Induced Expression of the Legionella pneumophila Gene Encoding a 20-Kilodalton Protein during Intracellular Infection

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Kwaik, Y. A.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Kwaik, Y. A.

Previous Article | Next Article

Infect Immun, January 1998, p. 203-212, Vol. 66, No. 1
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Induced Expression of the Legionella pneumophila Gene Encoding a 20-Kilodalton Protein during Intracellular Infection

Yousef Abu Kwaik^*

Department of Microbiology and Immunology, University of Kentucky Chandler Medical Center, Lexington, Kentucky 40536-0084

Received 5 March 1997/Returned for modification 16 June 1997/Accepted 17 October 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

The eukaryotic protein synthesis inhibitor cycloheximid has been used by many investigators to selectively radiolabel intracellularbacteria. Although cycloheximide has no direct effect on bacterialgene expression, there are concerns that long-term inhibitionof the host cell protein synthesis may have secondary effectson bacterial gene expression. Therefore, prior to further identificationand cloning of the macrophage-induced (MI) genes of Legionellapneumophila, the effects of cycloheximide on L. pneumophila-infectedU937 cells were evaluated by transmission electron microscopy.Inhibition of protein synthesis of the host cell for 6 h had nomajor effect on the ultrastructure of the host cell, on the formationof rough endoplasmic reticulum-surrounded replicative phagosome,or on initiation of intracellular bacterial replication. In contrast,by 15 h of cycloheximide treatment, there was profound deteriorationin the host cell as well as in the phagosome. To examine proteinsynthesis by L. pneumophila during the intracellular infection,U937 macrophage-like cells were infected with L. pneumophila,and intracellular bacteria were radiolabeled during a 2-h cycloheximidetreatment or following 12 h of cycloheximide treatment. Comparisonby two-dimensional sodium dodecyl sulfate-polyacrylamide gel electrophoresisof the protein profile of radiolabeled in vitro-grown L. pneumophilato that of intracellularly radiolabeled bacteria showed that 23proteins were induced in response to the intracellular environmentduring 2 h of inhibition of host cell protein biosynthesis. TwelveMI proteins of L. pneumophila were artifactually induced due toprolonged inhibition of the host cell protein synthesis. The geneencoding a 20-kDa MI protein was cloned by a reverse geneticstechnique. Sequence analysis showed that the cloned gene encodeda protein that was 80% similar to the enzyme inorganic pyrophosphatase.Studies of promoter fusion to a promoterless lacZ gene showedthat compared to in vitro-grown bacteria, expression of the pyrophosphatasegene (ppa) was induced fourfold throughout the intracellular infection.There was no detectable induction in transcription of the ppapromoter during exposure to stress stimuli in vitro. The ppa geneof L. pneumophila is the first example of a regulated ppa genewhich is selectively induced during intracellular infection andwhich may reflect enhanced capabilities of macromolecular biosynthesisby intracellular L. pneumophila. The data indicate caution inthe long-term use of inhibition of host cell protein synthesisto selectively examine gene expression by intracellular bacteria.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Legionella pneumophila is a ubiquitous organism in the natural aquatic environment where it is amplified by intracellularmultiplication within protozoa (reviewed in reference 17). Theability of L. pneumophila to cause Legionnaires' disease is dependenton its capacity to survive and to multiply within host alveolarmacrophages and possibly alveolar epithelial cells (14, 21,35).

Part of the uptake of L. pneumophila by macrophages is mediated by the complement receptor (36). We have recently shownthat uptake of L. pneumophila by the protozoan Hartmanella vermiformisis mediated by a $beta$ 2 integrin-like galactose lectin, which undergoesa time-dependent tyrosine dephosphorylation upon bacterial attachment(46). Although the mechanisms of L. pneumophila uptake by macrophagesand by protozoa are different (5, 25), the intracellularlife cycles of the bacterium within mammalian macrophages andwithin protozoa are highly similar (2, 18a, 19). In bothhost cells, the bacterium replicates in a phagosome that is inhibitedfrom maturation through the endosomal-lysosomal pathway and issurrounded by the rough endoplasmic reticulum (RER) (2, 10,19, 20, 43).

Pathogenic bacteria such as L. pneumophila and Salmonella typhimurium respond and adapt to the various local environmentalconditions that they encounter by coordinate regulation of geneexpression (1, 3, 16, 42). Upon phagocytosis and duringintracellular survival, facultative intracellular pathogens areexposed to a complex mixture of stimuli, and they respond to thesestimuli by a profound alteration in gene expression (1, 3,16). These phenotypic modulations allow intracellular bacteriato survive and adapt to environmental conditions that may be encounteredintracellularly, including nutrient limitation, temperature, oxidativeinjury, osmolarity, pH, and other stimuli (6, 33, 41).The phenotypic alteration by intracellular pathogens is controlledby multiple regulons and is most probably a simultaneous responseto a complex combination of unknown stimuli. Characterizationof the bacterial macrophage-induced (MI) genes and examinationof the kinetics of their expression during the intracellular infectionwill facilitate characterization of the phagosomal microenvironmentthat the organisms are exposed to within the host cell. We andothers have shown that intracellular L. pneumophila manifestsa stress response to the intracellular environment (3, 6,16). We have recently shown that the global stress gene (gspA)of L. pneumophila is induced in response to in vitro stress stimuliand is also induced throughout the intracellular infection period(4, 6). Differential expression of gspA by a $sigma$ ³²-regulated promoter throughout the intracellular infection isindicative of a continuous stress response manifested by intracellularbacteria (6). Besides the evidence of exposure of intracellularL. pneumophila to unidentified stress stimuli (3, 6, 16),the intracellular niche of L. pneumophila is not well identified.

To start understanding the nature of the microenvironment within the replicative vacuole and the biochemical signals thatintracellular L. pneumophila is exposed to, the technique of reversegenetics was utilized to isolate and characterize one of the 23L. pneumophila MI genes that are specifically induced during intracellularinfection.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Bacterial strains and vectors. The virulent AA100 strain of L. pneumophila has been described previously (3, 15). Escherichia coli XL1-Blue was usedas the host for the genomic library. E. coli K-12 derivative strain $chi$ 2981 is an asd insertion mutant that renders it auxotrophic fordiaminopimelic acid (7).

The plasmids pBluescript and pBC were purchased from Stratagene (La Jolla, Calif.). The plasmid pUC-4K was purchased fromPharmacia Biotechnologies (Piscataway, N.J.), and was the sourceof the kanamycin resistance gene in generating the insertionalmutations. The single-copy plasmid pEU730 is a spectinomycin-resistantplasmid containing a promoterless lacZ gene, kindly provided byR. Perry (University of Kentucky, Lexington) (18). Bacteriaharboring pEU730 or its derivative (pPPZ) were maintained by growthon agar plates supplemented with 0.5 mg of spectinomycin per ml.The high concentration of spectinomycin is required to selectfor extrachromosomal locus on the plasmid, since L. pneumophilacontains a chromososmal spectinomycin resistance gene (12a).The plasmid pBOC20 (kindly provided by N. Cianciotto, NorthwesternUniversity, Chicago, Ill.) is a chloramphenicol-resistant plasmidthat contains oriT and the sacB gene, which is lethal to L. pneumophilagrown in the presence of sucrose (13). The conjugative plasmidpRK212.1 was used as a helper plasmid to mobilize the pBOC20 vectorand its recombinant derivatives by triparental conjugation intoL. pneumophila (8).

DNA manipulations. Chromosomal DNA preparations, transfection, in situ colony hybridization, end radiolabeling of oligonucleotides, restrictionenzyme digestion, and DNA ligation were performed as describedelsewhere (39) unless specified. Restriction enzymes, T4 polynucleotidekinase, and T4 DNA ligase were obtained from Bethesda ResearchLaboratories (BRL) (Gaithersburg, Md.).

Plasmid DNA preparations were done by using the QIAGEN (Chatsworth, Calif.) plasmid kit according to manufacturer's recommendations.Transformations were carried out by electroporation with a Bio-Rad(Hercules, Calif.) gene pulser as recommended by the manufacturer.Purification of DNA fragments from agarose gels for subcloningor labeling for Southern hybridization was done by using a QIAEXkit (QIAGEN) according to manufacturer's recommendations. Transferof DNA from agarose gels onto membranes, fluorescein labelingof DNA probes, hybridizations, and detection were done as describedpreviously (4). For DNA sequencing, the dideoxy chain terminationmethod of Sanger et al. (40) was employed. Oligonucleotide primerswere synthesized commercially (BRL).

Tissue culture. Macrophage-like U937 cells were maintained at 37°C and 5% CO₂ in RPMI 1640 tissue culture medium supplemented with 10% heat-inactivatedfetal calf serum (Sigma Chemical Co., St. Louis, Mo.). Prior toinfection, the cells were differentiated with phorbol 12-myristate13-acetate for 48 h, as described previously (3). Differentiatedcells are nonreplicative adherent macrophage-like cells. Monolayerswere washed three times with the tissue culture medium prior toinfection. For infection of monolayers, L. pneumophila grown for48 h at 37°C on BCYE agar plates were resuspended in RPMI 1640.The infection was carried out as described for each experiment.

Transmission electron microscopy. U937 cell monolayers were treated with cycloheximide for 30 min prior to the beginning of the infection by L. pneumophilaat a multiplicity of infection (MOI) of 10, followed by extensivewashing of extracellular bacteria with tissue culture medium.To examine phagocytosis, infection was carried out for 3 min atan MOI of 500. At several time intervals, infected U937 cell monolayerswere fixed in 3.5% glutaraldehyde in 0.1 M phosphate buffer (pH7.4) for 1 h on ice followed by 1% OsO₄ in 0.1 M phosphate bufferfor 1 h on ice. Dehydration was accomplished by serial exposureto ethanol (50 to 100%) for 10 min at room temperature. The cellswere embedded in Eponate 12 resin (Ted Pella, Redding, Calif.)according to the manufacturer's recommendations. Ultrathin sectionswere stained with uranyl acetate followed by lead citrate andexamined with a Hitachi model H-7000/STEM electron microscopeat 75 kV.

Radiolabeling of bacteria and two-dimensional polyacrylamide gel electrophoresis (PAGE). A modification of a previously reported protocol (3) was used to radiolabel intracellular L. pneumophila. Monolayers ofdifferentiated U937 cells were infected for 1 h with L. pneumophilaAA100 resuspended in RPMI 1640 (Gibco, Gaithersburg, Md.) at abacterium-to-U937 ratio of 10:1. The monolayers were subsequentlywashed and treated with gentamicin (50 µg/ml) for 1 h to killextracellular bacteria. Two sets of infected monolayers were used;in one set, cycloheximide (200 µg/ml) was added immediately tothe monolayers after the gentamicin treatment, while for the secondinfected monolayers, cycloheximide was added after 12 h of theinfection, prior to radiolabeling of intracellular bacteria. [³⁵S]methionine (150 µCi/ml) was added to both sets of infected monolayersfor an additional 2 h to permit incorporation of the label. UninoculatedU937 cells monolayers and monolayers infected with heat-killedL. pneumophila were also radiolabeled under the same experimentalconditions to confirm the complete inhibition of protein synthesisof the macrophage. Intracellular radiolabeled organisms were harvestedas described previously (3). For comparison, bacteria wereradiolabeled in vitro in defined medium during mid-log growthphase in a manner similar to that of intracellular bacteria, exactlyas described previously (3).

Cell extracts of the radiolabeled bacterial pellet were prepared by the methods of O'Farrel, as described previously (3).Equal amounts of tricarboxylic acid-precipitated radiolabeledproteins were subjected to equilibrium isoelectric focusing priorto separation in the second dimension on sodium dodecyl sulfate(SDS)-11.5% PAGE slab gels. After electrophoresis, the gels weredried and autoradiographed by using Kodak BIO-MAX film.

Protein isolation and partial N-terminal sequence analysis. The protein spot on two-dimensional SDS-PAGE corresponding to the MI protein was isolated for N-terminal sequencing, as describedpreviously (3). Briefly, after electrophoresis gels were soakedin transfer buffer [10 mM 3-(cyclohexylamino)-1-propanesulfonicacid-10% methanol (pH 11.0)] for 10 min and the proteins weretransferred onto a polyvinylidene difluoride membrane (Immobilon;Millipore) for 30 min at 50 V (150 to 170 mA) in a Trans-Blotcell (Bio-Rad, Richmond, Calif.). The membranes were stained withCoomassie brilliant blue R-250 (Sigma), and the stained proteinspots were subjected to direct, automated Edman degradation.

Cloning. A degenerate oligonucleotide corresponding to the amino acid sequence of the N terminus of the MI protein was synthesized(BRL). The sequence of the degenerate oligonucleotide was 5'-GGI(C/A)GIGA(T/C)GTICCIAA,where I is inosine. The oligonucleotide was radiolabeled and usedas a probe for in situ colony hybridizations to screen the L.pneumophila partial genomic library (39). The partial genomiclibrary was constructed by ligating gel-purified 2- to 2.5-kbEcoRI fragments into plasmid pBC and transformed into E. coli.The in situ colony hybridizations were performed exactly as describedpreviously (4).

Transposon mutagenesis. To facilitate subsequent allelic exchanges of insertion mutations in the cloned 2.2-kb insert, it was subcloned into plasmidpBOC20 to generate pJA2a. Transposon mutagenesis of pJA2 was performedby using lambda 1105 containing mini-Tn10-kan, exactly as describedpreviously (7). Selected insertions were introduced into L.pneumophila AA100 by triparental conjugation (8).

Primer extension. Total RNA was isolated from BCYE-grown L. pneumophila and from intracellular bacteria in U937 monolayers, exactly as describedpreviously (7). The isolated RNA was used immediately or storedat $-$ 20°C. For 5' primer extensions, an oligonucleotide with thesequence 5'-CTTCATACTTTACAGGTTCTCCGTGCATAG was used, and the reactionswere carried out exactly as described previously (4).

In vitro transcription-translation. A coupled in vitro transcription-translation system was used to examine the polypeptides expressed by pJA2 (Promega Biotech,Madison, Wis.). [³⁵S]methionine was used to radiolabel the polypeptides. The reactionproducts were resolved by SDS-PAGE and autoradiography.

Fusion of the ppa promoter to a promoterless lacZ gene and $beta$ -galactosidase ( $beta$ -Gal) assays. The sequence encompassing the promoter region upstream of the initiation codon of ppa was amplified by PCR with the primers5'-CGCTTAATTAAGTGGTAAACTTCCTGCCC and 5'-GCGGGTACCTTACGCACCCTTAATAAT.The PCR reaction was carried out in the presence of 2.5 mM Mg²⁺-0.25 mM deoxynucleoside triphosphates-0.2 µg of each primer-50ng of the template PJA2a-2.5 U of Taq polymerase (Stratagene)in a 100-µl reaction mixture. The PCR protocol included one stepof denaturation at 94°C for 5 min, 5 cycles of annealing at 48°Cfor 1 min, and extension at 72°C for 30 s followed by 25 cyclesof annealing at 58°C and extension at 72°C for 1 min each. ThePCR product was purified from an agarose gel and directionallycloned into the PacI-KpnI sites of the single-copy plasmid pEU730(18), which places the promoterless lacZ gene under the controlof the ppa promoter. The in-frame construct was confirmed by DNAsequencing of the junction. The recombinant was designated pPPZand electroporated into L. pneumophila.

$beta$ -Gal expression was monitored during several stages of growth in vitro. Culture aliquots for each $beta$ -Gal determination wereplated to determine the number of CFU per milliliter, and thus, $beta$ -Gal activity could be expressed as units per CFU (34). Toassess $beta$ -Gal activity in response to stress stimuli, mid-log-phaseL. pneumophila grown in BYE (optical density at 550 nm of 0.6to 0.7) was exposed to stress stimuli, as described previously(3). Bacteria were pelleted immediately after exposure to thestress stimuli and resuspended in BYE for determination of $beta$ -Galactivity.

To determine $beta$ -Gal activity from intracellularly grown L. pneumophila at several stages of the intracellular infection, monolayersof differentiated U937 cells were infected with L. pneumophilaharboring pPPZ or pEU730. The infection was accomplished withan MOI of 10 for 1 h followed by three washes with tissue culturemedium to remove most of the extracellular bacteria. Gentamicintreatment (50 µg/ml) was done for 1 h to kill any remaining extracellularbacteria, followed by three washes with tissue culture medium.At several time intervals, monolayers were washed three timeswith tissue culture medium and lysed hypotonically with distilledwater. Aliquots of the lysate were diluted and plated to determinethe number of intracellular CFU per milliliter. $beta$ -Gal activitywas determined for each lysate and calculated in terms of Millerunits per CFU (34). To determine whether the $beta$ -Gal assay wasaffected by debris of the lysed U937 cells, mid-log-phase BYE-grownL. pneumophila was pelleted and resuspended in a lysate of uninfectedmonolayers for 30 to 60 min prior to measurement of $beta$ -Gal activity.

Nucleotide sequence accession number. The nucleotide sequence of the predicted open reading frame encoding the 178-amino-acid protein identified in this study hasbeen assigned GenBank accession no. AFO31464.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Effects of long-term inhibition of host cell protein biosynthesis on phagosomal ultrastructure. Cycloheximide is a protein synthesis inhibitor of eukaryotic cells that has been used by many investigators to examine proteinsynthesis by intracellular bacterial pathogens (1, 3). However,the long-term use of this inhibitor may have secondary effectson bacterial gene expression due to possible physiological changesin the host cell. To examine this possibility, the effect of inhibitionof protein synthesis of the host cell was examined at severaltimes during the intracellular infection of the U937 macrophage-likecells. In these experiments, cycloheximide was added to the monolayers30 min prior to the infection. At several intervals (3 min and1 h, 2, 4, 6, 8, and 15 h), the monolayers were fixed and processedfor transmission electron microscopy. Control untreated, infectedmonolayers were also examined. Complete inhibition of host cellprotein synthesis was confirmed by the failure of uninfected U937cells to incorporate [³⁵S]methionine compared to that of untreated cells (data not shown).Compared to that in untreated infected cells, there was no detectableeffect of cycloheximide on recruitment of the host cell organellesaround the L. pneumophila phagosome or on formation of the RER-surroundedreplicative vacuole during the first 6 h of treatment (Fig. 1)(19, 43). Inhibition of host cell protein synthesis for 8h did not have any detectable effect on the ability of L. pneumophilato initiate bacterium replication as detected by transmissionelectron microscopy at 8 h postinfection (Fig. 1 and 2A) and bythe number of intracellular bacteria, which had increased forat least two generations (data not shown). There were no majorultrastructural alterations in the host cell during the first8 h of inhibition of protein synthesis, with the exception ofincreased frequency of fusion of cellular vesicles to the phagosome,and there may have been some minor changes in the host cell at6 h as well (Fig. 1 and 2). These data showed that inhibitionof protein synthesis of the host cell for 6 h during infectiondid not have a major effect on the ultrastructure of the replicativevacuole or the rest of the infected cell.

View larger version (166K):
[in this window]
[in a new window]

FIG. 1. Electron micrographs of infected U937 cells during inhibition of host cell protein synthesis at 1 h (a), 2 h (b), 4 h (c), 6 h (d), 8 h (e), and 15-h (f) postinfection. Arrowheads indicate the smooth multilayer phagosomal membrane, arrows indicate the RER surrounded phagosome, M indicates mitochondria, and B indicates bacteria. Note the vesicles making contact and possibly fusing with the phagosomal membrane at 8 h in panel e. Note the absence of a defined membrane around the phagosome at 15 h in panel f. Bars, 0.5 µm.

View larger version (151K):
[in this window]
[in a new window]

FIG. 2. Electron micrographs of untreated infected U937 cells at 8 h (A) and 15 h (B) postinfection. Arrowheads indicate the RER-surrounded phagosome.

In contrast, after 15 h of inhibition of protein synthesis of the host cell, there was a clear evidence of deterioration ofthe ultrastructure of the replicative vacuole and the rest ofthe host cell as well (Fig. 1f and 2B). Although L. pneumophilaappeared to be in clusters, there was no definitive visible phagosomalmembrane and no visible RER around the vacuole. These observationsindicated that long-term inhibition of host cell protein synthesishad dramatic effects on cell physiology and ultrastructure. Thesechanges may have a secondary effect on bacterial gene expression.The data indicated that caution should be taken with interpretationof data obtained with the long-term use of this inhibitor to examinegene expression of other slow-growing intracellular bacterialpathogens, such as Mycobacterium tuberculosis, for which bacterialprotein synthesis has been examined after 23 h of cycloheximidtreatment of infected cells (31).

Protein synthesis by intracellular L. pneumophila. The protein profile of radiolabeled intracellular L. pneumophila has been previously reported (3). In that report, theU937 macrophage-like cells were treated with cycloheximide formore than 20 h during radiolabeling of intracellular bacteria.Since inhibition of protein synthesis of the host cell for 15h had profound effects on the host cell biology, we reevaluatedprotein synthesis by intracellular L. pneumophila radiolabeledduring cycloheximide treatment of infected cells. In the previousstudy cycloheximide was added to the monolayers at the beginningof the infection, and intracellular bacteria were radiolabeledat mid-log phase (3). In this study, mid-log-phase intracellularbacteria were radiolabeled for 2 h in U937 cells treated withcycloheximide at the beginning of the infection or just priorto the 2 h radiolabeling of intracellular bacteria. Examinationof infected cells at the end of the cycloheximide treatment showedthat in contrast to cellular deteriorations after prolonged inhibitionof protein synthesis of the host cell, this short-term treatmentdid not have any detectable effect on the ultrastructural characteristicsof the replicative phagosome or on multiplication of intracellularbacteria (data not shown).

Extracts of intracellular radiolabeled L. pneumophila were subjected to two-dimensional SDS-PAGE, and the protein profilewas compared to that of in vitro-grown bacteria radiolabeled duringthe same growth phase. Equal amounts of radioactivity (in countsper minute) were loaded for intracellular and in vitro-grown bacteria.Figure 3 shows the protein profile of radiolabeled intracellularL. pneumophila in which cycloheximide was added just prior toradiolabeling of intracellular bacteria. Compared to the proteinprofile of in vitro-grown organisms (3), the spots marked byarrowheads (Fig. 3) indicate the 23 proteins that were inducedin response to the intracellular environment (3). In contrastto the detection of 35 MI proteins in intracellular L. pneumophilafollowing 12 h of cycloheximide treatment of infected cells (3),there was an induction of only 23 of the 35 MI proteins inducedduring prolonged inhibition of the host cell protein biosynthesis(3). There was no detectable difference in the repressed proteins.It has been previously shown that there is no detectable differencein the protein profiles of intracellular bacteria labeled at 10to 12 h postinfection compared to that radiolabeled at 20 to 22h postinfection (3). Thus, long-term inhibition of proteinsynthesis of the host cell had a secondary effect of artifactualinduction of expression of at least 12 L. pneumophila proteins(marked by small and large bold arrows in Fig. 3).

View larger version (73K):
[in this window]
[in a new window]

FIG. 3. Autoradiograph of two-dimensional SDS-PAGE of L. pneumophila proteins radiolabeled intracellularly in U937 cells during 2 h of cycloheximide treatment and compared to the protein profile of intracellular bacteria radiolabeled during the same growth phase after 12 h of inhibition of host cell protein synthesis and to in vitro-grown bacteria during the same growth phase (3). The alkaline-to-acid gradient is from left to right. Arrowheads indicate the proteins that were induced in response to the intracellular environment. Closed arrows indicate the proteins that were artifactually induced as a result of prolonged inhibition of host cell protein synthesis (3). The open arrow indicates the 20-kDa PPase that is uniquely induced in response to the intracellular environment. The spots in squares represent the two major spots shown in Fig. 4 on both sides of the 20 kDa PPase. The spot in the circle represents the protein to which the levels of 20-kDa PPase was normalized.

Cloning of one of the MI genes of L. pneumophila. The microenvironment of the RER-surrounded phagosome containing L. pneumophila and the biochemical signals to which the bacteriaare exposed in their specialized and unique niche are not known.To start understanding this microenvironment, one of the MI genesthat was specifically induced during the intracellular infectionand not induced by in vitro stress stimuli was cloned and characterized(3). The protein spot marked by an open arrow (Fig. 3 and 4),which was shown by phosphorimaging semiquantitation to be inducedby approximately 3.4-fold, was subjected to N-terminal amino acidsequencing by Edman degradation. The sequence obtained was SLMEIPSGRDVPNEVNVIIE,with serine as the N-terminal amino acid. A degenerate oligonucleotidecorresponding to the underlined sequence was synthesized. In Southernhybridizations, the probe hybridized to single 1.8-kb BamHI, 11-kbClaI, 2.2-kb EcoRI, 3.2-kb EcoRV, and 8-kb HindIII fragments ofL. pneumophila chromosomal DNA (Fig. 5). A partial genomic libraryof the ~2.2-kb EcoRI fragments was constructed in plasmid pBC.Screening was performed by in situ colony hybridizations withthe degenerate oligonucleotide as a probe. Two positive cloneswere isolated, and one clone, designated pJA2, was chosen forfurther analysis (Fig. 5).

View larger version (85K):
[in this window]
[in a new window]

FIG. 4. Magnification of portions of two-dimensional gels to illustrate the protein level of the PPase protein expressed in vitro-grown bacteria (A) compared to that expressed by intracellular bacteria (B). The arrows indicate the 20-kDa PPase that is uniquely induced in response to the intracellular environment. Although three spots on the left of PPase seem to be slightly induced in this gel, they were not reproducible in multiple experiments.

View larger version (39K):
[in this window]
[in a new window]

FIG. 5. (Top) Restriction map of pJA2 insert; (bottom) Southern hybridization of chromosomal DNA of L. pneumophila digested and probed with the degenerate oligonucleotide corresponding to the N-terminus sequence of the 20-kDa MI protein. Lanes: 1, 1.8-kb BamHI; 2, 11-kb ClaI; 3, 2.2-kb EcoRI; 4, 3.2-kb EcoRV; 5, 8-kb HindIII. The second signal in lane 4 is an artifact. The sizes were based on a 1-kb ladder (BRL).

Sequence analysis. The degenerate oligonucleotide corresponding to the N-terminal sequence was used for an initial sequencing reaction, and subsequentoligonucleotides were synthesized. The DNA sequence revealed thepresence of a predicted open reading frame consisting of 534 nucleotidesencoding a 178-amino-acid protein (Gen Bank accession no. AF031464.There was a Shine-Dalgarno sequence 8 nucleotides upstream ofthe initiation codon, strongly suggesting that this initiationcodon represented a translational initiation site.

To identify the promoter regulating transcription of the MI gene, we identified the transcriptional initiation site by 5'primer extension analysis. By comparing the synthesized cDNA tothe DNA from a sequencing reaction primed with the same oligonucleotide,the 5' primer end of the cDNA was mapped to 30 nucleotides upstreamof the initiation codon (Fig. 6). Analysis of the DNA sequenceupstream from the transcriptional start site suggested the presenceof potential -10 and -35 regions that appeared to be similar to $sigma$ ⁷⁰-regulated promoters.

View larger version (69K):
[in this window]
[in a new window]

FIG. 6. Primer extension analysis of ppa transcript. A radiolabeled oligonucleotide was annealed to RNA isolated from BYE-grown bacteria, and reverse transcriptase was added to produce cDNA. The same oligonucleotide was used to prime the dideoxy sequencing reaction of pJA2 DNA. The letters above each lane indicate the dideoxy nucleotide used to terminate each reaction. The arrow indicates the 5' end of the mRNA specie corresponding to nucleotide 140.

Translation of the predicted open reading frame revealed that it encoded a protein with a predicated molecular mass of 20kDa and an estimated isoelectric point of 5.22. These resultsare in agreement with the size of the protein and its migrationin the acidic portion of the two-dimensional SDS-PAGE (Fig. 3).Expression of the 20-kDa MI protein by the cloned fragment wasconfirmed by in vitro transcription-translation, which showedsynthesis of the 20-kDa polypeptide encoded by pJA2 compared tothe pBC vector (Fig. 7). Furthermore, the N-terminal sequencederived by Edman degradation completely matched the predictedN-terminal sequence of the open reading frame. It is possiblethat the protein is processed posttranslationally to remove theN-terminal methionine from the mature protein. These data confirmedthat the predicted open reading frame encoded the 20-kDa MI protein.

View larger version (32K):
[in this window]
[in a new window]

FIG. 7. In vitro transcription-translation of pJA2 (lane 2) and the vector pBC (lane 1). The arrow indicates the 20-kDa ³⁵S-labeled protein. Sizes were estimated based on Bio-Rad low-molecular-mass prestained protein standards.

Alignment with sequences in GenBank showed that the MI protein was 62% identical and 80% similar to the inorganic pyrophosphatase(PPase) of E. coli (Fig. 8) (27). Similar identities to inorganicpyrophosphatase of other organisms were also observed (data notshown). Similarly, the N-terminal sequence of the mature PPaseof E. coli is also posttranslationally processed by an aminopeptidaseto remove the N-terminal methionine (27).

View larger version (29K):
[in this window]
[in a new window]

FIG. 8. Alignment of L. pneumophila (Lpn) PPase to the E. coli (Ec) homolog. Conservative substitutions are indicated by colons. The amino acid residues that have been shown to be crucial for structural and catalytic activity of the enzyme in E. coli (see Discussion) are indicated in bold.

Construction of null mutation in ppa. A mini-Tn10::kan was used to construct an insertion mutation in the ppa gene in pJA2a. Three different insertions within thegene and many insertions in the sequences flanking the gene wereobtained. The mutagenized plasmids were introduced into L. pneumophilaby triparental conjugation (see Materials and Methods). Allelicexchange was achieved by selection on kanamycin-containing platesin the presence of sucrose. Allelic exchange was achieved forall four insertions (attempted) in the flanking regions of theppa gene at a frequency of approximately 10⁴ to 10⁵. In contrast, many trials for allelic exchange of the three differentinsertion mutations within the ppa gene were unsuccessful, withthe exception of occasional integration of the whole plasmid intothe chromosome, creating a merodiploid (data not shown). Theseallelic exchanges are performed routinely in our laboratory (6,7), and this is the first example of our inability to achievethe proper allelic exchange. Although these data suggested butdid not confirm that PPase was essential to L. pneumophila, theobservations that PPase is essential for the viability of bothE. coli and yeast and our inability to construct a mutation inppa suggested that this gene is probably essential for the viabilityof L. pneumophila (12, 32). Considering the essential andubiquitous role of this protein in macromolecular biosynthesis(see Discussion), it is not surprising that it would be essentialfor all living organisms.

Induction in transcription of the ppa gene of L. pneumophila within macrophages. The PPase gene (ppa) of E. coli is constitutively expressed and is not regulated in vitro. Interestingly, synthesis of the20-kDa MI protein corresponding to PPase of L. pneumophila wasinduced in response to the intracellular environment but was notinduced upon exposure to in vitro stress stimuli (3). Theseobservations indicated that certain unique stimuli within thephagosomal microenvironment triggered expression of the 20-kDaprotein. To examine the kinetics of transcription of ppa throughoutthe intracellular infection, we constructed a fusion of the ppapromoter to a promoterless lacZ gene. The promoter fusion construct(pPPZ) or the vector (pEU730) was introduced into L. pneumophila.

Monolayers of differentiated U937 cells were infected with L. pneumophila harboring pPPZ or pEU730, followed by gentamicintreatment to kill extracellular bacteria, and further incubatedwithout gentamicin (see Materials and Methods). At several times,monolayers were lysed hypotonically and $beta$ -Gal activity was determined(34). To determine whether the $beta$ -Gal assay was affected by debrisof the lysed U937 cells, BYE-grown L. pneumophila in growth phasessimilar to those of intracellular bacteria was pelleted and resuspendedin a lysate of uninfected monolayers, prior to measurement of $beta$ -Gal activity. Compared to that of in vitro-grown bacteria, transcriptionof the ppa gene was induced during intracellular logarithmic replicationby approximately fourfold (Fig. 9). There was an induction inppa transcription upon entry to the logarithmic phase by approximatelytwo- and eightfold by in vitro-grown and intracellular bacteria,respectively. These data indicated that expression of ppa wasinduced in response to the intracellular microenvironment. Sincethe density of the bacteria may affect the level of expressionthrough the lacZ fusion, the $beta$ -Gal levels were evaluated for invitro cultures of different densities (10⁵ to 10⁹ CFU/ml), and the density of the culture had no detectable effecton the expression of $beta$ -Gal per CFU (data not shown).

View larger version (15K):
[in this window]
[in a new window]

FIG. 9. Kinetics of $beta$ -Gal expression by in vitro-grown (A) and macrophage-grown (B) L. pneumophila harboring a ppa promoter (pPPZ) fused to the promoterless lacZ gene of pEU730. Data are expressed as the mean $beta$ -Gal activity for triplicate samples (34). L. pneumophila harboring the vector pEU730 did not show any detectable $beta$ -Gal activity (data not shown).

In contrast to the intracellular induction of the ppa promoter, there was no induction in expression following exposure ofL. pneumophila to heat shock, osmotic shock, acid shock, and oxidativestress (data not shown). These data further confirmed the stableexpression of ppa upon exposure to stress stimuli and furthershowed that ppa was specifically induced in response to the intracellularenvironment of the host cell.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Radiolabeling of intracellular bacterial pathogens during a period of inhibition of host cell protein synthesis has been usedby many investigators to examine bacterial gene expression duringintracellular infection (1, 3). Cycloheximide has no directeffect on bacterial viability, growth rate, or pattern of proteinsynthesis in vitro (1, 3). However, prior to further cloningof L. pneumophila MI genes, the effects of this inhibitor on thehost cell physiology were evaluated to ensure that some L. pneumophilaMI proteins were not artifactually induced as a secondary effectof prolonged inhibition of protein synthesis of the host cell.Transmission electron microscopy was used to evaluate the effectsof this inhibitor on the intracellular infection by L. pneumophilaand on the ability of the bacterium to form the RER-surroundedreplicative phagosome. Inhibition of protein synthesis of L. pneumophila-infectedU937 cells for up to 6 h did not cause any detectable structuralchanges in the host cell. By 15 h posttreatment, there was clearevidence of dramatic structural deteriorations in the host celland in the vacuole containing intracellular bacteria. These detectablestructural deteriorations in the host cell caused a secondaryeffect of an artifactual induction of 12 bacterial proteins. Ourdata caution that extended use of this inhibitor to selectivelyradiolabel intracellular bacterial pathogens (3, 31) hasprofound effects on the host cell physiology, which may lead tochanges in bacterial gene expression. It is recommended that toexclude any possible secondary effects on expression by intracellularbacteria, this inhibitor not to be used for more than 6 h.

Formation of the RER-surrounded replicative phagosome of L. pneumophila was not affected by inhibition of protein synthesisof the host cell. These data indicated that formation of the replicativevacuole is dictated at the biochemical level of signal transductionand that new host cell proteins are not required for this process.Bacterial replication within the RER-surrounded phagosome wasalso independent of the host cell protein synthesis. The dataalso excluded the possibility that degradation of newly synthesizedproteins is required for bacterial replication.

Expansion of the phagosome was also independent of host cell protein synthesis. The data suggested that expansion of the membraneof the replicative phagosome was due to incorporation of hostcell vesicles of presynthesized proteins or of bacterial componentsor both. The incorporation of bacterial components into the phagosomalmembrane has been described previously. For example, protein antigensof the intracellular pathogens Chlamydia trachomatis and Chlamydiapsittaci are incorporated into the phagosomal membrane (37,44). Incorporation of bacterial proteins into the phagosomalmembrane by L. pneumophila has yet to be determined. Such incorporationmay have significant effects on the biochemical interaction betweenL. pneumophila and the host cell.

The PPase of L. pneumophila was 80% similar to the E. coli PPase (EC 3.6.1.1). The "housekeeping" function of PPase mayexplain its highly conserved domains that are involved in catalyticand structural integrity. The PPase of E. coli has been extensivelycharacterized at the biochemical, structural, and ultrastructurallevels. Many residues of the PPase have been shown to be criticalfor activity and structural integrity of the enzyme. The E. coliPPase is composed of six identical subunits (47) arranged inan octahedral configuration. Residues that are involved in structuralstability of the homohexamer (H136 and H140) (9, 45), inbinding to the Mg²⁺ cofactor (D65, D70, N24, D26, E98, Y141, and D102) (23, 28,29, 38), and in catalytic activity of the enzyme (K29, R43,K142, D97, D102, Y55, and E20) (24, 28, 38) are all conservedin L. pneumophila. X-ray crystallography of the three-dimensionalstructure of the E. coli PPase clearly showed the presence ofa group of functionally important residues that are conservedamong all identified PPases (22). The consensus sequence isD-hyd-D-P-ali-D-ali-ali (hyd is a small hydrophilic residue likeS, G, or N; ali, an aliphatic hydrophobic residue like C, I, L,M, or V) (22). All of these residues are also conserved in theL. pneumophila PPase (D-G-D-P-V-D-V-L). These data clearly demonstratedthat the 20-kDa MI protein of L. pneumophila is a PPase. Thesedata further confirmed the highly conserved nature of this enzyme,which is underlined by its vital housekeeping functions in macromolecularbiosynthesis.

The data suggested that the PPase may be essential for viability of L. pneumophila. PPase is essential for survival in E.coli as well as in yeast (12, 32). It catalyzes reversibletransfer of the phosphoryl group from pyrophosphate to water,providing a thermodynamic pull for essential biosynthetic processessuch as tRNA charging and DNA, RNA, protein, and polysaccharidebiosynthesis (reviewed in reference 26). It may also have animportant role in evolutionary events by affecting the accuracyby which DNA molecules are copied during chromosomal replication(30). Therefore, it may not be surprising that this enzyme isessential for viability (12, 32).

The predicted sequence of the ppa promoter had some similarity to $sigma$ ⁷⁰-regulated promoters. Induction in transcription of ppa by intracellularL. pneumophila indicated the presence of other factors and/orother unidentified upstream sequences that are involved in transcriptionalregulation of this gene. Mutational analysis of the upstream regionmay provide an explanation of the inducible nature of this geneand whether this induction is essential for survival of L. pneumophilawithin the intracellular environment.

Although the levels of PPase have been shown to be constitutive for E. coli (11), regulation in expression of none of thecharacterized PPase genes has been examined. L. pneumophila ppais the first example of a regulated ppa gene during growth ina unique niche. Transcription of L. pneumophila ppa was specificallyinduced during intracellular multiplication but was not inducedin response to in vitro stress stimuli. It is expected that activelygrowing organisms would require a higher rate of macromolecularbiosynthesis including that of DNA, RNA, protein, and polysaccharides.Since pyrophosphate is a by-product of these reactions, higherlevels of PPase activity would be required to provide the thermodynamicpull for these biosynthetic reactions. The short generation timeof intracellular L. pneumophila compared to that of in vitro-grownbacteria in rich medium (21) indicates that intracellular L.pneumophila undergoes macromolecular biosynthesis at a higherrate than do in vitro-grown bacteria. These observations suggestthat for replication of L. pneumophila, the microenvironment withinmacrophages is a more favorable niche than is rich medium. Whetherenhanced macromolecular biosynthesis is the only factor requiredfor induction of ppa transcription by intracellular bacteria orwhether ppa induction is triggered by other signals to which intracellularL. pneumophila is exposed is still to be determined. Future studiesto examine regulation of expression of ppa by other intracellularpathogens would shed light on whether induction of ppa in theintracellular environment is a general phenomenon among intracellularpathogens.

In summary, short-term radiolabeling of intracellular bacteria during inhibition of protein synthesis of the host cell doesnot have any detectable effect on the host cell biology, on theformation of the RER-surrounded replicative phagosome, or on replicationof L. pneumophila. One of the MI proteins was identified as PPase,a protein highly conserved through evolution. The ppa gene ofL. pneumophila is regulated intracellularly and is the first exampleof a regulated ppa gene. Regulation of ppa during intracellularinfection may reflect enhanced capabilities of macromolecularbiosynthesis by intracellular L. pneumophila compared to thoseof in vitro-grown bacteria.

	ACKNOWLEDGMENTS

Y.A.K. is supported by Public Health Service grant no. 1R29AI38410.

I thank R. Perry for the pEU730 plasmid gift, J. Abbott for technical assistance, members of my laboratory for their valuablecomments on the manuscript, and Mary G. Engle for her valuableelectron microscopy expertise.

	FOOTNOTES

^* Mailing address: Department of Microbiology and Immunology, University of Kentucky Chandler Medical Center, Lexington, KY40536-0084. Phone: (606) 323-3873. Fax: (606) 257-8994. E-mail:yabukw{at}pop.uky.edu.

Editor: J. G. Cannon

	REFERENCES

Top Abstract Introduction Materials & Methods Results Discussion References

1.	Abshire, K. Z., and F. C. Neidhardt. 1993. Analysis of proteins synthesized by Salmonella typhimurium during growth within host macrophage. J. Bacteriol. 175:3734-3743[Abstract/Free Full Text].
2.	Abu Kwaik, Y. 1996. The phagosome containing Legionella pneumophila within the protozoan Hartmanella vermiformis is surrounded by the rough endoplasmic reticulum. Appl. Environ. Microbiol. 62:2022-2028[Abstract].
3.	Abu Kwaik, Y., B. I. Eisenstein, and N. C. Engleberg. 1993. Phenotypic modulation by Legionella pneumophila upon infection of macrophages. Infect. Immun. 61:1320-1329[Abstract/Free Full Text].
4.	Abu Kwaik, Y., and N. C. Engleberg. 1994. Cloning and molecular characterization of a Legionella pneumophila gene induced by intracellular infection and by various in vitro stress stimuli. Mol. Microbiol. 13:243-251[Medline].
5.	Abu Kwaik, Y., B. S. Fields, and N. C. Engleberg. 1994. Protein expression by the protozoan Hartmannella vermiformis upon contact with its bacterial parasite Legionella pneumophila. Infect. Immun. 62:1860-1866[Abstract/Free Full Text].
6.	Abu Kwaik, Y., L.-Y. Gao, O. S. Harb, and B. J. Stone. 1997. Transcriptional regulation of the macrophage-induced gene (gspA) of Legionella pneumophila and phenotypic characterization of a null mutant. Mol. Microbiol. 24:629-642[Medline].
7.	Abu Kwaik, Y., and L. L. Pederson. 1996. The use of differential display-PCR to isolate and characterize a Legionella pneumophila locus induced during the intracellular infection of macrophages. Mol. Microbiol. 21:543-556[Medline].
8.	Arroyo, J., M. C. Hurley, M. Wolf, M. S. McClain, B. I. Eisenstein, and N. C. Engleberg. 1994. Shuttle mutagenesis of Legionella pneumophila: identification of a gene associated with host cell cytopathicity. Infect. Immun. 62:4075-4080[Abstract/Free Full Text].
9.	Baykov, A. A., V. Y. Dudarenkov, J. Kapyla, T. Salminen, T. Hyytia, V. N. Kasho, S. Husgafvel, B. S. Cooperman, A. Goldman, and R. Lahti. 1995. Dissociation of the hexameric Escherichia coli inorganic pyrophosphatase into trimers on His136Gln or His140Gln substitution and its effect on enzyme catalytic properties. J. Biol. Chem. 270:30804-30812[Abstract/Free Full Text].
10.	Bozue, J. A., and W. Johnson. 1996. Interaction of Legionella pneumophila with Acanthamoeba catellanii: uptake by coiling phagocytosis and inhibition of phagosome-lysosome fusion. Infect. Immun. 64:668-673[Abstract].
11.	Burton, P. M., D. C. Hall, and J. Josse. 1970. Constitutive inorganic pyrophosphatase of Escherichia coli: chemical studies of protein structure. J. Biol. Chem. 245:4346-4352[Abstract/Free Full Text].
12.	Chen, J., A. Brevet, M. Fromant, F. Leveque, J.-M. Schmitter, S. Blanquet, and P. Plateau. 1990. Pyrophosphatase is essential for growth of Escherichia coli. J. Bacteriol. 172:5686-5689[Abstract/Free Full Text].
12a.	Cianciotto, N. Personal communication.
13.	Cianciotto, N. P., R. Long, B. I. Eisenstein, and N. C. Engleberg. 1988. Site-specific mutagenesis in Legionella pneumophila by allelic exchange using counterselectable ColE1 vectors. FEMS Microbiol. Lett. 56:203-208.
14.	Cianciotto, N. P., J. K. Stamos, and D. W. Kamp. 1995. Infectivity of Legionella pneumophila mip mutant for alveolar epithelial cells. Curr. Microbiol. 30:247-250[Medline].
15.	Edelstein, P. H., D. J. Brenner, C. W. Moss, A. G. Steigerwalt, E. M. Francis, and W. L. George. 1982. Legionella wadsworthii species nova: a cause of human pneumonia. Ann. Intern. Med. 97:809-813.
16.	Fernandez, R. C., S. Logan, S. H. S. Lee, and P. S. Hoffman. 1996. Elevated levels of Legionella pneumophila stress protein Hsp60 early in infection of human monocytes and L929 cells correlated with virulence. Infect. Immun. 64:1968-1976[Abstract].
17.	Fields, B. S. 1996. The molecular ecology of legionellae. Trends Microbiol. 4:286-290[Medline].
18.	Froehlich, B., L. Husmann, J. Caron, and J. R. Scott. 1994. Regulation of rns, a positive regulatory factor for pili of enterotoxigenic Escherichia coli. J. Bacteriol. 176:5385-5392[Abstract/Free Full Text].
18a.	Gao, L.-Y., O. S. Harb, and Y. Abu Kwaik. 1997. Utilization of similar mechanisms by Legionella pneumophila to parasitize two evolutionarily distant hosts, mammalian and protozoan cells. Infect. Immun. 65:4738-4746[Abstract].
19.	Horwitz, M. A. 1983. Formation of a novel phagosome by the Legionnaires' disease bacterium (Legionella pneumophila) in human monocytes. J. Exp. Med. 158:1319-1331[Abstract/Free Full Text].
20.	Horwitz, M. A. 1983. The Legionnaires' disease bacterium (Legionella pneumophila) inhibits phagosome-lysosome fusion in human monocytes. J. Exp. Med. 158:2108-2126[Abstract/Free Full Text].
21.	Horwitz, M. A., and S. C. Silverstein. 1980. Legionnaires' disease bacterium (Legionella pneumophila) multiples intracellularly in human monocytes. J. Clin. Invest. 66:441-450.
22.	Kankare, J., G. S. Neal, T. Salminen, T. Glumhoff, B. S. Cooperman, R. Lahti, and A. Goldman. 1994. The structure of E. coli soluble inorganic pyrophosphatase at 2.7 A resolution. Protein. Eng. 7:823-830[Abstract/Free Full Text].
23.	Kankare, J., T. Salminen, R. Lahti, B. S. Cooperman, A. A. Baykov, and A. Goldman. 1996. Crystallographic identification of metal-binding sites in Escherichia coli inorganic pyrophosphatase. Biochemistry 35:4670-4677[Medline].
24.	Kapyla, J., T. Hyytia, R. Lahti, A. Goldman, A. A. Baykov, and B. S. Cooperman. 1995. Effect of D97E substitution on the kinetic and thermodynamic properties of Escherichia coli inorganic pyrophosphatase. Biochemistry 34:792-800[Medline].
25.	King, C. H., B. S. Fields, E. B. Shotts, Jr., and E. H. White. 1991. Effects of cytochalasin D and methylamine on intracellular growth of Legionella pneumophila in amoebae and human monocyte-like cells. Infect. Immun. 59:758-763[Abstract/Free Full Text].
26.	Lahti, R. 1983. Microbial inorganic pyrophosphatases. Microbiol. Rev. 47:169-179[Free Full Text].
27.	Lahti, R., T. Pitkaranta, E. Valve, I. Ilta, E. Kukko-Kalske, and J. Heinonen. 1988. Cloning and characterization of the gene encoding inorganic pyrophosphatase of Escherichia coli K-12. J. Bacteriol. 170:5901-5907[Abstract/Free Full Text].
28.	Lahti, R., K. Pohjanoksa, T. Pitkaranta, P. Heikinheimo, T. Salminen, P. Meyer, and J. Heinonen. 1990. A site-directed mutagenesis study on Escherichia coli inorganic pyrophosphatase. Glutamic acid-98 and lysine-104 are important for structural integrity, whereas aspartic acids-97 and -102 are essential for catalytic activity. Biochemistry 29:5761-5766[Medline].
29.	Lahti, R., T. Salminen, S. Latonen, P. Heikinheimo, K. Pohjanoska, and J. Heinonen. 1991. Genetic engineering of Escherichia coli inorganic pyrophosphatase: Tyr55 and Tyr141 are important for the structural integrity. Eur. J. Biochem. 198:293-297[Medline].
30.	Lecomte, P., O. P. Doupleday, and M. Radman. 1986. Evidence for an intermediate in DNA synthesis involving pyrophosphate exchange. A possible role in fidelity. J. Mol. Biol. 189:643-652[Medline].
31.	Lee, B. Y., and M. A. Horwitz. 1995. Identification of macrophage and stress-induced proteins of Mycobacterium tuberculosis. J. Clin. Invest. 96:245-249.
32.	Lundin, M., H. Baltscheffsky, and H. Ronne. 1991. Yeast PPA2 gene encodes a mitochondrial inorganic pyrophosphatase that is essential for mitochondrial function. J. Biol. Chem. 266:12168-12172[Abstract/Free Full Text].
33.	Mekalanos, J. J. 1992. Environmental signals controlling expression of virulence determinants in bacteria. J. Bacteriol. 174:1-7[Free Full Text].
34.	Miller, J. H. 1992. . A short course in bacterial genetics: a laboratory manual and handbook for Escherichia coli and related bacteria. Cold Spring Harbor Press, Plainview, N.Y.
35.	Mody, C. H., R. Paine III, M. S. Shahrabadi, R. H. Simon, E. Pearlman, B. I. Eisenstein, and G. B. Toews. 1993. Legionella pneumophila replicates within rat alveolar epithelial cells. J. Infect. Dis. 167:1138-1145[Medline].
36.	Payne, N. R., and M. A. Horwitz. 1987. Phagocytosis of Legionella pneumophila is mediated by human monocyte complement receptors. J. Exp. Med. 166:1377-1389[Abstract/Free Full Text].
37.	Rockey, D. D., and J. L. Rosquist. 1994. Protein antigens of Chlamydia psittaci present in infected cells but not detected in the infectious elementary body. Infect. Immun. 62:106-112[Abstract/Free Full Text].
38.	Salminen, T., J. Kapyla, P. Heikinheimo, J. Kankare, A. Goldman, J. Heinonen, A. A. Baykov, B. S. Cooperman, and R. Lahti. 1995. Structure and function analysis of Escherichia coli inorganic pyrophosphatase: is a hydroxide ion the key to catalysis? Biochemistry 34:782-791[Medline].
39.	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.
40.	Sanger, F., S. Nicklen, and A. R. Coulson. 1977. DNA sequencing with chain-terminating inhibitors. Proc. Natl. Acad. Sci. USA 74:5463-5467[Abstract/Free Full Text].
41.	Sorger, K. P. 1991. Heat shock factor and heat shock response. Cell 65:363-366[Medline].
42.	Susa, M., J. Hacker, and R. Marre. 1996. De novo synthesis of Legionella pneumophila antigens during intracellular growth in phagocytic cells. Infect. Immun. 64:1679-1684[Abstract].
43.	Swanson, M. S., and R. R. Isberg. 1995. Formation of the Legionella pneumophila replicative phagosome. Infect. Agents Dis. 2:269-271.
44.	Taraska, T., D. M. Ward, R. S. Ajioka, P. B. Wyrick, S. R. Davis-Kaplan, C. H. Davis, and J. Kaplan. 1996. The late chlamydial inclusion membrane is not derived from the endocytic pathway and is relatively deficient in host proteins. Infect. Immun. 64:3713-3727[Abstract].
45.	Velichko, I., S. E. Volk, V. Y. Dudarenkov, N. N. Magretova, V. Y. Chernyak, A. Goldman, B. S. Cooperman, R. Lahti, and A. A. Baykov. 1995. Cold lability of the mutant forms of Escherichia coli inorganic pyrophosphatase. FEBS Lett. 359:20-22[Medline].
46.	Venkataraman, C., B. J. Haack, S. Bondada, and Y. Abu Kwaik. 1997. Identification of a Gal/GalNAc lectin in the protozoan Hartmanella vermiformis as a potential receptor for attachment and invasion by the Legionnaires' disease bacterium, Legionella pneumophila. J. Exp. Med. 186:537-547[Abstract/Free Full Text].
47.	Wong, S. C., D. C. Hall, and J. Josse. 1970. Constitutive inorganic pyrophosphatase of Escherichia coli. III. Molecular weight and physical properties of the enzyme and its subunits. J. Biol. Chem. 245:4335-4345[Abstract/Free Full Text].

This article has been cited by other articles:

Fontan, P., Aris, V., Ghanny, S., Soteropoulos, P., Smith, I. (2008). Global Transcriptional Profile of Mycobacterium tuberculosis during THP-1 Human Macrophage Infection. Infect. Immun. 76: 717-725 [Abstract] [Full Text]
Molmeret, M., Horn, M., Wagner, M., Santic, M., Abu Kwaik, Y. (2005). Amoebae as Training Grounds for Intracellular Bacterial Pathogens. Appl. Environ. Microbiol. 71: 20-28 [Full Text]
Park, Y., Yilmaz, O., Jung, I.-Y., Lamont, R. J. (2004). Identification of Porphyromonas gingivalis Genes Specifically Expressed in Human Gingival Epithelial Cells by Using Differential Display Reverse Transcription-PCR. Infect. Immun. 72: 3752-3758 [Abstract] [Full Text]
Molmeret, M., Bitar, D. M., Han, L., Kwaik, Y. A. (2004). Disruption of the Phagosomal Membrane and Egress of Legionella pneumophila into the Cytoplasm during the Last Stages of Intracellular Infection of Macrophages and Acanthamoeba polyphaga. Infect. Immun. 72: 4040-4051 [Abstract] [Full Text]
Rajagopal, L., Clancy, A., Rubens, C. E. (2003). A Eukaryotic Type Serine/Threonine Kinase and Phosphatase in Streptococcus agalactiae Reversibly Phosphorylate an Inorganic Pyrophosphatase and Affect Growth, Cell Segregation, and Virulence. J. Biol. Chem. 278: 14429-14441 [Abstract] [Full Text]
Rankin, S., Li, Z., Isberg, R. R. (2002). Macrophage-Induced Genes of Legionella pneumophila: Protection from Reactive Intermediates and Solute Imbalance during Intracellular Growth. Infect. Immun. 70: 3637-3648 [Abstract] [Full Text]
Broudy, T. B., Pancholi, V., Fischetti, V. A. (2002). The In Vitro Interaction of Streptococcus pyogenes with Human Pharyngeal Cells Induces a Phage-Encoded Extracellular DNase. Infect. Immun. 70: 2805-2811 [Abstract] [Full Text]
Pedersen, L. L., Radulic, M., Doric, M., Abu Kwaik, Y. (2001). HtrA Homologue of Legionella pneumophila: an Indispensable Element for Intracellular Infection of Mammalian but Not Protozoan Cells. Infect. Immun. 69: 2569-2579 [Abstract] [Full Text]
Broudy, T. B., Pancholi, V., Fischetti, V. A. (2001). Induction of Lysogenic Bacteriophage and Phage-Associated Toxin from Group A Streptococci during Coculture with Human Pharyngeal Cells. Infect. Immun. 69: 1440-1443 [Abstract] [Full Text]
Monahan, I. M., Betts, J., Banerjee, D. K., Butcher, P. D. (2001). Differential expression of mycobacterial proteins following phagocytosis by macrophages. Microbiology 147: 459-471 [Abstract] [Full Text]
Harb, O. S., Abu Kwaik, Y. (2000). Essential Role for the Legionella pneumophila Rep Helicase Homologue in Intracellular Infection of Mammalian Cells. Infect. Immun. 68: 6970-6978 [Abstract] [Full Text]
Alli, O. A. T., Gao, L.-Y., Pedersen, L. L., Zink, S., Radulic, M., Doric, M., Abu Kwaik, Y. (2000). Temporal Pore Formation-Mediated Egress from Macrophages and Alveolar Epithelial Cells by Legionella pneumophila. Infect. Immun. 68: 6431-6440 [Abstract] [Full Text]
Gao, L.-Y., Abu Kwaik, Y. (1999). Activation of Caspase 3 during Legionella pneumophila-Induced Apoptosis. Infect. Immun. 67: 4886-4894 [Abstract] [Full Text]
Freitag, N. E., Jacobs, K. E. (1999). Examination of Listeria monocytogenes Intracellular Gene Expression by Using the Green Fluorescent Protein of Aequorea victoria. Infect. Immun. 67: 1844-1852 [Abstract] [Full Text]
Stone, B. J., Kwaik, Y. A. (1999). Natural Competence for DNA Transformation by Legionella pneumophila and Its Association with Expression of Type IV Pili. J. Bacteriol. 181: 1395-1402 [Abstract] [Full Text]
Gao, L.-Y., Abu Kwaik, Y. (1999). Apoptosis in Macrophages and Alveolar Epithelial Cells during Early Stages of Infection by Legionella pneumophila and Its Role in Cytopathogenicity. Infect. Immun. 67: 862-870 [Abstract] [Full Text]
Abu Kwaik, Y., Gao, L.-Y., Stone, B. J., Venkataraman, C., Harb, O. S. (1998). Invasion of Protozoa by Legionella pneumophila and Its Role in Bacterial Ecology and Pathogenesis. Appl. Environ. Microbiol. 64: 3127-3133 [Full Text]
Abu Kwaik, Y., Venkataraman, C., Harb, O. S., Gao, L.-Y. (1998). Signal Transduction in the Protozoan Host Hartmannella vermiformis upon Attachment and Invasion by Legionella micdadei. Appl. Environ. Microbiol. 64: 3134-3139 [Abstract] [Full Text]
Harb, O. S., Kwaik, Y. A. (1998). Identification of the Aspartate-beta -Semialdehyde Dehydrogenase Gene of Legionella pneumophila and Characterization of a Null Mutant. Infect. Immun. 66: 1898-1903 [Abstract] [Full Text]
Stone, B. J., Kwaik, Y. A. (1998). Expression of Multiple Pili by Legionella pneumophila: Identification and Characterization of a Type IV Pilin Gene and Its Role in Adherence to Mammalian and Protozoan Cells. Infect. Immun. 66: 1768-1775 [Abstract] [Full Text]
Gao, L.-Y., Harb, O. S., Kwaik, Y. A. (1998). Identification of Macrophage-Specific Infectivity Loci (mil) of Legionella pneumophila That Are Not Required for Infectivity of Protozoa. Infect. Immun. 66: 883-892 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation m