Identification and Characterization of a New Lipoprotein, NlpI, in Escherichia coli K-12

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Journal of Bacteriology, July 1999, p. 4318-4325, Vol. 181, No. 14
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Identification and Characterization of a New Lipoprotein, NlpI, in Escherichia coli K-12

Masaru Ohara,¹ Henry C. Wu,¹^, Krishnan Sankaran,¹^, and Paul D. Rick¹^,^*

Department of Microbiology and Immunology, Uniformed Services University of the Health Sciences, Bethesda, Maryland 20814-4799¹

Received 5 March 1999/Accepted 26 April 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

We report here the identification of a new lipoprotein, NlpI, in Escherichia coli K-12. The NlpI structural gene (nlpI) islocated between the genes pnp (polynucleotide phosphorylase) anddeaD (RNA helicase) at 71 min on the E. coli chromosome. The nlpIgene encodes a putative polypeptide of approximately 34 kDa, andmultiple lines of evidence clearly demonstrate that NlpI is indeeda lipoprotein. An nlpI::cm mutation rendered growth of the cellsosmotically sensitive, and incubation of the insertion mutantat an elevated temperature resulted in the formation of filaments.The altered phenotype of the mutant was a direct consequence ofthe mutation in nlpI, since it was complemented by the wild-typenlpI gene alone. Overexpression of the unaltered nlpI gene inwild-type cells resulted in the loss of the rod morphology andthe formation of single prolate ellipsoids and pairs of prolateellipsoids joined by partial constrictions. NlpI may be importantfor an as-yet-undefined step in the overall process of celldivision.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

More than 130 different lipoproteins have been identified in a wide variety of both gram-positive and gram-negative bacteria(39). Indeed, more than 16 chromosomally encoded lipoproteinshave been identified in Escherichia coli (7, 18, 22, 25,27, 39, 40). In addition, several lipoproteins that areplasmid encoded have been identified in E. coli and other organisms(11, 35, 39). Although the primary amino acid sequencesof the mature forms of these lipoproteins differ considerably,their respective unmodified prolipoprotein forms share certaingeneral structural features. These features include a signal sequencethat contains a lipid modification, or "lipobox" sequence, whichin turn includes the cysteine residue destined for lipid modification.The consensus lipobox has the sequence Leu(Ala, Val)₄-Leu₃-Ala(Ser)₂-Gly(Ala)₁-Cys₊₁(39). The posttranslational lipid modification of these lipoproteinspresumably occurs by a common biosynthetic pathway. This pathwayinvolves three posttranslational reactions catalyzed by the enzymesphosphatidylglycerol:prolipoprotein diacylglyceryltransferase,prolipoprotein signal peptidase (signal peptidase II), and phospholipid:apolipoproteintransacylase (N-acyltransferase). These enzymes are encoded bythe lgt, lsp, and lnt genes, respectively, and their activitiesculminate in the synthesis of an N-terminal N-acyl-S-sn-1,2-diacylglyceryl-modifiedcysteine residue, the signature structural component of bacteriallipoproteins (39).

The isolation and characterization of mutants possessing temperature-sensitive alleles of the lgt, lsp, and lnt genes haverevealed that these genes are essential. In addition, the antibioticglobomycin is a specific inhibitor of signal peptidase II, andinhibition of this enzyme by globomycin is lethal (17, 19,20). These observations have led to the proposal that bacteriapossess one or more lipoproteins that are required for normalcell growth and function (39). However, attempts to identifyan essential lipoprotein have thus far beenunsuccessful.

Previous studies identified a single open reading frame of unknown function located downstream of the pnp (polynucleotidephosphorylase) gene and immediately upstream of the deaD (ATP-dependentRNA helicase) gene at 71 min on the E. coli chromosome (4,33, 36). The studies reported here demonstrate that this openreading frame encodes a previously unrecognized lipoprotein whichwe have designated new lipoprotein I (NlpI). Characterizationof an nlpI::cm insertion mutant suggests that NlpI may be requiredfor an as-yet-undefined step in the overall process of celldivision.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains, plasmids, and growth conditions. The bacterial strains and plasmids used in this study are listed in Table 1. Bacteria were grown in Luria-Bertani (LB) broth(30) or in M9 minimal medium (30) containing magnesium sulfateand calcium chloride at final concentrations of 0.1 and 0.01 mM,respectively. Ampicillin and kanamycin were added to culture mediawhen appropriate to give final concentrations of 50 and 25 µg/ml,respectively.

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TABLE 1. Bacterial strains and plasmids

DNA techniques. All DNA manipulations were performed by standard techniques (28). Restriction enzymes were purchased from New England Biolabs(Beverly, Mass.). PCR amplifications were carried out with Taqpolymerase (Perkin-Elmer, Foster City, Calif., or Takara Shuzo,Shiga,Japan).

Cloning and sequencing of the nlpI gene. Oligonucleotide primers for PCR amplification of the nlpI gene were designed in accordance with nucleotide sequence data obtainedfrom investigations of the pnp (33) and deaD (36) genes ofE. coli K-12. The oligonucleotide primer U1F1 (5'-TCGGGAATTCGAAATGAAGCCT-3';forward) includes the putative translational start codon (ATG,in bold) of nlpI; the underlined nucleotides indicate alterationsof the wild-type sequence which were made in order to create anEcoRI site immediately upstream of the start codon. The oligonucleotideprimer U1F2 (5'-CGTATCCGTCTGAGCATTAA-3'; forward) correspondsto nucleotides 2713 to 2732 in the 3' region of the pnp gene.The oligonucleotide primer U1R (5'-CTGAAGCTTACGTCAGCTATTGC-3';reverse) is complementary to the 3' terminus of nlpI as well asto the 16 flanking nucleotides located beyond the translationalstop codon; the underlined nucleotides designate changes in thewild-type sequence which were made in order to incorporate a HindIIIrestriction site. PCR amplifications were carried out with chromosomalDNA obtained from E. coli DH5 $alpha$ and RM4606. The products of PCRamplifications with primer pairs U1F1-U1R and U1F2-U1R were ligatedinto pCR2.1 to yield pCU11 and pCU21, respectively. The resultingconstructs were used to transform E. coli INV $alpha$ F'. Bidirectionalnucleotide sequencing of cloned nlpI was carried out with ABIPRISM dye terminator cycle sequencing kits (Perkin-Elmer), complementaryoligonucleotide primer pairs 277F (5'-CGGATATGCCTGAAGTATTCA-3';forward)-277R (5'-TGAATACTTCAGGCATATCCG-3'; reverse) and 576F(5'-AATCGGATAAGGAACAGTGGG-3'; forward)-576R (5'-CCCACTGTTCCTTATCCGATT-3';reverse), and M13 forward ( $-$ 21) and reverseprimers.

Construction of nlpI knockout mutants through gene replacement. Null mutations in the E. coli nlpI gene were generated through allelic exchange with the pBIP3 suicide vector as describedby Slater and Maurer (34). Briefly, the 886-bp chloramphenicolresistance determinant of plasmid pACYC184 was obtained by PCRamplification with the forward and reverse primer sequences 5'-CTGAACCGACGACCGGGTCGA-3'and 5'-TGAGACGTTGATCGGCACGTAAG-3', respectively. The resultingproduct was inserted into the middle of the nlpI gene carriedby pCU21 by blunt ligation into the unique BstBI site of the nlpIgene. The nlpI::cm insertion was then excised with restrictionenzymes ApaI and SpeI and subcloned into the corresponding sitesof plasmid pBIP3. The ntp-sacB cassette of plasmid pBIP3 confersresistance to kanamycin and sensitivity to 5% sucrose (34).Thus, the resulting construct was introduced into E. coli JM109by electroporation, and transformants were selected on LB agarplates containing both chloramphenicol and kanamycin. The pBIP-nlpI::cmderivative was isolated from the transformants, and incorporationof the nlpI::cm construct into the polylinker site of pBIP3 wasverified by nucleotide sequencing. Transformants harboring pBIP3-nlpI::cmwere infected with helper phage f1R189, and the resulting lysateswere used to infect strain RM4606. Chloramphenicol-resistant colonieswere plated on salt-free LB agar plates containing 5% sucroseto resolve cointegrates, and colonies resistant to both chloramphenicoland 5% sucrose were screened for sensitivity to kanamycin. Kanamycin-sensitivederivatives were examined by Southern blot analyses with the nlpIand cm genes as probes to identify nlpI::cm insertion mutants.One such mutant, WU620, was used for furtherstudies.

Southern hybridization. Chromosomal DNA was isolated from wild-type and mutant cells of E. coli with Puregene DNA isolation kits (Gentra Systems,Inc., Minneapolis, Minn.). The isolated DNA was digested withEcoRV at 37°C overnight, and the resulting fragments were separatedby electrophoresis in a 0.7% agarose gel (60 V, 5 to 6 h) withTBE buffer (90 mM Tris-borate, 2 mM EDTA [pH 8.0]). DNA fragmentswere visualized by ethidium bromide staining, and the DNA wassubsequently denatured by incubating the gel with gentle shakingin denaturing buffer (0.5 M NaOH, 1.5 M NaCl) for 30 min at roomtemperature. The gel was next incubated in neutralizing buffer(1 M Tris-HCl [pH 7.4], 1.5 M NaCl), and the denatured DNA fragmentswere transferred to a Hybond N nylon membrane filter (AmershamLife Science, Inc., Arlington Heights, Ill.) by capillary blottingovernight with 10× SSC buffer (1.5 M NaCl, 0.15 M sodium citrate[pH 7.0]). The filter was air dried, and the DNA was cross-linkedto the filter by UV treatment (StratalinkerR; Stratagene, La Jolla,Calif.). Subsequent steps, including the preparation of labeledprobes as well as hybridization and detection steps, were carriedout with enhanced chemiluminescence direct nucleic acid labelingand detection systems (Amersham Life Science). Probes were preparedfrom the nlpI coding region (PCR product obtained with primersU1F1 and U1R) and the 886-bp chloramphenicol resistance cassetteobtained by PCR amplification as describedabove.

Expression of nlpI and radiolabeling experiments. High-level expression of nlpI was made possible by subcloning of the PCR product in pCU11 into the expression vector pBAD24(10). Subcloning of the PCR product into the multicloning siteof this vector was facilitated by use of the EcoRI and HindIIIrestriction sites that were created in the U1F1 and U1R PCR primers,respectively. The construct resulting from subcloning of thisfragment into pBAD24 was designated pBU142. Plasmid pBU142 wasintroduced into E. coli DH5 $alpha$ by transformation, giving rise tostrainMO101.

Radiolabeling of NlpI was carried out with either [9,10-³H]palmitic acid (specific activity, 56.5 Ci/mmol; Dupont NEN, Wilmington,Del.) or [2-³H]glycerol (specific activity, 6.35 Ci/mmol; New England NuclearCorp., Boston, Mass.). Cells were grown overnight at 37°C in M9minimal medium containing glucose (0.4%) and supplemented with5% LB broth (medium A). A portion of the culture (3 ml) was harvestedby centrifugation, and the cells were washed with M9 minimal mediumcontaining L-arabinose and LB broth at final concentrations of0.2 and 5%, respectively (medium B). The cells were then resuspendedin 3 ml of medium B to give an A₆₀₀ of 0.2 to 0.3, and the mixturewas incubated with shaking at 37°C for 1 h. Control cultures (3ml) were grown overnight at 37°C in medium A, washed with mediumA, and subsequently resuspended in 3 ml of medium A to give anA₆₀₀ of 0.2 to 0.3, and the mixture was incubated with shakingat 37°C for 1 h. Ampicillin (50 µg/ml) was included in culturemedia to ensure the maintenance of plasmids. To each of the cultureswas added either [9,10-³H]palmitate (100 µCi) or [2-³H]glycerol (100 µCi), and the cultures were incubated with shakingat 37°C for 5 to 6 h. The cells were harvested by centrifugation,washed with 3 ml of ice-cold 10 mM sodium phosphate buffer (pH7.0), and resuspended in 3 ml of the same buffer. The labeledcells were subsequently disrupted by sonication, and unbrokencells were removed by centrifugation at 5,000 × g for 5 min at4°C. The crude cell envelope fraction was isolated by centrifugationof the supernatant solution at 200,000 × g for 1.5 h at 4°C. Thecell envelope fraction was washed with 1 ml of cold acetone, andthe washed membranes were dried at 60 to 70°C. The dried membraneswere solubilized by boiling for 5 min following the addition of30 to 50 µl of sample buffer (62.5 mM Tris-HCl [pH 6.8], 2% sodiumdodecyl sulfate [SDS], 5% 2-mercaptoethanol, 20% glycerol, 0.01%bromophenol blue). The samples were analyzed by SDS-polyacrylamidegel electrophoresis (PAGE) either by the procedure of Ito et al.(21) or by the procedure described by Laemmli (23). The resultinggels were soaked in Amplify (Amersham Life Science) with gentleshaking for 20 to 30 min at room temperature and dried, and thelocation of radioactivity on the gels was determined by fluorographywith Kodak X-Omat AR film (Eastman Kodak, New Haven, Conn.).

Inhibition of NlpI posttranslational modification by globomycin. Strain MO101 was cultured overnight with shaking in medium A at 37°C. The cells contained in 3 ml of the overnight culturewere washed with 3 ml of medium B and diluted with medium B togive an A₆₀₀ of 0.5 to 0.6, and 3-ml portions of the resultingsuspension were incubated with shaking at 37°C for 1 h. Globomycinwas then added from a stock solution of 10 mg/ml in dimethyl sulfoxide(DMSO) to separate 3-ml cultures to give final concentrationsof 0, 50, 100, and 200 µg/ml. The cells were incubated with shakingfor an additional 10 min at 37°C, and either [9,10-³H]palmitic acid or [2-³H]glycerol was added to give a final concentration of 100 µCi/ml.The cells were subsequently incubated with the radiolabeled compoundsat 37°C for 1 h with vigorous aeration. Radiolabeling was terminatedby placing the cultures in an ice bath; this step was followedimmediately by the addition of cold trichloroacetic acid to givea final concentration of 5%, and the cells were incubated on icefor 15 min. The cells were harvested by centrifugation, and thepellets were washed with 1 ml of acetone and dried at 60 to 70°C.The dried pellets were resuspended in 25 µl of sample buffer togetherwith 1.25 µl of 5 N NaOH, and radiolabeled NlpI was solubilizedby boiling for 5 min. The solubilized samples were analyzed bySDS-PAGE by the procedure of Ito et al. (21) or by SDS-PAGE(12% acrylamide) as described by Laemmli (23). The locationof radioactivity on the gels was determined by fluorography asdescribedabove.

Purification of radiolabeled NlpI. SDS-solubilized cell envelope proteins were obtained from strain MO101 following incubation of the cells in medium B in thepresence of either [9,10-³H]palmitate or [2-³H]glycerol by the procedures described above. The solubilizedproteins were subjected to SDS-PAGE (12% acrylamide) as describedby Laemmli (23) and subsequently located on the gels by stainingwith Coomassie brilliant blue by standard procedures. A thin bandcontaining 32-kDa NlpI was excised from the gel, and the gel slicewas placed in a Spectrapor dialysis tube (molecular weight cutoff,3,500; Spectrum, Los Angeles, Calif.) containing 5 ml of Laemmlirunning gel buffer (25 mM Tris-glycine [pH 8.4], 1% SDS). RadiolabeledNlpI was electroeluted from the gel slice by electrophoresis for4 h at a constant voltage (150 V) by use of a horizontal mini-submarinegel apparatus filled with Laemmli running gel buffer. The proteinwas exhaustively dialyzed against water and lyophilized untilfurtheruse.

Identification of glyceryl-cysteine. The occurrence of glyceryl-cysteine in NlpI was demonstrated by previously described procedures (14). Briefly, purified[2-³H]glycerol-labeled NlpI was dissolved in 1 ml of a mixture ofH₂O₂ and 88% formic acid (1:9 [vol/vol]), and the mixture wasincubated overnight in a closed screw-cap tube at 4°C. The mixturewas transferred to a glass hydrolysis ampoule and lyophilizedto remove performic acid. One milliliter of constant-boiling HClwas added to the ampoule, and the ampoule was sealed and incubatedin vacuo for 20 h at 100°C. The hydrolysate was lyophilized toremove HCl. The dried sample was dissolved in 20 to 30 µl of electrophoresisbuffer (0.47 M formic acid, 1.4 M acetic acid [pH 2.3 to 2.4])and analyzed by high-voltage paper electrophoresis at 2,000 Vfor 2 h with cooling by use of Whatman 3MM paper and electrophoresisbuffer. Standards of cysteic acid, cysteine, methionine sulfone,and methionine were included in the analyses. The electrophoreticmobilities of radiolabeled components in the sample were determinedby cutting the sample lane into 1-cm segments and determiningthe amount of radioactivity in each segment by standard liquidscintillation counting procedures. The electrophoretic mobilitiesof standard compounds were determined by spraying the dried electrophoretogramwith a ninhydrin solution (0.2% ninhydrin inacetone).

Mild alkali treatment of [9,10-³H]palmitate-labeled NlpI. A dried sample of purified [9,10-³H]palmitate-labeled NlpI was incubated with 8 µl of 0.5 N NaOH for 2 h at 37°C with occasionalmixing. The sample was neutralized by the addition of 10 µl of0.4 N HCl and subsequently mixed with 9 µl of sample buffer. Asecond, control sample containing the same amount of radioactivitywas incubated with 15 µl of sample buffer. Both samples were analyzedby SDS-PAGE (12% acrylamide) with a minigel apparatus. The gelwas dried without staining, and individual lanes were cut into1-mm segments. The segments were incubated overnight with 0.5ml of 0.1% SDS at 37°C, and the amount of radioactivity in eachsegment was determined by standard liquid scintillation countingprocedures.

Miscellaneous techniques. Cellular morphology was examined by light microscopy of crystal violet-stained cells. Nucleoids were stained with 4',6-diamidino-2-phenylindole(DAPI) and visualized by fluorescence microscopy with a Zeisstype 741 fluorescence microscope interfaced with a PhotometricsCE200A camera essentially as described by Hiraga et al. (15).The osmolarity of various media was determined with a 5100B vaporpressure osmometer (Wescor, Inc.).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

The nlpI gene encodes a lipoprotein. Previous studies reported the occurrence of a gene of unknown function, gene yhbM, located between genes pnp and deaD at 71min on the E. coli chromosome (4). The predicted polypeptideencoded by yhbM contains 294 amino acid residues and has a calculatedmolecular mass of 33,619 Da (Fig. 1). Inspection of the aminoacid sequence of the predicted polypeptide encoded by yhbM suggestedthat this gene product is a lipoprotein. Thus, the N terminuspossesses the characteristics of a typical bacterial signal sequence;it contains a charged amino acid (lysine) in proximity to theN terminus as well as a short hydrophobic region (residues 3 to15). In addition, the hydrophobic region is followed by the sequenceLeu₁₆-Ala-Gly-Cys₁₉, which conforms to the parameters that definea lipobox, or lipoprotein modification and processing sequence(39).

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FIG. 1. (A) Predicted amino acid sequence of the product of the nlpI gene. The nlpI gene encodes a 34-kDa polypeptide containing 294 amino acids including a putative signal sequence consisting of 18 amino acids (italic type). The amino acids comprising the lipobox sequence, Leu-Ala-Gly-Cys, are underlined. The sequence delineated by amino acid residues 62 to 163 contains three TPRs. The eight consensus amino acids of the TPR motif are indicated in italics above the first TPR. The amino acid residues in NlpI that conform to the consensus TPR motif are indicated in bold type. (B) Genetic map of the region containing the nlpI gene between 71.0 and 71.1 min on the E. coli chromosome. An nlpI::cm insertion mutant was constructed by insertion of an 886-bp chloramphenicol resistance cassette into the BstBI site of nlpI as indicated. Southern blot analyses revealed 2.6- and 3.5-kb fragments in EcoRV digests of chromosomal DNAs obtained from the wild type and the nlpI::cm insertion mutant, respectively.

The yhbM gene was amplified by PCR with genomic DNA from E. coli DH5 $alpha$ . It was subsequently subcloned into expression vectorpBAD24, placing the expression of yhbM under the control of theara_BAD promoter; the resulting construct was designated pBU142.Significant incorporation of radioactivity into a protein withan apparent molecular mass of 32 kDa was observed when strainMO101 (DH5 $alpha$ /pBU142) was incubated with [³H]palmitate under conditions where the expression of yhbM wasinduced with L-arabinose (Fig. 2A, lane 2). This radiolabeledprotein was not detected when strain MO101 was incubated with[³H]palmitate under noninducing conditions (Fig. 2A, lane 1). Similarresults were obtained when strain MO101 was incubated with [2-³H]glycerol under inducing and noninducing conditions (Fig. 2B).

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FIG. 2. (A and B) In vivo incorporation of [³H]palmitic acid (A) and [2-³H]glycerol (B) into polypeptides following overexpression of the nlpI gene in E. coli. In vivo labeling and SDS-PAGE were performed as described in Materials and Methods. In each case, strain MO101 was grown overnight in medium A and subsequently incubated in medium A (lane 1) or medium B (lane 2) immediately prior to the addition of radiolabeled palmitic acid or glycerol. The location of 32-kDa NlpI is indicated by an arrow. The electrophoretic mobilities of marker proteins with known molecular masses are indicated in kilodaltons. (C) Effect of globomycin on the maturation of NlpI. Strain MO101 was grown overnight in medium A, and the cells were harvested and washed in medium B. The washed cells were resuspended in medium B containing globomycin at a final concentration of 0 µg/ml (lane 1), 50 µg/ml (lane 2), 100 µg/ml (lane 3), or 200 µg/ml (lane 4). Globomycin was dissolved in DMSO to yield a stock solution of 10 mg/ml; accordingly, 20 µl of DMSO was added to a control culture (lane 5). The cells were subsequently incubated with either [³H]palmitic acid or [2-³H]glycerol, and the incorporation of radiolabel into NlpI was determined by SDS-PAGE and fluorography. Experimental details are provided in Materials and Methods. The upper and lower arrows in each panel indicate the locations of modified pro-NlpI (MPNlpI) and mature NlpI, respectively.

Signal peptidase II is required for the conversion of diacylglyceryl-modified prolipoproteins to apolipoproteins (39). Theantibiotic globomycin is a specific inhibitor of signal peptidaseII, and this inhibition is characterized by the accumulation ofdiacylglyceryl-modified prolipoproteins which are slightly largerthan their corresponding mature lipoproteins owing to the presenceof the signal peptide (17). The incorporation of radioactivityinto the 32-kDa protein was clearly inhibited by globomycin followingthe expression of yhbM in strain MO101 in the presence of either[2-³H]glycerol or [³H]palmitate (Fig. 2C). Partial inhibition was observed when globomycinwas added to cultures at a final concentration of 100 µg/ml, whereassignificantly greater inhibition occurred when the drug was presentat a final concentration of 200 µg/ml. The inhibition of synthesisof the 32-kDa protein was also accompanied by the appearance ofa radiolabeled 34-kDa protein. Taken together, the above observationssupport the conclusion that the yhbM gene encodes a lipoprotein,and we have renamed the gene nlpI, for new lipoproteinI.

Characterization of the lipid modification in NlpI. Bacterial lipoproteins are characterized by the occurrence of an N-terminal N-acyl-S-sn-1,2-diacylglyceryl-modified cysteineresidue. In E. coli, the N-acyl-linked substituent of Lpp is primarilypalmitate; however, other fatty acids have also been found tooccur at this position (13). In contrast, the O-acyl-linkedsubstituents of Lpp are similar to those found in bulk phospholipids(13). The thioether linkage in the glyceryl-cysteine moietyis more acid stable than a peptide bond, and performic acid oxidationof bacterial lipoproteins followed by acid hydrolysis characteristicallyresults in the formation of glyceryl-cysteine sulfone (14).Thus, [2-³H]glycerol-labeled NlpI purified by preparative SDS-PAGE was examinedfor the presence of glyceryl-cysteine by established methods (14).Performic acid oxidation of [2-³H]glycerol-labeled NlpI followed by acid hydrolysis resulted inthe release of a radiolabeled compound whose electrophoretic mobilitywas the same as that reported for glyceryl-cysteine sulfone analyzedby high-voltage paper electrophoresis at pH 2.3 to 2.4 (14)(Fig. 3).

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FIG. 3. Identification of glyceryl-cysteine sulfone in total acid hydrolysates of performic acid-oxidized NlpI. [2-³H]glycerol-labeled NlpI was purified by preparative SDS-PAGE and treated with performic acid at 4°C overnight. Total acid hydrolysates of performic acid-oxidized lipoprotein were then analyzed by high-voltage paper electrophoresis at pH 2.3 to 2.4 along with the indicated standards. The distance of electrophoretic movement (centimeters) from the origin toward the cathode is indicated by the negatively prefixed scale on the abscissa. Additional experimental details are provided in Materials and Methods.

[³H]palmitate-labeled NlpI was also examined for the presence of ester- and amide-linked fatty acyl substituents. Incubationof [³H]palmitate-labeled Lpp with mild alkali results in the hydrolysisof ester-linked fatty acyl moieties, and such treatment typicallyresults in the loss of at least 50% of the radioactivity as freefatty acids. Treatment of [³H]palmitate-radiolabeled NlpI with mild alkali followed by SDS-PAGEresulted in the release of approximately 62% of the radioactivity.The remainder of the radioactivity migrated as a single componentwith an apparent electrophoretic mobility identical to that ofuntreated NlpI. These data clearly demonstrate the occurrenceof N-acyl-S-diacylglyceryl-modified cysteine inNlpI.

Isolation of an nlpI::cm insertion mutant. A chloramphenicol resistance cassette was inserted into the E. coli nlpI gene, and the interrupted gene was introduced intothe chromosome of E. coli RM4606 by allelic exchange, yieldingthe insertion mutant WU620. The presence of a single insertionallyinactivated nlpI gene in the chromosome was confirmed by Southernblot analyses of WU620 and two transductants, WU62 and WU63; thetransductants were obtained by introduction of the mutation inWU620 into the chromosome of the parental strain, RM4606, by P1-mediatedtransduction. In wild-type cells, the nlpI gene is flanked byEcoRV sites which delineate a 2.6-kb fragment (Fig. 1B). Insertionof the 886-bp Cm^r cassette into the BstBI site of the nlpI gene would increasethe size of this fragment to approximately 3.5 kb. Southern blotanalyses revealed a single DNA fragment of approximately 3.5 kbin an EcoRV digest of the chromosome of each of the transductantsand strain WU620 with the chloramphenicol resistance gene as theprobe (data not shown). In contrast, this fragment was not detectedin an EcoRV digest of the chromosome of the wild-type parentalstrain, RM4606. Similar results were obtained with labeled nlpIas the probe, except that a single 2.6-kb fragment correspondingto the wild-type nucleotide sequence was detected in an EcoRVdigest of the chromosome of strainRM4606.

Phenotype of the nlpI::cm insertion mutant. The null mutation in nlpI had no apparent effect on the ability of strain WU62 to grow in standard LB liquid medium or onLB solid medium at 30, 37, and 42°C. However, microscopic examinationrevealed pronounced filamentation of the mutant cells when brothcultures were incubated at 42°C (Fig. 4A). No obvious morphologicaldifferences between mutant and wild-type cells were observed whencells were grown in broth at either 30 or 37°C (Fig. 4B). In addition,the thermosensitive phenotype of the mutant was complemented byplasmid pCU21, which contains the wild-type nlpI gene as wellas a 195-bp sequence upstream of the putative translational startcodon (Fig. 4C). The filamentation of mutant strain WU62 at anelevated temperature did not appear to affect nucleoid numbersor segregation (Fig. 4D).

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FIG. 4. (A to C) Effect of the nlpI::cm mutation on the morphology of cells at an elevated temperature. Cells were incubated in LB broth at 42°C with shaking until the optical density (A₆₀₀) reached 0.4 to 0.5. The cells were subsequently stained with crystal violet and visualized by light microscopy. (A) WU62 (nlpI::cm). (B) RM4606 (wild type). (C) WU62 carrying plasmid pCU21. Bars, 2 µm. (D) DNA segregation in strain WU62. Cells were incubated in LB broth at 42°C until the optical density (A₆₀₀) of the culture reached 0.4 to 0.5, and nucleoids were subsequently visualized by fluorescence microscopy after DAPI staining. Additional details are provided in Materials and Methods.

Although the nlpI::cm insertion did not preclude the growth of strain WU62 in standard LB liquid medium or on LB solid mediumcontaining 0.5% NaCl, the growth of the mutant was severely restrictedon low-salt LB medium. The mutant was able to form only smallcolonies at 30°C on LB agar lacking NaCl, and no growth was observedon this medium at 37 and 42°C (data not shown). The growth ofthe mutant at an elevated temperature was rescued when NaCl inLB agar was replaced by either KCl or LiCl at the same final concentration(85.86 mM). These observations appear to reflect a sensitivityof the mutant to osmotic conditions, since growth at an elevatedtemperature on LB medium was also rescued when NaCl in the mediumwas replaced by 2.5% sucrose. The effect of low salt on the growthof the mutant in LB broth at various temperatures was somewhatmore complex. The apparent rate of growth of strain WU62 becameprogressively lower as the growth temperature was increased from30 to 42°C, and the growth of the mutant appeared to be almostcompletely inhibited at 42°C (data not shown). Similarly, cellfilamentation became increasingly apparent as the growth temperaturewas increased; however, filamentation was most pronounced at 42°C.

The phenotype of the nlpI::cm insertion mutant was unaltered following introduction of the recA56 mutant allele into strainWU62. Thus, we conclude that the thermosensitive cell divisionand osmotic sensitivity of the nlpI::cm insertion mutant are notindirectly due to an induction of the SOSresponse.

Effect of nlpI overexpression. The phenotype of the nlpI null mutation prompted an examination of the effect of nlpI overexpression on growth and cellularmorphology. Overexpression of nlpI in strain MO101 was clearlyevident following growth of the cells at 37°C in medium B (inductionwith 0.2% arabinose), as indicated by the appearance of the 32-kDaNlpI lipoprotein when cell envelope preparations were analyzedby SDS-PAGE and Coomassie brilliant blue staining (data not shown).The overexpression of nlpI in cells grown in medium B resultedin a loss of the rod morphology, accompanied by the striking appearanceof swollen prolate ellipsoids as well as pairs of prolate ellipsoidsjoined by partial constrictions (Fig. 5A). This morphology wasalso observed when strain MO101 was grown in LB broth containing0.2% L-arabinose. The overexpression of nlpI also affected thegrowth of cells. Accordingly, strain MO101 grew with a decreasedgeneration time in medium B at 37°C, and growth ceased after theapparent cell mass had increased by approximately 1.5 doublings(data not shown). In contrast, the NlpI protein was not detectedin cell envelopes obtained from wild-type cells that were grownsimilarly or from strain MO101 grown at 37°C in medium A (repressionwith 0.4% glucose) when these preparations were analyzed in thesame manner. Furthermore, the growth of strain MO101 was unaffectedwhen cells were incubated at 37°C in medium A, and the morphologyof these cells also appeared to be normal (Fig. 5B).

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FIG. 5. Morphology of cells following the overexpression of nlpI. (A) The overexpression of nlpI from the ara_BAD promoter was induced by the growth of strain MO101 (DH5 $alpha$ /pBU142) at 37°C in medium B with shaking for 4 to 5 h. (B) Control cultures were grown in medium A under the same conditions. The cells were subsequently stained with crystal violet and visualized by light microscopy. Bars, 2 µm.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We describe here the identification and characterization of a previously unrecognized lipoprotein in E. coli K-12 which wehave designated NlpI. The function of NlpI is not yet known. However,NlpI is the first example of a bacterial lipoprotein whose mutationalalteration has a direct effect on cellular morphology. Indeed,the phenotype of the nlpI::cm insertion mutant suggests that thislipoprotein may be important for some step in the overall processof cell division. In this regard, it is interesting that severalof the phenotypic characteristics of the nlpI::cm insertion mutantare similar to those expressed by mutants that are conditionallydefective in fts (filamenting temperature-sensitive) genes involvedin cell division (26). Accordingly, incubation of the nlpI::cminsertion mutant at an elevated temperature resulted in filamentationof the cells and rendered the cells osmotically sensitive. Filamentationof bacterial cells commonly occurs secondarily as a consequenceof the SOS response elicited by damage to DNA or as a result ofa blockage in DNA replication. However, filamentation of the nlpI::cminsertion mutant at a nonpermissive temperature did not appearto be due to any of these causes, since the synthesis of DNA andthe partitioning of chromosomes within filaments were not alteredand the same phenotype was observed for recA56 nlpI::cm doublemutants. In addition, it is unlikely that the phenotype of thenlpI::cm insertion mutant is due to a polar effect of the insertionin nlpI on downstream genes, since normal cell growth and morphologywere restored when the nlpI::cm insertion mutant was complementedby the wild-type nlpI gene alone. Furthermore, the deaD gene islocated immediately downstream of nlpI, and it appears to be transcribedindependently of the rpsO-pnp genes and the nlpI gene (36).

The overall process of cell division is a complex process that involves the coordinated activities of numerous proteins. Indeed,it is now clear that the actual division event or septum formationrequires the coordinated function of several proteins that comprisea macromolecular complex. This complex is localized at the siteof circumferential invagination (26), and it has been variouslytermed a divisome (31), a septalsome (16), and a septator(37). The available data suggest the possibility that NlpI mightbe a previously unrecognized component of this complex. However,it is important to stress that the identification of NlpI as acomponent of either the cytoplasmic or the outer membrane remainsto be established. Additional studies are also required to ascertainwhether or not NlpI is localized in the vicinity of circumferentialinvagination during cell division. Nevertheless, it is interestingto note that analyses of the deduced amino acid sequence of NlpIhave revealed the presence of the tetratricopeptide repeat (TPR)unit (5) (Fig. 1A). The TPR consists of a degenerate 34-amino-acidmotif which is tandemly repeated, and this motif is defined bythe occurrence of the loosely conserved consensus sequence W...LG...Y...A...F...A...P(6, 9, 24). The TPR motif occurs widely in nature, andTPR-containing proteins participate in a diverse array of relatedand unrelated biological processes. The TPR motif appears to mediateintermolecular protein-protein interactions, leading to the formationof protein complexes (6), and it has been suggested that theTPR motif may also facilitate intramolecular protein interactions(24).

Altered cell morphology has been observed following the overexpression of several genes known to be involved in cell divisionand related processes in E. coli. For example, moderate overexpressionof ftsZ results in the formation of minicells (2, 26, 38),whereas higher levels of ftsZ expression result in the formationof filaments (26, 38). Additional examples include the formationof spherically shaped cells and chains of cells following theoverexpression of dacA (D,D-carboxypeptidase 1A; penicillin-bindingprotein 5) (29) and cafA (formation of cytoplasmic axial filaments)(32), respectively. The overexpression of nlpI resulted in theloss of rod morphology and the formation of both single prolateellipsoids and what appear to be pairs of prolate ellipsoids joinedby partial constrictions. This result was unexpected, since prolateellipsoids have only been observed in double mutants conditionallydefective in both cell elongation and in an early step of celldivision following a shift to nonpermissive conditions. For example,RodA is required for cell elongation and maintenance of the rodshape of E. coli (1), whereas FtsZ is required for the initialstep in the assembly of the septal ring structure, the formationof the FtsZ ring (1, 3, 8, 12). Mutants possessingthe temperature-sensitive rodA52 allele grow as spherical cellsat a nonpermissive temperature (1). However, prolate ellipsoidsare formed by double mutants possessing the rodA52 allele anda temperature-sensitive allele of ftsZ when incubated at a nonpermissivetemperature (1). This morphology is believed to result fromcontinued peptidoglycan synthesis in the absence of both chainelongation and the formation of the FtsZ ring (1). The formationof prolate ellipsoids following the overexpression of nlpI suggeststhat increased levels of NlpI might disrupt both of these processes.In addition, the appearance of pairs of prolate ellipsoids joinedby partial constrictions may be due to the deleterious effectsof elevated NlpI levels on both chain elongation and continuedseptum formation in cells in which septum formation has alreadybegun prior to the onset of nlpIoverexpression.

The basis for the temperature-sensitive phenotype of the nlpI::cm insertion mutant is not yet understood. It is possible thatNlpI is required only for normal cell growth and morphology atan elevated temperature. However, this possibility seems unlikelyin view of the observation that the nlpI::cm insertion mutationrendered the mutant osmotically sensitive at 30 and 37°C as wellas at 42°C. Alternatively, it is possible that the mutant expressesa truncated protein, since the cm insertion is located at theapproximate midpoint of the nlpI gene. In this event, the putativetruncated protein might be "functional" at the permissive temperature,whereas it is rendered "nonfunctional" at the nonpermissive temperatureor in media of reduced osmotic strength. Additional biochemicalstudies are required to determine whether or not the mutant synthesizesa truncated lipoprotein. In addition, it will also be of interestto determine the phenotype of mutants that either lack the nlpIgene or contain insertions more proximal to the 5' terminus ofthe gene. In this regard, the results of numerous investigationshave prompted the proposal that E. coli and related organismspossess a minor lipoprotein(s) that is required for growth andviability (39); however, an essential lipoprotein has not yetbeen identified. Accordingly, attempts to isolate additional nlpInull mutants may provide insights into whether or not NlpI isindeed an essentiallipoprotein.

	ACKNOWLEDGMENTS

We thank H. Suginaka, M. Sugai, A. Maurelli, Y. Ishi, M. Yamashita, and A. Iwagaki for helpful advice and suggestions. Wealso thank S. D. Gupta, A. Rahman, K. Barr, and A. DeJesus fortechnical assistance. Finally, we are grateful to M. Arai forthe kind gift ofglobomycin.

This work was supported by NIGMS grant GM28811 to P.D.R.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, Uniformed Services University of the HealthSciences, 4301 Jones Bridge Rd., Bethesda, MD 20814-4799. Phone:(301) 295-3418. Fax: (301) 295-1545. E-mail: Rickp{at}usuhs.mil.

Deceased 12 February1996.

Present address: Centre for Biotechnology, Anna University, Madras 600 025,India.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Begg, K., and W. D. Donachie. 1985. Cell shape and division in Escherichia coli: experiments with shape and division mutants. J. Bacteriol. 163:615-622[Abstract/Free Full Text].

2. Begg, K., Y. Nikolaichik, N. Crossland, and W. D. Donachie. 1998. Roles of FtsA and FtsZ in activation of division sites. J. Bacteriol. 180:881-884[Abstract/Free Full Text].

3. Bi, E., and J. Lutkenhaus. 1991. FtsZ ring structure associated with division in Escherichia coli. Nature (London) 354:161-164[Medline].

4. Blattner, F. R., G. Plunkett III, C. A. Bloch, N. T. Perna, V. Burland, M. Riley, J. Collade-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].

5. Borodovsky, M., K. E. Rudd, and E. V. Koonin. 1994. Intrinsic and extrinsic approaches for detecting genes in a bacterial genome. Nucleic Acids Res. 22:4756-4767[Abstract/Free Full Text].

6. Das, A. K., P. T. W. Cohen, and D. Barford. 1998. The structure of the tetratricopeptide repeats of protein phosphatase 5: implications for TPR-mediated protein-protein interactions. EMBO J. 17:1192-1199[Medline].

7. Ehlert, K., J.-V. Höltje, and M. F. Templin. 1995. Cloning and expression of a murein hydrolase lipoprotein from Escherichia coli. Mol. Microbiol. 16:761-768[Medline].

8. Erickson, H. P. 1995. FtsZ, a prokaryotic homolog of tubulin? Cell 80:367-370[Medline].

9. Goebl, M., and M. Yanagida. 1991. The TPR snap helix: a novel protein repeat motif from mitosis to transcription. Trends Biochem. Sci. 16:172-177[Medline].

10. Guzman, L.-M., D. Belin, M. J. Carson, and J. Beckwith. 1995. Tight regulation, modulation, and high-level expression by vectors containing the arabinose P_BAD promoter. J. Bacteriol. 177:4121-4130[Abstract/Free Full Text].

11. Haase, J., M. Kalkum, and E. Lanka. 1996. TrbK, a small cytoplasmic membrane lipoprotein, functions in entry exclusion of the IncP $alpha$ plasmid RP4. J. Bacteriol. 178:6720-6729[Abstract/Free Full Text].

12. Hale, C. A., and P. A. J. de Boer. 1997. Direct binding of FtsZ to ZipA, an essential component of the septal ring structure that mediates cell division in E. coli. Cell 88:175-185[Medline].

13. Hantke, K., and V. Braun. 1973. Covalent binding of lipid to protein. Diglyceride and amide-linked fatty acid at the N-terminal end of the murein-lipoprotein of the Escherichia coli outer membrane. Eur. J. Biochem. 34:284-296[Medline].

14. Hayashi, S., and H. C. Wu. 1992. Identification and characterization of lipid-modified proteins in bacteria, p. 261-285. In N. M. Hooper, and A. J. Turner (ed.), Lipid modification of proteins: a practical approach. Oxford University Press, Oxford, England.

15. Hiraga, S., H. Niki, T. Ogura, C. Ichinose, H. More, B. Ezaki, and A. Jaffé. 1989. Chromosome partitioning in Escherichia coli: novel mutants producing anucleate cells. J. Bacteriol. 171:1496-1505[Abstract/Free Full Text].

16. Holland, I. B. 1987. Genetic analysis of the E. coli division clock. Cell 48:361-362[Medline].

17. Hussain, M., S. Ichihara, and S. Mizushima. 1980. Accumulation of glyceride-containing precursor of the outer membrane lipoprotein in the cytoplasmic membrane of Escherichia coli treated with globomycin. J. Biol. Chem. 255:3707-3712[Abstract/Free Full Text].

18. Ichihara, S., M. Hussain, and S. Mizushima. 1981. Characterization of new membrane lipoproteins and their precursors of Escherichia coli. J. Biol. Chem. 256:3125-3129[Abstract/Free Full Text].

19. Inukai, M., M. Takeuchi, K. Shimizu, and M. Arai. 1978. Mechanism of action of globomycin. J. Antibiot. 31:1203-1205[Medline].

20. Inukai, M., M. Takeuchi, K. Shimizu, and M. Arai. 1979. Existence of the bound form of prolipoprotein in Escherichia coli B cells treated with globomycin. J. Bacteriol. 140:1098-1101[Abstract/Free Full Text].

21. Ito, K., T. Date, and W. Wickner. 1980. Synthesis, assembly into the cytoplasmic membrane, and proteolytic processing of the precursor of coliphage M13 coat protein. J. Biol. Chem. 255:2123-2130[Free Full Text].

22. Kraft, A. R., M. F. Templin, and J.-V. Höltje. 1998. Membrane-bound lytic endotransglycosylase in Escherichia coli. J. Bacteriol. 180:3441-3447[Abstract/Free Full Text].

23. Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature (London) 227:680-685[Medline].

24. Lamb, J. R., S. Tudendreich, and P. Hieter. 1995. Tetratrico peptide repeat interactions: to TPR or not to TPR? Trends Biochem. Sci. 20:257-259[Medline].

25. Lommatzsch, J., M. F. Templin, A. R. Kraft, W. Vollmer, and J.-V. Höltje. 1997. Outer membrane localization of murein hydrolase: MltA, a third lipoprotein lytic transglycosylase in Escherichia coli. J. Bacteriol. 179:5465-5470[Abstract/Free Full Text].

26. Lutkenhaus, J., and A. Mukherjee. 1996. Cell division, p. 1615-1626. In F. C. Neidhardt, R. Curtiss III, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. S. Reznikoff, M. Riley, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed. ASM Press, Washington, D.C.

27. Ma, J., A. Katsonouri, and R. B. Gennis. 1997. Subunit II of the cytochrome bo₃ ubiquinol oxidase from Escherichia coli is a lipoprotein. Biochemistry 36:11298-11303[Medline].

28. Maniatis, T., E. F. Fritsch, and J. Sambrook. 1989. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

29. Markiewicz, Z., J. K. Broome-Smith, U. Schwarz, and B. G. Spratt. 1982. Spherical E. coli due to elevated levels of D-alanine carboxypeptidase. Nature (London) 297:702-704[Medline].

30. Miller, J. H. 1992. A short course in bacterial genetics: a laboratory manual and handbook for Escherichia coli and related bacteria. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

31. Nanninga, N. 1991. Cell division and peptidoglycan assembly in Escherichia coli. Mol. Microbiol. 5:791-795[Medline].

32. Okada, Y., M. Wachi, A. Hirata, K. Suzuki, K. Nagai, and M. Matsuhashi. 1994. Cytoplasmic axial filaments in Escherichia coli cells: possible function in the mechanism of chromosome segregation and cell division. J. Bacteriol. 176:917-922[Abstract/Free Full Text].

33. Régnier, P., M. Grunberg-Manago, and C. Portier. 1987. Nucleotide sequence of the pnp gene of Escherichia coli encoding polynucleotide phosphorylase. J. Biol. Chem. 262:63-68[Abstract/Free Full Text].

34. Slater, S., and R. Maurer. 1993. Simple phagemid-based system for generating allele replacements in Escherichia coli. J. Bacteriol. 175:4260-4262[Abstract/Free Full Text].

35. Theisen, M. 1996. Molecular cloning and characterization of nlpH, encoding a novel, surface-exposed, polymorphic, plasmid-encoded 33-kilodalton lipoprotein of Borrelia afzelii. J. Bacteriol. 178:6435-6442[Abstract/Free Full Text].

36. Toone, W. M., K. E. Rudd, and J. D. Friesen. 1991. deaD, a new Escherichia coli gene encoding a presumed ATP-dependent RNA helicase, can suppress a mutation in rpsB, the gene encoding ribosomal protein S2. J. Bacteriol. 173:3291-3302[Abstract/Free Full Text].

37. Vicente, M., S. R. Kushner, T. Garrido, and M. Aldea. 1991. The role of the `gearbox' in the transcription of essential genes. Mol. Microbiol. 5:2085-2091[Medline].

38. Ward, J. E., and J. Lutkenhaus. 1985. Overproduction of FtsZ induces minicell formation in E. coli. Cell 42:941-949[Medline].

39. Wu, H. C. 1996. Biosynthesis of lipoproteins, p. 1005-1014. In F. C. Neidhardt, R. Curtiss III, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. S. Reznikoff, M. Riley, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed. ASM Press, Washington, D.C.

40. Yu, F., S. Inouye, and M. Inouye. 1986. Lipoprotein-28, a cytoplasmic membrane lipoprotein from Escherichia coli. Cloning, DNA sequence, and expression of its gene. J. Biol. Chem. 261:2284-2288[Abstract/Free Full Text].

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	ALL ASM JOURNALS

1.	Begg, K., and W. D. Donachie. 1985. Cell shape and division in Escherichia coli: experiments with shape and division mutants. J. Bacteriol. 163:615-622[Abstract/Free Full Text].
2.	Begg, K., Y. Nikolaichik, N. Crossland, and W. D. Donachie. 1998. Roles of FtsA and FtsZ in activation of division sites. J. Bacteriol. 180:881-884[Abstract/Free Full Text].
3.	Bi, E., and J. Lutkenhaus. 1991. FtsZ ring structure associated with division in Escherichia coli. Nature (London) 354:161-164[Medline].
4.	Blattner, F. R., G. Plunkett III, C. A. Bloch, N. T. Perna, V. Burland, M. Riley, J. Collade-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].
5.	Borodovsky, M., K. E. Rudd, and E. V. Koonin. 1994. Intrinsic and extrinsic approaches for detecting genes in a bacterial genome. Nucleic Acids Res. 22:4756-4767[Abstract/Free Full Text].
6.	Das, A. K., P. T. W. Cohen, and D. Barford. 1998. The structure of the tetratricopeptide repeats of protein phosphatase 5: implications for TPR-mediated protein-protein interactions. EMBO J. 17:1192-1199[Medline].
7.	Ehlert, K., J.-V. Höltje, and M. F. Templin. 1995. Cloning and expression of a murein hydrolase lipoprotein from Escherichia coli. Mol. Microbiol. 16:761-768[Medline].
8.	Erickson, H. P. 1995. FtsZ, a prokaryotic homolog of tubulin? Cell 80:367-370[Medline].
9.	Goebl, M., and M. Yanagida. 1991. The TPR snap helix: a novel protein repeat motif from mitosis to transcription. Trends Biochem. Sci. 16:172-177[Medline].
10.	Guzman, L.-M., D. Belin, M. J. Carson, and J. Beckwith. 1995. Tight regulation, modulation, and high-level expression by vectors containing the arabinose P_BAD promoter. J. Bacteriol. 177:4121-4130[Abstract/Free Full Text].
11.	Haase, J., M. Kalkum, and E. Lanka. 1996. TrbK, a small cytoplasmic membrane lipoprotein, functions in entry exclusion of the IncP $alpha$ plasmid RP4. J. Bacteriol. 178:6720-6729[Abstract/Free Full Text].
12.	Hale, C. A., and P. A. J. de Boer. 1997. Direct binding of FtsZ to ZipA, an essential component of the septal ring structure that mediates cell division in E. coli. Cell 88:175-185[Medline].
13.	Hantke, K., and V. Braun. 1973. Covalent binding of lipid to protein. Diglyceride and amide-linked fatty acid at the N-terminal end of the murein-lipoprotein of the Escherichia coli outer membrane. Eur. J. Biochem. 34:284-296[Medline].
14.	Hayashi, S., and H. C. Wu. 1992. Identification and characterization of lipid-modified proteins in bacteria, p. 261-285. In N. M. Hooper, and A. J. Turner (ed.), Lipid modification of proteins: a practical approach. Oxford University Press, Oxford, England.
15.	Hiraga, S., H. Niki, T. Ogura, C. Ichinose, H. More, B. Ezaki, and A. Jaffé. 1989. Chromosome partitioning in Escherichia coli: novel mutants producing anucleate cells. J. Bacteriol. 171:1496-1505[Abstract/Free Full Text].
16.	Holland, I. B. 1987. Genetic analysis of the E. coli division clock. Cell 48:361-362[Medline].
17.	Hussain, M., S. Ichihara, and S. Mizushima. 1980. Accumulation of glyceride-containing precursor of the outer membrane lipoprotein in the cytoplasmic membrane of Escherichia coli treated with globomycin. J. Biol. Chem. 255:3707-3712[Abstract/Free Full Text].
18.	Ichihara, S., M. Hussain, and S. Mizushima. 1981. Characterization of new membrane lipoproteins and their precursors of Escherichia coli. J. Biol. Chem. 256:3125-3129[Abstract/Free Full Text].
19.	Inukai, M., M. Takeuchi, K. Shimizu, and M. Arai. 1978. Mechanism of action of globomycin. J. Antibiot. 31:1203-1205[Medline].
20.	Inukai, M., M. Takeuchi, K. Shimizu, and M. Arai. 1979. Existence of the bound form of prolipoprotein in Escherichia coli B cells treated with globomycin. J. Bacteriol. 140:1098-1101[Abstract/Free Full Text].
21.	Ito, K., T. Date, and W. Wickner. 1980. Synthesis, assembly into the cytoplasmic membrane, and proteolytic processing of the precursor of coliphage M13 coat protein. J. Biol. Chem. 255:2123-2130[Free Full Text].
22.	Kraft, A. R., M. F. Templin, and J.-V. Höltje. 1998. Membrane-bound lytic endotransglycosylase in Escherichia coli. J. Bacteriol. 180:3441-3447[Abstract/Free Full Text].
23.	Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature (London) 227:680-685[Medline].
24.	Lamb, J. R., S. Tudendreich, and P. Hieter. 1995. Tetratrico peptide repeat interactions: to TPR or not to TPR? Trends Biochem. Sci. 20:257-259[Medline].
25.	Lommatzsch, J., M. F. Templin, A. R. Kraft, W. Vollmer, and J.-V. Höltje. 1997. Outer membrane localization of murein hydrolase: MltA, a third lipoprotein lytic transglycosylase in Escherichia coli. J. Bacteriol. 179:5465-5470[Abstract/Free Full Text].
26.	Lutkenhaus, J., and A. Mukherjee. 1996. Cell division, p. 1615-1626. In F. C. Neidhardt, R. Curtiss III, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. S. Reznikoff, M. Riley, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed. ASM Press, Washington, D.C.
27.	Ma, J., A. Katsonouri, and R. B. Gennis. 1997. Subunit II of the cytochrome bo₃ ubiquinol oxidase from Escherichia coli is a lipoprotein. Biochemistry 36:11298-11303[Medline].
28.	Maniatis, T., E. F. Fritsch, and J. Sambrook. 1989. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
29.	Markiewicz, Z., J. K. Broome-Smith, U. Schwarz, and B. G. Spratt. 1982. Spherical E. coli due to elevated levels of D-alanine carboxypeptidase. Nature (London) 297:702-704[Medline].
30.	Miller, J. H. 1992. A short course in bacterial genetics: a laboratory manual and handbook for Escherichia coli and related bacteria. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
31.	Nanninga, N. 1991. Cell division and peptidoglycan assembly in Escherichia coli. Mol. Microbiol. 5:791-795[Medline].
32.	Okada, Y., M. Wachi, A. Hirata, K. Suzuki, K. Nagai, and M. Matsuhashi. 1994. Cytoplasmic axial filaments in Escherichia coli cells: possible function in the mechanism of chromosome segregation and cell division. J. Bacteriol. 176:917-922[Abstract/Free Full Text].
33.	Régnier, P., M. Grunberg-Manago, and C. Portier. 1987. Nucleotide sequence of the pnp gene of Escherichia coli encoding polynucleotide phosphorylase. J. Biol. Chem. 262:63-68[Abstract/Free Full Text].
34.	Slater, S., and R. Maurer. 1993. Simple phagemid-based system for generating allele replacements in Escherichia coli. J. Bacteriol. 175:4260-4262[Abstract/Free Full Text].
35.	Theisen, M. 1996. Molecular cloning and characterization of nlpH, encoding a novel, surface-exposed, polymorphic, plasmid-encoded 33-kilodalton lipoprotein of Borrelia afzelii. J. Bacteriol. 178:6435-6442[Abstract/Free Full Text].
36.	Toone, W. M., K. E. Rudd, and J. D. Friesen. 1991. deaD, a new Escherichia coli gene encoding a presumed ATP-dependent RNA helicase, can suppress a mutation in rpsB, the gene encoding ribosomal protein S2. J. Bacteriol. 173:3291-3302[Abstract/Free Full Text].
37.	Vicente, M., S. R. Kushner, T. Garrido, and M. Aldea. 1991. The role of the `gearbox' in the transcription of essential genes. Mol. Microbiol. 5:2085-2091[Medline].
38.	Ward, J. E., and J. Lutkenhaus. 1985. Overproduction of FtsZ induces minicell formation in E. coli. Cell 42:941-949[Medline].
39.	Wu, H. C. 1996. Biosynthesis of lipoproteins, p. 1005-1014. In F. C. Neidhardt, R. Curtiss III, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. S. Reznikoff, M. Riley, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed. ASM Press, Washington, D.C.
40.	Yu, F., S. Inouye, and M. Inouye. 1986. Lipoprotein-28, a cytoplasmic membrane lipoprotein from Escherichia coli. Cloning, DNA sequence, and expression of its gene. J. Biol. Chem. 261:2284-2288[Abstract/Free Full Text].