTGCTGCTGGCA-3' [2472 to 2489 nt]) and JQ76
(5'-CTTGTATTGCAGGGTATCAG-3' [5404 to 5385 nt]) were used for construction of pKK38.
DNA sequencing.
Plasmids pUC129 and pUC18 containing
insertions from the phnA gene region were used as templates
for the Taq Dye-Deoxy Terminator Cycle sequencing kit
(Applied Biosystems). DNA sequences were obtained using an automatic
DNA sequencer (model 373A; Applied Biosystems). The nucleotide
sequences of both strands were determined. Primer synthesis was
performed by C. Stevenson (School of Biology and Biochemistry, The
Queen's University of Belfast, Ireland). Initial computer analysis of
the sequences was performed using the DNASIS (Hitachi) software
package. The alignment of sequences was performed by using CLUSTALW
software (25) with parameters set at default values.
Searches for nucleotide and amino acid sequence similarities were
carried out on the National Center for Biotechnology Information
web
server (
http://www.ncbi.nlm.nih.gov) in the nonredundant
nucleotide
(nr-nt) or amino acid (nr-aa) databases using the FASTA and
BLAST
programs (
22).
RNA analysis.
P. fluorescens 23F cells were grown
in mineral salts medium to an OD600 of 0.7. In
the case of induction with PA, cells were harvested by centrifugation,
washed, and resuspended in the same medium without a source of carbon
and phosphorus. PA was added to a final concentration of 10 mM, and
cells were incubated for 24 h. Cells were lysed with a solution
containing 4 M guanidine thiocyanate, 0.5% (wt/vol) laurylsarcosine,
and 100 mM -mercaptoethanol. An equal volume of phenol saturated
with 0.3 M sodium acetate (pH 5.5) was added, and the preparation was
mixed thoroughly and heated at 80°C for 4 min. It was then cooled,
and 0.1 volume of chloroform was added. Following centrifugation the
aqueous phase was collected. This procedure was repeated 3 to 4 times.
The RNA preparation was ethanol precipitated and dissolved in diethyl pyrocarbonate-treated water. Northern blot analysis was carried out
essentially according to the method of Sambrook et al.
(23). Aliquots of total RNA (20 µg) were fractionated in
0.8% or 1.2% agarose-formaldehyde gels electroblotted onto
Hybond-N+ membranes (Amersham) in formaldehyde
gel-running buffer for 3 h at a constant current of 150 mA using
the Mini Trans-Blot cell (Bio-Rad) and were UV cross-linked to the
filter. Either 5'-32P-labeled oligonucleotides or
uniformly 32P-labeled single-stranded DNA
fragments were used in hybridization. Primer JQ86
(5'-CGCCGTGAGTCAGGTTCAGTTCCCGGGCCG-3') complementary to mRNA
for phnR (positions 3803 through 3832 in the sequence) was
5'-32P-labeled with T4 polynucleotide kinase
(Promega) by the recommendations of the suppliers. The probe used for
phnA mRNA analysis was obtained as follows. First a DNA
fragment (positions 3948 through 4682), corresponding to the 5' end of
the phnA gene, was amplified by PCR using primers JQ87
(5'-TTGTGTGAGAAAGATGCTCAGAATACGGTG-3' [positions 3948 through 3977]) and JQ84 (5'-TGCCTGGCGCATGTTTGTGTTG-3'
[positions 4682 through 4661]). Residual primers, any
extraneous single-stranded DNA produced by PCR, and the remaining
deoxynucleoside triphosphates were removed from the PCR mixture with
exonuclease I (USB) and shrimp alkaline phosphatase (USB), using the
supplier's recommendations. Second, a uniformly
32P-labeled single-stranded DNA fragment was
synthesized by asymmetric PCR using JQ84 as the primer and the product
of the previous PCR as the template. RNA immobilized on filters was
hybridized overnight with 5'-32P-labeled JQ86 or
the uniformly 32P-labeled, single-stranded DNA
fragment, in 6× SSC (1× SSC is 0. 15 M NaCl, 0.015 M sodium citrate)
at 52°C or 68°C, respectively. Following hybridization, membranes
were washed with hybridization buffer under the same conditions for 30 min and subsequently washed at room temperature in 2× SSC, 0.5× SSC,
and 0.1× SSC.
Primer extension experiments were carried out according to the method
of Sambrook et al. (
23). Primers JQ86 (see above)
and JQ88
(5'-CAGGCGATAGGAGCGCGAGTTCACGCTGAT-3' [positions 4090
through 4060]), which are complementary to mRNA for
phnR
and
phnA,
respectively, were employed for these purposes.
5'-
32P labeling was carried out as described
above. Labeled primers
(500 to 1,000 × 10
3
cpm) were annealed with 10 to 30 µg of RNA. Hybridization was
performed at 30°C in a solution containing 40 mM
piperazine-
N,N'-bis(2
ethanesulfonic acid) (PIPES), pH 6.4, 1 mM EDTA, 0.4 M NaCl, and
80% formamide. Primer extension was carried
out with RNase H minus
Moloney murine leukemia virus reverse
transcriptase (Promega).
The products synthesized were analyzed by
electrophoresis in 6%
polyacrylamide 8 M urea
gels.
GC-MS determination of propionate.
Aliquots from enzyme
assays containing 2PP were derivatized as the phenylphenacyl
derivative of the target compound and analyzed by gas
chromatography-mass spectrometry (GC-MS) with the mass spectrometer
(MS) operating in the selected ion-monitoring mode. Fluoroacetate was
used as an internal standard for quantitation purposes. Fluoroacetate
(0.25 ml, 1 mM) was added to cell extract (1 ml), and the mixture was
frozen. Following sample lyophilization, the dried powder was suspended
in toluene-acetonitrile (1:1 [vol/vol], 1 ml);
1,4,7,10,13,16-hexaoxacyclooctadecane (10 mg) and 4-(bromoacetyl) biphenyl (10 mg) were added; and the mixture was heated at 75°C for
12 h. The derivatized samples were cooled and analyzed by GC-MS on
a Hewlett Packard 5890 series II gas chromatograph linked to a Hewlett
Packard 5971 mass selective detector controlled by a HP vectra computer
using ChemStation software. The gas chromatograph was fitted with an HP
Ultra 2 fused-silica wall-coated open tubular capillary column (12 m by
0.22 mm internal diameter) with 5% biphenyl-95% dimethyl
polysiloxane as the bonded phase. Helium was used as the carrier gas at
a flow rate of 0.8 ml min1, and samples (1 µl) were injected at a split ratio of 80:1. After injection of
samples, the oven temperature was held at 130°C for 1 min, then
programmed upwards at 10°C min1 to 300°C.
The mass selective detector was operated in selected ion
monitoring mode monitoring ion currents at m/z 181 and 268 atomic mass units for propionate and m/z 181 and 272 atomic mass units for fluoroacetate. To quantify propionate, the peak
area for ion m/z 181 at the expected retention time of
propionate was compared to a standard response curve after correcting
for the response of the internal standard.
Nucleotide sequence accession number.
The nucleotide
sequence reported in this work was deposited in GenBank under accession
number L49465.
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RESULTS |
Nucleotide sequence analysis of the phnA gene
region.
The construction of the P. fluorescens 23F
genomic library, and cloning and sequencing of the PA-hydrolase
structural gene (phnA) were reported earlier
(14). Here we describe the sequencing analysis of the
regions (9.5 kbp) adjacent to the phnA gene (Fig. 1 and Table
1). The nucleotide sequences of
orf1, phnR, phnB, and part of
orf2 were obtained using subclones produced from the pLA82
insert (Fig. 1). For sequencing of the distal part of orf2 and the whole of orf3, plasmids pUA45 and pUA6 were used
(Fig. 1). The latter plasmid was produced by the cloning from the
P. fluorescens 23F genomic library of the
HindIII fragment overlapping with the pLA82 insert.
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FIG. 1.
Physical and genetic map of the phnA gene
region. Restriction sites are indicated as follows: E,
EcoRI; RV, EcoRV; K, KpnI;
S, SalI; H, HindIII; IR, region of
imperfect inverted repeats; phnA, PA-hydrolase gene
locus; phnR, putative transcriptional regulator of the
PA-hydrolase gene cluster; phnB, putative transporter
gene for 2PP; putative genes with unknown functions found in the region
are designated as orf1, orf2, and
orf3. The direction of transcription of each gene is
shown by the arrows ( ). The most important clones analyzed in this
work are shown; the fragments containing the phnA gene
were subcloned into pLAFR5 (designated as pLA plasmids), pUC129
(designated as pUA plasmids), or pUC18 (designated as pCA plasmids).
Plasmid pKK2-26 was constructed by cloning a 2.8-kb PCR fragment
(primers JQ96 and JQ92) into plasmid pKK232-8, and plasmid pKK6-4
was constructed by cloning a 3.78-kb PCR fragment (primers JQ93 and
JQ92) into the same vector.
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Five open reading frames (ORFs), apart from the
phnA gene,
were found; they showed various degrees of similarity to existing
database entries (Table
1):
(i) ORF1 is preceded by a putative ribosome-binding site (RBS)
and encodes a putative protein with a molecular mass of 41,681
Da. This
protein shows similarity to the hydroxyphenylpropionic
acid transporter
(
6) and to several hypothetical metabolite
transport
proteins.
(ii) The ORF found immediately upstream of
phnA (Fig.
1) was
designated as the
phnR gene. This gene is encoded by a
complementary
chain (the direction of transcription is opposite to that
of the
phnA gene) and begins 140 bp upstream of the
phnA gene. This ORF
is also preceded by a putative RBS and
encodes a putative protein
of 32,827 Da. PhnR showed significant
similarity to several transcriptional
regulators belonging to the LysR
family. The alignment of the
PhnR amino acid sequence with the amino
acid sequences of three
proteins belonging to the LysR family is
presented in Fig.
2.
Analysis of this
alignment clearly demonstrates that the PhnR
gene product had a high
degree of similarity (identical aa residues)
to other LysR proteins in
its N-terminal part, the first 66 amino
acid residues, and much lower
similarity in the C-terminal half.
This mode of similarity distribution
has been shown to be typical
for the LysR family of transcriptional
regulators (
24). Evidence
for the regulation of
PA-hydrolase activity by the
phnR gene is
presented later in
this paper.
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FIG. 2.
Alignment of the LysR family transcriptional regulators.
PhnR, the putative transcriptional regulator encoded by the
phnR gene; AmpR, the positive regulator of expression of
cephalosporinase from Rhodobacter capsulatus
(3); GcvA, regulatory protein for glycine cleavage enzyme
system from E. coli (28); TrpI, tryptophan
biosynthesis transcriptional activator from Pseudomonas
syringae (1). Residues identical in all four
proteins are indicated by asterisks (*); positions where PhnR
residues are identical to two proteins are indicated by dots. The
amino-terminal DNA-binding domain, which was shown to be the most
highly conserved in all LysR proteins (24), is
underlined.
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(iii) An ORF found 96 bp downstream of
phnA was designated
as the
phnB gene. This ORF (Fig.
1) was preceded by a
putative
RBS. It encoded a putative protein of 428 amino acids. The
amino
acid sequence of this protein was shown to be similar to several
transporter proteins; for example, it showed 25% of aa identity
with
the glycerol-3-phosphate transporter (
20). The possible
role of PhnB in the biodegradation of 2PP is analyzed later in
this
paper.
(iv) ORF2 encoded a putative protein of 377 amino acids. This protein
was found to be very similar (55% aa identity) to the
spermidine/putrescine-binding protein precursor from
E. coli
(
21)
and to several other similar
proteins.
(v) ORF3 encoded a putative protein of 209 amino acids. Significant
similarity between this protein (44% aa identity) and
the peptide
methionine sulfoxide reductase from
Bacillus subtilis and
several other sulfoxide reductases was
found.
Identification of phnA and phnR
transcripts and mapping of their 5' termini.
To identify the
phnA and phnR transcripts, total RNA isolated
from PA-induced and uninduced P. fluorescens 23F cells was
fractionated by electrophoresis, transferred to nylon membranes, and
hybridized with 32P-labeled probes. Transcripts
for phnA were detected only in those RNA preparations
obtained from induced cells (Fig. 3A). In
contrast, mRNA for phnR was found in cells grown in either
the presence or the absence of the inducer; it migrated as a single
band, which corresponded to mRNA of ~1.5 kb (Fig. 3B). A more complex
picture was observed in the case of phnA mRNA (Fig. 3A).
Three main bands were detected: an upper band of less intensity, which
may correspond to the full-length phnAB transcript of ~2.6
kb, and two bands representing transcripts of ~2.0 and 1.4 kb.
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FIG. 3.
Northern blot analysis of phnA (A) and
phnR (B) mRNA. Equal amounts of total RNA (20 µg)
isolated from P. fluorescens 23F cells grown in the
presence (+) or in the absence ( ) of PA were separated on denaturing
gels, transferred onto positively charged nylon membrane, and
hybridized with 32P-labeled probes specific for
phnA (A) and phnR (B). (See Materials and
Methods.)
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Precise mapping of the
phnA and
phnR
5'-transcriptional termini was carried out by primer extension
analysis. In these experiments,
oligonucleotides complementary to the
sequence regions downstream
of the 5' ends of the
phnA and
phnR ORFs were used. The results
of the analysis are
presented in Fig.
4. In the case of the
primer
specific to
phnA, a cDNA product was synthesized only
with the
RNA obtained from induced cells (Fig.
4A), whereas for
phnR cDNA
products were detected in both cases (Fig.
4B).
These data are
in perfect agreement with the results of Northern blot
analysis
(Fig.
3). The transcription start sites were mapped at
positions
68 nt upstream of the translation start codon for the
phnA ORF
and 101 nt upstream of the start codon for the
phnR ORF (Fig.
4C). It is also worth mentioning that a minor
band was observed
when mapping the
phnR transcript (Fig.
4B). As transcripts usually
begin with a purine (predominantly A), it
is unlikely that the
above-mentioned band (with an initial C) indicated
a transcription
start site for the
phnR gene. Examination of
the nucleotide sequence
upstream of the transcription start site for
phnA revealed
10
and
35 consensus-like hexamers typical
for
70 promoters (TACGGT and TTGTGT,
respectively), followed by a putative
recognition site for positive
regulators belonging to the LysR
family (from
70 to
58). There were
no consensus-like sequences
typical of
70 or
54 promoters in the region preceding the
transcription start site
for
phnR.
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FIG. 4.
Identification of phnA and
phnR transcript initiation sites and putative regulatory
sequences. Total RNA (30 µg) isolated from P.
fluorescens 23F cells grown in the presence (+) or in the
absence () of PA was annealed with 32P-labeled primers
JQ88 (A), and 10 µg of the same RNA was annealed to JQ86 (B) as
described in Materials and Methods. Aliquots from the primer extension
reactions (lanes + and ) were separated by electrophoresis in
denaturing 6% polyacrylamide gels along with the sequence ladders
generated with the same oligonucleotides (lanes A, G, C, and T). The
corresponding primer extension products are indicated by arrows. The
nucleotide sequence of the intergenic region and the 5' ends of
phnA and phnR genes are presented (C).
N-terminal amino acids translated from ORFs for both genes are shown in
one-letter codes. Transcription start sites for PA and
PR promoters are indicated by bent arrows. Putative
10 and 35 sequences of PA and RBS are shown. The putative
recognition site for PhnR is boxed.
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Substrate specificity of PA hydrolase.
Surprisingly, only one
xenobiotic (PA) was known to be degraded by the PA hydrolase encoded by
the phnA gene of P. fluorescens 23F
(15). To analyze the activity of this enzyme in greater detail, clones with different hybrid plasmids containing the
phnA gene were examined with respect to their ability to use
several structurally analogous phosphonates (2PP,
3-phosphonopropionate, 2-phosphonobutyrate, and
phosphonoformate) as sources of phosphorus. It was found that P. putida AC577 containing the hybrid plasmids pLA82 and pLA45
(Fig. 1) as well as the original P. fluorescens 23F strain
was able to use all tested compounds except phosphonoformate as a
source of phosphorus. However, these strains released
Pi only when 2PP served as a source of phosphorus
(Fig. 5). This suggested that degradation
of 2PP was mediated by the PhnA gene product (PA hydrolase) rather than
by a classical C-P lyase since the latter enzyme is subject to
repression by Pi and no net
Pi release should occur as a result of its
activity.
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FIG. 5.
Phosphate release during growth of
Pseudomonas strains on 2PP. Strains were grown in batch
cultures. 2PP (2 mM) was used as a source of phosphorus and sodium
gluconate (2 g l1) as a source of carbon. Pi
release was measured as described in Materials and Methods.  ,
P. fluorescens 23F;  , P. putida AC577;
 , P. putida AC577(pLA45);  , P.
putida AC577(pLA82).
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Cleavage of the C-P bond of 2PP was detected only in cell extracts of
P. putida and
E. coli recombinant strains with
hybrid
plasmids containing the
phnA gene. No activity was
detected when
the
phnA gene was deleted. C-P cleavage
activities towards 2PP
were rather low, at most some 2% of the
hydrolase's activity against
PA (Table
2). To prove that the degradation of 2PP
is determined
by the enzymatic activity of the PA hydrolase encoded by
the
phnA gene, P
i release and
accumulation of propionate were analyzed
when 2PP was incubated with
cell extract known to contain PA-hydrolase
activity (Table
3). Although only low levels of C-P
cleavage
activity were found, near equimolar release of
P
i and propionate
from 2PP was obtained. These
results confirmed that the hydrolase
encoded by
phnA was
also active against 2PP.
Regulation of PA-hydrolase activity by the phnR
gene.
It has been shown above that the phnR gene
encodes a protein similar to a number of positive regulators belonging
to the LysR family. To further investigate a possible role for PhnR in
the expression of PA hydrolase, plasmids containing either
phnR and phnA or only phnA were
constructed. Plasmid pLA45, in which phnR was deleted, still
contained the whole of the phnA gene and 120 nt of upstream
region which included a promoter sequence (Fig. 1 and 4). Plasmid pLA82
contained both phnR and phnA. Plasmids pLA82 and
pLA45 (pLAFR5 vector) were transferred into P. putida AC577
using the helper plasmid pRK2013.
Phosphate release was assayed in the corresponding cell extracts
using PA and 2PP as substrates after the induction of
phnA with PA (2 mM) or 2PP (2 mM) or in the absence of any inducer
(Table
2). These results showed that PA and 2PP were similarly
effective
inducers of expression of the
phnA gene in clones of
P. putida that contained both
phnA and
phnR. Uninduced activities
of PA hydrolase in these clones
were 30 to 100 times lower. In
those clones in which the
phnR gene was deleted, induction with
either PA or 2PP was
not required for the effective expression
of the PA hydrolase
(Table
2). Transcription of the
phnA gene
in these cases was
probably achieved from the
lac promoter of
the pLAFR5
vector. Similar results were obtained with these plasmids
in
E. coli DH5
cells (data not shown). To distinguish between
possible expression from the
lac promoter and expression
regulated
by
phn-regulatory elements, a promoter probe
vector pKK232-8 was
used for analysis of the expression of
phn genes in
E. coli. For
the latter analysis,
two clones were constructed: pKK6-4 (Fig.
1), containing the
phnR,
phnA, and
phnB genes with a
putative
promoter region, and pKK2-26, which lacked most of the
putative
transcriptional-regulator gene sequence
phnR but
contained
phnA and
phnB genes and a putative
promoter region.
E. coli DH5
strains
containing these
plasmids were analyzed for the ability to grow
in liquid medium with PA
as phosphorus source. Only
E. coli DH5
(pKK6-4)
showed
the ability to grow in this medium and release
P
i. In vitro
activity of the PA-hydrolase gene
(
phnA) was measured using cell
extracts from induced and
uninduced strains. The results of these
experiments showed that,
without induction, PA-hydrolase activity
is low (0.22 to 0.25 nmol
min
1 mg
1). Induction by
PA led to an 11-fold increase in PA-hydrolase
activity (2.5 nmol
min
1 mg
1) and by 2PP to
a 9-fold increase (1.9 nmol min
1
mg
1) (Table
2). Since this effect was observed
only in the clone
with the
phnR gene, it is clear that the
phnR gene is essential
as a positive regulator for the PA-
or 2PP-dependent induction
of PA
hydrolase.
Role of phnB in the utilization of 2PP.
As
discussed above, the putative product of the phnB gene
showed similarity to several transport proteins. To analyze the possible involvement of phnB in the transport of PA and/or
2PP into bacterial cells, the activity of PA hydrolase towards these substrates was analyzed using both cell extracts and resting cell cultures. For these experiments clones were constructed (Fig. 1) in
which both the phnA and phnB genes were present
(plasmid pCA455) or in which the phnB gene was deleted
(plasmid pCA452). The results are summarized in Table
4. It is clear that PA-hydrolase activity
against PA is present in both cell extracts and resting cell cultures
induced with PA, irrespective of the presence of the phnB
gene. By contrast, Pi release from 2PP was
dependent on the presence of the phnB gene in the case of
the resting cell cultures but not of cell extracts. These results
suggest that the phnB gene product was needed for the
transport of 2PP into the bacterial cell. Induction of PA-hydrolase
activity by PA but not by 2PP was observed in clones with plasmid pKK38
which lacked the phnB gene (Fig. 1, Table 2). This
observation supported the conclusion that the phnB gene
product was involved in 2PP transport.
View this table:
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|
TABLE 4.
Phosphate release from PA and 2PP in cell-free extracts
and resting cells of E. coli DH5 with different
plasmids, preinduced with PA
|
|
| |
DISCUSSION |
PA hydrolase has been reported to be a C-P bond cleavage enzyme of
unique specificity; the purified enzyme showed no detectable activity
towards 39 organophosphonate and analogous compounds tested (17,
15). The cloning of the PA-hydrolase structural gene
phnA and adjacent genes has, however, allowed us to analyze expression of PA hydrolase in different genetic environments using E. coli and P. putida host strains. We have now
demonstrated that the phnA gene product from P. fluorescens 23F can hydrolyze the C-P bond not only of PA but also
of 2-phosphonopropionate (Table 3). Activity against 2PP was
nevertheless very low, constituting no more than 2% of that on PA; the
compound did not serve as sole carbon and energy source for either
P. fluorescens 23F or any recombinant strain containing the
cloned phnA gene. However, both PA and 2PP served as
similarly effective inducers of the phnA gene in the
original P. fluorescens 23F strain and in hybrid plasmids expressed in both E. coli DH5 and P. putida
AC577 (Table 2). This induction was dependent on the presence in the
clones of the phnR gene. phnR is located
immediately upstream of the phnA gene and shows remarkable
similarity to the group of transcriptional regulators belonging to the
LysR family (24): (i) phnR encodes a putative
protein of 299 amino acids, typical of the members of the LysR family
which range from 276 to 324 residues; (ii) its direction of
transcription is divergent to that of phnA, and it is
located 140 bp upstream of the structural gene; (iii) since regulation
of the expression of phnA is dependent on the presence of PA
or 2PP, each of these may be considered as a coinducer essential for
the PhnR regulator protein; (iv) the amino acid sequence of PhnR shows
significant homology to other members of the LysR family; this homology
is almost entirely restricted to the N-terminal part of the protein,
which is characteristic of the homology distribution among LysR family
regulators (Fig. 2); (v) a putative site for PhnR recognition was found
in the PA promoter at position 65 (Fig. 4);
this structure included dyadic symmetry and a
T-N11-A motif which has been proven to be
critical for binding of the NodD, NahR, and MetR transcriptional
regulators (9).
Our finding was not unusual, since transcriptional regulators belonging
to the LysR family are the most common group in bacteria, with more
than 50 reported members that regulate a diversity of genes and complex
regulons in many prokaryotic genera (24). However, the
involvement of a transcriptional regulator of this type in the
regulation of the expression of PA hydrolase, a unique enzyme of its
class, is of particular interest; all other C-P cleavage enzymes
studied have been shown to be under Pho regulon control
(10).
Three ORFs, which may encode proteins involved in phosphonate
utilization, were found downstream of the phnA gene. Of
these, only the role of the phnB gene has been analyzed; it
seems probable that its product is involved in the transportation of
2PP into the bacterial cell. The data obtained, however, do not rule
out the possibility that PA can also be transported by phnB.
Deletion of phnB cannot be used to prove this because
E. coli DH5 can use PA but not 2PP as a source of
phosphorus (A. Kulakova, data not shown). Significantly, in view
of the 25% homology between phnB and the
glycerol-3-phosphate transporter in B. subtilis
(20) (Table 1), it is known that the antibacterial
antibiotic fosfomycin (phosphonomycin;
cis-1,2-epoxypropylphosphonic acid) which has close
structural similarity to 2PP, is transported into bacterial cells by
the glycerol-3-phosphate pathway (11). It should be noted
that expression of the phnB gene has been investigated using E. coli DH5 as a host. Accordingly, extrapolation of
these results to the original P. fluorescens 23F host should
be made with care. However, it is significant that cloned PA hydrolase
was expressed to equally high levels in P. putida and
E. coli hosts (results not shown). The inducible nature of
this expression (Table 2) is likely to be due to the function of the
positive regulator encoded by the phnR locus.
In the course of Northern blot analysis (Fig. 3), a transcript of
~2.6 kb was identified in RNA preparations obtained from induced
cells, using a DNA probe specific to phnA. In terms of its
size, this transcript could represent mRNA for phnA and
phnB. Transcripts of similar lengths could be synthesized if
termination of transcription occurred in the intergenic region between
the phnB gene and ORF2. There were two inverted repeats in
this region (positions 6742 to 6773 and 6923 to 6942). The presence of
these repeats might lead to formation of stem and loop structures in RNA with free energies (
G25) of 8.0 kcal and
9.4 kcal, respectively. It is likely that one or both of these
repeats serve as a terminator(s) of transcription.
Analysis of the expression of different clones containing the
phn region (Tables 1 and 2) in P. putida and
E. coli cells indicated that neither ORF2 nor ORF3 was
necessary for the degradation of PA and 2PP. Furthermore the results of
Northern hybridization experiments (Fig. 3) did not reveal transcripts
of lengths greater than that of a dimeric transcript for
phnA and phnB. Therefore, we could suppose that
ORF2 and ORF3 do not belong to the phnAB operon and are
transcribed independently.
It was also evident from Northern blot analysis that phnR
was transcribed in the form of monocistronic mRNA. A region of tandem inverted repeats localized at the 3' end of ORF1 (positions 2610 to
2828) might serve for termination of its transcription.
Northern blot analysis of the phnA region also revealed two
transcripts of ~2.0 and ~1.4 kb as the major products. The former may represent the whole phnA ORF and the 5' part of the
phnB ORF, and the latter may represent phnA only.
These transcripts might be produced as a result of the termination of
the transcription inside the phnB gene and in the
phnA and phnB intergenic region, respectively. We
also can not exclude the possibility that these transcripts originated
from the processing of a phnAB transcript.
In conclusion, our study has indicated a probable mechanism by which
the inducible expression of PA hydrolase occurs in P. fluorescens 23F. In light of other studies in this laboratory (16) which show that 2-aminoethylphosphonic acid,
phosphonomycin, and phosphonoalanine can also be degraded by
environmental microorganisms in a P-insensitive manner, it is likely
that the expression of a number of other C-P cleavage enzymes may prove
to be similarly regulated.
| |
ACKNOWLEDGMENTS |
This project was supported by the Queen's University
Environmental Science and Technology Research Centre (QUESTOR), the
European Regional Development Fund
Technology Development Programme,
and BBSRC grant 81/P11488.
We are most grateful to anonymous reviewers for their suggestions for
the improvement of an earlier version of this article.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: The Questor
Centre, David Keir Building, The Queen's University of Belfast,
Belfast BT9 5AG, Northern Ireland. Phone: (44) 2890 272250; Fax: (44) 2890 661462. E-mail: A.Kulakova{at}qub.ac.uk.
| |
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Journal of Bacteriology, June 2001, p. 3268-3275, Vol. 183, No. 11
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.11.3268-3275.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
