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Infection and Immunity, January 1999, p. 80-87, Vol. 67, No. 1
Department of Biochemistry and Molecular
Biology, Wright State University School of Medicine, Dayton, Ohio
45435
Received 12 May 1998/Returned for modification 29 July
1998/Accepted 19 October 1998
We have shown that Pasteurella multocida toxin (PMT)
directly causes transient activation of Gq Pasteurella multocida
toxin (PMT) is a major virulence factor associated with progressive
atrophic rhinitis in domestic and wild animals (1, 12),
respiratory disease in cattle and laboratory rabbits (3-6, 8,
14), and dermonecrosis and bacteremia resulting from bite wounds
or animal exposure in humans (15, 16, 20, 23, 28, 35, 41).
PMT is a 1,285-amino-acid protein (7, 22, 26, 32) that
appears to bind to and enter mammalian cells via receptor-mediated
endocytosis (34, 36) and acts intracellularly to initiate
DNA synthesis and cytoskeletal rearrangements (9, 17, 18, 21, 24,
29, 36). Some of the intracellular events that have been observed
upon exposure to PMT in cultured fibroblasts and osteoblasts include
enhanced hydrolysis of inositolphospholipids to increase intracellular
inositol phosphates and diacylglycerol (29, 30, 38);
mobilization of intracellular Ca2+ pools (29, 30, 38,
40); decreased ADP-ribosylation of GRP78/BiP (39);
increased protein phosphorylation (40); and tyrosine
phosphorylation of p125Fak and paxillin, as well as actin
stress fiber formation and focal adhesion assembly (9, 24).
Recently, we used voltage-clamped Xenopus oocytes to
demonstrate direct PMT-mediated stimulation of the During our earlier studies, we observed that specific antibodies
against an N-terminal peptide of PMT, anti-toxA28-42, were
able to block the PMT-mediated response in Xenopus oocytes (43). On the other hand, specific antibodies to a C-terminal peptide of PMT, anti-toxA1239-1253, did not block the
activity, strongly implying that the N terminus of PMT is critical for
its intracellular activity. The N-terminal half of the related
cytotoxic necrotizing factor type 1 (CNF1) and CNF2 from pathogenic
Escherichia coli show homology to the N terminus of PMT
(10, 31). Comparisons of the amino acid sequence of PMT with
those of other bacterial dermonecrotic toxins has been reported
elsewhere (10, 27, 31, 42). While there is homology in the C
termini of the CNFs and the dermonecrotic toxin from Bordetella
bronchiseptica (DNT), the C-terminal region of PMT does not have
this similarity with those of the CNFs and DNT (10, 27, 31,
42). As has been shown for PMT, both DNT and the CNFs induce DNA
synthesis, as well as actin stress fiber formation and focal adhesion
assembly (19, 25, 31). For the CNFs and DNT, this activity
has been shown to occur through constitutive activation of the small G protein RhoA by deamidation of Gln-63 (11, 19, 31, 37). The
RhoA deamidase activity was reported to be localized to the C terminus
of CNF1 (27), and the receptor-binding activity was postulated to be in the N terminus. While all of these toxins have been
shown to induce stress fiber formation and focal adhesion assembly, the
molecular and functional organization of this group of toxins remains
unclear. It is also not clear how the modification of RhoA by the CNFs
and DNT and the modification of Gq To define the functional domain of PMT responsible for intracellular
activity, we cloned the entire toxA gene from P. multocida and expressed the corresponding recombinant PMT (rPMT)
as a hexahistidine (His)-tagged fusion protein in E. coli.
We confirmed that the full-length rPMT protein is as active as native
PMT in both oocyte and cell culture assays. We then constructed a
series of N- and C-terminal deletion mutants of the toxA
gene and expressed the corresponding recombinant His-tagged PMT
fragments (ToxAN and ToxAC, respectively) in E. coli. To
screen for the functional domain of PMT responsible for activation of
the intracellular Gq-PLC Materials.
Rabbit polyclonal antisera against two synthetic
peptides, comprising residues 28 to 42 of PMT (NSDFTVKGKSADEIF) and
residues 1239 to 1253 of PMT (PVDDWALEIAQRNRA), were obtained from
Bio-Synthesis, Inc., using multiple antigen peptide conjugation
methodology. The anti-peptide immunoglobulin G (IgG) antibodies
(anti-toxA28-42 and anti-toxA1239-1253) were
purified by using a protein A-agarose column (PURE-1; Sigma). Goat
anti-rabbit IgG antibodies conjugated to alkaline phosphatase and
tetramethylrhodamine B isothiocyanate (TRITC)-conjugated phalloidin
were obtained from Sigma. E. coli BL21(DE3) and the plasmid
vectors pET-15b, pET-21b, and pET-33b were obtained from Novagen.
E. coli XL-1 Blue was obtained from Stratagene. TA-cloning
kits, E. coli TOP10 and competent TOP10F' One-Shot cells,
and plasmid vectors pTrcHisC and pCR3-Uni were obtained from
Invitrogen. LipofectAMINE, the plasmid vector pROEX-1, and tissue
culture media, sera, and reagents were obtained from Gibco/BRL. The
plasmid vector pEGFP-N1 was obtained from Clontech.
Ni2+-nitrilotriacetic acid (NTA)-agarose and Qiaex II DNA
purification kits were obtained from Qiagen. PCR primers were obtained
from Bio-Synthesis and Gibco/BRL. Restriction enzymes were obtained from Gibco/BRL or New England Biolabs. Centricon, Ultra-Free, and
Centricon Plus-20 concentrators were obtained from Amicon/Millipore. Xenopus laevis frogs were obtained from Xenopus I, Dexter,
Mich. African green monkey kidney (Vero) cells (CCL-81) and murine
Swiss 3T3 (CCL-92) and NIH 3T3 (CRL-1658) fibroblast cells were
obtained from the American Type Culture Collection. P. multocida subsp. multocida 45/78 (NCTC 12178) was
obtained from the National Collection of Type Cultures and grown at
37°C on Trypticase soy agar supplemented with 5% defibrinated sheep
blood (BBL 11043). Native PMT was purchased from Sigma as a lyophilized
powder with bovine serum albumin and resuspended in 50 mM Tris-HCl (pH
7.5) containing 5% glycerol prior to use. Native PMT, purified to
homogeneity, quantified, and titered by Vero cell cytotoxicity assays
as described elsewhere (8), was a generous gift from
Clarence Chrisp. All other reagents were of the highest quality
commercially available.
Construction of plasmids containing deletion mutants of PMT.
All recombinant proteins were engineered to have either an N- or a
C-terminal fusion peptide containing a His tag, with all N-terminal
fusion peptides also containing a thrombin proteolytic recognition site
(Fig. 1). All cloning was carried out
with either E. coli XL-1 Blue or E. coli TOP10F'
One-Shot cells.
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Localization of the Intracellular Activity Domain
of Pasteurella multocida Toxin to the N Terminus
ABSTRACT
Top
Abstract
Introduction
Materials and methods
Results
Discussion
References
protein that is coupled
to phosphatidylinositol-specific phospholipase C
1 in
Xenopus oocytes (B. A. Wilson, X. Zhu, M. Ho, and L. Lu, J. Biol. Chem. 272:1268-1275, 1997). We found that antibodies
directed against an N-terminal peptide of PMT inhibited the
toxin-induced response in Xenopus oocytes, but antibodies
against a C-terminal peptide did not. To test whether the intracellular
activity domain of PMT is localized to the N terminus, we conducted a
deletion mutational analysis of the PMT protein, using the
Xenopus oocyte system as a means of screening for toxin
activity. Using PCR and conventional cloning techniques, we cloned from
a toxinogenic strain of P. multocida the entire
toxA gene, encoding the 1,285-amino-acid PMT protein, and
expressed the recombinant toxin as a His-tagged fusion protein in
Escherichia coli. We subsequently generated a series of
N-terminal and C-terminal deletion mutants and expressed the His-tagged
PMT fragments in E. coli. These proteins were screened for
cytotoxic activity on cultured Vero cells and for intracellular
activity in the Xenopus oocyte system. Only the full-length
protein without the His tag exhibited activity on Vero cells. The
full-length PMT and N-terminal fragments containing the first 500 residues elicited responses in oocytes, but the C-terminal 780 amino
acid fragment did not. Our results confirm that the intracellular
activity domain of PMT is localized to the N-terminal 500 amino acids
of the protein and that the C terminus is required for entry into cells.
INTRODUCTION
Top
Abstract
Introduction
Materials and methods
Results
Discussion
References
1 isoform of
phospholipase C (PLC1) and the inositol 1,4,5-trisphosphate
(IP3) signaling pathway and to identify the immediate
intracellular target of PMT as the free, monomeric subunit of the
Gq protein (43).
by PMT lead to each of the
observed intracellular changes.
1-IP3 signaling pathway, the
recombinant toxin proteins were microinjected into voltage-clamped
Xenopus oocytes to observe the toxin-induced
Ca2+-dependent Cl
current. Our results
localize the functional domain of PMT responsible for intracellular
activity to the N terminus. To determine if this functional domain
alone possessed cytotoxic activity on intact cells, we also tested each
of the recombinant proteins for effects on cultured Vero cells and
found that only the full-length rPMT protein is able to cause the
morphological effects induced by native PMT.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and methods
Results
Discussion
References
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FIG. 1.
Localization of deletion mutant proteins used in this
study relative to full-length PMT. Open bar, sequence derived from the
toxA gene; closed bar, location of the His tag in each
recombinant protein.
Expression of recombinant toxin proteins in E. coli.
Recombinant proteins were expressed in E. coli BL21(DE3) for
constructs generated in expression vector pET15b, pET21b, pET33b, or
pROEX-1 or in E. coli TOP10 for constructs generated in
expression vector pTrcHisC. Seed flasks containing 50 ml of LB with the
appropriate antibiotic, ampicillin (100 µg/ml) or kanamycin (25 µg/ml), were inoculated with the desired bacterial colonies and
incubated with vigorous shaking overnight at 37°C. Fermentation
flasks containing 500 ml of LB with ampicillin (100 µg/ml) or
kanamycin (25 µg/ml) were inoculated with 8 to 10 ml of the overnight
seed culture and incubated with vigorous shaking at 37°C until an
optical density at 600 nm of 0.6 to 0.8 was reached. Expression of the
recombinant proteins was induced by addition of
isopropyl--D-thiogalactopyranoside (IPTG) to a final
concentration of 1 mM, and growth was continued for 3 h. Cells
were harvested by centrifugation at 5,000 × g for 10 min in a Sorvall RC-5C Plus centrifuge. Cell pellets were suspended in
lysis buffer (100 ml per 2.5-liter starting culture volume; 50 mM
potassium phosphate [pH 7.5] containing 100 mM KCl, 0.1% Tween 20, 5% glycerol, 5 µg each of pepstatin, leupeptin, and aprotinin per
ml, 2 mM benzamidine, 2 mM phenylmethylsulfonyl fluoride, 0.2 mg of
lysozyme per ml, 200 U of RNase A, and 1,500 U of DNase I). The cell
suspension was sonicated for four rounds of 1-min pulses at a
duty cycle of 0.7 in a Brau-Sonic-U cell disruptor, with 1-min cooling
intervals on ice. The cellular debris was removed by centrifugation at
20,000 × g for 90 min, and the supernatants were
immediately used as cell extracts for further purification.
Purification of recombinant toxin proteins. The His tag affinity handle allowed for essentially one-step purification of the full-length and deletion mutant toxins by nickel chelate affinity chromatography. Cell extracts were passed twice through a 5-ml/Ni2+-NTA-agarose column (Qiagen). The column was washed twice with 50 ml of Ni column buffer (50 mM potassium phosphate [pH 7.5], 100 mM KCl, 0.1% Tween 20, 5% glycerol, 10 mM imidazole), followed by stepwise elution with 50 ml each of Ni column buffer containing 20, 30, 60, 110, 160, and 500 mM imidazole. Column fractions were analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and Western blotting, and fractions containing the toxin proteins were pooled and concentrated in Centricon/Millipore concentrators to remove the imidazole and to exchange the buffer with 50 mM Tris-HCl (pH 7.5) containing 5% glycerol. To further desalt the samples, the concentrated solutions were passed through a PD-10 desalting column (Pharmacia).
SDS-PAGE and Western analysis. To analyze dilute protein fractions or fractions containing high salt concentrations, samples were precipitated with an equal volume of cold 20% trichloroacetic acid and microcentrifuged at 15,000 × g at 4°C for 20 min, washed twice with cold acetone, and then air dried. Protein pellets were redissolved in a mixture of 100 mM Tris-HCl (pH 9.0), SDS-PAGE sample buffer, and tracking dye. Alternatively, SDS-PAGE sample buffer and tracking dye were added directly to protein samples. The protein samples were then separated by SDS-PAGE on 8, 10, 11, or 16% gels. Protein bands were visualized by Coomassie or silver staining and by Western blotting. For Western blot analysis, proteins were first transferred onto nitrocellulose membrane and immunoblotted with rabbit polyclonal antibodies to PMT, followed by secondary goat anti-rabbit IgG antibodies conjugated to alkaline phosphatase. The images of gels and Western blots shown in Fig. 2 and 3 were obtained by using a ScanJet 3C (Hewlett-Packard) with DeskScan II (Hewlett-Packard) image acquisition software, and the graphics were produced by using Adobe Photoshop on an Apple Macintosh G3 computer.
Removal of the His tag by thrombin treatment. The His tag peptide was removed from recombinant toxin proteins possessing N-terminal His tags (rPMT, ToxAN2, and ToxAN3) by thrombin treatment. The His-tagged protein (4 to 5 mg) and biotinylated thrombin (5 U; Novagen) in thrombin cleavage buffer (500 µl; 20 mM Tris-HCl [pH 8.4], 150 mM NaCl, 2.5 mM CaCl2) were incubated at room temperature for 16 to 20 h. Completion of reaction was assessed by SDS-PAGE analysis. To terminate the reaction, streptavidin-agarose beads (20 µl; Novagen) were added and the suspension was incubated for an additional hour with gentle shaking. The beads were pelleted by centrifugation at 400 × g for 30 s, and the supernatant was diluted with Ni column buffer (1 to 2 ml) and passed twice through a 2- to 3-ml Ni2+-NTA-agarose column (Qiagen) to remove the His tag peptide. Samples were desalted on PD-10 columns (Pharmacia) against 50 mM Tris-HCl (pH 7.5) containing 5% glycerol and concentrated in Centricon concentrators.
Quantitation of recombinant toxin proteins. The concentration of His-tagged rPMT was determined by Coomassie Plus protein assay (Pierce), with bovine serum albumin as a standard. The concentration of the commercial native PMT sample was determined by image quantitation analysis of silver-stained SDS-polyacrylamide gels, using His-tagged rPMT as a standard. The concentrations of rPMT without the His tag, ToxAN2 without the His tag, ToxAN4, ToxAN5, and ToxAC1 were determined by image quantitation analysis of the appropriate bands on Western blots with either anti-toxA28-42 or anti-toxA1239-1253 as the primary antibody, using His-tagged rPMT as a standard. The concentrations of ToxAN3 without the His tag, ToxAN6, ToxAN7, and ToxAC2 were determined by image quantitation analysis of the appropriate bands on Western blots with either anti-toxA28-42 or anti-toxA1239-1253 as the primary antibody, using ToxAN4 as a standard. Western blots were imaged as described above, and images were quantitated by using NIH Image (National Institutes of Health) image analysis software and Microsoft Office Excel (Microsoft) data analysis software.
Cell culture assays. Cultured cells were maintained at 37°C and 10% carbon dioxide in Dulbecco modified Eagle medium (DMEM; Gibco/BRL), pH 7.4, supplemented with 10% heat-inactivated fetal bovine serum (Gibco/BRL) for Vero cells and NIH 3T3 cells) or 15% heat-inactivated calf serum (Gibco/BRL) for Swiss 3T3 cells, containing penicillin G (100 U/ml) and streptomycin (100 µg/ml) (Gibco/BRL). After trypsinization, cells were plated onto 12-well plates (Falcon) at a density of 4 × 104 (Vero cells) or 2 × 104 (Swiss 3T3 cells) per well, and incubation was continued with a change of medium after 24 h. Vero cells and Swiss 3T3 cells were allowed to reach confluency 5 days after plating, and then the medium was changed to DMEM-1% fetal bovine or calf serum (pH 7.4) containing antibiotics. Two days after quiescence with low-serum media, the medium was replaced with filter-sterilized, low-serum medium containing 200 ng of the native PMT, rPMT, and ToxAN4 proteins per ml, as well as controls containing the corresponding heat-inactivated proteins and no protein. The cells were visualized after 1, 4, and 6 days of toxin exposure for morphological changes by phase-contrast microscopy using an Olympus IX-70 inverted microscope. Heat-inactivated controls of the protein samples were prepared by heating the samples at 70°C for 45 min.
Transfection of NIH 3T3 cells with mammalian expression plasmids containing an N-terminal fragment of PMT or green fluorescent protein (GEP). Cells were cotransfected with a 1:1 ratio of pCR3-Uni(1&3) and pEGFP-N1 or with pEGFP-N1 alone, using LipofectAMINE reagent (Gibco/BRL) according to the manufacturer's protocol. Briefly, 1 day prior to transfection, NIH 3T3 cells were plated at a density of 2 × 105 cells/well on six-well plates in antibiotic-free medium. DNA plasmids (1 µg of each) in 100 µl of Opti-MEM (Gibco/BRL) and 4 µl of LipofectAMINE reagent in 100 µl of Opti-MEM were combined, incubated at room temperature for 15 min, and then added to each well containing 800 µl of Opti-MEM. After 3 h of incubation at 37°C, 1 ml of antibiotic-free, low-serum medium was added, and cells were further incubated at 37°C for 24 h prior to staining and visualization.
Fluorescence staining of transfected NIH 3T3 cells expressing an N-terminal fragment of PMT. The cells were washed twice with phosphate-buffered saline (PBS), fixed with 3.7% formaldehyde in PBS for 10 min, washed with PBS, permeabilized with 0.5% Triton X-100 in PBS for 10 min, washed twice with PBS, incubated for 1 h at room temperature with TRITC-conjugated phalloidin (2 µM; Sigma) in PBS, washed twice with PBS, and visualized by fluorescence microscopy using an Olympus IX-70 inverted microscope, equipped with U-MWB and U-MWIG fluorescence cubes for observing GFP and TRITC, respectively. Images were captured by using NIH Image 1.61, and micrographs were generated by using Adobe Photoshop 4.0.
Oocyte preparation. Adult female X. laevis frogs (Xenopus I) were anesthetized by immersion in a 0.1% tricaine methanesulfonate (Sigma), adjusted to pH 7.4 with NaHCO3. A small incision was made on one side of the abdomen to remove several ovarian lobes. The lobes were gently torn apart and immersed in a Ca2+-free OR-2 solution (100 mM NaCl, 2 mM KCl, 1 mM MgCl2, 5 mM HEPES-Tris [pH 7.5]). Oocytes were defolliculated by incubation with collagenase (2 mg/ml; Sigma type 1A) at room temperature (22 to 24°C) for 1 to 2 h. The oocytes were then washed five times with OR-2 solution and five times with a modified Barth's solution [88 mM NaCl-1 mM KCl-2.4 mM NaHCO3-0.3 mM Ca(NO3)2-0.4 mM CaCl2-0.8 mM MgSO4-15 mM Tris-HCl (pH 7.6) containing penicillin G (100 µg/ml) and streptomycin (100 µg/ml)]. Stage 5-6 oocytes were selected and stored at 18°C in modified Barth's solution.
Two-microelectrode voltage clamp. Two microelectrodes, made by a vertical puller (model PP-83, Narishige) and filled with 3 M KCl to give a resistance of 1.5 to 2.0 megaohms, were used for voltage clamping. Voltage clamp experiments were performed in a continuously perfused bath (10 ml/min) at room temperature (22 to 24°C). The bath was connected through an Ag-AgCl-agar-3 M KCl bridge to the two-electrode voltage clamp system (TEV-200 voltage clamp; Dagan). Membrane currents were measured in normal Ringer's solution (96 mM NaCl, 2 mM KCl, 1 mM MgCl2, 11.8 mM CaCl2, 5 mM HEPES-NaOH [pH 7.4]). Data acquisition was performed by using MacLab/8s (ADInstruments) linked to a Macintosh Quadra 800 computer with Chart and Scope application software (ADInstruments). Graphics were obtained by using Cricket Graph III (Computer Associates).
Oocyte microinjections.
Microinjections of toxins, toxin
fragments, and antibodies were performed under voltage-clamped
conditions at 
80-mV holding potential, using a pulse-controlled
microinjector (Dagan model PMI-200). Toxins and other reagents were
prepared in 50 mM Tris-HCl (pH 7.5) with 5% glycerol prior to
injection. For experiments involving anti-toxA28-42
inhibition of ToxAN4, protein A-purified antibodies were passed through
a PD10 column in 50 mM Tris-HCl (pH 7.5) with 5% glycerol and
concentrated such that an equal volume could neutralize the rPMT
response in oocytes. This antibody preparation was then incubated in a
1:1 ratio with ToxAN4 on ice for 1 h prior to injection.
Data analysis and determination of EC50s.
In all
experiments reported here, each group of oocytes was tested for
positive responses elicited by rPMT. All results are expressed as the
mean ± standard error of the maximal inward current assayed in
oocytes from the same donor group. For the titration experiments, the
same group of oocytes from a given donor was used for all doses tested.
The number of oocytes used for data analysis at each dose is given in
parentheses in Fig. 5. Fifty percent effective concentrations
(EC50s) were calculated with SigmaPlot (Jandell Scientific)
by fitting data points to a logistic function f(x) = a/{1 + exp[b*(x c)]}, where
a is the maximum response observed, b is the
slope, and c is the EC50. The EC50 curves shown in Fig. 5 were plotted by using Cricket Graph III (Computer Associates).
Protein sequence and structure comparison between PMT and the CNFs and DNT. Primary sequence comparison between PMT, CNF1, CNF2, and DNT was performed by using the BestFit sequence analysis program from the Genetics Computer Group Wisconsin Package with BLOSUM30 and BLOSUM62 amino acid alignment scoring matrices. The secondary structure prediction for PMT and CNF1 was performed with the GOR-IV program available at http://absalpha.dcrt.nih.gov:8008/gor.html. The area plot shown in Fig. 7 was generated from the GOR-IV analysis results, with an additional smoothing window of 11 amino acid residues for the helical probability, 5 amino acid residues for the extended strand probability, and the remainder for the coil probability.
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RESULTS |
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Top
Abstract
Introduction
Materials and methods
Results
Discussion
References
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Construction of N-terminal and C-terminal deletion mutants of
PMT.
To define the specific region of PMT responsible for
activation of the intracellular Gq-PLC1-IP3 signaling
pathway, we cloned the toxA gene, encoding the full-length
PMT protein, and designed a series of N- and C-terminal deletion
mutants (Fig. 1). Expression plasmids containing the entire
toxA gene or various deletion fragments thereof were
constructed by using PCR and conventional cloning techniques. A plasmid
containing the full-length toxA gene, pTHC-toxA, was
generated by splicing three overlapping toxA fragments from cloning vectors containing the corresponding PCR products,
pET15b-toxAN1, pCR3-Uni(1&3), and pCR3-Uni(4&5). The N- and
C-terminal deletion mutants were obtained from regions of the
toxA gene encoding the N- and C-terminal portions of the PMT
protein. The deletion mutants were designed such that all regions of
the entire protein would be included in at least one of the deletion
fragments. The ToxAN4 fragment containing the N-terminal 568 amino
acids of PMT included the region showing homology with the CNFs.
Sequentially shorter N-terminal fragments, which could be used to
further define the activity domain, were also designed; these included
the N-terminal 505, 450, 400, 300, 293, and 93 amino acids of PMT
(ToxAN2, ToxAN5, ToxAN6, ToxAN7, ToxAN1, and ToxAN3, respectively). The
two C-terminal fragments included the C-terminal 780 amino acids of PMT
(ToxAC1) and the C-terminal 226 amino acids (ToxAC2). The various
toxA deletion fragments were subcloned into E. coli expression vectors which incorporated a His tag affinity
handle at either the N- or C terminus of the protein, as indicated in
Fig. 1.
Expression, purification, and quantitation of rPMT and PMT deletion mutant proteins. We expressed the recombinant toxin proteins under IPTG-inducible promoters in E. coli as His-tagged fusion peptides for ease in purification. The His tag allowed for essentially one-step purification of the proteins, thereby reducing the amount of sample handling and decreasing the likelihood of protein denaturation or inactivation. During the course of our initial studies, we observed that the His tag placed at the N terminus of rPMT interfered with the activity of the protein in the Xenopus oocyte assay system, as well as in tissue culture assays (data not shown). Hence, following Ni2+ chelate chromatography, we opted to remove the His tag by thrombin cleavage from all of the N-terminal fragments having His tag at their N-termini, including rPMT, ToxAN1, ToxAN2, and ToxAN3. The ToxAN1 protein with a His tag at the N terminus was difficult to purify (Fig. 2) and was not stable to subsequent thrombin treatment, and we could not obtain quantities adequate to assay for activity. ToxAN7 was similar in length to ToxAN1. The His tag was placed at the C termini of ToxAN4, ToxAN5, ToxAN6, and ToxAN7. The C-terminal His tag was not removed from these recombinant proteins. For ToxAC1 and ToxAC2, the N-terminal His tag was placed at the N terminus but was not removed.
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Comparison of rPMT with native PMT. Figure 3 shows a silver-stained SDS-polyacrylamide gel of rPMT before and after thrombin cleavage in comparison to native PMT from two different sources. Anti-toxA28-42 and anti-toxA1239-1253 were reactive with recombinant toxin samples in Western blots (Fig. 2). Native and recombinant toxins gave comparable responses in oocyte experiments (Fig. 4A and B), although the highly purified PMT and rPMT samples were at least 20-fold more active than the commercial native PMT sample. However, after determining the concentrations of the impure native PMT samples by analyzing silver-stained SDS-polyacrylamide gels, using purified rPMT as a standard, we found that the commercial native PMT was as active as rPMT. When the EC50s were adjusted accordingly, the native and recombinant toxins exhibited similar responses in oocytes, with EC50s of 5.2 and 3.6 fmol/oocyte, respectively (Fig. 5A and B). Anti-toxA28-42, but not anti-toxA1239-1253, specifically inhibited the activities of both native and recombinant toxin samples in oocyte experiments (reference 43 and data not shown). As depicted in Fig. 6, rPMT caused dramatic morphological effects on confluent, quiescent Vero cells, showing focus formation surrounded by enlarged cells, as well as proliferative effects on confluent, quiescent Swiss 3T3 cells. Native PMT caused similar effects (data not shown), although the rPMT sample consistently appeared to be more potent than the commercial native PMT sample. The results from these studies are summarized in Table 1.
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Activities of N- and C-terminal deletion fragments of PMT. The C-terminal PMT fragments, ToxAC1 and ToxAC2, and the smaller N-terminal fragments, ToxAN3, ToxAN6, and ToxAN7, exhibited no detectable responses in the oocyte assay at concentrations as high as 1 pmol/oocyte. In contrast, ToxAN4, consisting of the N-terminal 568 amino acids, gave reproducible responses in oocytes (Fig. 4C) with an EC50 of 22 fmol/oocyte (Fig. 5C), compared to 3.6 fmol/oocyte for the full-length rPMT. ToxAN2, consisting of the N-terminal 505 amino acids, also showed a reproducible activity (Fig. 4D), with an EC50 of 140 fmol/oocyte (Fig. 5D), about 40-fold lower than that for full-length rPMT. ToxAN5, consisting of the N-terminal 450 amino acids, gave detectable responses in oocytes (Fig. 4E), but the responses were so weak that it was not possible to accurately determine an EC50 for this mutant protein with injection of as much as 3 pmol. Unlike the full-length rPMT, none of the N- or C-terminal deletion mutants exhibited an effect on cultured Vero cells (data not shown). The results from these studies are summarized in Table 1.
To determine whether the N terminus of PMT could also trigger downstream signaling events in mammalian fibroblasts, leading to changes in cellular morphology, a mammalian expression plasmid containing the N-terminal 521 amino acids of PMT under the cytomegalovirus promoter was cotransfected into NIH 3T3 cells along with a reporter plasmid containing GFP under the same promoter. In vitro translation assays using pCR3-Uni(1&3) were also performed to ensure that the construct was indeed capable of expressing truncated toxin protein (data not shown). We found that cells cotransfected with both plasmids underwent significant morphological responses compared to control cells transfected with reporter plasmid alone. As shown in Fig. 7, control cells expressing only the GFP protein have a characteristic spread-out fibroblast morphology, whereas cells expressing the N-terminal fragment of PMT and GFP have a more retracted and spindly appearance, with evidence of more intense TRITC-phalloidin staining.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and methods
Results
Discussion
References
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Evidence from previous studies suggests that the mode of action of
PMT involves binding to cell surface receptors and internalization via
receptor-mediated endocytosis (34, 36), followed by
activation of various signaling pathways (29, 30, 38-40,
43), leading eventually to morphological and proliferative events
(9, 17, 18, 21, 24, 29, 36). In our earlier studies, we
demonstrated that intact PMT protein could directly activate the
Gq-PLC1-IP3 signaling pathway in Xenopus
oocytes (43). Using this system, we bypassed the
cell-binding and internalization process by direct microinjection
of the toxin, apparently without the requirement for further
intracellular processing or activation. In the present work, we report
the cloning, expression, and purification of fully active recombinant
PMT from E. coli. This full-length recombinant protein has
an activity in oocytes similar to that of the native toxin isolated
from P. multocida. We have also shown that rPMT has an
effect on cultured Vero cells similar to that of the native toxin.
We have demonstrated that a recombinant deletion mutant consisting of
the N-terminal 568 amino acids of PMT could elicit a PMT-like response
in oocytes, while two mutants consisting of the C-terminal 780 and 226 amino acids gave no detectable response at higher doses. Weaker
responses were also observed with mutants consisting of the N-terminal
505 and 450 amino acids but not with shorter N-terminal fragments. We
thus conclude that the functional domain responsible for activating the
intracellular Gq-PLC1-IP3 signaling pathway in
Xenopus oocytes is localized to the N terminus of PMT.
The N-terminal 500 residues of PMT have 24 to 27% homology to the N-terminal 500 residues of CNF1 and CNF2 (10, 31). As can be seen from the area plot shown in Fig. 8, the predicted secondary structures of PMT and CNF1 also have limited similarity in this region, particularly in the region with 30% homology between residues 200 and 450 of PMT. We have shown that deletion mutations made within this conserved region resulted in loss of intracellular activity. With localization of the intracellular activity domain to the N-terminal 500 amino acid residues of PMT, the sequence and structural similarity in the N-terminal region between the two toxins suggests that CNF1 and CNF2 may have an intracellular activity similar to that of PMT. However, there are sufficient differences between the toxins within this region, as indicated in the secondary structure prediction profiles (Fig. 8), for it to be feasible that they have different intracellular activities and target preferences. CNF1 and CNF2 possess deamidase activity on RhoA (11, 19, 31, 37). The deamidase activity domain of CNF1 has been reported to be located in the C-terminal 300 residues (27), which shares about 20% homology with the C-terminal 300 residues of DNT but has no discernible sequence similarity with PMT. It is possible that the N-terminal region of CNF1 with homology to the N-terminal region of PMT possesses an intracellular activity different from the activity associated with the C-terminal 300 residues of CNF1.
|
In our previous study (43), we showed that antibodies
specific for the N terminus of PMT blocked the PMT-induced response in
oocytes, but antibodies against the C terminus did not. The N-terminal
toxin fragments ToxAN4 and ToxAN2 are able to elicit responses in
oocytes similar to those elicited by full-length rPMT. Antibodies to
the N terminus of PMT also blocked the ToxAN4-induced response in
oocytes, yet ToxAN4 had no effect on cultured Vero cells. Moreover,
none of the deletion mutants exhibited an effect on Vero cells. This is
consistent with earlier findings that deletion mutants lacking
N-terminal (
28-149 and 175-247) or C-terminal (1130-1285)
portions of the PMT protein had no toxic activity in assays for
cytopathicity on embryonic bovine lung (EBL) cells, dermonecrosis in
guinea pigs, or mouse lethality (33). Previous studies also
showed that monoclonal antibodies recognizing an epitope in the
C-terminal 155 amino acids of PMT blocked the cytopathic effect of PMT
on EBL cells (13, 33). The C-terminal fragments ToxAC1 and
ToxAC2 were inactive in the oocyte assay and had no effect on cultured
Vero cells, thus supporting the notion that only the N terminus of PMT
has intracellular activity and the C terminus of PMT is required for
toxin entry into cells. Further study is required to determine the
precise biochemical activity of PMT that induces the
Gq-PLC1-IP3 signaling pathway and to understand how
this PMT-associated activity and the CNF-associated deamidase activity
could result in the observed changes in cells caused by these toxins.
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ACKNOWLEDGMENTS |
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This work was supported by grant AI38396 from the National Institutes of Health/NIAID (to B.A.W.).
We thank Xinjun Zhu, Brooke Murphy, Tina Caserta, April Buehler, James Burgett, and Jennifer Williams for technical assistance. We especially thank Adrian Corbett for helpful discussions and generous assistance in setting up the electrophysiological equipment, Hangjun Zhan for helpful discussions and assistance in the initial cloning stages of this project, and Steven Berberich for assistance with in vitro translation assays. We are grateful to Clarence Chrisp for generously providing purified samples of native PMT.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Biochemistry and Molecular Biology, Wright State University School of Medicine, 3640 Col. Glenn Hwy., Dayton, OH 45435. Phone: (937) 775-4803. Fax: (937) 775-3730. E-mail: bwilson{at}wright.edu.
Editor: J. T. Barbieri
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REFERENCES |
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Top
Abstract
Introduction
Materials and methods
Results
Discussion
References
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Infection and Immunity, January 1999, p. 80-87, Vol. 67, No. 1
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