Biochemistry and Regulation of a Novel Escherichia coli K-12 Porin Protein, OmpG, Which Produces Unusually Large Channels

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Journal of Bacteriology, September 1998, p. 4452-4459, Vol. 180, No. 17
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Biochemistry and Regulation of a Novel Escherichia coli K-12 Porin Protein, OmpG, Which Produces Unusually Large Channels

Daniel A. Fajardo,¹ Joyce Cheung,² Chikako Ito,³ Etsuko Sugawara,³ Hiroshi Nikaido,³ and Rajeev Misra¹^,²^,^*

Department of Microbiology¹ and Molecular and Cellular Biology Program,² Arizona State University, Tempe, Arizona 85287-2701, and Department of Molecular and Cell Biology, University of California, Berkeley, California 94720-3206³

Received 10 April 1998/Accepted 26 June 1998

	ABSTRACT

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A novel porin, OmpG, is produced in response to a chromosomal mutation termed cog-192. Molecular characterization of cog-192revealed that it is a large chromosomal deletion extending fromthe 3' end of pspA through to the 5' end of an open reading framelocated immediately upstream of ompG. As a result of this 13.1-kbdeletion, the expression of ompG was placed under the controlof the pspA promoter. Characterization of OmpG revealed that itis quite different from other porins. Proteoliposome swellingassays showed that OmpG channels were much larger than those ofthe OmpF and OmpC porins, with an estimated limited diameter ofabout 2 nm. The channel lacked any obvious solute specificity.The folding model of OmpG suggests that it is the first 16-stranded $beta$ -barrel porin that lacks the large external loop, L3, which constrictsthe channels of other nonspecific and specific porins. Consistentwith the folding model, circular dichroism showed that OmpG containslargely a $beta$ -sheet structure. In contrast to other Escherichiacoli porins, there is no evidence that OmpG exists as stable oligomers.Although ompG DNA was present in all E. coli strains examinedso far, its expression under laboratory conditions was seen onlydue to rare chromosomal mutations. Curiously, OmpG was constitutivelyexpressed, albeit at low levels, in Salmonella, Shigella, andPseudomonas species.

	INTRODUCTION

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The outer membrane of gram-negative bacteria provides a barrier against noxious agents in the environment. Escherichia coliK-12 contains a set of outer membrane porin proteins that formchannels allowing an influx of nutrients (for reviews, see references3, 21, and 25). Two porins, OmpF and OmpC, often regardedas the classical porins, allow the flow of water-soluble soluteswith molecular weights of around 500 or less (20, 25). Althoughthese general pores lack any pronounced solute specificity, theyare weakly cation selective. The PhoE porin is structurally similarto the classical porins and forms general diffusion pores witha preference for anionic solutes (26). Other porins can specificallyfacilitate the uptake of substrates such as maltodextrins (LamB[40]) and nucleosides (Tsx [15]). OmpA was initially thoughtto play only a structural role, but recent in vitro studies haveshown that this protein also displays weak channel activity (37).Similarly, TolC has been shown to form channels in vitro (3).

In the last decade, publications pertaining to structure-function analysis of the porins provided a better understanding oftheir molecular anatomy. A major breakthrough came with the three-dimensionalstructural resolutions of OmpF (6) and PhoE (6, 10). Themonomeric subunit of each of these homotrimeric porins consistsof 16-stranded antiparallel $beta$ barrels enclosing the transmembranepore. The pore entrance is narrowed by long external loops, andthe middle of the channel is constricted by the inward foldingof loop L3, while its cross section increases abruptly just afterthis constriction zone (facing the periplasm). Proof that theconstricted area defines the filtering ability of the channelscame from genetic studies (2, 16, 17).

The classical porin proteins exist as trimers that display unusually stable structural properties (28). They form trimersthat resist denaturation by strong anionic detergents such assodium dodecyl sulfate (SDS). This high stability results fromhydrophobic and electrostatic interactions between the subunits(6). Porin proteins do not contain long stretches of hydrophobicresidues; instead, every alternate residue facing the lipid bilayeris hydrophobic. The presence of negatively charged residues onthe outer surface allows these exposed surfaces to interact withthe negatively charged groups of lipopolysaccharide via divalentcation bridges (25).

Porin proteins are critical for bacterial growth. Porin-deficient strains grow slowly and accumulate mutations that permitexpression of new porin proteins. This finding led to the isolationof E. coli strains that acquired the ability to synthesize a newporin protein, NmpC (4). The origin of NmpC was linked to adefective prophage, QSR. Similarly, another porin, Lc, encodedby a lambdoid bacteriophage, was isolated (8). The OmpG porinwas discovered among mutants that gained increased outer membranepermeability in the absence of OmpF and LamB (18). However,unlike NmpC and Lc, OmpG is not encoded by a prophage genome.Normally LamB is required for transport of maltodextrins, sugarsthat are excluded from OmpF and OmpC channels because of theirlarge size. Thus, a LamB OmpF⁺ OmpC⁺ strain displays a maltodextrin-minus (Dex) phenotype. Strains with this composition revert to Dex⁺ at a low frequency (10⁹ to 10¹⁰). The mutations were mapped to four loci: ompF (2), ompC (16,17), imp (30), and cog (18). cog (for control of ompG) mutationsresulted in the appearance of a new outer membrane protein, OmpG.Growth and uptake experiments showed that OmpG displays a porin-likeactivity. Genetic experiments indicated that cog itself may codefor a negative regulator of OmpG expression (18).

In this report, we provide data showing that OmpG defines a novel class of porin protein whose sequence, biochemical properties,and channel properties are distinct from those of known bacterialporins.

	MATERIALS AND METHODS

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Media. Luria broth and MacConkey media (both from Gibco) were prepared as described previously (33). The amount of maltodextrins(Pfsanstiehl) added to the MacConkey medium differed between preparationsof the maltodextrin stock solution. The stock solution of maltodextrinswas titered by determining the amount of maltodextrins neededto yield red colonies for an OmpG⁺ strain (RAM123) and white colonies for an OmpG strain (DME553).

Bacterial strains and lambda phages from Kohara library. The laboratory E. coli K-12 strains used in this study were derived from DME553 ( $Delta$ lamB106 $Delta$ ompF80). RAM123 is a Dex⁺ derivative of DME553 that produces OmpG due to the cog-192 mutation(18). RAM194 was derived from RAM123 by transducing the $Delta$ ompC178allele through a linked Tn10, thus making the resulting strainOmpC. HS3169 (malK::Tn10) was obtained from Howard Shuman. StrainsK1342 [ $lambda$ psp3.2; $Phi$ (pspA'-lacZ)] and K1472 ( $Delta$ pspABC::kan) were kindlyprovided by Peter Model. All other E. coli strains were obtainedfrom E. coli Genetic Stock Center. Salmonella typhimurium LT2(ompD⁺) and CH338 (ompD) were kindly provided by Ken Sanderson. Shigellaflexneri serotype 2a (ATCC 9473) was obtained from the AmericanType Culture Collection. Pseudomonas aeruginosa PAO1 was fromour laboratory strain collection. Clinical isolates of Salmonellastrains were made available to us by Micah Williams. Lambda clones250 through 260 from Kohara phage library (12) and E. coli LE392for their propagation were kindly provided by Frederick Blattner.

Protein methods. Cell envelopes were prepared by the French press lysis method as described previously (19). Proteins were analyzed by electrophoresisthrough SDS-polyacrylamide (11%) gels (SDS-PAGE) (14). The followingmethods were used for OmpG purification. When OmpG was neededfor raising antibodies or protein sequencing, envelopes obtainedfrom a strain lacking OmpA, OmpC, OmpF, and LamB but producingOmpG from a plasmid were treated with 0.5% SDS in 50 mM Tris-HCl(pH 8.0) for 1 h at 37°C. SDS-solubilized proteins were removedby centrifugation at 18,000 × g for 30 min. The pellet was resuspendedin the SDS sample buffer (2% SDS, 10% glycerol, 5% $beta$ -mercaptoethanol,50 mM Tris-HCl [pH 6.8]) and solubilized by boiling for 5 min.Solubilized samples were analyzed by SDS-PAGE, and the gel wasstained with Coomassie blue. The OmpG band was excised and electroelutedin a Bio-Rad electroelutor. Eluted OmpG samples were concentratedby ethanol precipitation at $-$ 20°C. The pellet was resuspendedin 20 mM HEPES (pH 7.4) or double-distilled H₂O for protein sequencedetermination.

For proteoliposome swelling assays, OmpG was partially purified from envelopes by a two-step detergent solubilization method.Envelopes lacking all major outer membrane proteins except OmpGwere resuspended in 0.5% n-octylglucoside (OG)-10 mM HEPES (pH7.4) and incubated for 30 min at 37°C. The pellet recovered bycentrifuging samples at 436,000 × g for 30 min was resuspendedin 1.0% OG-10 mM HEPES (pH 7.4). After incubation for 30 min at37°C, samples were centrifuged as described above, and the supernatantcontaining primarily OmpG was recovered. Extract containing 0.2µg of protein was used for reconstitution of proteoliposomes asdescribed previously (13) except that (i) a 30:2 mixture ofacetone-washed phosphatidylcholine (Avanti Polar Lipids) and dicetylphosphate(Sigma) was used instead of E. coli phospholipids and (ii) dextranT-40 (Pharmacia) was used instead of dextran T-20. Proteoliposomescontaining the dextran were diluted into iso-osmotic solutionsof various solutes, and the permeation rates were measured bythe initial rates of decrease of optical density of proteoliposomesuspension (13).

OmpG for circular dichroism measurement was purified as follows. The outer membrane fraction of RAM194 was isolated by sucrosedensity centrifugation and extracted with 2% octyl-polyoxyethylene(Alexis Biochemicals). The extract was applied to a Bio-Rad DEAE-5PWhigh-pressure liquid chromatography column, which was eluted witha 0 to 0.5 M linear gradient of NaCl in 10 mM Tris-HCl (pH 8.0)-1mM EDTA-0.2% Lubrol PX. The fraction containing essentially pureOmpG was dialyzed against the buffer just mentioned but withoutNaCl, and its spectrum was measured, after concentration by ultrafiltrationwith Amicon PM-10 membrane, with an Aviv model 62DS circular dichroismspectrometer.

Antibodies were raised as described previously (19). For protein sequence analysis, electroeluted OmpG in double-distilledH₂O was acidified with trichloroacetic acid and dissolved withacetonitrile. Approximately 100 pmol of OmpG protein was spottedon a fiberglass disk (Beckman) and sequenced in a Proton 2090protein sequencer (Beckman). For Western blot analysis, proteinsamples analyzed by PAGE were transferred to Immuno-Lite membranes(Bio-Rad), using a Mini Trans-Blot electrophoretic transfer cell(Bio-Rad). The Western blot analysis was carried out with solutionsobtained from Bio-Rad and a 1:5,000 dilution of the OmpG antiserum.

DNA and RNA methods. ompG⁺ plasmid clones were obtained by transforming an OmpG strain with a Sau3A chromosomal gene bank, prepared from an ompG⁺ strain, and selecting for Dex⁺ (red) colonies on MacConkey-maltodextrin-ampicilliln (50 µg/ml)medium. Confirmation that the Dex⁺ phenotype was conferred by the expression of OmpG from a plasmidwas obtained by retransforming the plasmid into an OmpG strain and observing the Dex phenotype of transformants. cog⁺ plasmid clones were also obtained from a Sau3A chromosomal genebank. The DNA sequence of cloned DNA was determined by the dideoxy-chaintermination method (31). Sequence analysis was carried out withsoftware packages from Genetics Computer Group Inc. (Universityof Wisconsin, Madison) and DNAMAN (Lynnon BioSoft). Lambda phageswere purified through CsCl isopycnic gradients, and DNA was extractedas described previously (29). Chromosomal DNA and total RNAwere isolated by a kit obtained from Amersham Life Science. Restrictionenzyme digestions were carried out as instructed by the manufacturer.Southern and Northern analyses were carried out by standard protocols(29). Nucleic acids were cross-linked to Quantum Yield filters(Promega) in a Stratalinker (Stratagene). Nonradioactive hybridizationprobes were prepared by using a random-primer fluorescein labelingkit (Du Pont-NEN).

Nucleotide sequence accession number. Nucleotide sequences of the ompG gene and an upstream open reading frame (orf1) were assigned GenBank accession no. ECU49400.

	RESULTS

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Genetic mapping and cloning of ompG. Genetic mapping of ompG was facilitated by the isolation of linked transposon insertions. To obtain such insertions, a transposon(Tn10) insertion pool was prepared in a wild-type strain. TheTc^r (from Tn10) marker from this pool was transduced into an ompG⁺ (Dex⁺ Cog) strain so as to obtain insertion mutations that prevented OmpGexpression (Dex phenotype). These Tn10s were genetically mapped and found tobe located at the 29-min region of the chromosome where cog hadbeen previously mapped (18). Once ompG sequencing was completed(see below), ompG-specific primers were used to confirm the geneticlocation of ompG by using Kohara clones encompassing the 29-minregion of the chromosome (12). Of the several Kohara clonesused, two covering min 29.5 to 29.7 of the E. coli chromosomeyielded ompG-specific fragments. Also, Southern blot analysisof Kohara clones with an ompG-specific probe confirmed its geneticlocation in the chromosome (data not shown).

The Tn10 insertion mutations resulting in a Dex (OmpG) phenotype were found to be recessive, which allowed procurement ofan ompG⁺ (Dex⁺) clone by complementation using an E. coli gene library. Theoriginal ompG⁺ plasmid clone contained a 5.5-kb chromosomal DNA insert. Subsequentsubcloning showed that a 2.6-kb DNA fragment contains sufficientinformation for OmpG expression. The expression of OmpG from theseplasmid clones was not repressible by either chromosomal or plasmid-borneCog (data not shown). Gene dosage experiments showed that thelack of repression was not due to a possible titration of therepressor by an excessive number of operator sites. A reorientationof the ompG⁺ DNA insert with respect to the plasmid-borne Tc^r gene promoter resulted in no detectable OmpG expression, showingthat the ompG⁺ clone lacked promoter sequences and possibly the site neededfor Cog-mediated repression.

Nucleotide sequence analysis of the ompG region. The nucleotide sequence of the entire 2.6 kb of insert DNA was determined and found to match perfectly the published sequence(5). Two ORFs (orf1 and orf2) within the ompG⁺ DNA insert were identified; orf2 corresponded to OmpG. orf2 starts157 bp downstream from the end of orf1 and encodes a 301-residue-longprotein. The amino-terminal end of Orf2 contains a typical signalsequence motif of 21 amino acid residues. A 14-amino-acid NH₂-terminalsequence of the purified OmpG was identical to residues 22 to35 deduced from DNA sequence of orf2, confirming that OmpG iscoded by orf2.

OmpG is a novel porin protein. At the amino acid sequence level, OmpG shows no significant homology with other proteins in the data bank. Direct alignmentof the OmpG sequence with the OmpF and OmpC sequences displayeda low overall random identities of 22% (16 alignment gaps) and16% (13 alignment gaps), respectively. That these identities areonly superficial became apparent when we compared the primarysequence of OmpA with those of structurally and functionally unrelatedproteins, OmpF and OmpC. Here again, the overall random identitieswere 22% (17 alignment gaps) between OmpA and OmpF and 17% (11alignment gaps) between OmpA and OmpC. Finally, a low overallrandom identity of 17% (10 alignment gaps) was observed betweenOmpG and OmpA. On the other hand, between the two related proteinsOmpF and OmpC, a striking 64% overall identity was observed withonly seven alignment gaps.

Immunoblot analysis of filters containing purified E. coli OmpG, OmpC, OmpF, and LamB proteins showed no cross-reactivityof polyclonal OmpG antibodies with these proteins (data not shown).Furthermore, blotting of envelopes containing OmpA also gave negativesignals. As expected, antibodies reacted strongly with eitherthe purified OmpG protein or OmpG present in envelopes. Thus,OmpG is novel, as it shares neither sequence similarity nor antigenicoverlap with the previously characterized outer membrane proteinsof E. coli.

In certain respects, however, OmpG is related to other outer membrane proteins of E. coli. (i) Apart from its signal sequence,OmpG lacks any long hydrophobic stretches. (ii) OmpG, like someother porin proteins, lacks cysteine residues in its mature portion.(iii) The last residue of OmpG is phenylalanine, which is thoughtto be important for the proper insertion or assembly of outermembrane proteins (36). (iv) Like many outer membrane proteins,OmpG contains a preponderance of negatively charged residues (50Asp and Glu, compared to 22 Arg and Lys), with an estimated pIof 4.4.

Circular dichroism and folding patterns of OmpG. To gain a better understanding of the secondary structure of OmpG, detergent-solubilized OmpG retaining its full channel activitywas analyzed by circular dichroism (Fig. 1). The ellipticity patternshowed a minimum of a fairly small magnitude, close to 210 nm.This showed that in contrast to OmpA (38), there was littlecontribution from $alpha$ -helical structures and that OmpG had a largely $beta$ -sheet structure, similar to the classical porins. Based on thefolding prediction methods of Schirmer and Cowan (predicts transmembranestretches [32]) and Paul and Rosenbusch (predicts turns [27]),the mature portion of OmpG is predicted to have 16 transmembranesegments (Fig. 2, boxed regions). The amino acids at alternatepositions within transmembrane segments are primarily hydrophobicresidues that are predicted to have their side chains orientedoutward toward the lipid environment. In general, the internalloops are smaller than those present on the outside, where thereis a distinctive absence of an especially large loop, L3, a hallmarkof the classical porins, where such a loop is shown to narrowthe middle of the channel (6). The predicted OmpG folding modelcan now be tested by genetic and molecular means.

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FIG. 1. Circular dichroism analysis of purified OmpG. Purification and measurement were carried out as described in Materials and Methods. The magnitude of mean residue ellipticity (about $-$ 5,000 deg² dmol¹) is significantly smaller than that found with OmpA or P. aeruginosa OprF ( $-$ 9,000 to $-$ 10,000 deg² dmol¹ [38]), two outer membrane proteins that contain substantial $alpha$ -helical domains. The spectrum also does not show the two sharp negative peaks at 208 and 220 nm, which are characteristic of $alpha$ helices.

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FIG. 2. Predicted folding pattern of OmpG. The OmpG amino acid sequence was analyzed by using computer programs based on the algorithms of Schirmer and Cowan (32) and Paul and Rosenbusch (27). Transmembrane $beta$ strands were predicted whenever a high value of hydrophobicity on alternate residues in a 10-residue stretch was found, and this prediction was strengthened by the presence of turn-promoting sequences on either side. Most of the transmembrane segments could be assigned unequivocally, but the presence of the 12th and 13th segments is less convincing, as the hydrophobicity of the alternate residues is not high.

OmpG is a heat-modifiable protein. We have previously reported that unlike OmpF and OmpC, OmpG is not strongly associated within the cell envelope, as it canbe completely solubilized with 1% SDS or Triton X-100 in the absenceof high salt concentrations (18), a condition that does notallow solubilization of the classical porins. However, under mildersolubilization conditions, such as treatment with 0.5% SDS orOG, the majority of OmpG remained associated with the membrane(Fig. 3). Interestingly, under these solubilization conditionswhen envelopes were analyzed by SDS-PAGE without heating, OmpGdid not migrate at its denatured position of 34,000 mol wt butinstead appeared as a faster-migrating species of 28,000 mol wt(Fig. 3, lane 7). Immunoblot analysis confirmed that this faster-migratingpolypeptide corresponds to OmpG (data not shown). The treatmentof envelopes with 1% OG led to the complete solubilization ofOmpG without altering its heat-modifiable property. However, subsequentremoval of OG by dialysis led to loss of this property (Fig. 3,lane 8). As shown below, both dialyzed and undialyzed preparationsof OmpG were competent in forming active channels in proteoliposomeswelling assays. The dialysis therefore appears to make the OmpGmore susceptible to complete denaturation by SDS, presumably byremoving stabilizing factors.

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FIG. 3. SDS-PAGE analysis of envelopes and detergent-solubilized OmpG. Lane 1, untreated envelopes obtained from a strain lacking OmpF, OmpC, LamB, and OmpA; lane 2, pellet after OG extraction; lane 3, supernatant of 0.5% OG extraction; lane 4, supernatant of 0.5 and 1% OG extraction; lane 5, same as lane 4 but dialyzed against 10 mM HEPES (pH 7.4) buffer; lane 6, unheated envelopes; lane 7, same as lane 4 but unheated; lane 8, same as lane 5 but unheated. Positions of denatured OmpG and heat-modifiable OmpG (OmpG*) are shown. Samples present in lanes 1 to 5 were heated by boiling for 5 min prior to SDS-PAGE analysis.

In vitro channel properties of OmpG. In vivo growth and uptake experiments showed that OmpG has a porin-like activity that allows the influx of larger solutesthan do the classical porins (18). Proteoliposome swelling assays(22, 23) were carried out to confirm the in vivo data.

Proteoliposomes were reconstituted from phosphatidylcholine and unfractionated outer membrane fragments from a strain lackingOmpF, OmpC, and LamB but containing OmpG. The influx of sugarswas measured by the osmotic swelling of these vesicles. Severalconclusions can be made from these experiments (Fig. 4). (i) OmpGproduces fairly efficient channels. The rate of influx for a pentose,L-arabinose, was similar to that seen for proteoliposomes reconstitutedwith similar amounts of OmpC. Thus, at least for sugars, OmpGfunctions as well as the classical trimeric porins of E. coli.(ii) OmpG channels behaved strikingly differently from OmpF andOmpC when disaccharides were used. OmpF and OmpC showed disaccharidediffusion rates around 1 to 2% of the rate of L-arabinose diffusion(also see reference 24). In contrast, OmpG channels behavedas though they were much larger, allowing the diffusion of disaccharidesat rates corresponding to 15 to 30% of the rates of L-arabinose.This behavior is very similar to that of the P. aeruginosa porinOprF, where a limiting pore diameter of 2.0 nm has been calculated(42). OprF, however, is different from OmpG in its low efficiency.Isolated OmpG (purified by solubilization in OG and fractionatedby ion-exchange chromatography) and OmpF preparations were alsoused in proteoliposome swelling assays. The results validatedthe above finding, showing that OmpG channels were functionallylarger than those of OmpF when a disaccharide (sucrose) and atrisaccharide (raffinose) were used. Calculations by the approachof Nikaido and Rosenberg (22) show that the dependence of permeabilityon solute size fits best with a pore diameter of about 20 Å. Sincethe distance between neighboring $beta$ strands is 4.5 Å, a $beta$ barrelwith 16 transmembrane strands will have a diameter of 23 Å, measuredbetween $alpha$ -carbon atoms. With the amino acid side chains protrudinginto the interior of this barrel, the 20-Å average diameter isconsistent with our model.

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FIG. 4. Rates of penetration of various sugars through the OmpG channel. Proteoliposomes containing OmpG extract were made as described in Material and Methods, and portions of the suspension were diluted into iso-osmotic solutions of sugars to determine the rates of osmotic swelling of the vesicles. The rates were normalized to the swelling rate in L-arabinose, which was taken as 100%. The sugars used (and, in parentheses, their molecular weights) were L-arabinose (150), D-glucose (180), N-acetylglucosamine (221), 2,3-diacetamido-2,3-dideoxy-D-glucose (262), lactose (342), sucrose (342), and maltose (342). As a control, proteoliposomes containing OmpC extract were used.

Dialyzed and undialyzed preparations yielded very similar solute diffusion rates, suggesting that the loss of heat modifiability(Fig. 3) did not result from the denaturation of the protein.Using maltose, lactose, sucrose, trehalose, and (GIY)₄ peptidein proteoliposome swelling assays, we failed to see any evidenceof solute specificity for OmpG channels.

Outer membrane permeability of OmpG⁺ strains. We have shown above that OmpG produces a larger channel than OmpF or OmpC. Furthermore, OmpG is expressed in strain RAM194at a level similar to that of the classical porins in other K-12strains (18). We might expect that an abundant expression ofa large-channel porin would make the cells hypersensitive to inhibitorsand antibiotics. We therefore tested the susceptibility of strainsDME553 (OmpC⁺), RAM123 (OmpC⁺ OmpG⁺), and RAM194 (OmpG⁺) to hydrophilic (ampicillin and chloramphenicol) and hydrophobic(novobiocin and rifampin) antibiotics. Cells expressing OmpG showedhypersensitivity to hydrophilic antibiotics: paper disks (7-mmdiameter) presoaked with 10 µg of ampicillin or 5 µg of chloramphenicolgave inhibition zones of 13 mm in DME553 but around 18 mm in RAM123or RAM194. In contrast, only a slight increase in sensitivitytoward hydrophobic antibiotics was noted in cells expressing OmpG.These results further corroborated the above finding that thechannel formed by OmpG is larger than those formed by the classicalporins.

OmpG lacks stable oligomeric forms. The majority of porin proteins exist as homotrimers. However, the following experiments suggest that OmpG is monomeric porin.First, we carried out two-dimensional PAGE analysis (first dimensionunder native and second dimension under SDS-denaturing conditions)to look for evidence that OmpG is an oligomeric porin. We coulddetect OmpF trimers but no oligomeric forms of OmpG. Second, wecarried out cross-linking experiments using dimethylsuberimidateand formaldehyde. In these experiments, either purified envelopes,OG-solubilized extracts, or whole cells were used. SDS-PAGE followedby immunoblot analysis did not reveal any evidence of cross-linkedOmpG, although oligomeric forms were visible with OmpF (data notshown).

Expression of OmpG in other gram-negative bacteria. Immunoblot analysis using OmpG-specific antibodies showed the presence of a cross-reacting protein band with similar sizesin membranes of S. flexneri and S. typhimurium and even in P.aeruginosa, which does not belong to the family Enterobacteriaceae(Fig. 5). In addition to being detected in S. typhimurium LT2,OmpG expression was detected in several clinical Salmonella isolatesgrown under our standard laboratory conditions (data not shown).It is curious that unlike in our E. coli strains, where OmpG isnot expressed, it is produced, albeit apparently at a low level,in other bacterial species. It is conceivable that the lack ofOmpG expression in our contemporary K-12 strains was due to chromosomalaberrations caused by the heavy mutagenesis used to constructthese strains in the first place or that optimum growth conditionsfor its expression have not been found. Attempts to define growthconditions under which OmpG is expressed without mutations haveso far been unsuccessful. To test the first hypothesis, we examinedwild-type E. coli K-12 strains 679, Y10, W1, and AB1157, E. coliB, E. coli C, and E. coli K1 for OmpG expression by Western blotanalysis. We failed to see OmpG from these strains. However, allstrains yielded ompG-specific DNA fragments by PCR analysis.

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FIG. 5. Immunoblot analysis of OmpG from envelopes of various gram-negative bacteria. Lanes 1 and 2 contain envelopes (1.5 µg of protein) from OmpG and OmpG⁺ E. coli strains, respectively; lanes 3 to 7 contain 0.75, 1.5, 3, 6, and 12 µg of total protein, respectively. Gels were blotted with polyclonal antibodies raised against E. coli OmpG.

Unlike E. coli, S. typhimurium contains three constitutively expressed porins, OmpD in addition to OmpF and OmpC (25). Immunoblotanalysis using OmpG antibodies on envelopes prepared from OmpD⁺ and OmpD (ompD::Tn10) strains showed the presence of a cross-reactingprotein band in both strains (data not shown). That OmpG is unrelatedto OmpD was not surprising because we already knew that OmpG isunrelated to OmpF and OmpC, which show high antigenic and sequenceconservation with OmpD (34, 35).

Regulation of OmpG: cloning of cog⁺. By using conventional genetic mapping methods, cog-192 was mapped at 29 min on the chromosome (18). Diploid analysis revealedthat cog-192 was recessive, suggesting that it may disable theactivity of a repressor protein that negatively controls ompGexpression. However, the low frequency by which cog-192 was isolatedsuggested that it is not a simple null mutation. The recessivenature of the cog-192 mutation permitted the isolation of a plasmidclone containing the wild type cog⁺ gene from an E. coli gene bank by genetic complementation. TheDNA insert carrying cog⁺ was roughly 10 kb long and thus likely to contain other genesthat may or may not be relevant to cog function. The originalcog⁺ clone was reduced to half its size by removing a restrictionfragment. When introduced into an OmpG⁺ (Dex⁺) strain, this shorter clone still conferred an OmpG (Dex) phenotype. Partial DNA sequencing from either end of the clonerevealed the presence of truncated aldH on the one end and truncatedpspC on the other. Four ORFs organized in the order aldH-goaG-pspF-pspA-pspB-pspChave been identified between these two genes (5, 11). Twosmaller plasmid clones retaining both pspA and pspB (a 1.8-kbBglII-SalI fragment) or just pspA (an 800-bp BglII-EcoRI fragmentin which the EcoRI site was created immediately downstream frompspA by site-directed mutagenesis) also complemented the cog-192mutation. This showed a possible involvement of pspA in the regulationof OmpG expression.

Three additional observations strengthened the notion that cog-192 allows OmpG expression by somehow affecting the psp operon:(i) both cog-192 and psp map at 29 min on the E. coli chromosome,(ii) an introduction of $Delta$ pspA::Km^r abolishes OmpG expression; and (iii) consistent with a proposalthat pspA is autoregulated (41), we found that the presenceof the cog-192 mutation elevates the activity of a pspA::lacZconstruct 10-fold.

Molecular characterization of cog-192. Complementation of cog-192 by plasmid clones bearing just the pspA gene provided evidence that cog-192 may define a chromosomalaberration affecting pspA gene function. When we used pspA-specificprimers to amplify DNA from cog⁺ and cog-192 strains by PCR, only the cog⁺ strain yielded the pspA fragment. The psp region was also examinedby Southern blot analysis using three different probes, specificto pspA, b1312 to 1313, and ompG (Fig. 6). The data revealed thatin the cog-192 strain, regions corresponding to the pspA and b1312to 1313 probes were missing (Fig. 6). The ompG-specific proberevealed a substantial alteration in the genome immediately upstreamto the ompG gene (Fig. 6).

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FIG. 6. Molecular organization of the chromosomal region encompassing ompG and the psp operon. Ten uncharacterized genes (b1309 to 1317 and orf1) are present between ompG and the psp operon. These 10 ORFs as well as a significant portion of the psp operon are deleted (marked by dotted lines) in the cog-192 strain. The deletion aligns ompG with the pspA promoter; precise ends of the deletion are shown in a close-up diagram below. Double-headed arrows show DNA probes used in Southern and/or Northern blot analysis. Locations of various primers and of restriction enzyme sites are shown at the top. Abbreviations: B, BglII; C, ClaI; N, NcoI; and S, SalI.

cog-192 defines a large chromosomal deletion. In the cog⁺ strain, the pspF and ompG genes are separated by about 14.0 kb. Thus, under standard PCR conditions, it may notbe possible to amplify a 14.0-kb intervening DNA fragment withprimers specific to pspF and ompG. However, if this distance issignificantly reduced, it should become possible to PCR amplifyDNA by pspF forward and ompG reverse primers. To test this, weused two forward primers that were complementary to the goaG/pspFregion and four reverse primers that were complementary to theorf1/ompG region (Fig. 6). As anticipated, no DNA fragments couldbe amplified from the cog⁺ strain. On the other hand, all but one set of primers yieldedDNA fragments from the cog-192 strain. Amplified DNA fragments,however, were much shorter than expected from a genome where theregion between pspF and ompG was intact, showing that these tworegions are now immediately adjacent to each other in the cog-192strain.

PCR-amplified DNA from the cog-192 strain was used for nucleotide sequence analysis to pinpoint the deletion junction. Theresults showed that the region between pspA and orf1, includingthe last 369 (of 666) bp of the pspA gene and the first 685 (of969) bp of orf1 were deleted in the cog-192 strain (Fig. 6). Thisshowed that cog-192 defined a large chromosomal deletion of atotal of 13,127 bp between the pspF and ompG genes.

cog-192 creates a transcriptional fusion between pspA' and ompG. As mentioned above, the expression of OmpG in the cog-192 strain was turned off by the presence of a pspA⁺ plasmid, indicating that PspA somehow controls OmpG expressionin this strain. One explanation for this observation could bethat the cog-192 deletion resulted in ompG being placed underthe control of a pspA promoter. Since the pspA promoter is regulatedby the pspA gene product (41), the presence of a multicopy pspA⁺ plasmid would be expected to have a negative effect on its activityand hence ompG expression. This possibility was tested by Northernblot analysis of ompG mRNA (Fig. 7).

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FIG. 7. Northern blot analysis to detect ompG-specific transcripts. Total RNA (3 µg) obtained from DME553 (cog⁺; lanes 1 and 7), RAM123 (cog-192; lanes 2 and 8), RAM123 recA::Km^r (lane 3), RAM123 recA::Km^r/pBR322 (lane 4), RAM123 recA::Km^r/pBR322-pspFAB (lane 5), and RAM123 recA::Km^r/pBR322-pspA (lane 6) was probed with an ompG-specific probe. Molecular sizes of the two ompG-specific mRNA species are 1.4 and 2.0 kb.

No ompG-specific transcripts were detected from a cog⁺ strain (Fig. 7; lanes 1 and 7). In contrast, two ompG-specific transcriptswere detected from the cog-192 strain (lanes 2 and 8). These transcriptswere either absent (lane 5) or present in a greatly reduced amount(lane 6) when the cog-192 strain was transformed with a plasmidbearing pspFAB or pspA, respectively. These results showed thata promoter that is negatively regulated by the pspA gene productcontrols ompG transcription in the cog-192 strain. Northern analysisalso revealed the presence of two ompG-related transcripts thatwere regulated in the same fashion (Fig. 7). One interpretationof this observation is that the two transcripts initiated fromthe same promoter but were terminated at different points.

Chromosomal deletions are necessary for OmpG expression. We sought additional Dex⁺ revertants from DME553 (cog⁺ Dex) to examine whether mutations other than deletions could permit OmpGexpression. Dex⁺ revertants were obtained from 10 independent cultures. Dex⁺ isolates expressing OmpG were estimated to be around 1% of thetotal Dex⁺ revertants obtained, as judged by Western blotting. PCR and Southernanalyses of the chromosomal DNA from five independently obtainedDex⁺ isolates revealed deletions upstream of ompG. In two isolates,the deletion extended beyond the entire psp operon; in three,the deletions retained pspA. As was the case for the cog-192 strain,OmpG expression in the latter three isolates was inhibited bya plasmid carrying pspA⁺. These results support the notion that deletions upstream ofthe ompG structural gene are necessary for OmpG expression underlaboratory growth conditions. These deletions must create noveljunctions between ompG and an upstream promoter element that maynot be genetically related to ompG in the parental strain.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The molecular and biochemical analyses presented in this study showed that OmpG is a unique class of porin. Consistent withour previous in vivo findings (18), the in vitro data revealedthat OmpG channels are functionally larger than those of the classicalporins. The major reason for large OmpG channels may be the absenceof a large external loop, L3, which in classical porins foldsback into the channel and serves to restrict pore size (6).Since the distance between neighboring strands in a $beta$ sheet is0.45 nm, the 16-membered $beta$ barrel predicted for OmpG (Fig. 2)will produce a channel with the diameter 0.45 × 16/ $pi$ = 2.3 nm.Considering that side chains will narrow the channel somewhat,this value is in perfect agreement with the diameter determinedby the solute size dependence of sugar flux (Fig. 6). If our modelis correct, OmpG is the first porin with such a simple barrelstructure.

Large OmpG channels mean that a greater variety of nutrients can be taken up by the bacteria, which would provide a growthadvantage to bacterial strains producing OmpG. Yet, OmpG expressionhas not been observed in wild-type E. coli strains obtained fromlaboratory collections. In contrast, OmpG expression has beenobserved in Salmonella and Shigella strains analyzed so far. Thelevel of expression, however, appears to be in the range of 10to 20% of the levels of classical porins, which may explain whythe presence of this porin was not noticed earlier. Future workshould address the significance of OmpG in these organisms. Itis conceivable that OmpG was a functional porin in the ancestorof present day Enterobacteriaceae and that its expression wasdown regulated or abolished in E. coli, which confronts the constantchallenge of toxic bile salts (39).

The discovery of OmpG showed the potential of bacterial genomes to code for a number of porin proteins. Of course, not allporins are expressed at the same time. Some, such as general porins,may be required under all growth conditions, although their relativelevels fluctuate in response to physiological parameters. Theseproteins are present in large quantities (around 10⁵ molecules/cell). However, solute diffusion through OmpF and OmpCchannels is not efficient, which may have contributed to the evolutionof bacteria with specialized porins, such as LamB and Tsx, whichare needed only under conditions of specific nutrient availability.Solute specificity for OmpG channels and physiological parametersregulating its expression are not known.

OmpG expression was achieved under laboratory conditions where the entry of large sugars was not possible through generalchannels. A mutation, cog-192, permitting OmpG expression turnedout to be a chromosomal deletion that removed 13.1 kb of DNA immediatelyupstream of ompG. This deletion placed ompG expression under thecontrol of the pspA promoter. The regulation data contrasted withour previous hypothesis that operator or repressor mutations derepressOmpG expression (18). Indeed, the recessive nature of cog-192and plasmid complementation data supported a repressor theory.Molecular analysis of cog mutations, however, demonstrated thatregulated expression of OmpG was the result of a novel gene fusion.Jacob and colleagues (1, 9) reported deletions fusing twounrelated operons where the downstream genes were also placedunder the transcriptional control of an upstream promoter forunrelated operon. Computer analysis of the nucleotide sequenceupstream of ompG did not reveal the existence of a $sigma$ ⁷⁰-dependent promoter element. It is conceivable that ompG and 10other ORFs sandwiched between it and the psp operon are not expressedin E. coli due to the absence of an active promoter.

Sequence homology data showed that several of these 10 uncharacterized ORFs may code for proteins involved in the transportor metabolism of sugars (5). Interestingly, orf1, located immediatelyupstream of ompG, shows a strikingly high identity with the ATPasecomponent of various ABC transporters (7). These componentsare usually associated with other proteins dedicated to the transportof a specific substrate, and genes coding for these other componentsare present in the vicinity of orf1. At this point it is unclearwhether orf1 and ompG are part of the same operon. Our data showedthat the OmpG-mediated Dex⁺ phenotype is dependent on the malK gene product of the mal operonbut not on orf1. Curiously, we found that orf1 sequences fromE. coli B and E. coli C strains had the capacity to encode a 360-residueprotein (compared to the 322-residue Orf1 from K-12). A truncationof Orf1 in E. coli K-12 was due to the presence of a natural frameshiftmutation (deletion of G) close to the end of the gene. The truncationof Orf1 may render the protein nonfunctional and/or highly susceptibleto proteolysis.

	ACKNOWLEDGMENTS

We thank Howard Shuman and Peter Model for bacterial strains. We are grateful to Peter Model for numerous valuable discussions.

This work was supported in part by grants from the Arizona Disease Control Research Commission and from the Public HealthService (GM-RO1 48167-06) to R.M. and by Public Health Servicegrant AI-09644 to H.N. D.A.F. was a recipient of a predoctoralfellowship from NIGMS. J.C. was supported from a graduate fellowshipfrom the Molecular and Cellular Biology program at ASU.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, Arizona State University, Tempe, AZ 85287-2701. Phone:(602) 965-3320. Fax: (602) 965-0098. E-mail: rajeev.misra{at}asu.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Ames, B. N., P. E. Hartman, and F. Jacob. 1963. Chromosomal alterations affecting the regulation of histidine biosynthetic enzymes of Salmonella. J. Mol. Biol. 7:23-42[Medline].

2. Benson, S. A., J. L. Occi, and B. A. Sampson. 1988. Mutations that alter the pore function of the OmpF porin of Escherichia coli K-12. J. Mol. Biol. 203:961-970[Medline].

3. Benz, R. 1994. Uptake of solutes through bacterial outer membranes, p. 397-423. In J.-M. Ghuysen, and R. Hakenbeck (ed.), Bacterial cell wall. Elsevier Science, Amsterdam, The Netherlands.

4. Blasband, A. J., W. R. Marcotte, Jr., and C. A. Schnaitman. 1986. Structure of the lc and nmpC outer membrane porin protein genes of lambdoid bacteriophage. J. Mol. Biol. 261:12723-12732.

5. Blattner, F. R., G. Plunkett III, C. A. Bloch, N. T. Perna, V. Burland, M. Riley, J. Collado-Vides, J. D. Glasner, C. K. Rode, G. F. Mayhew, J. Gregor, N. W. Davis, H. A. Kirkpatrick, M. A. Goeden, D. J. Rose, B. Mau, and Y. Shao. 1997. The complete genome sequence of Escherichia coli K-12. Science 277:1453-1462[Abstract/Free Full Text].

6. Cowan, S. W., T. Schirmer, G. Rummel, M. Steiert, R. Ghosh, R. A. Paupit, J. N. Jansonius, and J. P. Rosenbusch. 1992. Crystal structures explain functional properties of two E. coli porins. Nature 358:727-733[Medline].

7. Higgins, C. F. 1992. ABC transporters: from microorganism to man. Annu. Rev. Cell Biol. 8:67-113.

8. Highton, P. J., Y. Chang, W. R. Marcotte, Jr., and C. A. Schnaitman. 1985. Evidence that the outer membrane protein gene nmpC of Escherichia coli lies with the defective qsr' prophage. J. Bacteriol. 162:256-262[Abstract/Free Full Text].

9. Jacob, F., A. Ullman, and J. Monod. 1965. Deletions fusing the lactose and purine operons of Escherichia coli. J. Mol. Biol. 31:704-719.

10. Jap, B. K., P. J. Walian, and K. Gehring. 1991. Structural architecture of an outer membrane channel as determined by electron crystallography. Nature 350:167-170[Medline].

11. Jovanovic, G., and P. Model. 1997. The RIB element in the goaG-pspF intergenic region of Escherichia coli. J. Bacteriol. 179:3095-3102[Abstract/Free Full Text].

12. Kohara, Y., K. Akiyama, and K. Isono. 1987. The physical map of the whole E. coli chromosome: application of a new strategy for rapid analysis and sorting of a larger genomic library. Cell 50:495-508[Medline].

13. Luckey, M., and H. Nikaido. 1980. Specificity of diffusion channels produced by $lambda$ phage receptor protein of Escherichia coli. Proc. Natl. Acad. Sci. USA 77:167-171[Abstract/Free Full Text].

14. Lugtenberg, B., J. Meijers, R. Perters, P. van der Hoek, and L. van Alphen. 1975. Electrophoretic resolution of the major outer membrane proteins of Escherichia coli K-12 into four bands. FEBS Lett. 58:254-258[Medline].

15. Maier, C., E. Bremer, A. Schmid, and R. Benz. 1988. Pore-forming activity of the Tsx protein from the outer membrane of Escherichia coli. Demonstration of a nucleoside-specific binding site. J. Biol. Chem. 263:2493-2499[Abstract/Free Full Text].

16. Misra, R., and S. A. Benson. 1988. Isolation and characterization of OmpC porin mutants with altered pore properties. J. Bacteriol. 170:528-533[Abstract/Free Full Text].

17. Misra, R., and S. A. Benson. 1988. Genetic identification of pore domain of the OmpC porin of Escherichia coli K-12. J. Bacteriol. 170:3611-3617[Abstract/Free Full Text].

18. Misra, R., and S. A. Benson. 1989. A novel mutation, cog, which results in the production of a new porin protein (OmpG) of Escherichia coli K-12. J. Bacteriol. 171:4105-4111[Abstract/Free Full Text].

19. Misra, R., A. Peterson, T. Ferenci, and T. J. Silhavy. 1991. A genetic approach for analyzing the pathway of LamB assembly into the outer membrane of Escherichia coli. J. Biol. Chem. 266:13592-13597[Abstract/Free Full Text].

20. Nakae, T. 1976. Identification of the outer membrane protein of E. coli that produces transmembrane channels in reconstituted vesicle membranes. Biochem. Biophys. Res. Commun. 71:877-884[Medline].

21. Nikaido, H. 1994. Porins and specific diffusion channels in bacterial outer membrane. J. Biol. Chem. 269:3905-3908[Free Full Text].

22. Nikaido, H., and E. Y. Rosenberg. 1981. Effect on solute size on diffusion rates through the transmembrane pores of the outer membrane of Escherichia coli. J. Gen. Physiol. 77:121-135[Abstract/Free Full Text].

23. Nikaido, H., and E. Y. Rosenberg. 1983. Porin channels in Escherichia coli: studies with liposomes reconstituted from purified proteins. J. Bacteriol. 153:241-252[Abstract/Free Full Text].

24. Nikaido, H., E. Y. Rosenberg, and J. Foulds. 1983. Porin channels in Escherichia coli: studies with beta-lactams in intact cells. J. Bacteriol. 153:232-240[Abstract/Free Full Text].

25. Nikaido, H., and M. Vaara. 1985. Molecular basis for bacterial outer membrane permeability. Microbiol. Rev. 49:1-32[Free Full Text].

26. Overbeeke, N., and B. Lugtenberg. 1980. Expression of outer membrane protein e of Escherichia coli K-12 by phosphate limitation. FEBS Lett. 112:229-232[Medline].

27. Paul, C., and J. P. Rosenbusch. 1985. Folding patterns of porin and bacteriorhodopsin. EMBO J. 4:1593-1597[Medline].

28. Rosenbusch, J. P. 1974. Characterization of the major envelope protein from Escherichia coli: regular arrangement on the peptidoglycan and unusual dodecylsulfate binding. J. Biol. Chem. 249:8019-8029[Abstract/Free Full Text].

29. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

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1.	Ames, B. N., P. E. Hartman, and F. Jacob. 1963. Chromosomal alterations affecting the regulation of histidine biosynthetic enzymes of Salmonella. J. Mol. Biol. 7:23-42[Medline].
2.	Benson, S. A., J. L. Occi, and B. A. Sampson. 1988. Mutations that alter the pore function of the OmpF porin of Escherichia coli K-12. J. Mol. Biol. 203:961-970[Medline].
3.	Benz, R. 1994. Uptake of solutes through bacterial outer membranes, p. 397-423. In J.-M. Ghuysen, and R. Hakenbeck (ed.), Bacterial cell wall. Elsevier Science, Amsterdam, The Netherlands.
4.	Blasband, A. J., W. R. Marcotte, Jr., and C. A. Schnaitman. 1986. Structure of the lc and nmpC outer membrane porin protein genes of lambdoid bacteriophage. J. Mol. Biol. 261:12723-12732.
5.	Blattner, F. R., G. Plunkett III, C. A. Bloch, N. T. Perna, V. Burland, M. Riley, J. Collado-Vides, J. D. Glasner, C. K. Rode, G. F. Mayhew, J. Gregor, N. W. Davis, H. A. Kirkpatrick, M. A. Goeden, D. J. Rose, B. Mau, and Y. Shao. 1997. The complete genome sequence of Escherichia coli K-12. Science 277:1453-1462[Abstract/Free Full Text].
6.	Cowan, S. W., T. Schirmer, G. Rummel, M. Steiert, R. Ghosh, R. A. Paupit, J. N. Jansonius, and J. P. Rosenbusch. 1992. Crystal structures explain functional properties of two E. coli porins. Nature 358:727-733[Medline].
7.	Higgins, C. F. 1992. ABC transporters: from microorganism to man. Annu. Rev. Cell Biol. 8:67-113.
8.	Highton, P. J., Y. Chang, W. R. Marcotte, Jr., and C. A. Schnaitman. 1985. Evidence that the outer membrane protein gene nmpC of Escherichia coli lies with the defective qsr' prophage. J. Bacteriol. 162:256-262[Abstract/Free Full Text].
9.	Jacob, F., A. Ullman, and J. Monod. 1965. Deletions fusing the lactose and purine operons of Escherichia coli. J. Mol. Biol. 31:704-719.
10.	Jap, B. K., P. J. Walian, and K. Gehring. 1991. Structural architecture of an outer membrane channel as determined by electron crystallography. Nature 350:167-170[Medline].
11.	Jovanovic, G., and P. Model. 1997. The RIB element in the goaG-pspF intergenic region of Escherichia coli. J. Bacteriol. 179:3095-3102[Abstract/Free Full Text].
12.	Kohara, Y., K. Akiyama, and K. Isono. 1987. The physical map of the whole E. coli chromosome: application of a new strategy for rapid analysis and sorting of a larger genomic library. Cell 50:495-508[Medline].
13.	Luckey, M., and H. Nikaido. 1980. Specificity of diffusion channels produced by $lambda$ phage receptor protein of Escherichia coli. Proc. Natl. Acad. Sci. USA 77:167-171[Abstract/Free Full Text].
14.	Lugtenberg, B., J. Meijers, R. Perters, P. van der Hoek, and L. van Alphen. 1975. Electrophoretic resolution of the major outer membrane proteins of Escherichia coli K-12 into four bands. FEBS Lett. 58:254-258[Medline].
15.	Maier, C., E. Bremer, A. Schmid, and R. Benz. 1988. Pore-forming activity of the Tsx protein from the outer membrane of Escherichia coli. Demonstration of a nucleoside-specific binding site. J. Biol. Chem. 263:2493-2499[Abstract/Free Full Text].
16.	Misra, R., and S. A. Benson. 1988. Isolation and characterization of OmpC porin mutants with altered pore properties. J. Bacteriol. 170:528-533[Abstract/Free Full Text].
17.	Misra, R., and S. A. Benson. 1988. Genetic identification of pore domain of the OmpC porin of Escherichia coli K-12. J. Bacteriol. 170:3611-3617[Abstract/Free Full Text].
18.	Misra, R., and S. A. Benson. 1989. A novel mutation, cog, which results in the production of a new porin protein (OmpG) of Escherichia coli K-12. J. Bacteriol. 171:4105-4111[Abstract/Free Full Text].
19.	Misra, R., A. Peterson, T. Ferenci, and T. J. Silhavy. 1991. A genetic approach for analyzing the pathway of LamB assembly into the outer membrane of Escherichia coli. J. Biol. Chem. 266:13592-13597[Abstract/Free Full Text].
20.	Nakae, T. 1976. Identification of the outer membrane protein of E. coli that produces transmembrane channels in reconstituted vesicle membranes. Biochem. Biophys. Res. Commun. 71:877-884[Medline].
21.	Nikaido, H. 1994. Porins and specific diffusion channels in bacterial outer membrane. J. Biol. Chem. 269:3905-3908[Free Full Text].
22.	Nikaido, H., and E. Y. Rosenberg. 1981. Effect on solute size on diffusion rates through the transmembrane pores of the outer membrane of Escherichia coli. J. Gen. Physiol. 77:121-135[Abstract/Free Full Text].
23.	Nikaido, H., and E. Y. Rosenberg. 1983. Porin channels in Escherichia coli: studies with liposomes reconstituted from purified proteins. J. Bacteriol. 153:241-252[Abstract/Free Full Text].
24.	Nikaido, H., E. Y. Rosenberg, and J. Foulds. 1983. Porin channels in Escherichia coli: studies with beta-lactams in intact cells. J. Bacteriol. 153:232-240[Abstract/Free Full Text].
25.	Nikaido, H., and M. Vaara. 1985. Molecular basis for bacterial outer membrane permeability. Microbiol. Rev. 49:1-32[Free Full Text].
26.	Overbeeke, N., and B. Lugtenberg. 1980. Expression of outer membrane protein e of Escherichia coli K-12 by phosphate limitation. FEBS Lett. 112:229-232[Medline].
27.	Paul, C., and J. P. Rosenbusch. 1985. Folding patterns of porin and bacteriorhodopsin. EMBO J. 4:1593-1597[Medline].
28.	Rosenbusch, J. P. 1974. Characterization of the major envelope protein from Escherichia coli: regular arrangement on the peptidoglycan and unusual dodecylsulfate binding. J. Biol. Chem. 249:8019-8029[Abstract/Free Full Text].
29.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
30.	Sampson, B. A., R. Misra, and S. A. Benson. 1989. Identification and characterization of a new gene of Escherichia coli K-12 involved in outer membrane permeability. Genetics 122:491-501[Abstract/Free Full Text].
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