Lead Stimulates Lymphocyte Proliferation Through Enhanced T Cell-B Cell Interaction

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Vol. 288, Issue 2, 714-719, February 1999

Lead Stimulates Lymphocyte Proliferation Through Enhanced T Cell-B Cell Interaction¹

Seddigheh Razani-Boroujerdi, Bruce Edwards and Mohan L. Sopori

Pathophysiology Division, The Lovelace Respiratory Research Institute, Albuquerque, New Mexico

	Abstract

Top Abstract Introduction Materials and methods Results Discussion References

We have studied the in vitro effects of lead (Pb) as Pb-acetate (0.1-1000 ppm) on the activation of rat spleen (SP) cells.At a concentration of 0.5 to 200 ppm, Pb augmented the uptakeof [³H]thymidine, progression of SP cells through the cell cycle, andallogeneic and syngeneic mixed lymphocyte reactions. However,at concentrations above 200 ppm, Pb inhibited the proliferationof these cells. To understand the cellular and molecular basisof these responses, we examined the effects of Pb on the proliferationof isolated T and/or B cell populations. Pb failed to stimulatethe proliferation of isolated T and B cells; however, the additionof $gamma$ -irradiated B cells to T cell cultures or irradiated T cellsto B cell cultures resulted in Pb-induced incorporation of [³H]thymidine. On the other hand, macrophages were unable to reconstitutethis response. Pb also induced a significant rise in the intracellularconcentration of inositol 1,4,5-trisphosphate in SP cells; however,unlike the activation of lymphocytes through the antigen receptors,Pb did not significantly stimulate protein tyrosine kinase activity.These observations suggest that Pb facilitates the T cell-B cellinteraction-dependent proliferation of lymphocytes through a signalingpathway(s) independent of the antigenreceptor.

	Introduction

Top Abstract Introduction Materials and methods Results Discussion References

Lead (Pb) is a ubiquitous environmental contaminant and belongs to the group of most toxic heavy elements in the atmosphere.In many countries, Pb poisoning continues to be a common occupationaldisease affecting several organ systems (Feldman and White, 1992;Gennart et al., 1992; Xuezhi et al., 1992). In the last 25 years,there has been an increased concern about the accumulation oflead in the environment. Many studies have demonstrated that Pbaffects the function of a variety of cell types, including thoseof the nervous system (Cohen and Coryslechta, 1994; Struzynskaand Rafalowska, 1994), the microvascular endothelium (Bressleret al., 1994), the kidney (Fowler et al., 1994), and the immunesystem (Luster et al., 1978; Lawrence, 1981, 1985; Fischbein etal., 1993; Cohen et al., 1994: McCabe, 1994). In vivo studieshave shown that Pb is an immunotoxicant depressing humoral immunity(Koller and Kovacic, 1974; Luster et al., 1978), increasing hostsusceptibility to bacterial (Hemphil et al., 1971; Lawrence, 1981),and viral infections (Gainer, 1974).

The manner in which Pb affects the immune cells is not well understood. Although Pb treatment in vivo may result in immunosuppression,Pb has been observed to enhance lymphocyte proliferation in vitro(Shenker et al., 1977; Gaworski and Sharma, 1978; Lawrence, 1981;Warner and Lawrence, 1986; McCabe and Lawrence, 1990). This apparentdiscrepancy between the in vitro and in vivo findings may be dueto complex interactions between tissues that form the in vivotargets of Pb, the ability of Pb to accumulate in various tissues,and/or the doses of Pb used in various studies. Moreover, immunosuppressionand autoimmune-like conditions coexist in several diseases (Rosen,1987). In this communication, we demonstrate that, depending onthe concentration of Pb, in vitro proliferation of splenic lymphocytesis either stimulated or inhibited in the presence ofPb.

	Materials and Methods

Top Abstract Introduction Materials and methods Results Discussion References

Animals. Pathogen-free male LEW (Lewis) and F344 (Fischer 344) rats were purchased from Harlan Sprague-Dawley Farms (Indianapolis,IN), housed in class-100 air quality rooms, and routinely monitoredfor common rat infections. Food (Lab Blox, Teklad, Madison, WI)and water were provided ad libitum, and animals 8 to 12 weeksof age were used in thesestudies.

Reagents. Phycoerythrin (PE)-conjugated monoclonal rat-specific antibodies to T cells (W3/13) and B cells (anti-IgM) were purchasedfrom Serotec (Indianapolis, IN). PE or fluorescein isothiocyanate(FITC)-labeled monoclonal antibodies (mAbs) to CD4⁺ T cells (W3/25), CD8⁺ T cells (OX-8), and appropriate antibody isotype controls werepurchased from PharMingen (San Diego, CA). DNase-free RNase, propidiumiodide, and lead acetate trihydrate were obtained from Sigma (St.Louis, MO). Mouse antiphosphotyrosine mAb was obtained from UpstateBiotechnology (Lake Placid,NY).

Pb Treatment. We examined the effects of 0.1 to 1000 ppm (0.26 µM to 2.6 mM) Pb on lymphocyte responses. For some experiments, the maximallystimulating dose of Pb (50 ppm $approx$ 131 µM) was used in order toobserve effects that might otherwise have beenmissed.

Tissue and Cell Preparations. Rats were sacrificed by CO₂ inhalation and spleen (SP) cell suspensions were prepared as previously described (Razani-Boroujerdiet al., 1994). Briefly, spleens were pressed through stainlesssteel mesh and red blood cells were lysed by treatment with NH₄Clsolution. T and B cells were purified as described previously(Sopori et al., 1984). Briefly, SP cells (1 × 10⁸ cells) in 25 ml of complete tissue culture medium (RPMI 1640supplemented with 10% heat-inactivated fetal calf serum, 2 mML-glutamine, 50 µM 2-mercaptoethanol, 1 mM sodium pyruvate, 10µg/ml gentamicin, minimal essential medium nonessential aminoacids, and polyvitamines) were depleted of macrophages by incubatingthe cells on a 100- × 15-mm glass Petri dish at 37°C for 1 h.T cells were purified by the passage of macrophage-depleted SPcells over a nylon-wool column (nylon-wool nonadherent cells).Enriched B cells were obtained from the macrophage-depleted populationby a negative selection in which T cells were removed by panningon dishes coated with W3/13 mAb (Sopori et al., 1985). The purityof T and B cell preparations was about 90% by fluorescence-activatedcell sorter analysis with an EPICS C (Coulter Electronics, Hialeah,FL) flowcytometer.

Assay for Mitogenesis. Proliferative responses were performed as previously described (Sopori et al., 1990). Briefly, in a final volume of 0.2 mlof complete medium, 2 × 10⁵ cells (SP, T, B, or T+B) were cultured in triplicates in flat-bottomed96-well microtiter plates (Corning, NY) in the presence and absenceof concanavalin A (Con A)/lipopolysaccharide (LPS) and indicatedconcentrations of Pb. Plates were incubated at 37°C in a 5% CO₂atmosphere. After 48 h, cultures were labeled with 0.5 µCi of[³H]thymidine per well (New England Nuclear, Waltham, MA) and, after24 h, cells were harvested using a Skatron cell harvester (Skatron,Sterling, VA). Samples were counted in a liquid scintillationcounter. Proliferation results are presented as the mean cpm ±S.D. of triplicatecultures.

Allogeneic and Syngeneic Mixed Lymphocyte Reactions. The allogeneic mixed lymphocyte reaction (MLR) and syngeneic mixed lymphocyte reaction (SMLR) were determined essentiallyas described previously (Sopori et al., 1984). Briefly, for MLR,2 × 10⁵ SP cells from LEW (RT1^l) were stimulated with 2 × 10⁵ of $gamma$ -irradiated (2000 rad) ACI (RT1^a) SP cells in a final volume of 0.2 ml in microtiter wells asdescribed under the assay for mitogenesis. On day 4, cells werelabeled with [³H]thymidine and harvested 16 h later. SMLR was carried out asthe MLR cultures were except that LEW SP cells were stimulatedwith $gamma$ -irradiated (2000 rad) syngeneic SPcells.

Determination of Percentages of B Cells, T Cells, and T Cell Subsets by Flow Cytometry. To determine the percentage of lymphocyte populations, cells were stained with PE or FITC-labeled antibodies specific fora given lymphocyte subpopulation and then analyzed by flow cytometryas described previously (Razani et al., 1994). Briefly, in a V-bottom96-well microtiter plate, 3 × 10⁵ cells were added to each well and washed twice with wash medium[phosphate-buffered saline (PBS) containing 5% fetal calf serumand 0.01% sodium azide]. Cells were pelleted and incubated onice for 1 h with 5 µl of predetermined optimal concentration ofPE or FITC-labeled mAb specific for various lymphocyte subpopulations.After washing, cells were resuspended in 200 µl of wash mediumand analyzed by flow cytometry. At least 10,000 cells were scoredfor each analysis. Percentages of positive cells were calculatedby subtracting the nonspecific (isotype controls) from the specificantibody fluorescentprofiles.

Cell Cycle Studies. DNA content and cell volumes were determined by flow cytometry according to the protocol described by Kusewitt et al. (1992).Briefly, 2 × 10⁶/ml SP cells, T cells, or B cells were cultured at 37°C in thepresence of indicated concentrations of Pb for various periods.Cells were pelleted and resuspended in 0.5 ml of cold PBS andpermeabilized by adding, in a dropwise fashion, 4 ml of prechilled( $-$ 20°C) 95% ethanol. Cells were stored at $-$ 20°C until furtherprocessing. To prepare cells for flow cytometric analysis, cellswere washed with 4 ml of PBS at room temperature, resuspendedin 0.5 ml of PBS, and treated with 10 µl of RNase (50 mg/ml; Sigma)and 20 µl of propidium iodide (1 mg/ml; Sigma). Cells were incubatedin the dark for 30 min at 37°C and analyzed by a flow cytometerwith excitation from an argon ion laser at 488 nm and detectionat 610 nm. To eliminate doublets, cells were gated on peak redfluorescence. At least 10,000 cells were analyzed for eachsample.

Inositol 1,4,5-Trisphosphate (IP₃) Assay. IP₃ was measured using [³H]inositol 1,4,5-trisphosphate radioreceptor assay kit (DuPont, Wilmington, DE), as described previously(Geng et al., 1996). Briefly, SP cells (1 × 10⁷/ml) were cultured in the presence of 50 ppm Pb or 5 µg/ml anti-clusterof differentiation 3 (CD3) for 0 to 10 min. The reaction was stoppedby adding 0.2 volumes of ice-cold 100% trichloroacetic acid solution.Samples were incubated on ice for 15 min and centrifuged in coldfor 1 min in a microfuge at 1000g. The supernatant was treatedwith a solution of 1,1,2-trichloro-1,2,2-trifluoroethane/trioctylamine(3:1) to remove trichloroacetic acid from the extracts. IP₃ wasmeasured in the aqueous (top) layer by radioreceptor assay asdescribed in instructions for thekit.

Tyrosine Phosphorylation Assays. Protein tyrosine phosphorylation was determined as described previously (Geng et al., 1996). Briefly, SP cells were incubatedwith different concentrations of Pb (0.1-100 ppm) at varying times(30 s to 48 h). The reaction was stopped with an excess of coldPBS and the cells were quickly pelleted, washed and lysed by alysis buffer containing Tris HCl (10 mM, pH, 7.0), NaCl (50 mM),sodium orthovanadate (10 mM), tetrasodium pyrophosphate (50 mM),NaF (50 mM), iodoacetamide (2.3 mM), ZnCl₂ (5 µM), Nonidet P-40(1%), phenlymethylsulfonyl fluoride (0.5 mM), and a concentration(5 µg/ml) of the following protease inhibitors: leupeptin, antipain,aprotinin, and pepstatin. Samples were stored at $-$ 70°C until theassay. Samples were thawed and boiled in a sample buffer containing125 mM Tris (pH 6.8), 0.1% SDS, 25 mM dithiothreitol, and 0.01%bromphenol blue for 3 min. Samples were loaded on a 10% SDS-polyacrylamidegel electrophoresis along with Kaleidoscope Prestained Standards(Bio-Rad, Hercules, CA) and electrophoresed on a minigel system(Bio-Rad) at 150 V for 45 min. The gel was blotted onto a nitrocellulosepaper, and the blot stained with Ponceu S (Sigma) to confirm thetransfer of proteins from the gel to the paper. The blots weretreated with 3% bovine serum albumin in Tris-buffered saline (pH7.2) for 30 min to block nonspecific binding. Blots were incubatedwith mouse antiphosphotyrosine mAb overnight and washed and incubatedwith goat anti-mouse horseradish peroxidase-conjugated antibodyfor 2 h. Blots were washed and developed for horseradish peroxidasedetection by either the chromogenic detection system (Renaissance4CN plus; DuPont) or chemiluminescence (enhanced chemiluminescenceWestern blotting solutions; Amersham, Uppsala,Sweden).

Statistical Analysis. Statistical comparisons between different treatments were performed using a one-way analysis of variance. A Scheffe post hoctest was used to determine the significance among groups. Thesestatistical procedures were performed using ABSTAT (Anderson-BellCorp., Parker,CO).

	Results

Top Abstract Introduction Materials and methods Results Discussion References

Pb Alters SP Cell Proliferation. Addition of Pb at concentrations from 0.1 to 200 ppm (0.1-200 µg/ml) to LEW SP cells significantly increased the incorporationof [³H]thymidine at doses above 0.5 ppm (Fig. 1). Maximal stimulationwas observed with 25 to 50 ppm of Pb (Fig. 1A). However, the proliferativeresponse dropped significantly below the background levels atPb concentrations of >500 ppm, reaching >90% inhibition of thebackground response at 1000 ppm (Fig 1B). Similar results wereobtained in F344 rats (data not shown). Thus, while the lowerconcentrations of Pb are immunostimulatory, higher concentrationsinhibit SP cell proliferation.

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Fig. 1. Pb induces proliferation of unfractionated SP cells and cultures containing both T and B cells, but not isolated T cells and B cells. Cells were cultured in triplicate wells, under the conditions described in Materials and Methods, in the presence or absence of indicated Pb concentrations. Each data point in the figure represents the mean ± S.D. of six independent experiments. For each experiment, cells were pooled from two animals. To compare the results from different experiments, the background proliferative response (i.e., response in the absence of Pb) of each animal was assigned a value of 100%. The data have been graphed in two ways. A, expanded graph to visualize the stimulatory effects of low Pb concentrations. B, extended dose range to show the inhibitory effects of high Pb concentrations.

Pb Increases Proliferation of Both T and B Cells. To determine whether Pb preferentially stimulated a subpopulation of lymphocytes, the percentages of B cells, T cells, CD4⁺ T cells, and CD8⁺ T cells were determined in SP cells cultured with 0.1 to 50 ppmPb for 3 days. Data presented in Table 1 (for a dosage of Pbwith highest mitogenic effect) show that, in spite of significantincreases in proliferation (see Fig. 1), percentages of thesesubpopulations were not significantly altered after Pb exposure,indicating that the Pb treatment increased the proliferation ofthese lymphocyte subsets to the same extent. Similar results wereobtained in cell cultures exposed to lower Pb treatments (notshown).

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TABLE 1
Pb does not stimulate the proliferation of selective lymphocyte subpopulations^a

Pb-Induced Proliferation Requires Participation of Both T and B Cells. Unlike unfractionated SP cells, proliferation of enriched T and B cell fractions was not significantly stimulated by Pb (Fig.1, A and B). Nevertheless, in the absence of Pb, the T cell fractiondid respond to Con A (not shown), indicating that the lack ofresponse to Pb is not due to limiting numbers of accessory cellsin the T cell fraction. However, the proliferative response toPb was restored after the T and B cell fractions were combined(Fig. 1). Thus, the Pb-induced proliferative response of lymphocytesmay require the presence of both B and T cells. Moreover, in thepresence of $gamma$ -irradiated SP cells, both T cells (Fig. 2A) andB cells (Fig. 2B), exhibited a significant proliferative responseto 50 ppm Pb. Similar but less pronounced proliferation was obtainedwith lower Pb levels (0.5-5 ppm, not shown). Furthermore, whilepurified $gamma$ -irradiated B and T cells could replace the SP cellsin stimulating the proliferation of purified T and B cells, respectively,addition of $gamma$ -irradiated macrophages did not restore this response(Fig. 2). These results suggest that both T and B cells are essentialfor Pb-induced proliferation and that Pb may cause an increasedinteraction between T and B cells. Since stimulation of T cellswith syngeneic B cells represents the SMLR response (Savage etal., 1993), these results suggest that Pb enhances SMLR.

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Fig. 2. Pb stimulates the SMLR response. T cells (A) and B cells (B) from the LEW rat spleen were cultured in the presence of $gamma$ -irradiated syngeneic cells: spleen (SPX), macrophages (MX), B cells (BX), or T cells (TX). Where indicated, Pb was added to a final concentration of 50 ppm. Cells were harvested on day 4 after pulsing with [³H]thymidine (see Materials and Methods). Data bars, mean ± S.E.M. from six separate experiments as described in Fig. 1.

Pb Stimulates the MLR. Figure 3 shows that 50 ppm Pb dramatically increases the MLR response of LEW (RT1^l) SP cells to $gamma$ -irradiated (2000 rad) SP cells from a major histocompatibilitycomplex-disparate strain ACI (RT1^a) (ACIX). In conjunction with the results shown in Fig. 2, theseresults suggest that Pb stimulates both the MLR and SMLR responses.

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Fig. 3. Pb enhances the allogenic MLR response. LEW SP cells were stimulated with $gamma$ -irradiated (2000 rad) ACI spleen cells (ACIX) in the presence or absence of 50 ppm Pb. Experimental conditions are as described in Materials and Methods. Data bars, mean ± S.E.M. from six different experiments (one or two rats/experiment).

Pb Stimulates the Entry of Lymphocytes into the Cell Cycle. We examined the effects of various Pb concentrations on the kinetics of entry of splenocytes into the cell cycle. Treatmentof SP cells with 50 ppm Pb significantly increased the entry ofthese cells into the S (area 2) and G₂-M (area 1) phases of thecell cycle within less than 6 h of Pb exposure (Fig. 4). Thisunusually fast cell-cycle response suggests that Pb treatmentmay trigger the progression of preexisting G₁ cells into the cellcycle. Thus, Pb may stimulate the transition of lymphocytes fromthe G₁ to the S phase of the cell cycle. The magnitude of theeffect obtained with 0.5 to 12 ppm Pb treatment was smaller (notshown). However, at Pb concentrations of 500 and 1000 ppm, therewas a significant increase in the cell population with less than1× DNA content (Fig. 4, area 4), suggesting increased death ofcells at these Pb concentrations. These results further supportthe inference that, although lower Pb concentrations (<200 ppm)are mitogenic, higher concentrations may be lymphotoxic.

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Fig. 4. Pb treatment stimulates the progression of G₁ cells into the cell cycle. LEW SP cells were cultured in medium alone (BK), 0.5 µg/ml Con A, and 50 and 1000 ppm Pb. Histograms represent the distribution of cells in the various phases of the cell cycle after 6 h of incubation. Areas 1, 2, and 3 correspond to the cell cycle phases of G₂-M, S, and G₀-G_1, respectively. Area 4 represents cells with less than 1× DNA content (apoptotic). Con A- and low Pb- (50 ppm) treated cells have significantly (p < .05) higher numbers of cells in the G₂-M and S phases of the cell cycle relative to BK. High Pb (1000 ppm) treated cells show a significant (p < .001) increase in the apoptotic fraction (area 4) compared with BK.

Pb Augments the Response of Spleen Cells to T and B Cell Mitogens. In the presence of 50 ppm Pb, the proliferative response of SP cells to the T cell mitogen, anti-CD3 antibody, and the B cellmitogen, LPS, is significantly increased (Fig. 5). Smaller increasesin anti-CD3 and LPS-induced proliferation were observed with lowerPb levels (0.5-5 ppm, not shown). In the presence of 50 ppm Pb,Con A typically induced greater spleen cell proliferation thanin the absence of Pb. However, this effect was not statisticallysignificant (not shown). Thus, Pb may enhance the response oflymphocytes to relatively weak mitogens.

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Fig. 5. Pb (50 ppm) increases proliferation of LEW SP cells in response to anti-CD3 antibody (A) and LPS (B). Solid line (control) and dotted line (with Pb). Each data point represents the mean ± S. D. of four to five experiments (n = 8).

Pb Increases IP₃ Levels in Splenocytes without Stimulating Protein Tyrosine Kinase (PTK) Activity. One of the earliest events in the antigen-induced activation of lymphocytes is an increase in the PTK activity, which in turnactivates phospholipase C $gamma$ (PLC $gamma$ ) catalyzing the hydrolysis ofphosphatidylinositol 4,5-bisphosphate (PIP₂) to IP₃ and diacylglycerol(Cambier et al., 1994; Chan et al., 1994). To determine whetherPb stimulated lymphocyte proliferation through a similar pathway,we determined the concentration of IP₃ in SP cells following exposureto 50 ppm Pb or anti-CD3. Results presented in Fig. 6 indicatethat, within 5 to 7 min, Pb significantly increased IP₃ levelsin these cells and the magnitude of response was similar to thatobtained with anti-CD3. However, as seen by Western blot analysisof tyrosine phosphorylation (Fig. 7), unlike treatment with anti-CD3or anti-IgM, there is no significant increase in the PTK activityin Pb-treated SP cells over the 0-time controls. These resultssuggest that Pb may stimulate the PLC activity through a mechanismthat is independent of PTK activation and is, therefore, differentfrom the antigen receptor-mediated lymphocyte activation.

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Fig. 6. Pb increases IP₃ production by SP cells. LEW SP cells were incubated with 50 ppm Pb or anti-CD3 antibody (5 µg/ml) for 0 to 10 min at 37°C. Lysates were assayed for IP₃ concentrations. Values represent an average of five experiments. IP₃ levels were significantly (p < .05) elevated by both treatments.

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Fig. 7. Pb does not stimulate the activity of PTKs in SP cells. SP cells were incubated with anti-CD3 (5 µg/ml), anti-IgM (5 µg/ml), and indicated Pb concentrations for 5 min. The lysates were examined for PTK activity by Western blot analysis. Similar results were obtained with longer Pb treatments (10 min to 24 h). BK, response in the absence of Pb; mw, molecular weight of standards.

	Discussion

Top Abstract Introduction Materials and methods Results Discussion References

Results presented herein suggest that Pb is a weak mitogen for lymphocytes and stimulates the proliferation of both T andB cells. At higher concentrations (>200 ppm), however, Pb is immunosuppressive,causing inhibition of background proliferation. While the enhancementof lymphocyte proliferation has also been reported by others (Shenkeret al., 1977; Gaworski and Sharma, 1978; Lawrence, 1981; Warnerand Lawrence, 1986; McCabe and Lawrence, 1990), our results indicatethat Pb has no significant effect on isolated populations of Tand B cells. However, addition of $gamma$ -irradiated B cells to T cellsor $gamma$ -irradiated T cells to B cells reconstituted the Pb-inducedproliferative response of these cell cultures; addition of $gamma$ -irradiatedmacrophages was ineffective in restoring this response. We havepreviously demonstrated that the rat SMLR response is dependenton the interaction between T cells and B cells resulting in theproliferation and differentiation of both cell types (Sopori etal., 1990; Savage et al., 1993). Thus, Pb may facilitate T cell-Bcell interaction accounting for the enhancement of the SMLR andMLR responses (i.e., responses where T cell-B cell interactionplays a pivot role in the response) (Singer and Hodes, 1983; Savageet al., 1993). The ability of Pb to enhance the SMLR responsecould potentially play a role in the increased frequency of someautoimmune diseases observed in Pb-exposed individuals (Wedeenet al., 1979).

To understand the mechanism through which Pb treatment increases lymphocyte proliferation, we investigated the effects ofPb on the progression of SP cells into the cell cycle. Culturingof SP cells with 50 ppm Pb caused a significant progression ofcells into the S and G_2-M phases of the cell cycle within 6 h.This relatively fast Pb-induced entry of lymphocytes into theS phase suggests that Pb may stimulate the progression of thesplenic lymphocyte fraction, which is in the G₁ phase at the timeof cell isolation. This could also explain the manner throughwhich Pb enhances proliferation of lymphocytes to relatively weakmitogens (i.e., anti-CD3, LPS); in the rat, LPS is a relativelypoor B cell mitogen. The ability of heavy metals to induce cellcycle progression in murine splenocytes was also reported by others(Warner and Lawrence, 1986)

One of the earliest events in the antigen-mediated activation of lymphocytes is an increase in PTK activity (Cambier et al.,1994; Chan et al., 1994). An important consequence of this activationis tyrosine phosphorylation of PLC $gamma$ leading to hydrolysis of PIP₂into diacylglycerol and IP₃ (Berridge, 1993; Robey and Allison,1995). IP₃ causes an increase in the intracellular calcium level(Berridge, 1993), leading to a progression of G₀-G₁ cells intothe S phase of the cell cycle (Crabtree and Clipstone, 1994).Because Pb enters into cells and binds to commonly used indicatorsfor measuring ionized calcium, Pb interferes with Ca⁺⁺ detection by standard methods (Schanne et al., 1989). Therefore,instead of measuring Ca⁺⁺ we determined whether Pb treatment had any effect on PIP₂ metabolismby measuring the intracellular IP₃ levels. As shown in Fig. 6,within minutes of Pb treatment, lymphocytes had significantlyhigher levels of IP₃, suggesting that Pb stimulates PLC activity.An increase in IP₃ levels in Pb-treated rat astrocytes has beenreported by Dave et al. (1993). However, unlike activation oflymphocytes through ligation of antigen receptors, the Pb-mediatedincrease in PLC $gamma$ activity in SP cells does not appear to dependon the activation of PTK activity. Therefore, it is unlikely thatincreased IP₃ levels in Pb-treated cells result from the activationof PLC $gamma$ . [Although the modulation of PTK by Pb⁺⁺ has not been reported, the inhibitory effects of Pb⁺⁺ on other protein kinase activities (e.g., protein kinase C) iswell documented (Saijoh et al., 1988; Rajanna et al., 1995).]The other known pathway for IP₃ synthesis involves the G-protein-dependentactivation of PLC $beta$ (Gilman, 1987); at present, we have no directevidence to suggest that Pb stimulates the G-protein-dependentsignaling pathway in lymphocytes. Nonetheless, our results suggestthat the lymphoproliferative effects of Pb may result from increasedIP₃ synthesis which is independent of antigen receptoractivation.

	Footnotes

Accepted for publication July 27, 1998.

Received for publication April 2, 1998.

¹ This work was supported in part by grants from the National Institutes of Health (DAO4208) and Lovelace Respiratory ResearchInstitute.

Send reprint requests to: M.L. Sopori, Ph.D., The Lovelace Respiratory Research Institute, P.O. Box 5890, Albuquerque, New Mexico 87185. E-mail: msopori{at}lrri.org

	Abbreviations

Pb, lead; PE, phycoerythrin; FITC, fluorescein isothiocyanate; mAb, monoclonal antibody; SP, spleen; LPS, lipopolysaccharide; SMLR, synergic mixed lymphocyte reaction; PBS, phosphate-buffered saline; IP₃, inositol 1,4,5-trisphosphate; PLC, phospholipase C; PTK, protein tyrosine kinase; PIP₂, phosphatidylinositol 4,5-bisphoshate.

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Lead Stimulates Lymphocyte Proliferation Through Enhanced T Cell-B Cell Interaction1

Lead Stimulates Lymphocyte Proliferation Through Enhanced T Cell-B Cell Interaction¹