Regulation of Adherence and Virulence by the Entamoeba histolytica Lectin Cytoplasmic Domain, Which Contains a beta 2 Integrin Motif

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Vol. 9, Issue 8, 2069-2079, August 1998

Regulation of Adherence and Virulence by the Entamoeba histolytica Lectin Cytoplasmic Domain, Which Contains a $beta$ 2 Integrin Motif

Richard R. Vines,^* Girija Ramakrishnan, Joshua B. Rogers, Lauren A. Lockhart, Barbara J. Mann,^* and William A. Petri Jr.^*^§

Departments of ^*Microbiology, Medicine, and ^§Pathology, University of Virginia, Charlottesville, Virginia 22908

Submitted March 2, 1998; Accepted May 13, 1998
Monitoring Editor: W. James Nelson

	ABSTRACT

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Killing of human cells by the parasite Entamoeba histolytica requires adherence via an amebic cell surface lectin. Lectinactivity in the parasite is regulated by inside-out signaling.The lectin cytoplasmic domain has sequence identity with a regionof the $beta$ 2 integrin cytoplasmic tail implicated in regulation ofintegrin-mediated adhesion. Intracellular expression of a fusionprotein containing the cytoplasmic domain of the lectin has adominant negative effect on extracellular lectin-mediated celladherence. Mutation of the integrin-like sequence abrogates thedominant negative effect. Amebae expressing the dominant negativemutant are less virulent in an animal model of amebiasis. Theseresults suggest that inside-out signaling via the lectin cytoplasmicdomain may control the extracellular adhesive activity of theamebic lectin and provide in vivo demonstration of the lectin'srole in virulence.

	INTRODUCTION

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The intestinal protozoan parasite Entamoeba histolytica is the causative agent of the disease amebiasis. E. histolytica infectionresults in 50 million cases of invasive amebiasis and 100,000deaths annually, and is surpassed only by malaria and schistosomiasisas the leading parasitic cause of death. E. histolytica is foundworldwide, with the highest morbidity and mortality seen in Centraland South America, Africa, and India (WHO, 1997).

Carbohydrate-protein interactions are responsible for the contact-dependent cytotoxicity for which E. histolytica was named.Contact of E. histolytica to host cells is mediated by an amebiclectin specific for galactose (Gal) and N-acetyl-D-galactosamine(GalNAc) (Petri et al., 1987). Amebae are unable to adhere toor kill Chinese hamster ovary (CHO) cell glycosylation mutantswhich lack Gal/GalNAc-terminal oligosaccharides. Adherence andcytolysis of human colonic epithelial cells, neutrophils, macrophages,and T lymphocytes is blocked in vitro by 50 mM Gal or GalNAc (Ravdinand Guerrant, 1981; Ravdin et al., 1985; Burchard and Bilke, 1992).

The Gal/GalNAc lectin is a heterodimeric molecule composed of a transmembrane heavy (170-kDa) subunit and a glycosylphosphatidylinositol-anchoredlight (31/35-kDa) subunit which are linked by disulfide bonds(Petri, 1996). The light subunit is encoded by a family of atleast seven genes (lgl) which share 79-85% amino acid sequenceidentity. There are five heavy subunit (hgl) gene family membersin E. histolytica strain HM1:IMSS which exhibit >89% nucleotidesequence identity (Ramakrishnan et al., 1996). The amino-terminal1209 residues are extracellular, with the carbohydrate-bindingdomain located between amino acids 898-998 of the heavy subunit(Mann et al., 1991; Dodson, Mann, and Petri, unpublished data).The carboxyl-terminal 41 amino acids of the heavy subunit comprisethe only cytoplasmic portion of the lectin.

The carbohydrate-binding function of the lectin is regulated, apparently due to changes in the structure of the lectin asopposed to changes in lectin number. For example, mAbs againstepitopes 1 and 2 of the heavy subunit enhance trophozoite adherenceby activating the Gal/GalNAc lectin (Petri et al., 1990). CytochalasinsB and D inhibit lectin-mediated adherence, presumably by disruptinglectin interactions with the cytoskeleton (Ravdin and Guerrant,1981). The ability to control lectin activity may be especiallyimportant because lectin binding to Gal/GalNAc oligosaccharidesis of extremely high affinity (K_d = 8.2 × 10¹¹ M¹) (Chadee et al., 1988). Without a mechanism to modulate lectinactivity, amebae might be unable to detach from mucins and epithelialcells as they invade the host.

The integrin family of adherence proteins is a well-studied example of dynamic regulation of adhesive function. Several integrinsare activated to a high-affinity state by extracellular signalsor by anti-integrin antibodies. Activation is independent of changesin integrin number or microenvironment. The cytoplasmic tailsof the integrin subunits are crucial regulators of integrin activity,both via interaction with the cytoskeleton and by transductionof signals to the extracellular integrin domains. The lectin-heavysubunit cytoplasmic domain has sequence identity with the $beta$ 2 and $beta$ 7 integrin cytoplasmic tails, including amino acids implicatedin control of integrin adhesiveness (Figures 1 and 2A).

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Figure 1. Sequence identity of the lectin-heavy subunit (hgl1) cytoplasmic tail with the $beta$ 2 and $beta$ 7 integrin cytoplasmic tails. Identical amino acids are in bold, amino acids implicated in integrin inside-out signaling are highlighted (*), and gaps placed to maximize sequence alignment are shown as (:).

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Figure 2. Lectin-GFP fusion protein constructs. (A) Schematic representation of the heavy subunit of the Gal/GalNAc lectin. SP, signal peptide; C-W, cysteine and tryptophan-rich region (3% cysteine, 2% tryptophan); C-free, cysteine-free region; C-rich, cysteine-rich region (11% cysteine); TM, transmembrane; CT, cytoplasmic tail. (B) 224, lectin-GFP fusion protein. (C). 324, lectin-GFP fusion protein lacking the cytoplasmic tail.

For this reason we focused on the potential role of the lectin cytoplasmic domain in control of adhesiveness of the lectin.We hypothesized that an intracellular factor interacts with thelectin cytoplasmic domain to regulate amebic adherence. Inducibleexpression of a fusion protein containing the cytoplasmic tailof the lectin resulted in a dominant negative effect on the extracellularadhesive activity of the wild-type lectin. The dominant negativeeffect appeared to be at the level of regulation of lectin activity,since the structure and cell surface concentration of the wild-typelectin were unaltered. The dominant negative effect was lost uponmutation of the lectin cytoplasmic domain amino acids with identityto the $beta$ integrins. Amebae induced to express the dominant negativelectin mutant were defective in the ability to form liver abscesses,providing the first in vivo evidence of the importance of thelectin, and its adhesive regulation, in virulence.

	MATERIALS AND METHODS

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Entamoeba histolytica and CHO Cells $---$ Culture and Other Methods

E. histolytica strain HM1:IMSS trophozoites were grown in TYI-S-33 medium containing penicillin (100 U/ml¹) and streptomycin sulfate (100 µg/ml¹) in either 12-ml screw cap tubes, 75-cm² flasks, or 25-cm² flasks at 37°C (Diamond et al., 1978). Amebae to be used forstable transfection were grown in 75-cm² flasks to a density of 5.3-6.6 × 10⁴ trophozoites/ml¹ (logarithmic phase growth). CHO cells were grown in 25-cm² flasks in 5 ml of MEM- $alpha$ (Life Technologies, Grand Island, NY)supplemented with 10% FBS, penicillin (100 U/ml¹), and streptomycin (100 µg/ml¹) at 37°C and 5% CO₂. For use in in vitro assays, CHO cells werereleased from the monolayer by a 3-min incubation in 0.25% trypsin.

E. histolytica adherence and cytolysis were assayed using the method of Ravdin and Guerrant (1981). Electroporation of E.histolytica followed the protocol described previously by Ramakrishnanet al. (1997). Erythrophagocytosis was measured according to themethod of Trissl et al. (1978).

Construction of Inducible Expression Vector

As described previously, the tetO operator sequence was introduced downstream of the TATA box of the hgl5 promoter by ligatingin annealed oligonucleotides that generate a BglII site at oneend (Ramakrishnan et al., 1997). Plasmid pGIR208 described previouslyhas the BglII site proximal to the TATA box; companion plasmidpGIR209 had the BglII site distal to the TATA box. Target genesfor inducible expression were cloned at the BglII site of pGIR209,thus placing their translational start very close to the transcriptionstart within the tetO sequence.

Construction of Lectin-Green Fluorescent Protein (GFP) Fusion Expression Vectors

A lectin-heavy subunit-GFP fusion protein was constructed in the following manner: First, an NcoI digest was performed ona full-length hgl clone (kindly provided by J. M. Dodson, Universityof Virginia). This was followed by blunt-ending with Klenow enzyme(Life Technologies) and ligation of an XbaI linker onto the bluntend. Next, an EcoRI digest was performed which liberated bp 179-3460of hgl. The entire ORF of GFP was PCR amplified (Pfu DNA polymerase)with the forward primer 5'-ctactgtctagaCATATGAGTAAA GGAGAAGA-3'and the reverse primer 5'-ctactggaattcTTTGTA TAGTTCATCCATGC-3'.After digestion with XbaI and EcoRI, GFP was ligated into thesesites of the hgl construct. The construct was then digested withXbaI and filled in with Klenow to yield an in-frame product. Thelectin-GFP fusion was then PCR amplified with the forward primer5'-ctactgggatccAAATGAAATTATTAT TATTAA-3' and the reverse primer5'-ctactggtcgacTTATCCATT GAATGTTGCTG-3'. After digestion withBamHI and SalI, the fragment was ligated into the BglII and SalIsites of pGIR209 creating plasmid pGIR224.

As a control, a vector to inducibly express the lectin-GFP fusion protein, which lacked the lectin cytoplasmic domain, wasconstructed. Using pGIR224 as template with the forward primer5'-cta ctgggatccAAATGAAATTATTATTATTAA-3' and the reverse primer5'-cagtaggtcgacttaAAATAATCCAATAGAAAC-3', the desired lectin-GFPDNA was PCR amplified using Pfu DNA polymerase. Following digestionwith BamHI and SalI, the fragment was ligated into the BglII andSalI sites of pGIR209 creating plasmid pGIR324. Constructs weresequenced in their entirety to rule out cloning or PCR artifacts.

Mutations in the cytoplasmic tail of the 224 construct were created using a two-step PCR method. For each mutation, one newprimer was synthesized to replace the original bases. The primerused for the Y $right-arrow$ A transition was 5'-ACTAATGAAAATGCAGAAGCTGTTGGAGCAGATAATGAA-3'. (The bases in bold represent the desiredmutations.) This primer was used with a second primer, 5'-AAATGATGTTCACTTTATTT-3',which hybridized to the 3' end of hgl 3' region approximately100 bp downstream of the stop codon. This first round productwas then used as a primer for a second round of PCR with a newprimer, 5'-CTACTGGGATCC AAATGAAATTATTATTATTAAA-3' (BamHIsite used for cloning underlined, bold bases represent start codon),which hybridized in the hgl 5' region, allowing the synthesisof the entire hgl-GFP fusion protein with the appropriate mutation.The TIT... Y $right-arrow$ AAA... A mutation was synthesized utilizing the samestrategy except with primer 5'-ATGAAGAATGCCATTGCAGCAGCTAATGAAAATGCAGAAGCTGTTGGAGCAGATAAT-3' (bold bases indicate mismatch).The second round PCR products were then digested with BamHI andSalI, and ligated into vector pGIR209 which had been digestedwith BglII and SalI. Colonies were screened by restriction analysisand then sequenced to ensure that there were no PCR-induced errorsand that our base substitutions had been incorporated.

FACS Analysis

Trophozoites (1-2 × 10⁶) were first washed with cold PBS and resuspended in 180 µl of PBS and incubated on ice for 45 min with20 µl of lectin mAb ascites or 40 µg of purified lectin mAb. Amebaewere washed twice in cold PBS, resuspended in 180 µl of PBS, and20 µl of antimouse IgG conjugated to FITC (Sigma, St. Louis, MO)were added and incubated for 45 min on ice. After two washes inPBS, amebae were resuspended in 1 ml of TYI-S-33 medium. Sampleswere analyzed using a Becton Dickinson FACScan Flow Cytometerequipped with an air-cooled argon laser at an excitation of 488nm. An acquisition gate was set on forward scatter (relative size)× side scatter (granularity or complexity) to exclude debris.The instrument was adjusted based on negative and background controls.Fifteen thousand gated events were collected and analyzed. Fluorescencedata was collected in a 4-decade log mode, forward scatter andside scatter were collected in a linear mode.

Immunofluorescence and Confocal Microscopy

For immunofluorescent staining, approximately 2 × 10⁵ amebae per sample were chilled and washed in PBS. Amebae were then fixedin 3% paraformaldehyde for 30 min at room temperature, permeabilizedin 0.25% Triton X-100 for 30 s, washed twice in PBS, and resuspendedin a rabbit-derived primary antibody at a dilution of 1:33 for1 h. Amebae were then washed twice in PBS and resuspended in goatanti-rabbit-FITC (Sigma) at a dilution of 1:64 for 1 h. Amebaewere washed twice in PBS and mounted on glass slides in VectaShield (Vector Laboratories, Burlingame, CA). Amebae were visualizedusing a Zeiss LSM 410 laser scanning confocal microscope equippedwith an argon/krypton laser. To generate final images, four averagesat 8 s each were compiled via a Zeiss 63×, plan-apochromat (numericalaperture, 1.40) objective, with laser excitation at 488 nm appropriatefor FITC.

Amebic Liver Abscess Model

One day prior to challenge, amebae strains 224 and 324 were induced with 5 µg/ml doxycycline in TYI-S33 medium. The gerbilsin the induced group received drinking water containing 2.5 mg/mldoxycycline and 5% sucrose. The control animals received watercontaining 5% sucrose alone. The animals were challenged by directhepatic inoculation with 5 × 10⁵ amebic trophozoites using the method of Chadee and Meerovitch(1985). Gerbils were killed 5-8 d after challenge and liver abscessweights were determined.

	RESULTS

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Optimization of the tetO Inducible Promoter System for Protein Expression

In the tetracycline-inducible system previously developed for use in E. histolytica, the tetO sequence was incorporated intothe 5' untranslated region of the induced luciferase RNA in plasmidconstruct pGIR204 (Ramakrishnan et al., 1997). Although the inducedtranscription was efficient, the induced RNA was not very welltranslated, presumably due to the presence of a dyad structureconferred by the inverted repeats of the tetO sequence. The expressionvector was therefore redesigned so as to prevent the formationof the dyad structure. It has been shown that the site of transcriptioninitiation in the hgl5 promoter is primarily determined by thepresence of the TATA box at about $-$ 30 from the transcription start(Singh et al., 1997). The endogenous sequences downstream of theTATA box in the expression vector were replaced with the tetOsequence so that transcription would initiate within the invertedrepeats of the operator sequence, thereby generating a transcriptthat cannot form a hairpin loop at the 5' end. Mapping of theRNA by primer extension showed that transcription initiation occurredwithin the tetO sequence, as predicted (our unpublished results).The luciferase expression of this construct showed good repressionunder normal conditions (0.3 U/cell) and was induced 100-foldon addition of 5 mg/ml tetracycline (40 U/cell) at 15 µg/ml hygromycinand 6 µg/ml G418 for maintenance of episomes. The fold inductionand induced levels with this construct were approximately fivefoldhigher than with previous constructs.

Inducible Expression of a Fusion Protein Containing the Lectin Cytoplasmic Domain

To investigate the role of the lectin-heavy subunit cytoplasmic tail in adherence and cell killing, a portion of the codingregion of the hgl gene was fused in-frame with the GFP (Cormacket al., 1996), generating the lectin-GFP fusion protein 224 (Figure2B). This protein maintained the amino-terminal signal peptide,the putative transmembrane domain, and the cytoplasmic tail ofthe lectin (Mann et al., 1991). Lectin-GFP fusion protein 324was created by deleting the cytoplasmic tail sequences from the224 construct via PCR (Figure 2C). These lectin-GFP fusion proteinswere designed to be expressed from the pGIR209 plasmid to allowfor inducible expression when introduced into E. histolytica (Ramakrishnanet al., 1997).

After establishment of stable transfected amebae lines, a Western blot was performed to verify expression of the lectin-GFPproteins. (Detection of the lectin-GFP fusion proteins was alwaysthrough the use of antibody to GFP because the fusion proteinswere not autofluorescent and were not recognized by antibodiesto the lectin-heavy subunit.) Figure 3A shows the expression ofthe 324 and 224 proteins during a time course of induction with5 µg/ml¹ tetracycline. Expression of the two proteins was approximatelyequivalent, as judged by Western blot. The 324 protein migratedat the expected size of approximately 47 kDa. With the additionof the 4-kDa cytoplasmic tail, 224 migrated as predicted at approximately51 kDa. The expression of both proteins was repressed in the absenceof tetracycline.

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Figure 3. Inducible expression of the 224 and 324 fusion proteins in E. histolytica. (A) Time course of expression of lectin-GFP fusion proteins after induction with tetracycline. Stably transfected pGIR324/308 and pGIR224/308 amebae were induced to express the 324 and 224 fusion proteins, respectively, with tetracycline for the indicated times. Amebic proteins were analyzed by SDS-PAGE followed by Western blotting with anti-GFP antibodies. The positions of the 324 and 224 fusion proteins and the 46-kDa size marker are shown. (B-D) Intracellular location of lectin-GFP fusion proteins. Control amebae (B) and amebae induced to express the 224 (C) or 324 (D) fusion proteins were fixed in paraformaldehyde, permeabilized, and immunostained with polyclonal antibody to the lectin (B) or to GFP (C and D). Amebae were then incubated with FITC-conjugated sheep anti-rabbit IgG, mounted, and visualized by confocal microscopy. (E) Surface expression of the endogenous lectin is not altered by expression of the 224 lectin-GFP fusion protein. Amebae were incubated with antilectin antibody. After incubation with an FITC-conjugated secondary antibody, amebae (uninduced or induced to express 224 for 24 h) were analyzed by single parameter FACS for surface fluorescence.

To ascertain the percentage of stable, transfected amebae that were actually expressing the lectin-GFP proteins, 224 amebaewere induced for 24 h and immunostained using antibody to GFP.Stained amebae were visualized by both bright field and fluorescentmicroscopy to assess the expression of the 224 protein by individualamebae. All amebae examined were expressing the lectin-GFP protein(our unpublished results). In addition, the intensity of fluorescencesuggested that the amebae were expressing the protein at similarlevels. Background staining was minimal as staining for lectin-GFPproteins was only evident upon induction, and omission of theGFP antibody yielded no significant staining of cells.

Intracellular Location of the Lectin-GFP Fusion Proteins 224 and 324

As these lectin-GFP proteins maintained the membrane signal sequence, it was theoretically possible that the proteins wouldlocalize to the cell surface. The cellular locations of the lectin-GFPproteins were ascertained by immunofluorescent staining and confocalmicroscopy. Cell surface staining of amebae with lectin antibodyhas been previously demonstrated (Petri et al., 1987). The stainingof the lectin was evident at the cell surface as a border whichsurrounded the cells; lectin was also visualized within the cytoplasm(Figure 3B). In contrast, the pattern of staining for 324 (Figure3C) and 224 (Figure 3D) showed a decided lack of surface stainingand a punctate pattern of staining within the cytoplasm, suggestinga vesicular location. Consistent with these results, FACS analysesof amebae expressing 324 and 224 were also negative for surfaceexpression (our unpublished results).

Wild-Type Lectin Cell Surface Concentration and Structure Is Unchanged by 224 Expression

To verify that lectin-GFP fusion protein 224 expression did not alter the expression of the endogenous lectin at the surface,cell surface lectin was quantitated by FACS analysis using lectinmAb H85 (which did not recognize the lectin-GFP fusion proteins).Uninduced and 24-h induced 224 amebae were stained with mAb H85(Mann et al., 1993) followed by incubation with a FITC-conjugatedantimouse secondary antibody. Analysis of these amebae by singleparameter FACS showed that the cell surface expression of thelectin as assessed by antilectin mAb H85 was not significantlyaltered on induction of 224 (Figure 3E). Cell surface lectin expressionas measured by the lectin activating antilectin mAb 3F4 was alsounaltered by expression of the 224 fusion protein (our unpublishedresults). The lack of a difference in 3F4 mAb staining on inductionof the 224 fusion protein is consistent with the 3F4 mAb havingthe same affinity for active and inactive lectin (as 224 inductioninactivated the lectin, see below). A similar observation hasbeen made for the integrin activating mAb KIM-127 (Cai and Wright,1995). These data indicated that expression of 224 did not perturbendogenous lectin expression on the surface of amebae.

To determine whether 224 associated with the heavy or light subunits of the endogenous lectin, amebae expressing 224 werelysed under nonreducing conditions. Under nonreducing conditionsthe lectin migrated on SDS-PAGE as a 260-kDa heterodimer composedof the heavy and light subunits (Petri et al., 1989; McCoy etal., 1994). As shown in Figure 4, both the heavy and light subunitscomigrated as a single band of 260 kDa, with no new bands beingevident which would correlate to a heavy or light subunit/224complex. The GFP blot showed that 224 was only present at itspredicted monomeric size of 51 kDa. These data demonstrated thatby Western blot, 224 was not covalently associated with the endogenousheavy or light subunits of the lectin.

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Figure 4. Lack of association of lectin-GFP fusion protein 224 with endogenous lectin subunits. Amebic proteins were separated under nonreducing conditions by SDS-PAGE and transferred to PVDF membranes. The blot was cut into three equivalent blots and each blot was incubated with antibody to either a lectin-heavy subunit, lectin-light subunit, or GFP. The blots were then incubated in alkaline phosphatase-conjugated secondary antibody and developed in substrate for alkaline phosphatase. The position of the molecular mass markers (in kDa) is shown. 1, amebae expressing luciferase as a control; 2 and 3, independent amebae transfectants expressing the 224 fusion protein.

Inducible Expression of Lectin Cytoplasmic Domain Decreases Amebic Adherence

We hypothesized that the extracellular adhesive activity of the lectin is controlled via interactions of cytoplasmic regulatoryfactors with the cytoplasmic tail of the lectin. Expression ofthe 224 fusion protein containing the cytoplasmic tail would bepredicted to alter the regulation of the endogenous lectin ifit competes with the endogenous lectin for the regulatory protein(s).We therefore measured the ability of amebae to adhere (at 4°C)to target cells on induction of the 224 and 324 fusion proteins.As shown in Figure 5A, following induction of the 324 construct(which lacks the lectin cytoplasmic domain), the ability of amebaeto adhere to CHO cells was unchanged. However, when amebae wereinduced to express the 224 fusion protein containing the lectincytoplasmic domain, there was a marked decrease in the abilityof the amebae to adhere to CHO cells (58% decrease, p < 0.0001)(Figure 5B). The decrease in adherence was evidenced as an increasein the number of amebae that had $<=$ 1 CHO cells attached. Correspondingly,these was a decrease in the number of amebae that had 3 or $>=$ 4CHO cells attached. Photomicrographs showing examples of adherentuninduced 224 amebae and nonadherent induced 224 amebae are shownin Figure 6. Because the endogenous lectin's cell surface concentrationand subunit structure were unaltered and because recruitment tothe cell surface of cytoplasmic stores of the endogenous lectindoes not occur at 4°C, we concluded that the decreased adherencewas a dominant negative effect of the 224 protein on regulationof lectin activity.

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Figure 5. Effect of induction of lectin-GFP fusion proteins on amebic adherence to and killing of CHO cells. Amebae [uninduced or induced to express either 324 (A) or 224 (B) for 24 h] were incubated with CHO cells. An adherence assay was performed and the number of CHO cells adhered to each ameba was determined. (C) Inhibition of cytolysis of CHO cells on inducible expression of lectin-GFP fusion protein 224. Amebae (uninduced or induced to express 224 for 24 h) were incubated with ⁵¹Cr-labeled CHO cells and treated as in the adherence assay. Dextran was added to the amebae/CHO pellet to prevent further adherence events from occurring. The pellet was incubated at 37°C to allow for cytolysis of the CHO cells and the supernatant was removed and assayed for ⁵¹Cr release.

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Figure 6. Photomicrographs of amebae-expressing lectin-GFP fusion protein 224 adhering to CHO cells. An adherence assay was performed with amebae (uninduced or induced to express 224 for 24 h). Representative amebae were photographed using a microscope equipped with differential interference contrast (DIC) optics. (A-C) Uninduced 224 amebae and adhered CHO cells. (D-F) Induced 224 amebae and nonadhered CHO cells.

Effect of Expression of Lectin Cytoplasmic Domain on Amebic Cytolysis

Because killing of target cells by E. histolytica is contact dependent, a decrease in the ability to adhere to target cellsshould result in decreased killing (Ravdin and Guerrant, 1981).The effect of 224 expression on the ability of amebae to kill⁵¹Cr-labeled CHO cells was tested. Following adherence at 4°C, theamebae-CHO cell rosettes were resuspended in dextran (to preventadditional amebae-CHO cell interactions) and lysis of the attachedCHO cells was measured at 37°C. The amount of ⁵¹Cr released into the supernatant was quantitated and used as ameasure of cell lysis. Amebae that were induced to express 224showed a 54% decrease in comparison to uninduced amebae (p = 0.031)in their ability to lyse labeled CHO cells (Figure 5C). Therefore,adherence and cytolysis were proportionately decreased in amebaeexpressing the 224 fusion protein. The expression of the lectincytoplasmic domain apparently inhibited adherence but not thecytolytic event occurring after adherence.

Phagocytosis and Serum Resistance Are Unaltered in 224 Expressing Amebae

E. histolytica has been shown to phagocytose a number of cells and particles including starch grains, bacteria, protozoa,and erythrocytes (Trissl et al., 1978). Because the lectin mediatesadherence of erythrocytes to amebae, we tested whether phagocytosiswould be affected by the induction of the 224 fusion protein.To ascertain the ability of 224-expressing amebae to phagocytosehuman erythrocytes, a phagocytosis assay was performed on amebaeinduced to express 224 for 24 h. Amebic phagocytosis of erythrocyteswas unchanged on induction of 224 expression (amebae phagocytosingred blood cells was 48 ± 2% without induction and 51 ± 3% withinduction) (our unpublished results).

Amebae activate the complement system, but are able to evade this early host defense mechanism. This evasion has been shownto be mediated by the ability of the lectin to bind complementcomponents C8 and C9, thereby abrogating assembly of the membraneattack complex (Braga et al., 1992). Studies investigating theeffect of 224 expression on the ability of amebae to evade lysisby complement did not demonstrate any consistent effect upon resistanceto lysis by complement (our unpublished results). Thus, the alteredphenotype in 224-expressing amebae appeared to be specific tothe adherence function of the lectin, with no observed effectson cytolysis (independent of adherence), phagocytosis, or serumresistance.

Amebae Expressing the Lectin Cytoplasmic Domain Fusion Protein Are Less Virulent

We next wished to test whether the decreased adherence seen on induction of the 224 fusion protein would result in decreasedvirulence of E. histolytica in the gerbil model of amebic liverabscess. Gerbils were challenged by intrahepatic inoculation with5 × 10⁵ trophozoites. Gerbils challenged with amebae induced to express224 and 324 received drinking water containing 2.5 mg/ml doxycyclinefrom 1 d before challenge to the completion of the experiment.Amebic strains were induced to express the 224 and 324 fusionproteins 24 h before challenge. Gerbils challenged with amebaeinduced to express the 224 fusion protein containing the lectincytoplasmic domain had abscesses that were 84% smaller than thoseof animals challenged with the uninduced 224 amebae (median abscesssize of 23.6 mg without induction and 4.0 mg with 224 induction;p = 0.03). In contrast, challenge of the gerbils with amebae containingthe 324 construct lacking the cytoplasmic domain demonstratedno significant change in liver abscess size on induction of the324 fusion protein (14.0 mg without induction and 17.8 mg with324 induction; p = 0.92). Amebae cultured from the abscesses maintainedthe expression of the 224 and 324 fusion proteins. We concludedthat inducible expression of the 224 fusion protein containingthe lectin cytoplasmic domain, but not the 324 fusion proteinlacking the cytoplasmic domain, decreased the virulence of E.histolytica. These data are the first in vivo confirmation ofthe importance of the lectin, and specifically of adhesive regulation,in virulence.

Role of Integrin Motif in Regulation of Adherence

Finally, we wished to ascertain the role of lectin cytoplasmic domain amino acids T₁₂₅₃, I₁₂₅₄, T₁₂₅₅, and Y₁₂₆₁ in the decreasedadherence phenotype seen on induction of the cytoplasmic tail224 construct. We focused on this region of the cytoplasmic tailbecause of its identity to the region in the $beta$ 2 integrin cytoplasmictail known to be involved in regulation of integrin adhesiveness.Mutation of the corresponding residues in the $beta$ 2 integrin cytoplasmictail has been shown to have a deleterious effect on integrin adherenceand cytoskeletal interaction (Hibbs et al., 1991; Peter and O'Toole,1995). Induction of a mutated 224 construct containing a cytoplasmicdomain Y/A₁₂₆₁ substitution (Figure 7A, mut1) resulted in a decreasein adherence equivalent to that seen on 224 induction. However,mutation of the entire motif (T/A₁₂₅₃, I/A₁₂₅₄, T/A ₁₂₅₅, andY/A₁₂₆₁) in the 224 construct (mut2) resulted in loss of the decreasedadherence phenotype (Figure 7). All three constructs, 224, mut1,and mut2, were expressed to equal levels in E. histolytica asassessed by Western blots with GFP antibodies (our unpublishedresults). These observations raise the possibility that the integrinmotif present in the lectin cytoplasmic tail is involved in theregulation of lectin activity.

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Figure 7. Mutation of the lectin/integrin motif in the 224 fusion protein cytoplasmic tail abrogates the 224 phenotype. The cytoplasmic domain sequence in the 224 fusion protein was mutated to alanine at residue Y₁₂₆₁ (mut1) and at T₁₂₅₃, I₁₂₅₄, T ₁₂₅₅, and Y₁₂₆₁ (mut2). Adherence was measured in transfected amebae induced to express the 224, mut1, and mut2 fusion proteins for 24 h and compared with adherence of the uninduced amebae. For these experiments adherence was expressed as the percentage of adherence of the uninduced amebae, where an adherent ameba was counted as one containing at least three adherent CHO cells.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

In this study, the inducible expression of an intracellular fusion protein containing the cytoplasmic tail of the E. histolyticalectin was demonstrated to decrease the extracellular adhesiveactivity of the wild-type lectin. This dominant negative effecton the wild-type lectin appeared to be at the level of regulationof lectin activity, because the heterodimeric structure and cellsurface concentration of the wild-type lectin were unaltered.Mutation of the lectin cytoplasmic domain sequence with identityto the $beta$ 2 integrin adhesion regulatory region in the 224 fusionprotein resulted in loss of the dominant negative phenotype. Thesedata suggest that the molecular mechanisms of regulation of adhesivenessby $beta$ 2 integrins and the amebic lectin may be similar.

Amebae induced to express the dominant negative lectin mutant were markedly defective in the ability to form liver abscessesin animals, providing the first in vivo evidence of the role ofthe lectin, and its adhesive regulation, in virulence. Previousreports had implicated the Gal/GalNAc lectin in the in vitro adherenceand killing of target cells. The innovations of stable and inducibleexpression in E. histolytica allowed for a genetic investigationinto the role of the lectin in adherence and virulence. The datapresented here showed that through inducible expression of lectinmutants, it was possible to begin to address the role of specificlectin domains in lectin function.

Only 224 protein-expressing amebae exhibited the decreased adherence phenotype, indicating that aberrant expression of thecytoplasmic tail (and not the transmembrane region present inthe 324 fusion protein) of the lectin was responsible for thedominant negative capability of the lectin-GFP fusion protein.These data provided evidence that intracellular signals can elicitchanges in the ligand-binding capability of the lectin. Interactionsof the lectin cytoplasmic tail with other intracellular factorscould be the manner in which this inside-out signaling is mediatedin E. histolytica. Overexpression of the cytoplasmic tail whichis present in the 224 construct could have acted to titrate outintracellular protein(s) essential for optimal adherence by thelectin.

Mutation of lectin cytoplasmic domain amino acids T₁₂₅₃, I₁₂₅₄, T₁₂₅₅, and Y₁₂₆₁ in the 224 construct resulted in loss ofthe dominant negative phenotype. We focused on this region ofthe cytoplasmic tail because of its identity with a region inthe $beta$ 2 integrin cytoplasmic tail known to be involved in regulationof integrin adhesiveness. Mutation of the corresponding residuesin the $beta$ 2 integrin cytoplasmic tail had been shown to have a deleteriouseffect on integrin adherence and cytoskeletal interaction (Hibbset al., 1991; Peter and O'Toole, 1995). The 224 fusion proteincontaining a cytoplasmic domain Y/A₁₂₆₁ substitution (Figure 7A,mut1) had a dominant negative effect on adherence equivalent tothe unmutated 224 protein. However, mutation of the entire motif(T/A₁₂₅₃, I/A₁₂₅₄, T/A ₁₂₅₅, and Y/A₁₂₆₁) in the 224 construct(mut2) resulted in loss of the decreased adherence phenotype,as was the case for the $beta$ 2 integrin. Given these observations,it is tempting to propose a similar mechanism of adhesive regulationfor the amebic lectin and the mammalian $beta$ 2 integrin.

Regulation of integrin adherence involves essential, titratable cytoplasmic factors. Many of the cellular factors and eventsinvolved in regulating integrin adherence remain to be identified;however, several proteins have been described. CD98, a heterodimeric,integral membrane protein has been shown to be an essential, titratablefactor involved in $beta$ 1 integrin activation. Results indicated thatthe cytoplasmic tails of the $beta$ 1 integrin and CD98 mediate theassociation of the two molecules (Fenczik et al., 1997). The proteincytohesin-1 has been shown to functionally and physically interactwith the cytoplasmic domain of the integrin $beta$ 2 subunit. This interactionplays a role in the regulation of $alpha$ 1 $beta$ 2 (LFA-1, CD11a/CD18) integrin-mediatedadhesion. The amino acids in the $beta$ 2 integrin domain that interactwith cytohesin-1 have yet to be identified (Kolanus et al., 1996).Finally $beta$ 3-endonexin interacts specifically with the $beta$ 3 cytoplasmicdomain; its overexpression has been demonstrated to increase platelet $alpha$ _II $beta$ 3 affinity and adhesive function (Shattil et al., 1995).

The nature of the change within the integrin that activates its adhesive function is unknown, but working models have beenproposed based on the current data and conserved sequence motifsof the integrins. The "piston," "twist," "zipper," and "hinge"models involve the movement of one integrin subunit relative tothe other, resulting in a conformational change in the extracellulardomain (Williams et al., 1994). Clustering of integrins on thecell surface also has been shown to increase the avidity of theintegrin-ligand interaction (Figdor et al., 1990; van Kooyk etal., 1994). Clustering results in a change in the extracellularconformation of the integrins which is attributable to the interactionof integrin cytoplasmic domains with cytoplasmic proteins (Lubet al., 1997). The ability of antilectin mAbs to activate thelectin and of cytoskeletal-disrupting agents to inhibit the lectinsuggest similar mechanisms of integrin and lectin adhesive regulation.

Expression of the 224 protein had a dominant negative effect on adherence, but not on cytolysis of adherent amebae, phagocytosisof human erythrocytes, or avoidance of complement lysis. The lectinhas been implicated in all of these processes. Given these data,amebic adherence, cytolysis, phagocytosis, and serum resistanceappear to be distinct events. The lack of a dominant negativeeffect of the 224 fusion protein on all of the lectin-mediatedfunctions may reflect participation of other members of the hglfamily (such as hgl2) or a lack of participation of the hgl1 cytoplasmicdomain in these events.

Inducible expression of dominant negative lectin mutants allowed for the first time the validation of a virulence factor,and its regulation, in E. histolytica through reverse genetics.The role of the cytoplasmic domain in the altered regulation ofthe lectin is important because of its role in virulence and suggestssimilar mechanisms may be responsible for the regulation of adherencein the amebic lectin and mammalian $beta$ 2 integrin. Future studieswill be directed to the identification of the cytoplasmic factor(s)which regulates the lectin's activity.

	ACKNOWLEDGMENTS

We are grateful to Thomas Parsons, Robert Kadner, Robert Bloodgood, Carol Otey, and Douglas DeSimone for helpful discussionand advice. We thank Upinder Singh for help with primer extensionmapping of RNA. This research was supported by National Institutesof Health grant AI-26649. W.A.P. is a Burroughs Wellcome Scholarin Molecular Parasitology.

	FOOTNOTES

These authors contributed equally to this work.

Corresponding author: University of Virginia Health Sciences Center, Room 2115, MR4 Building, Charlottesville, VA 22908. e-mail:wap3g{at}virginia.edu.

REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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				X. Zhang, Z. Zhang, D. Alexander, R. Bracha, D. Mirelman, and S. L. Stanley Jr. Expression of Amoebapores Is Required for Full Expression of Entamoeba histolytica Virulence in Amebic Liver Abscess but Is Not Necessary for the Induction of Inflammation or Tissue Damage in Amebic Colitis Infect. Immun., February 1, 2004; 72(2): 678 - 683. [Abstract] [Full Text] [PDF]

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				S. L. Stanley Jr. and S. L. Reed Microbes and Microbial Toxins: Paradigms for Microbial-Mucosal Interactions: VI. Entamoeba histolytica: parasite-host interactions Am J Physiol Gastrointest Liver Physiol, June 1, 2001; 280(6): G1049 - G1054. [Abstract] [Full Text] [PDF]

				M. Frisardi, S. K. Ghosh, J. Field, K. Van Dellen, R. Rogers, P. Robbins, and J. Samuelson The Most Abundant Glycoprotein of Amebic Cyst Walls (Jacob) Is a Lectin with Five Cys-Rich, Chitin-Binding Domains Infect. Immun., July 1, 2000; 68(7): 4217 - 4224. [Abstract] [Full Text] [PDF]

				M. Espinosa-Cantellano and A. Martinez-Palomo Pathogenesis of Intestinal Amebiasis: From Molecules to Disease Clin. Microbiol. Rev., April 1, 2000; 13(2): 318 - 331. [Abstract] [Full Text] [PDF]

				H. Tachibana, X.-J. Cheng, K. Watanabe, M. Takekoshi, F. Maeda, S. Aotsuka, Y. Kaneda, T. Takeuchi, and S. Ihara Preparation of Recombinant Human Monoclonal Antibody Fab Fragments Specific for Entamoeba histolytica Clin. Vaccine Immunol., May 1, 1999; 6(3): 383 - 387. [Abstract] [Full Text] [PDF]

				F. Padilla-Vaca, S. Ankri, R. Bracha, L. A. Koole, and D. Mirelman Down Regulation of Entamoeba histolytica Virulence by Monoxenic Cultivation with Escherichia coli O55 Is Related to a Decrease in Expression of the Light (35-Kilodalton) Subunit of the Gal/GalNAc Lectin Infect. Immun., May 1, 1999; 67(5): 2096 - 2102. [Abstract] [Full Text] [PDF]

Regulation of Adherence and Virulence by the Entamoeba histolytica Lectin Cytoplasmic Domain, Which Contains a 2 Integrin Motif

Regulation of Adherence and Virulence by the Entamoeba histolytica Lectin Cytoplasmic Domain, Which Contains a $beta$ 2 Integrin Motif

				J. M. Schaenman, C. A. Gilchrist, B. J. Mann, and W. A. Petri Jr. Identification of Two Entamoeba histolytica Sequence-specific URE4 Enhancer-binding Proteins with Homology to the RNA-binding Motif RRM J. Biol. Chem., January 5, 2001; 276(2): 1602 - 1609. [Abstract] [Full Text] [PDF]

				C. A. Gilchrist, C. F. Holm, M. A. Hughes, J. M. Schaenman, B. J. Mann, and W. A. Petri Jr. Identification and Characterization of an Entamoeba histolytica Upstream Regulatory Element 3 Sequence-specific DNA-binding Protein Containing EF-hand Motifs J. Biol. Chem., April 6, 2001; 276(15): 11838 - 11843. [Abstract] [Full Text] [PDF]