Heterogeneity in the Attachment and Uptake Mechanisms of the Legionnaires' Disease Bacterium, Legionella pneumophila, by Protozoan Hosts

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Appl Environ Microbiol, January 1998, p. 126-132, Vol. 64, No. 1
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Heterogeneity in the Attachment and Uptake Mechanisms of the Legionnaires' Disease Bacterium, Legionella pneumophila, by Protozoan Hosts

Omar S. Harb, Chandrasekar Venkataraman, Bradley J. Haack, Lian-Yong Gao, and Yousef Abu Kwaik^*

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

Received 5 June 1997/Accepted 18 August 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Invasion and intracellular replication of Legionella pneumophila within protozoa in the environment plays a major role inthe transmission of Legionnaires' disease. Intracellular replicationof L. pneumophila within protozoa occurs in a rough endoplasmicreticulum (RER)-surrounded phagosome (Y. Abu Kwaik, Appl. Environ.Microbiol. 62:2022-2028, 1996). Since the subsequent fate of manyintracellular pathogens is determined by the route of entry, wecompared the mechanisms of attachment and subsequent uptake ofL. pneumophila by the two protozoa Hartmannella vermiformis andAcanthamoeba polyphaga. Our data provide biochemical and geneticevidence that the mechanisms of attachment and subsequent uptakeof L. pneumophila by the two protozoan hosts are, in part, different.First, uptake of L. pneumophila by H. vermiformis is completelyblocked by the monovalent sugars galactose and N-acetyl-D-galactosamine,but these sugars partially blocked A. polyphaga. Second, attachmentof L. pneumophila to H. vermiformis is associated with a time-dependentand reversible tyrosine dephosphorylation of multiple host proteins.In contrast, only a slight dephosphorylation of a 170-kDa proteinof A. polyphaga is detected upon infection. Third, synthesis ofH. vermiformis proteins but not of A. polyphaga proteins is requiredfor uptake of L. pneumophila. Fourth, we have identified L. pneumophilamutants that are severely defective in attachment to A. polyphagabut which exhibit minor reductions in attachment to H. vermiformisand, thus, provide a genetic basis for the difference in mechanismsof attachment to both protozoa. The data indicate a remarkableadaptation of L. pneumophila to attach and invade different protozoanhosts by different mechanisms, yet invasion is followed by a remarkablysimilar intracellular replication within a RER-surrounded phagosomeand subsequent killing of the host cell.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The Legionnaires' disease bacterium, Legionella pneumophila, is a common etiologic agent of bacterial pneumonia (13, 23,38, 53). Upon transmission to individuals through aerosolsgenerated in the environment, the bacteria invade and replicatewithin pulmonary macrophages and epithelial cells (20, 31,39).

In the environment, L. pneumophila is a parasite of at least 13 species of amoebae and ciliated protozoa (reviewed in reference24). In many outbreaks of Legionnaires' disease, the bacteriaand protozoa have been isolated from the same water source, andthe isolated protozoa have been shown to support intracellularmultiplication of the bacterial isolate (10, 16, 26, 37).Additionally, in many confirmed cases of Legionnaires' disease,the bacterium could only be isolated by its capacity to multiplywithin protozoa (8, 18, 28, 47).

Rowbotham has postulated that the infectious particle involved in transmission of Legionnaires' disease is L. pneumophila-infectedamoebae (44). Several lines of evidence indicate that protozoaplay major roles in the continued presence of L. pneumophila inthe environment as well as in the infectivity of the bacteriato humans. Intracellular replication of L. pneumophila withinprotozoa increases bacterial resistance to harsh environmentalconditions, which may allow the bacteria to survive extracellularlyfor prolonged periods of time in the environment (6, 11,12). Interestingly, it has been recently shown that viabilityand infectivity of nonculturable L. pneumophila can be "resuscitated"by intracellular replication within protozoa (45). Moreover,intracellular multiplication within protozoa enhances the infectivityof L. pneumophila to human-derived cells (21). These observationsmay explain why Legionnaires' disease is not transmitted betweenindividuals and why transmission occurs despite the presence oflow numbers of L. pneumophila from the source of aerosol (14,22, 40).

The hallmark of L. pneumophila infection of humans is the intracellular survival and replication of the bacteria within macrophagesin a rough endoplasmic reticulum (RER)-surrounded phagosome (2,24, 31). The intracellular infection of protozoa is similarto that of macrophages at the ultrastructural and molecular levels(1, 29). In addition, diaminopimelic acid auxotrophs of L.pneumophila are defective in intracellular growth within mammalianand protozoan cells (30a). During intracellular replication,changes in bacterial gene expression are manifested (2-4, 6,7, 48). Although protein synthesis by the RER is not requiredfor intracellular bacterial replication (2), the role of theRER in intracellular survival is not known.

The mechanisms involved in intracellular trafficking leading to survival and replication of the bacterium within mammalianand protozoan cells are not yet known. Several lines of evidenceindicate that the fate of some intracellular pathogens is determinedby the route of entry and the specific host cell receptor involved,which may trigger different host cell signal transduction mechanisms(9, 32, 35). We have recently shown that uptake of L. pneumophilaby the protozoan Hartmannella vermiformis is mediated by the Gal/GalNAclectin receptor and is associated with tyrosine dephosphorylationof this receptor (52). In this report, we extended our studieson the host cell processes involved in uptake of L. pneumophilato another protozoan host, Acanthamoeba polyphaga, and comparedits host cell response to that of H. vermiformis. The attachmentand subsequent cross talk between L. pneumophila and its hostsmay play a role in the intracellular fate of the bacterium.

Uptake of L. pneumophila by the protozoan H. vermiformis has been proposed to occur through a microfilament-independent butreceptor-mediated mechanism (36), but the processes involvedin bacterial uptake by other protozoan hosts have not been reported.This paper describes the investigation of the different mechanismsutilized for the attachment and uptake of L. pneumophila by twoprotozoa, H. vermiformis and A. polyphaga.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Bacterial strains. The virulent AA100 strain of L. pneumophila has been described previously (3, 5). The L. pneumophila mutants used inthis study (GF162, GG104, GB112, GM128, GO128, GP65, GQ262, andGT251) were generated by mini Tn10::kan transposon mutagenesisof the AA100 strain (29, 30). Southern hybridizations wereused to confirm that these mutants contained distinct insertionsin their chromosomes (29). L. pneumophila were grown on bufferedcharcoal yeast extract (BCYE) agar plates. Growth of the insertionmutants was on BCYE medium with 20 µg of kanamycin (Sigma ChemicalCo., St. Louis, Mo.)/ml.

Protozoan culture. Axenic A. polyphaga was obtained from B. S. Fields (Centers for Disease Control and Prevention, Atlanta, Ga.) and culturedas adherent cells in peptone-yeast-glucose medium (15). H. vermiformisCDC-19 (ATCC 50237) has been cloned and grown in axenic cultureas a model for the study of the pathogenesis of L. pneumophila(25). This strain has been isolated from a water source of anoutbreak of nosocomial Legionnaires' disease in a hospital inSouth Dakota, and its presence in the potable water sites correlatedwith the presence of the epidemic strain of L. pneumophila (16,25). H. vermiformis was maintained in ATCC culture medium 1034(5, 25).

Detection of tyrosine-phosphorylated proteins in H. vermiformis and A. polyphaga upon contact with L. pneumophila. Amoebae were incubated overnight in culture flasks in serum-free axenic medium or PYG medium for H. vermiformis and A. polyphaga,respectively. The amoebae were harvested by centrifugation andwere resuspended in the corresponding fresh medium. Aliquots of~2 × 10⁷ amoebae/ml were infected by 10⁹ L. pneumophila. At several time intervals of coincubation at37°C, amoebal cell lysates were prepared for Western blottingas described below.

Preparation of cell lysates and Western blotting. After incubation of amoebae with L. pneumophila, infections were stopped by using cold stop buffer (1X PBS, pH 7.2) containingthe phosphatase inhibitors NaF (5 mM) and Na₃VO₄ (1 mM) (SigmaChemical Co.). Cells were washed three times with cold stop bufferand pelleted by low-speed centrifugation at 735 × g for 2 min.The supernatant containing bacteria was discarded, and amoebaewere lysed by using cold 1% Triton X-100 lysis buffer (20 mM Tris-HCl[pH 7.6], 150 mM NaCl, 10 mM NaF, 1 mM Na₃VO₄, 1 mM EDTA, 1 mMphenylmethylsulfonyl fluoride, 2 µg of leupeptin/ml, and 2 µgof aprotinin/ml). The soluble and insoluble fractions were separatedby centrifugation at 16,000 × g for 30 min at 4°C in a microcentrifuge.Proteins from soluble fractions were resolved by sodium dodecylsulfate-10% polyacrylamide gel electrophoresis under reducingconditions. The transfer of proteins onto Immobilon-P membranes(Millipore, Bedford, Mass.) was performed in a Bio-Rad transfercell (Bio-Rad, Hercules, Calif.) for 1.5 to 2 h with 0.2 M Tris-0.025M glycine buffer containing 20% (vol/vol) methanol. After transferof proteins, membranes were incubated for 30 min in a blockingbuffer containing 1.5% bovine serum albumin. Membranes were probedwith antiphosphotyrosine antibody conjugated to horseradish peroxidase(RC-20) according to the manufacturer's recommendations (TransductionLaboratories, Lexington, Ky.). The blots were developed by usingan enhanced chemiluminescence kit (DuPont NEN, Boston, Mass.)according to the manufacturer's instructions. The specificityof the RC-20 antibody for protozoan phosphotyrosine-containingproteins was confirmed by Western blots probed with another antiphosphotyrosineantibody, clone 4G10 (Upstate Biotechnology Inc., Lake Placid,N.Y.) followed by a horseradish peroxidase-P conjugated goat anti-mousesecondary antibody (Santa Cruz Biotechnology Inc., Santa Cruz,Calif.) (data not shown).

Inhibition of L. pneumophila uptake by sugars. Infection of amoebae with L. pneumophila was performed exactly as described previously (5). To analyze the effects of differentsugars on invasion of amoebae by L. pneumophila, infections wereperformed in triplicate in the presence of a 100 mM concentrationof the following sugars: galactose (Gal), N-acetyl-D-galactosamine(GalNAc), glucose, lactose, and mannose (Sigma). Sugar solutionswere prepared in the medium used to maintain each of the amoebae.

The effects of the sugars on invasion were investigated by gentamicin protection invasion assays. In these assays, A. polyphagaor H. vermiformis was suspended in its respective medium at aconcentration of ~10⁷/ml. Amoebae were incubated in triplicate in the presence of differentsugars for 15 min prior to infection. L. pneumophila was addedto a final concentration of 10⁸/ml. The samples were incubated at 37°C for 4 h followed by theaddition of 50 µg of gentamicin/ml for 1 h to kill extracellularbacteria. Intracellular bacteria are protected from this antibiotic.The amoebae were washed with medium and lysed by the additionof a mild detergent (0.04% Triton X-100). Lysis of the amoebaewas monitored microscopically and was complete within 1 min. Thistreatment had no significant effect on the viability of the bacteria(data not shown). Dilutions were plated on BCYE plates for colonyenumeration. The percent invasion was calculated by dividing thenumber of CFU in the presence of each sugar by the number of CFUin the absence of the sugar.

The effects of the sugars on invasion of amoebae by L. pneumophila were also determined by examination of the growth kineticsof L. pneumophila within H. vermiformis and A. polyphaga in thepresence of each sugar. Amoebae were incubated in the presenceof each sugar for 15 min prior to infection with L. pneumophila.At several time intervals after infection (1, 3, 5, and 7 days),amoebae were lysed as described above, and samples were dilutedand plated on BCYE plates for colony enumeration. The percentinvasion was calculated as described above.

Uptake of L. pneumophila by amoebae in the presence of inhibitors of cytoskeletal integrity. Infection of amoebae with L. pneumophila was performed exactly as described previously (5). To analyze the effects of inhibitorsof cytoskeletal function on the uptake of L. pneumophila, amoebaewere incubated in the presence of each inhibitor for 1 h priorto infection. The inhibitors used were 2 µM cytochalasin D (microfilaments)and 10 µM colchicine (microtubules) (Sigma). Following a 3-h infection,extracellular bacteria were killed by the addition of 50 µg ofgentamicin/ml, and intracellular bacteria were plated for enumerationon BCYE plates.

Infection of A. polyphaga by L. pneumophila in the presence of cycloheximide. To assess the effect of cycloheximide on the uptake of L. pneumophila by A. polyphaga, ~10⁷ A. polyphaga was pretreated for 3 h with 200 µg of cycloheximide/mlto inhibit protein synthesis. Amoebae were infected with ~10⁸ L. pneumophila for 4 h in the presence of cycloheximide. Cycloheximidehas no detectable effect on the viability or gene expression ofL. pneumophila (5). Subsequently, nonadherent bacteria wereremoved by extensive washing, and extracellular bacteria werekilled by gentamicin, as described above. Intracellular bacteriawere recovered after lysis of the amoebae and were plated on BCYEfor colony enumeration, as described above.

Attachment of L. pneumophila mutants to H. vermiformis and A. polyphaga. H. vermiformis was infected with eight different miniTn10::kan insertion mutants that are defective in attachment to human-derivedU937 macrophages (29). To assess the ability of the mutant strainsto adhere to A. polyphaga and H. vermiformis, 5 × 10⁵ amoebae were infected for 20 min in triplicate with 10⁷ bacteria of each mutant. Infections were carried out in the presenceof 10 mM methylamine to prevent internalization of the bacteria(36). The amoebae were washed three times to remove unattachedbacteria and were subsequently lysed with a mild detergent (0.04%Triton X-100). Dilutions were plated on BCYE. Adherence of themutants was measured by comparison to the adherence of the wild-typestrain, AA100, to amoebae in the same assay. To ensure that theinhibitors were effective in the inhibition of uptake, controlmonolayers infected in the presence of the inhibitor were treatedwith gentamicin to kill extracellular bacteria. The data showedthat methylamine inhibited uptake by A. polyphaga and H. vermiformisby approximately 98% (data not shown).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Effects of sugars on the ability of L. pneumophila to invade A. polyphaga and H. vermiformis. We used two strategies to investigate the roles of several sugars in blocking the attachment and invasion of amoebae by L.pneumophila. First, a gentamicin protection invasion assay wasutilized to measure invasion of amoebae in the presence of varioussugars (see Materials and Methods). Our data showed that the presenceof specific sugars had different effects on bacterial uptake byA. polyphaga and H. vermiformis. Incorporation of 100 mM Gal orGalNAc in the infection assay had a dramatic effect on invasionof H. vermiformis by L. pneumophila (Fig. 1A). These sugar monomerswere able to block uptake of L. pneumophila by H. vermiformisby ~70 and 89%, respectively. Gal and GalNAc are not toxic toamoebae, and their inhibition of uptake of L. pneumophila is specific,dose dependent, and reversible (52). Other sugars (glucose,mannose, and lactose) at a concentration of 100 mM had no detectableeffect on the uptake of L. pneumophila by H. vermiformis (Fig.1A and data not shown).

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FIG. 1. Effects of different sugar monomers on invasion of H. vermiformis (A) and A. polyphaga (B) by L. pneumophila by gentamicin protection assays. Invasion of amoebae by L. pneumophila was performed in the absence or presence of various sugars. The percent invasion was determined by a comparison between the number of intracellular bacteria in the presence of sugars compared to that in untreated cultures. Values are the means of triplicate samples, and error bars represent standard deviations.

In contrast, Gal and GalNAc had slight effects on the uptake of L. pneumophila by A. polyphaga (Fig. 1B). These data showedthat uptake of L. pneumophila by H. vermiformis but not by A.polyphaga is dramatically blocked by Gal and GalNAc.

Second, a growth kinetics assay was performed in the presence of the above sugars. The data confirmed our results obtainedfrom the gentamicin protection invasion assays. Over the 7-dayinfection, 100 mM Gal or GalNAc caused a dramatic reduction ora complete inhibition in the growth kinetics of L. pneumophilawithin H. vermiformis (Fig. 2A). The inhibition of uptake of L.pneumophila by H. vermiformis in the presence of Gal or GalNAcis specific, reversible, and dose dependent (52). Other sugars(glucose, mannose, and lactose) at a concentration of 100 mM hadno detectable effect on the uptake of L. pneumophila by H. vermiformis(Fig. 1A and data not shown).

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FIG. 2. Growth kinetics of L. pneumophila in cocultures with H. vermiformis or A. polyphaga in the absence or presence of different sugars. The bacteria do not replicate extracellularly in the coculture, and thus, the increase in the number of bacteria is due to intracellular replication. Values are the means of triplicate samples, and error bars represent standard deviations.

In contrast, parallel experiments performed with A. polyphaga showed that the presence of Gal or GalNAc caused a slight reductionin the growth kinetics of L. pneumophila (Fig. 2B). These dataconfirmed the distinct difference in the effects of Gal and GalNAcon the uptake of L. pneumophila by H. vermiformis and A. polyphaga.

Protein tyrosine phosphorylation in A. polyphaga and H. vermiformis upon attachment to L. pneumophila. Tyrosine phosphorylation of host proteins has been shown to be important in the uptake of many intracellular pathogens (27,33, 41-43, 49). We have recently shown protein tyrosine dephosphorylationin the protozoan H. vermiformis upon attachment and invasion byL. pneumophila (52). In this report, we extended our studiesto another protozoan host, A. polyphaga, and compared its hostcell response to that of H. vermiformis. First, we examined hostcell signaling events in H. vermiformis and A. polyphaga uponcontact with their bacterial parasite, L. pneumophila. We utilizedWestern blots of amoebal proteins to examine the status of tyrosinephosphorylation of host proteins in resting amoebae and followingcontact with L. pneumophila. Examination of H. vermiformis celllysates showed several proteins that were tyrosine phosphorylatedin resting amoebae (Fig. 3A, lane 1) that underwent a time-dependentand reversible dephosphorylation upon contact with L. pneumophila.Dephosphorylation of several H. vermiformis proteins, includingthose with apparent molecular masses of 190, 170, 130, and 70kDa, was prominent and evident as early as 5 min (Fig. 3A, lane2), and was complete by 15 min (Fig. 3A, lane 3), confirming ourprevious observations (52).

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FIG. 3. Effects of attachment of L. pneumophila to H. vermiformis and A. polyphaga on tyrosine phosphorylation of host proteins. (A) Cell extracts were prepared from uninfected H. vermiformis (lane 1), from H. vermiformis infected with L. pneumophila for 5 min (lane 2) or for 15 min (lane 3), or from uninfected cells incubated for 15 min (lane 4). Lane 5 represents samples prepared from H. vermiformis infected for 15 min followed by removal of extracellular bacteria and further incubation for 15 min. (B) Extracts were prepared from uninfected A. polyphaga (lane 1) or from A. polyphaga infected with L. pneumophila for 5 min (lane 2) or for 15 min (lane 3). Lane 4 represents samples prepared from infection with dead L. pneumophila. Western blots were probed with antiphosphotyrosine antibody (see Materials and Methods). Arrows indicate the position of the 170-kDa protein.

To compare the host cell response in H. vermiformis to that of another protozoan host, we also examined the pattern of proteintyrosine phosphorylation in resting A. polyphaga and upon attachmentand invasion by L. pneumophila. Many tyrosine-phosphorylated proteinswere detected in resting A. polyphaga (Fig. 3B). The pattern oftyrosine-phosphorylated proteins in A. polyphaga was distinctlydifferent from that in H. vermiformis. However, in contrast toH. vermiformis, there was only a slight tyrosine dephosphorylationof a 170-kDa protein in A. polyphaga upon contact with L. pneumophila.These data demonstrated major differences in triggering the biochemicalevents involved in the attachment, and possibly the subsequentuptake, of L. pneumophila by the two amoebae.

Effects of inhibitors of cytoskeletal integrity on uptake of L. pneumophila by amoebae. To further characterize the differences in the mechanisms of uptake of L. pneumophila by H. vermiformis and A. polyphaga,the effects of two inhibitors of cytoskeletal function (cytochalasinD and colchicine) on uptake of L. pneumophila were examined bygentamicin protection invasion assay. After pre-incubating theamoebae with each inhibitor for 3 h, infections were performedfor 3 h. Subsequently, extracellular bacteria were killed, andthe number of intracellular bacteria was determined. The datashowed no detectable effect by either inhibitor on the uptakeof L. pneumophila by A. polyphaga (Fig. 4). Similar results wereobtained from H. vermiformis infected with L. pneumophila in thepresence of these inhibitors (data not shown). These data indicatedthat the uptake mechanisms of L. pneumophila by the two amoebaeare independent of microfilaments and microtubules. Our data areconsistent with previous observations that the uptake of L. pneumophilaby H. vermiformis is independent of the microfilaments (36).

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FIG. 4. Effects of disruption of A. polyphaga microtubules (by colchicine) and microfilament (by cytochalasin D) and inhibition of protein synthesis (by cycloheximide) on invasion by L. pneumophila. The percent invasion was determined by dividing the number of intracellular bacteria recovered following the invasion period after killing of extracellular bacteria by the number of intracellular bacteria in untreated samples. Values are the means of triplicate samples, and error bars represent standard deviations.

Effect of inhibition of protozoan protein synthesis on uptake of L. pneumophila. The uptake of L. pneumophila by H. vermiformis and macrophages is known to differ in the requirement for host protein synthesis.Our previous work showed that uptake of L. pneumophila by macrophagesis independent of protein synthesis of the host cell (5). Incontrast, synthesis of new host proteins is required for uptakeof the bacterium by H. vermiformis (5). We extended these observationsto the uptake of L. pneumophila by A. polyphaga. Our data showedthat inhibition of A. polyphaga protein synthesis had no detectableeffect on uptake of L. pneumophila (Fig. 4). In contrast, andconsistent with our previous observations, inhibition of H. vermiformisprotein synthesis completely inhibited the uptake of L. pneumophila(data not shown) (5). These data further substantiated ourobservations on the differences in the uptake mechanisms of L.pneumophila by A. polyphaga and H. vermiformis.

Attachment of mutants of L. pneumophila to A. polyphaga and H. vermiformis. We have recently isolated a group of mutants, generated through transposon mutagenesis, that are defective in attachment toA. polyphaga and to U937 human macrophage-like cells (29, 30).We examined the ability of these mutants to attach to H. vermiformisand compared it to their attachment to A. polyphaga. In theseassays, attachments were assessed in the presence of an inhibitorof uptake to prevent internalization of the bacteria (see Materialsand Methods). Our data showed that the 10 mutants were severelydefective in attachment to A. polyphaga but 4 of them (GP65, GM128,GT251, and GM224) attached at higher levels to H. vermiformis(Fig. 5). Interestingly, six of the mutants were severely defectivein attachment to both A. polyphaga and H. vermiformis, suggestingthat some of the bacterial ligands involved in attachment to bothprotozoa may be similar. These data indicated that L. pneumophilapossesses multiple ligands involved in distinct attachment toH. vermiformis or A. polyphaga, and some of these may be involvedin attachment to both protozoa.

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FIG. 5. Attachment levels of mutants of L. pneumophila to A. polyphaga and H. vermiformis. The number of attached bacteria is represented by the percentage of attached bacteria compared to that of the wild-type, strain AA100, in the presence of an inhibitor of uptake in both amoebae. Values are the means of triplicate measurements, and the error bars represent standard deviations. Some of the error bars cannot be seen due to their small values.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The replication of L. pneumophila within free-living amoebae is believed to be an integral component in the transmission ofLegionnaires' disease (24). It has been hypothesized that theintracellular infections of mammalian and protozoan cells by L.pneumophila are mediated by similar mechanisms (1, 19, 24).We have recently shown that 89 distinct insertion mutants of L.pneumophila exhibited similar defective phenotypes (severe tomodest) in their cytotoxicity and intracellular replication withinU937 macrophages and A. polyphaga (29), thus providing geneticevidence that many of the mechanisms utilized by L. pneumophilato parasitize the two evolutionarily distant hosts are similar.In contrast, processes involved in the uptake of L. pneumophilaby mammalian macrophages have been shown to differ from thoseby H. vermiformis (5, 36, 52), although the mechanismsof uptake by amoebae are not known.

Previous studies have shown that uptake of L. pneumophila by H. vermiformis is not inhibited by cytochalasin D, an inhibitorof microfilament-dependent endocytosis (36). In this report,we provide evidence that the attachment and uptake of L. pneumophilaby the two protozoa, A. polyphaga and H. vermiformis, occur bydifferent mechanisms, adding further complexity to the host-parasiteinteraction process. First, uptake of L. pneumophila by H. vermiformisis completely blocked by the monovalent sugars Gal and GalNAc,but these sugars partially blocked A. polyphaga. Second, attachmentof L. pneumophila to H. vermiformis is associated with a time-dependentand reversible tyrosine dephosphorylation of multiple host proteins.In contrast, only a slight dephosphorylation of a 170-kDa proteinof A. polyphaga is detected upon infection. Third, synthesis ofH. vermiformis proteins but not of A. polyphaga proteins is requiredfor uptake of L. pneumophila. Fourth, we have identified L. pneumophilamutants that are severely defective in attachment to A. polyphagabut which exhibit minor reductions in attachment to H. vermiformisand, thus, provide a genetic basis for the difference in mechanismsof attachment to both protozoa.

The dramatic inhibition of uptake of L. pneumophila by H. vermiformis compared to that by A. polyphaga in the presence ofGal or GalNAc indicates that the receptors utilized by L. pneumophilato attach to the two amoebae may be different or have differentaffinities. We have recently identified a 170-kDa Gal/GalNAc lectinas one of the tyrosine-phosphorylated proteins in resting H. vermiformisthat undergoes dephosphorylation upon attachment and invasionby L. pneumophila (52). Whether the slightly dephosphorylated170-kDa protein in A. polyphaga, as a result of bacterial infection,is related to the H. vermiformis lectin is still to be determined.

Therefore, A. polyphaga possesses another receptor or a similar receptor but with lower affinity to which L. pneumophila attachesduring the initial steps of interaction. The severe defect inattachment of the L. pneumophila mutant strain GM224 to A. polyphaga,but its normal attachment to H. vermiformis, provides strong geneticevidence for the presence of different receptors on both protozoafor attachment of L. pneumophila. Since these mutants are alsodefective in intracellular replication (29, 30), it is unlikelythat expression of the recently described pili of L. pneumophilais defective in any of these mutants (46). Future characterizationof the defective ligand in the mutant GM224 will allow us to characterizethe host cell receptor involved in attachment.

Attachment of L. pneumophila to H. vermiformis is associated with tyrosine dephosphorylation of multiple host proteins. Incontrast, there is only a slight reduction in the level of tyrosinephosphorylation of a 170-kDa protein (which may be related tothe Gal/GalNAc lectin of H. vermiformis) in A. polyphaga uponattachment to L. pneumophila. This host cell response may correlatewith the relative inhibition of bacterial uptake by Gal and GalNAcsugars, which was less pronounced in A. polyphaga. These datashowed a crucial difference in the initial steps involved in attachmentand subsequent cross talk between L. pneumophila and two of itsprotozoan hosts, A. polyphaga and H. vermiformis. Since thereare at least 13 species described to be environmental hosts forL. pneumophila (24), it would be interesting to examine theremarkable adaptation and the differential complexity of the interactionof this intracellular parasite with its numerous environmentalprotozoan hosts.

The fate of some intracellular parasites may be determined by the specific ligand-receptor interaction and subsequent signaltransduction involved in uptake by the host cell (9, 32,35). Our observations of tyrosine dephosphorylation of H. vermiformisproteins, including the Gal/GalNAc receptor, upon contact anduptake of L. pneumophila are rather intriguing since conventionalphagocytosis is associated with tyrosine phosphorylation of hostcell proteins (9, 52). Interestingly, attachment of manybacterial pathogens to host cell receptors and their exploitationof host cell processes is associated with tyrosine phosphorylationof host cell proteins (27). We speculate that attachment ofL. pneumophila to H. vermiformis is associated with disruptionof the classical phagocytic process. Additionally, cross talkbetween L. pneumophila and H. vermiformis activates host cellsignaling pathways that will trigger new protein synthesis inH. vermiformis, which is required for subsequent uptake of L.pneumophila (5). In contrast, adherence of L. pneumophila toA. polyphaga induces only minor changes in the host tyrosine phosphorylation,indicating that the initial cross talk does not induce the sameset of biochemical signaling events seen in H. vermiformis.

Many facultative intracellular pathogens exploit host signal transduction pathways to their own advantage (27). This exploitationincludes induced cytoskeletal rearrangement and subsequent internalizationof the bacterium. L. pneumophila invasion of both H. vermiformisand A. polyphaga, however, remains unaffected by inhibitors ofthe cytoskeleton that are commonly exploited by other bacterialpathogens (27). Both of these inhibitors have been found toperform their functions in protozoa in ways that are similar tothose in mammalian cells (34, 36, 50, 51). Therefore,our observations confirm previous reports that the mechanismsof invasion of amoebae by L. pneumophila are different from thoseutilized by other intracellular pathogens to invade their mammalianhost cells (5, 27, 36).

L. pneumophila is transmitted only from environmental sources, where protozoa play a major factor in transmission of Legionnaires'disease (24). Intracellular replication within protozoa increasesthe number of L. pneumophila in the environment (24), resuscitatesviability and infectivity of nonculturable bacteria (45), increasesbacterial resistance to harsh environmental conditions (6,11, 12), and enhances bacterial infectivity to human cellsand A/J mice (17, 21). Thus, understanding the mechanismsof uptake by protozoa will facilitate the design of measures toprevent uptake of L. pneumophila by protozoa, providing effectivepreventive approaches for controlling the transmission of Legionnaires'disease.

	ACKNOWLEDGMENTS

O.S.H. and C.V. made equal contributions to this work.

Y.A.K. was supported by Public Health Service grant no. 1R29AI38410. O.S.H. was supported by predoctoral national researchservice award no. TA09509.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, University of Kentucky Chandler MedicalCenter, Lexington, KY 40536-0084. Phone: (606) 323-3873. Fax:(606) 257-8994. E-mail: yabukw{at}pop.uky.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Abu Kwaik, Y. 1996. The phagosome containing Legionella pneumophila within the protozoan Hartmannella vermiformis is surrounded by the rough endoplasmic reticulum. Appl. Environ. Microbiol. 62:2022-2028[Abstract].

2. Abu Kwaik, Y. Induced expression of the Legionella pneumophila gene encoding a 20-kilodalton protein during intracellular infection. Infect. Immun., in press.

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. Adeleke, A., J. Pruckler, R. Benson, T. Rowbotham, M. Halablab, and B. S. Fields. 1996. Legionella-like amoebal pathogens $---$ phylogenetic status and possible role in respiratory disease. Emerg. Infect. Dis. 2:225-229.

9. Allen, L. H., and A. Aderem. 1996. Molecular definition of distinct cytoskeletal structures involved in complement- and Fc receptor-mediated phagocytosis in macrophages. J. Exp. Med. 184:627-637[Abstract/Free Full Text].

10. Barbaree, J. M., B. S. Fields, J. C. Feeley, G. W. Gorman, and W. T. Martin. 1986. Isolation of protozoa from water associated with a legionellosis outbreak and demonstration of intracellular multiplication of Legionella pneumophila. Appl. Environ. Microbiol. 51:422-424[Abstract/Free Full Text].

11. Barker, J., M. R. W. Brown, P. J. Collier, I. Farrell, and P. Gilbert. 1992. Relationship between Legionella pneumophila and Acanthamoeba polyphaga: physiological status and susceptibility to chemical inactivation. Appl. Environ. Microbiol. 58:2420-2425[Abstract/Free Full Text].

12. Barker, J., H. Scaife, and M. R. W. Brown. 1995. Intraphagocytic growth induces an antibiotic-resistant phenotype of Legionella pneumophila. Antimicrob. Agents Chemother. 39:2684-2688[Abstract].

13. Bates, J. H., G. D. Capmpbell, and A. L. Baron. 1992. Microbial etiology of acute pneumonia in hospitalized patients. Chest 101:1005-1012[Abstract/Free Full Text].

14. Bhopal, R. S., R. J. Fallon, E. C. Buist, R. J. Black, and J. D. Urquhart. 1991. Proximity of the home to a cooling tower and risk of non-outbreak Legionnaires' disease. Br. Med. J. 302:378-383.

15. 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].

16. Breiman, R. F., B. S. Fields, G. N. Sanden, L. Volmer, A. Meier, and J. S. Spika. 1990. Association of shower use with Legionnaires' disease: possible role of amoebae. JAMA 263:2924-2926[Abstract/Free Full Text].

17. Brieland, J. K., J. C. Fantone, D. G. Remick, M. LeGendre, M. McClain, and N. C. Engleberg. 1997. The role of Legionella pneumophila-infected Hartmanella vermiformis as an infectious particle in a murine model of Legionnaires' disease. Infect. Immun. 65:5330-5333[Abstract].

18. Britles, R. J., T. J. Rowbotham, D. Raoult, and T. G. Harrison. 1996. Phylogenetic diversity of intra-amoebal legionellae as revealed by 16S rRNA gene sequence comparison. Microbiology 142:3525-3530[Abstract/Free Full Text].

19. Cianciotto, N. P., and B. S. Fields. 1992. Legionella pneumophila mip gene potentiates intracellular infection of protozoa and human macrophages. Proc. Natl. Acad. Sci. USA 89:5188-5191[Abstract/Free Full Text].

20. 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].

21. Cirillo, J. D., L. S. Tompkins, and S. Falkow. 1994. Growth of Legionella pneumophila in Acanthamoeba castellanii enhances invasion. Infect. Immun. 62:3254-3261[Abstract/Free Full Text].

22. Dennis, P. J., A. E. Wright, D. A. Rutter, J. E. Death, and B. P. Jones. 1984. Legionella pneumophila in aerosols from shower baths. J. Hyg. 93:349-353[Medline].

23. Fang, G. D., M. Fine, and J. Orloff. 1990. New and emerging etiologies of community-acquired pneumonia with implications for therapy, a prospective multicenter study of 359 cases. Medicine (Baltimore) 69:307-316[Medline].

24. Fields, B. S. 1996. The molecular ecology of legionellae. Trends Microbiol. 4:286-290[Medline].

25. Fields, B. S., T. A. Nerad, T. K. Sawyer, C. H. King, J. M. Barbaree, W. T. Martin, W. E. Morrill, and G. N. Sanden. 1990. Characterization of an axenic strain of Hartmannella vermiformis obtained from an investigation of nosocomial legionellosis. J. Protozool. 37:581-583[Medline].

26. Fields, B. S., G. N. Sanden, J. M. Barbaree, W. E. Morrill, R. M. Wadowsky, E. H. White, and J. C. Feeley. 1989. Intracellular multiplication of Legionella pneumophila in amoebae isolated from hospital hot water tanks. Curr. Microbiol. 18:131-137.

27. Finlay, B. B., and P. Cossart. 1997. Exploitation of mammalian host cell functions by bacterial pathogens. Science 276:718-725[Abstract/Free Full Text].

28. Fry, N. K., T. J. Rowbotham, N. A. Saunders, and T. M. Embley. 1991. Direct amplification and sequencing of the 16S ribosomal DNA of an intracellular Legionella species recovered by amoebal enrichment from the sputum of a patient with pneumonia. FEMS Microbiol. Lett. 83:165-168.

29. 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].

30. Gao, L.-Y., O. S. Harb, and Y. Abu Kwaik. Submitted for publication.

30a. Harb, O. S., J. K. Brieland, and Y. Abu Kwaik. Submitted for publication.

31. 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].

32. 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].

33. Ireton, K., B. Payrastre, H. Chap, W. Ogawa, H. Sakaue, M. Kasuga, and P. Cossart. 1996. A role for phosphoinositide 3-kinase in bacterial adhesion. Science 274:780-782[Abstract/Free Full Text].

34. Isenberg, G., U. Aebi, and T. D. Pollard. 1980. An actin-binding protein from Acanthamoeba regulates actin filament polymerization and interactions. Nature 288:455-459[Medline].

35. Joiner, K. A., S. A. Fuhrman, H. M. Miettinen, L. H. Kasper, and I. Mellman. 1990. Toxoplasma gondii: fusion competence of parasitophorous vacuoles in Fc receptor-transfected fibroblasts. Science 249:641-646[Abstract/Free Full Text].

36. 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].

37. Kurtz, J. B., C. L. R. Bartlett, U. A. Newton, R. A. White, and N. L. Jones. 1982. Legionella pneumophila in cooling tower systems. J. Hyg. 88:369-381[Medline].

38. Marston, B. J. 1995. Epidemiology of community-acquired pneumonia. Infect. Dis. Clin. Pract. 4:S232-S239.

39. 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].

40. O'Brein, S. J., and R. S. Bhopal. 1993. Legionnaires' disease: the infective dose paradox. Lancet 342:5-6[Medline].

41. Rosenshine, I., V. Duronio, and B. B. Finlay. 1992. Tyrosine protein kinase inhibitors block invasin-promoted bacterial uptake by epithelial cells. Infect. Immun. 60:2211-2217[Abstract/Free Full Text].

42. Rosenshine, I., S. Ruschkowski, V. Foubister, and B. B. Finlay. 1994. Salmonella typhimurium invasion of epithelial cells: role of induced host cell tyrosine protein phosphorylation. Infect. Immun. 62:4969-4974[Abstract/Free Full Text].

43. Rosenshine, I., S. Ruschkowski, M. Stein, D. J. Reinscheid, S. D. Mills, and B. B. Finlay. 1996. A pathogenic bacterium triggers epithelial signals to form a functional bacterial receptor that mediates actin pseudopod formation. EMBO J. 15:2613-2624[Medline].

44. Rowbotham, T. J. 1980. Preliminary report on the pathogenicity of Legionella pneumophila for freshwater and soil amoebae. J. Clin. Pathol. 33:1179-1183[Abstract/Free Full Text].

45. Steinert, M., L. Emody, R. Amann, and J. Hacker. 1997. Resuscitation of viable but nonculturable Legionella pneumophila Philadelphia JR32 by Acanthamoeba castellanii. Appl. Environ. Microbiol. 63:2047-2053[Abstract].

46. Stone, B. J., and Y. Abu Kwaik Submitted for publication.

47. Stout, J. E., J. Joly, M. Para, J. Plouffe, C. Ciesielski, M. J. Blaser, and V. L. Yu. 1988. Comparison of molecular methods for subtyping patients and epidemiologically linked environmental isolates of Legionella pneumophila. J. Infect. Dis. 157:486-495[Medline].

48. 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].

49. Tang, P., I. Rosenshine, and B. B. Finlay. 1994. Listeria monocytogenes, an invasive bacterium, stimulates MAP kinase upon attachment to epithelial cells. Mol. Biol. Cell 5:455-464[Abstract].

50. Udezulu, I. A., and G. J. Leitch. 1987. A membrane-associated neuraminidase in Entamoeba histolytica trophozoites. Infect. Immun. 55:181-186[Abstract/Free Full Text].

51. Vazquez-Prado, J., and I. Meza. 1992. Fibronectin "receptor" in Entamoeba histolytica: purification and association with the cytoskeleton. Arch. Med. Res. 23:125-128[Medline].

52. 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].

53. Woodhead, M. A., J. T. Macfarlane, J. S. McCracken, D. H. Rose, and R. G. Finch. 1987. Prospective study of the aetiology and outcome of pneumonia in the community. Lancet i:671-674.

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1.	Abu Kwaik, Y. 1996. The phagosome containing Legionella pneumophila within the protozoan Hartmannella vermiformis is surrounded by the rough endoplasmic reticulum. Appl. Environ. Microbiol. 62:2022-2028[Abstract].
2.	Abu Kwaik, Y. Induced expression of the Legionella pneumophila gene encoding a 20-kilodalton protein during intracellular infection. Infect. Immun., in press.
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.	Adeleke, A., J. Pruckler, R. Benson, T. Rowbotham, M. Halablab, and B. S. Fields. 1996. Legionella-like amoebal pathogens $---$ phylogenetic status and possible role in respiratory disease. Emerg. Infect. Dis. 2:225-229.
9.	Allen, L. H., and A. Aderem. 1996. Molecular definition of distinct cytoskeletal structures involved in complement- and Fc receptor-mediated phagocytosis in macrophages. J. Exp. Med. 184:627-637[Abstract/Free Full Text].
10.	Barbaree, J. M., B. S. Fields, J. C. Feeley, G. W. Gorman, and W. T. Martin. 1986. Isolation of protozoa from water associated with a legionellosis outbreak and demonstration of intracellular multiplication of Legionella pneumophila. Appl. Environ. Microbiol. 51:422-424[Abstract/Free Full Text].
11.	Barker, J., M. R. W. Brown, P. J. Collier, I. Farrell, and P. Gilbert. 1992. Relationship between Legionella pneumophila and Acanthamoeba polyphaga: physiological status and susceptibility to chemical inactivation. Appl. Environ. Microbiol. 58:2420-2425[Abstract/Free Full Text].
12.	Barker, J., H. Scaife, and M. R. W. Brown. 1995. Intraphagocytic growth induces an antibiotic-resistant phenotype of Legionella pneumophila. Antimicrob. Agents Chemother. 39:2684-2688[Abstract].
13.	Bates, J. H., G. D. Capmpbell, and A. L. Baron. 1992. Microbial etiology of acute pneumonia in hospitalized patients. Chest 101:1005-1012[Abstract/Free Full Text].
14.	Bhopal, R. S., R. J. Fallon, E. C. Buist, R. J. Black, and J. D. Urquhart. 1991. Proximity of the home to a cooling tower and risk of non-outbreak Legionnaires' disease. Br. Med. J. 302:378-383.
15.	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].
16.	Breiman, R. F., B. S. Fields, G. N. Sanden, L. Volmer, A. Meier, and J. S. Spika. 1990. Association of shower use with Legionnaires' disease: possible role of amoebae. JAMA 263:2924-2926[Abstract/Free Full Text].
17.	Brieland, J. K., J. C. Fantone, D. G. Remick, M. LeGendre, M. McClain, and N. C. Engleberg. 1997. The role of Legionella pneumophila-infected Hartmanella vermiformis as an infectious particle in a murine model of Legionnaires' disease. Infect. Immun. 65:5330-5333[Abstract].
18.	Britles, R. J., T. J. Rowbotham, D. Raoult, and T. G. Harrison. 1996. Phylogenetic diversity of intra-amoebal legionellae as revealed by 16S rRNA gene sequence comparison. Microbiology 142:3525-3530[Abstract/Free Full Text].
19.	Cianciotto, N. P., and B. S. Fields. 1992. Legionella pneumophila mip gene potentiates intracellular infection of protozoa and human macrophages. Proc. Natl. Acad. Sci. USA 89:5188-5191[Abstract/Free Full Text].
20.	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].
21.	Cirillo, J. D., L. S. Tompkins, and S. Falkow. 1994. Growth of Legionella pneumophila in Acanthamoeba castellanii enhances invasion. Infect. Immun. 62:3254-3261[Abstract/Free Full Text].
22.	Dennis, P. J., A. E. Wright, D. A. Rutter, J. E. Death, and B. P. Jones. 1984. Legionella pneumophila in aerosols from shower baths. J. Hyg. 93:349-353[Medline].
23.	Fang, G. D., M. Fine, and J. Orloff. 1990. New and emerging etiologies of community-acquired pneumonia with implications for therapy, a prospective multicenter study of 359 cases. Medicine (Baltimore) 69:307-316[Medline].
24.	Fields, B. S. 1996. The molecular ecology of legionellae. Trends Microbiol. 4:286-290[Medline].
25.	Fields, B. S., T. A. Nerad, T. K. Sawyer, C. H. King, J. M. Barbaree, W. T. Martin, W. E. Morrill, and G. N. Sanden. 1990. Characterization of an axenic strain of Hartmannella vermiformis obtained from an investigation of nosocomial legionellosis. J. Protozool. 37:581-583[Medline].
26.	Fields, B. S., G. N. Sanden, J. M. Barbaree, W. E. Morrill, R. M. Wadowsky, E. H. White, and J. C. Feeley. 1989. Intracellular multiplication of Legionella pneumophila in amoebae isolated from hospital hot water tanks. Curr. Microbiol. 18:131-137.
27.	Finlay, B. B., and P. Cossart. 1997. Exploitation of mammalian host cell functions by bacterial pathogens. Science 276:718-725[Abstract/Free Full Text].
28.	Fry, N. K., T. J. Rowbotham, N. A. Saunders, and T. M. Embley. 1991. Direct amplification and sequencing of the 16S ribosomal DNA of an intracellular Legionella species recovered by amoebal enrichment from the sputum of a patient with pneumonia. FEMS Microbiol. Lett. 83:165-168.
29.	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].
30.	Gao, L.-Y., O. S. Harb, and Y. Abu Kwaik. Submitted for publication.
30a.	Harb, O. S., J. K. Brieland, and Y. Abu Kwaik. Submitted for publication.
31.	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].
32.	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].
33.	Ireton, K., B. Payrastre, H. Chap, W. Ogawa, H. Sakaue, M. Kasuga, and P. Cossart. 1996. A role for phosphoinositide 3-kinase in bacterial adhesion. Science 274:780-782[Abstract/Free Full Text].
34.	Isenberg, G., U. Aebi, and T. D. Pollard. 1980. An actin-binding protein from Acanthamoeba regulates actin filament polymerization and interactions. Nature 288:455-459[Medline].
35.	Joiner, K. A., S. A. Fuhrman, H. M. Miettinen, L. H. Kasper, and I. Mellman. 1990. Toxoplasma gondii: fusion competence of parasitophorous vacuoles in Fc receptor-transfected fibroblasts. Science 249:641-646[Abstract/Free Full Text].
36.	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].
37.	Kurtz, J. B., C. L. R. Bartlett, U. A. Newton, R. A. White, and N. L. Jones. 1982. Legionella pneumophila in cooling tower systems. J. Hyg. 88:369-381[Medline].
38.	Marston, B. J. 1995. Epidemiology of community-acquired pneumonia. Infect. Dis. Clin. Pract. 4:S232-S239.
39.	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].
40.	O'Brein, S. J., and R. S. Bhopal. 1993. Legionnaires' disease: the infective dose paradox. Lancet 342:5-6[Medline].
41.	Rosenshine, I., V. Duronio, and B. B. Finlay. 1992. Tyrosine protein kinase inhibitors block invasin-promoted bacterial uptake by epithelial cells. Infect. Immun. 60:2211-2217[Abstract/Free Full Text].
42.	Rosenshine, I., S. Ruschkowski, V. Foubister, and B. B. Finlay. 1994. Salmonella typhimurium invasion of epithelial cells: role of induced host cell tyrosine protein phosphorylation. Infect. Immun. 62:4969-4974[Abstract/Free Full Text].
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