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Journal of Bacteriology, September 2000, p. 5251-5255, Vol. 182, No. 18
Department of Microbiology and Immunology, University of
British Columbia, Vancouver, British Columbia, Canada V6T 1Z3
Received 9 March 2000/Accepted 18 May 2000
Pseudomonas aeruginosa OprF forms 0.36-nS channels and,
rarely, 2- to 5-nS channels in lipid bilayer membranes. We show that a
protein comprising only the N-terminal 162-amino-acid domain of OprF
formed the smaller, but not the larger, channels in lipid bilayers.
Circular dichroism spectroscopy indicated that this protein folds into
a OprF is a major outer membrane
protein in Pseudomonas aeruginosa that has been studied
extensively due to its proposed utility as a vaccine component, its
role in antimicrobial drug resistance, and its porin function (3,
6, 7, 13, 20). It has been shown to be required for cell growth
in low-osmolarity medium and for the maintenance of cell shape
(21). Through epitope-mapping experiments and linker
insertion mutagenesis, we originally proposed a 16-
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
The Amino Terminus of Pseudomonas aeruginosa
Outer Membrane Protein OprF Forms Channels in Lipid Bilayer Membranes:
Correlation with a Three-Dimensional Model
ABSTRACT
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-sheet-rich structure, and three-dimensional comparative modeling
revealed that it shares significant structural similarity with the
amino terminus of the orthologous protein Escherichia coli
OmpA, which has been shown to form a -barrel. OprF and OmpA share
only 15% identity in this domain, yet these results support the
utility of modeling such widely divergent -barrel domains in three
dimensions in order to reveal similarities not readily apparent through
primary sequence comparisons. The model is used to further hypothesize
why porin activity differs for the N-terminal domains of OprF and OmpA.
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Abstract
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-stranded
membrane topology model for OprF (19). However, on the basis
of deletion studies and secondary structure predictions, we recently
proposed a revised model with the N-terminal half of the protein
forming an eight-stranded -barrel domain that is inserted into the
outer membrane. The C-terminal half was proposed to form a domain that
is exposed and available to monoclonal antibody binding on the cell
surface (9) and binds peptidoglycan in the periplasm
(15). These two domains are linked by a proline-rich hinge-and-loop region that contains two disulfide bonds.
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FIG. 1.
Histograms of single-channel conductance measurements
showing channel size distributions for OprF (A) and
OprF1-162 (B).
A somewhat analogous structure has been proposed for the
Escherichia coli outer membrane protein OmpA (5, 12,
18), and these proteins, which also share some functional
similarities, are considered orthologs. Consistent with this concept,
significant amino acid sequence similarity has been detected between
OprF and OmpA, but only in their C-terminal domains (39% identity, 56% similarity). However, secondary structure predictions indicate that the N-terminal domains may also be similar, despite their lack of
substantial sequence identity (15% identity, with no regions of
similarity identified using BLAST2 with an "expect value" cutoff of
1,000). Recently, Pautsch and Schulz (12) solved a crystal structure for the N-terminal half of OmpA that was mutated at residues
23, 34, and 107 (in order to obtain crystals) and had been
reconstituted from inclusion bodies. Although the positioning of
surface loop regions could not be defined with certainty, the remainder
of the N terminus was shown to form an eight-stranded -barrel.
Pautsch and Schulz (12) also reported evidence (obtained through structural analysis and black lipid bilayer studies) that this
domain of OmpA did not form a membrane pore, although recently Arora et
al. (1) reported identifying very small channels, 0.05 to
0.08 nS, with this domain (using a protein containing four Trp-to-Phe
mutations and purified from outer membrane preparations under
denaturing conditions and refolded). Channels approximately 0.25 to 0.4 nS in size have been reported for the full-length OmpA protein (1,
16, 17). Since OprF has been previously shown reproducibly to
form small (0.36- to 0.38-nS) channels and, rarely, large (2- to 5-nS)
channels, and since in vivo experiments support this porin activity
(2, 3, 11, 20), we wondered whether the N-terminal domain of
OprF formed channels, and if so, whether the channels were of a size
similar to that of native OprF.
We therefore examined the pore-forming ability of a protein comprising
only the N-terminal domain of OprF (OprF1-162) that had
been purified under nondenaturing conditions from outer membranes. We
showed that this protein does indeed form small channels consistent
with those previously observed for native OprF, although no large
channels were observed. Circular dichroism (CD) spectral analysis and
three-dimensional modeling support a -barrel conformation for this
domain, and the modeling reveals similarities between OprF and OmpA in
this domain that are not apparent through primary sequence analysis.
These structural analyses permit us to hypothesize why the porin
activity differs for these domains of OprF and OmpA.
Purification of a protein comprising the N-terminal domain of OprF,
OprF1-162.
For this study, native OprF protein was
purified as previously described (2) from outer membrane
preparations of E. coli DH5
expressing OprF from plasmid
pRW5 (15). OprF1-162 was expressed in E. coli DH5 from the previously constructed plasmid pER163
(15). We found we were able to purify the
OprF1-162 by using the same procedure as for native OprF.
The identity of both proteins was confirmed through Western blot
analysis as described previously (10) using the monoclonal
antibody MA7-1, which is specific for an epitope within the N terminus
of OprF.
Planar lipid bilayer analysis of OprF and OprF1-162. OprF and OprF1-162 were assessed for pore-forming ability through planar lipid bilayer experiments, which were performed as previously described (3). Briefly, a 1 M KCl solution was placed within two compartments separated by a 0.1-mm3 circular hole that had been covered with a membrane formed from a solution of 1.5% oxidized cholesterol in n-decane. Electrodes were inserted into the KCl solutions in each compartment and a voltage of 50 mV was applied. When either an OprF or OprF1-162 protein sample (in 0.1% Triton X-100) was added to one of the compartments, stepwise increases in conductance were observed, indicating that channels were being formed in the membrane. Approximately 100 single-channel events were recorded for each experiment (Fig. 1).
For native OprF, small channels in the size range of those reported previously were observed (predominantly 0.4 nS) and, rarely (approximately 5% of events), larger channels (1 to 3 nS) were identified (Fig. 1). These larger channels were observed closely under conditions of low frequency of channel formation to ensure that they were not simply a reflection of multiple smaller channel events occurring simultaneously. For OprF1-162, small channel sizes in the range of 0.36 nS were frequently measured, but no channels of the larger size were observed (Fig. 1). These results suggest that the N-terminal half of OprF is able to form a pore and that the remainder of the protein, or a portion thereof, is required for the formation of the larger channels (perhaps through formation of alternate protein conformations). It should be noted that very small channels with a conductance of 0.04 to 0.08 nS were also frequently seen with both the OprF and OprF1-162 protein preparations (data not shown). However, similar-sized channels were also noted for a negative control sample that comprised a vector-only clone sample (E. coli with pUCP19) (14) after mock purification in the same manner as the OprF and OprF1-162 proteins.Structural analysis by indirect immunofluorescence of surface epitopes, and CD spectroscopy. To confirm that the OprF1-162 protein was folding in a conformation similar to that of the equivalent domain in wild-type OprF in our studies and was correctly localized to the cell surface, indirect intact E. coli/pER163 cells expressing OprF1-162 were examined by indirect immunofluorescence labeling using the monoclonal antibody MA7-1, which binds to a surface-exposed epitope, amino acids 55 to 62 in the OprF N terminus (14), as previously described (9). Cells expressing OprF1-162 were highly fluorescent, consistent with surface exposure of this epitope, while cells not expressing any OprF protein sequences showed no fluorescence (data not shown).
To evaluate the secondary structure of this OprF N-terminal domain, CD spectroscopy was performed on purified OprF1-162 by using a model J-70 spectropolarimeter (Jasco, Tokyo, Japan) connected to a Jasco data processor, using a quartz cell with a 1-mm path length. CD spectra were measured at 25°C, between 190 and 250 nm at a scanning speed of 10 m/min in 10 mM sodium phosphate buffer (pH 7.0) with 0.1% sodium dodecyl sulfate. The resulting spectrum (Fig. 2) was highly similar to that observed for antiparallel-sheet-rich proteins
(4), with a characteristic minimum at 217 nm. This is
consistent with the proposal that this domain forms a -barrel.
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Three-dimensional modeling.
The N-terminal half of OprF,
OprF1-162, shares only 15% identity with the
corresponding region of OmpA, OmpA1-171, yet secondary
structure prediction algorithms, CD spectroscopy results, and other
data (15) are consistent with these proteins sharing similar
-sheet secondary structures and thus indicate that
OprF1-162 may form a -barrel. Similarity of OprF and OmpA in the C terminus further supports an orthologous relationship between these proteins. We therefore attempted to model the OprF N
terminus using the published OmpA N-terminus crystal structure (12). We visually aligned the N-terminal 160 amino acids of OprF with the corresponding N-terminal 171 amino acids of OmpA used for
crystallization (Protein Data Bank Identification no. 1BXW)
(12). We used amino acid hydrophobicity, rather than identity, as a guide for constructing the alignment. The alignment was
further modified after a first round of modeling revealed that one
putative transmembrane -sheet strand was misaligned because a
charged residue was pointing out of the central barrel region into a
region of the lipid bilayer (final alignment shown in Fig.
3). Previous studies of OmpA
(8) and crystal structures of other outer membrane proteins
strongly indicate that charged residues are not permissive in such a
location in a -barrel protein. Using the Insight II (version 97.2)
molecular modeling program "Homology" (Molecular Simulations Inc.,
San Diego, Calif.), the OprF1-162 sequence was
threaded to the OmpA1-171 structure, constraining
regions that aligned with the -sheet regions of OmpA and allowing
more freedom in the formation of loop regions (which were not precisely
positioned in the OmpA model). The entire structure was then energy
minimized using the "Discover" program of Insight II (Fig.
4). The model is available from the
authors as a Protein Data Bank file, and animations and other images of the model may be viewed as supplementary data at
http://www.cmdr.ubc.ca/bobh/oprfmodel.html to aid visualization of its
three-dimensional structure.
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-barrel structures diverge
quickly in primary sequence from each other over time (relative to
other common protein folds) due to a lack of primary sequence
constraints while they remain structurally very similar.
There was one notable difference between the structure of
OmpA1-171 and the three-dimensional model of
OprF1-162 which we hypothesize could explain the
fact that no channels, or only very small channels (0.05 to 0.08 nS),
have been observed for the OmpA N-terminal domain, whereas we observed
channels of predominantly 0.36 nS with OprF1-162. Residues
previously implicated in blocking channel formation in the OmpA
N-terminal domain (12), or at minimum providing a
constriction in the pore, were noticeably not conserved in OprF, and
more significantly, the residues that replaced them in OprF permitted
the formation of a possible channel (Fig. 4B; see also supplementary
data). The previous study reporting this barrier in the pore
(12) also presented an alignment of OmpA orthologs,
suggesting that this barrier was conserved and that the OmpA -barrel
domain was more conserved than is noted for most porins. However, their
analysis was based on phylogenetically very similar organisms. Our
analysis of OprF suggests that this proposed constriction is not as
conserved as previously thought and that this -barrel domain is not
more conserved in primary sequence than has been observed for other porins.
The evidence presented here and in previous studies (15)
strongly suggests that the N-terminal half of OprF can form a
-barrel. A three-dimensional model for the N terminus of OprF is
proposed, and we support the benefit and utility of modeling proposed
orthologous outer membrane proteins in three-dimensional space, even if
they share little sequence identity. There is currently a need for better transmembrane -strand prediction algorithms for outer membrane proteins. Based on our experience studying outer membrane proteins and on the studies of others, we propose that an
amphipathicity plot that pays particular attention to the location of
hydrophobic residues and to preferential placement of aromatic residues
at the membrane-solvent interface, as well as some of the specific residue constraints reported by Koebnik (8), may be the most effective way to identify transmembrane -strands. This is
particularly important given the significant lack of sequence identity
constraints required by a -barrel structure.
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ACKNOWLEDGMENTS |
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We thank Annett Rozek for helpful comments regarding the three-dimensional modeling studies.
R.E.W.H. was a recipient of the Medical Research Council of Canada (MRC) Distinguished Scientist Award and received funding from MRC. This work was funded in part by the Canadian Cystic Fibrosis Foundation.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Microbiology and Immunology, 300-6174 University Blvd., University of British Columbia, Vancouver, British Columbia, Canada V6T 1Z3. Phone: (604) 822-2682. Fax: (604) 822-6041. E-mail: bob{at}cmdr.ubc.ca.
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Journal of Bacteriology, September 2000, p. 5251-5255, Vol. 182, No. 18
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Copyright © 2000, American Society for Microbiology. All rights reserved.
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