Enhancement of Splenic-Macrophage Fc{gamma} Receptor Expression by Treatment with Estrogens

doi:10.1128/CDLI.8.4.806-810.2001

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Clinical and Diagnostic Laboratory Immunology, July 2001, p. 806-810, Vol. 8, No. 4
1071-412X/01/$04.00+0 DOI: 10.1128/CDLI.8.4.806-810.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Enhancement of Splenic-Macrophage Fc $gamma$ Receptor Expression by Treatment with Estrogens

F. Gomez,^* P. Ruiz, J. A. Bernal, M. Escobar, A. Garcia-Egido, and J. J. B. Lopez-Saez

Hospital Universitario de Puerto Real/S.A.S. and Department of Medicine, School of Medicine, University of Cadiz, Cadiz, Spain

Received 19 January 2001/Returned for modification 15 March 2001/Accepted 7 May 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Splenic-macrophage Fc $gamma$ receptors (Fc $gamma$ Rs) participate in the pathophysiologies of immune-complex diseases and in host defenseagainst infection. Modulation of macrophage Fc $gamma$ R expression isan immuno-therapeutic target. Glucocorticoids, sex steroids, anddopaminergic drugs modulate macrophage Fc $gamma$ R expression. Previousdata indicate that estradiol increases macrophage Fc $gamma$ R expression.Nevertheless, the effects of clinically used estrogens upon macrophageFc $gamma$ R expression are unknown. We assessed the effects of treatmentwith commonly used estrogens on the expression of macrophage Fc $gamma$ Rsusing a guinea pig experimental model. Six estrogens have beenstudied: ethynylestradiol (Et), mestranol (M), chlortianisene(Ct), promestriene, 17-epiestriol, and 17 $beta$ -estradiol. Followingin vivo treatment of guinea pigs, we determined the clearanceof immunoglobulin G (IgG)-sensitized erythrocytes in vivo, thebinding of IgG-sensitized erythrocytes by isolated splenic macrophages,and splenic-macrophage Fc $gamma$ R cell surface expression. Estrogensenhance the clearance of IgG-sensitized erythrocytes by increasingsplenic-macrophage Fc $gamma$ R expression. Et, M, and Ct were more effectivethan the other estrogens. Flow cytometry and fluorescence microscopywith monoclonal antibodies demonstrated that estrogens increasethe cell surface expression of Fc $gamma$ R1 and -2 more than that ofFc $gamma$ R2. These data indicate that treatment with commonly used estrogensenhances the clearance of IgG-sensitized cells by improving splenic-macrophageFc $gamma$ Rexpression.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Splenic-macrophage Fc $gamma$ receptors (Fc $gamma$ Rs) play a important role in the clearance of immune complexes (2, 3, 5, 12,17, 18) and in host defense against infection (9, 16).Therefore, upregulation of macrophage Fc $gamma$ R expression is a potentialtherapeutic approach to those immunedisorders.

Sex hormones may affect the clinical manifestations of autoimmune disorders (10, 13). In vitro data indicate that sexhormones have regulatory effects on lymphocyte and macrophagefunctions (6, 11, 19, 24, 25). Although the precisemechanisms by which these steroid hormones affect the immune systemare not fully understood, our studies indicate that one effectis on macrophage Fc $gamma$ R expression (1, 7, 19, 20). Previousdata indicate that estradiol increases macrophage Fc $gamma$ R expression(6). Nevertheless, the effects of synthetic estrogens commonlyemployed in the treatment of human conditions upon macrophageFc $gamma$ R are presentlyunknown.

We have studied the effects of the treatment with estrogens approved for clinical use upon splenic-macrophage Fc $gamma$ R expressionusing a well-characterized experimental model, the guinea pig(7, 8, 15).

Treatment with estrogens of common clinical use improves the clearance of immunoglobulin G (IgG)-sensitized cells by enhancingthe expression of both guinea pig splenic-macrophage Fc $gamma$ Rs, Fc $gamma$ R2and Fc $gamma$ R1-Fc $gamma$ R2 (6, 11, 19). Therefore, estrogens are candidatedrugs for the treatment of disorders, like immune-complex diseases,whose sufferers benefit from an enhanced expression of the macrophageFc $gamma$ R.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

All experiments were performed with 500- to 600-g male Duncan-Hartley guinea pigs obtained from Criffa, Barcelona, Spain.Guinea pigs were injected with equal volumes of a homogeneoussuspension of estrogens in steroid suspension vehicle (SSV) (8,15). Sham controls received 1 ml of SSV not containing estrogen.All animals were injected subcutaneously in the dorsal neck fatpad every afternoon for seven consecutive days and studied onthe day after the last injection. The following estrogens wereobtained from Steraloids, Inc. (Wilton, N.H.): ethynilestradiol(Et), mestranol (M), 17-epiestriol (Ep), and 17 $beta$ -estradiol (E).Chlortianisene (Ct) and promestriene (Pm) were obtained from thepharmacy of our hospital. Doses of estrogens were selected onthe basis of those previously used in the treatment of human conditions:0.005 to 1 mg/kg of body weight for Et, 0.5 to 10 mg/kg for M,0.5 to 10 mg/kg for Ct, 0.1 to 5 mg/kg for Pm, 2.5 to 10 mg/kgfor Ep, and 2.5 to 10 mg/kg for E. Rabbit IgG anti-guinea pigred blood cell (RBC) antibodies were prepared as previously described,purified by Sephacryl S-300 gel filtration and quaternary aminoethylion-exchange chromatography (Pharmacia, Piscataway, N.J.), andfree of IgM as determined by Ouchterlony analysis and sodium dodecylsulfate-polyacrylamide gel electrophoresis (7, 8, 15).

Clearance of IgG-coated erythrocytes. Blood was drawn from anesthetized guinea pigs by cardiac puncture. Washed erythrocytes were radiolabeled with [⁵¹Cr]sodium chromate (Amersham, Madrid, Spain) and sensitized withan equal volume of IgG antibody, so as to be coated with approximately3,500 IgG molecules per erythrocyte as described previously (8,15). Treated animals were injected intravenously with 1.7 ×10⁸ ⁵¹Cr-labeled cells. Samples of blood were obtained 1 to 120 minafter injection, and cell-associated radioactivity was measuredin a gamma counter (Gamma 8000; Beckman Instruments, Inc., Fullerton,Calif.). Experiments were also performed with heat-altered erythrocytesto investigate splenic trapping mediated by nonimmune clearance,not only in sham controls but also in animals treated with high-doseestrogen (8, 15). Clearance curves were plotted by expressingthe number of blood counts per minute at each time point as apercentage of the number of counts per minute at 5 min. Levelsof clearance at 60, 90, and 120 min were analyzed to calculatea P value for the difference between control and experimentalclearance curves using Student's t test. Clearance at each timepoint represents the mean (± standard error of the mean [SEM])of results for at least six animals treated with a determineddose of estrogen, studied during 3 or more experimental days.Variations in levels of clearance among animals treated with variousdoses of estrogen was less than 10%. (In addition, for each day'sclearance study, the percent inhibition of clearance (mean ± SEM)above the level of inhibition of the control was calculated at90 and 120 min according to the formula 100 × [1 $-$ (cpm_c $-$ cpm_x)/(cpm_c $-$ cpm_ea)], where cpm_crefers to counts per minute for the untreated control animal injectedwith unsensitized cells, cpm_x refers to the experimentalanimal treated with steroid and injected with IgG-coated erythrocytes,and cpm_ea refers to control animals treated with SSVonly (no estrogen) and injected with the control IgG-sensitizederythrocytes. A negative value for percent inhibition indicatesenhancement of clearance. This formula compares results for treatedanimals with those for the control animals studied on the sameexperimental day and expresses the data as percentages of alterationof clearance, where 100% inhibition of clearance by estrogenscorresponds to the situation in which the clearance of IgG-sensitizederythrocytes (cpm_x) is identical to that of unsensitizederythrocytes (cpm_c) (7, 8, 15).

Binding of IgG-coated erythrocytes by splenic macrophages in vitro. Guinea pigs were sacrificed, splenectomy was performed immediately, and the spleens were placed in RPMI 1640 plus 10% heat-inactivatedfetal calf serum plus glutamine (complete RPMI). Splenic macrophageswere isolated by tissue grinding and sieving, discontinous Percollgradient centrifugation, and plastic adherence as previously described(7, 8, 15). More than 95% of the resultant cells wereviable mononuclear cells as determined by their ability to excludetrypan blue, and >90% of cells ingested latex beads and were stainedwith nonspecific sterase. Monolayers of adherent cells were preparedas previously described by incubating 10⁶ cells on a glass coverslip in a 35-mm-diameter plastic petridish at 37°C for 45 min under 5% CO₂ (1, 2, 7, 8,13, 20). More than 95% of the cells were adherent to glass.For experiments studying Fc $gamma$ R activity in vitro, guinea pig erythrocyteswere coated with 800 molecules of IgG per erythrocyte as describedabove and 1 ml of erythrocytes (5 × 10⁷ cells/ml) was incubated with the macrophage monolayers at 37°Cunder 5% CO₂ for 20 min. The monolayers were washed, air dried,and stained with Wright-Giemsa, and 200 consecutive macrophageswere inspected under an oil immersion lens for the number of erythrocytesbound per cell. The number of macrophages which bound $>=$ 3 IgG-sensitizederythrocytes was then determined (7, 8, 15, 20).

Flow cytometry. Monoclonal antibodies (MAbs) with specificities for guinea pig macrophage Fc $gamma$ R1-Fc $gamma$ R2 (VIA2 IgG1) and Fc $gamma$ R2 (VIIA1 IgG1) (22)were used in indirect immunofluorescence binding experiments toassess Fc $gamma$ R protein surface expression. These MAbs were the generousgift of I. Yamashita and T. Nakamura, Sapporo, Japan. Cells (5× 10⁵) were incubated with saturating concentrations of each MAb for60 min at 4°C and washed twice with phosphate-buffered salinecontaining 0.5% bovine serum albumin and 0.02% sodium azide. Tomeasure bound antibody, a fluorescein isothiocyanate-labeled goatanti-mouse antibody (Tago, Inc., Burlingame, Calif.) was addedfor 30 min at 4°C. The cells were again washed twice and fixedwith 4% paraformaldehyde. Cell-associated fluorescence was measuredusing a FACSTAR cytometer with Consort-32 software (Becton Dickinson& Co., Mountain View, Calif.). For all samples, 10,000 eventswere recorded on a logarithmic fluorescence scale and the meanfluorescence intensity (MFI) for each sample was determined usingConsort-32 software. In order to correct for autofluorescence,the MFI of a nonreactive murine IgG1 antibody (M3) was subtractedfrom the MFI of the anti-Fc $gamma$ R1-Fc $gamma$ R2- and anti-Fc $gamma$ R2-stained cells.Percent change in fluorescence intensity was calculated by theformula [(MFI of anti-Fc $gamma$ R-treated cells $-$ MFI of M3-treated cells)/(MFIof cells not treated with anti-Fc $gamma$ R $-$ MFI of cells not treatedwith M3)]¹ ×100.

To demonstrate the specificity of the estrogen effect on Fc $gamma$ R expression, we included an additional control with an irrelevantguinea pig pan-macrophage surface antigen, GPB (Seralab Ltd.,Sussex, England). Treatment with estrogens did not significantlyalter the cell surface expression of this pan-macrophage antigenand enhanced the expression of Fc $gamma$ R1-Fc $gamma$ R2 and Fc $gamma$ R2.

Effect of in vivo estrogens on membrane mobility of Fc $gamma$ R1-Fc $gamma$ R2 and Fc $gamma$ R2. Immunofluorescence capping experiments were performed in order to examine any possible effects of in vivo-administered estrogenson the membrane mobilities of Fc $gamma$ R1-Fc $gamma$ R2 and Fc $gamma$ R2. To this endin vitro capping experiments were performed comparing splenicmacrophages isolated from treated animals to those from sham controls.Et (0.01, 0.1, and 1 mg/kg), M (1, 5, and 10 mg/kg), and Ct (1,5, and 10 mg/kg) were the chosen estrogens. Splenic macrophages(5 × 10⁵) from guinea pigs treated with different doses of the most effectiveestrogens for 7 days or from sham-treated animals were incubatedwith saturating concentrations of MAbs for 30 min at 0°C on ice.After two washes at 0°C in phosphate-buffered saline-0.5% bovineserum albumin without sodium azide, fluorescein isothiocyanate-labeledgoat anti-mouse antibody was added as in the flow cytometry experiments.Cells were incubated at either 0 or 37°C for 20 min, washed, fixedin paraformaldehyde, and spun onto microscope slides in a centrifuge.Several hundred cells per slide were examined under epifluorescencewith a fluorescent microscope (Carl Zeiss, Oberkochen, Germany)(data notshown).

Statistics. To determine whether the difference between two means was significant, the unpaired or paired t test wasused.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Six estrogens, Et, M, Ct, Pm, Ep, and E, were studied. We examined the clearance of IgG-sensitized RBCs in animals treatedwith estrogens for 7 days to assess their in vivo effects on theexpression of splenic-macrophage Fc $gamma$ Rs. Treatment with any ofthe estrogens significantly enhanced the clearance of IgG-sensitizederythrocytes in more than 90% of the animals at 120 min comparedwith that of simultaneously tested sham controls (Fig. 1). Et,M, and Ct increased the clearance of IgG-sensitized RBCs moreefficiently than Pm, Ep, or E. The enhancement of clearance wasdose related (data not shown). No significant inhibition of clearancewas observed at doses of estrogens below those indicated in Fig.1.

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FIG. 1. In vivo clearance of IgG-sensitized RBCs in guinea pigs treated with minimal effective doses of estrogens. Numbers represent the doses of estrogens used (in milligrams per kilogram per day). Red cell survival is the percentage of ⁵¹Cr-labeled IgG-senstized RBCs (± SEM) remaining in the circulation at each indicated time point. Clearance of IgG-sensitized RBCs at 120 min was significantly enhanced by Et at 0.01 mg/kg (P < 0.001), M at 1 mg/kg (P < 0.001), Ct at 1 mg/kg (P < 0.001), Pm at 0.25 mg/kg (P < 0.01), Ep at 5 mg/kg (P < 0.01), and E at 5 mg/kg (P < 0.01). Survival of heat-damaged RBCs was not significantly different in estrogen-treated animals from that in sham controls (no estrogen).

The effect of estrogens on the function of the splenic-macrophage Fc $gamma$ Rs was assessed in vitro after splenic-macrophage isolation.Treatment with estrogens has no consistent effect on the yieldor viability of mononuclear cells isolated from the spleen. Fc $gamma$ Ractivity was determined by the in vitro binding of IgG-sensitizederythrocytes (Table 1). Following treatment with any of the estrogens,the percentage of isolated splenic macrophages binding $>=$ 3 IgG-sensitizederythrocytes was significantly higher than that of macrophagesisolated from sham animals. Et was the most active estrogen, enhancingthe recognition of IgG-sensitized RBCs by isolated splenic macrophages(P < 0.05). The lowest doses of estrogens that inhibited the bindingof IgG-sensitized erythrocytes by splenic macrophages are indicatedin Table 1.

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TABLE 1. In vitro binding of IgG-sensitized RBCs by isolated splenic macrophages and enhancement by treatment with estrogens

We further studied the effect of the treatment with estrogens on splenic macrophage Fc $gamma$ R cell surface expression. Guinea pigmacrophages express two classes of Fc $gamma$ Rs: Fc $gamma$ R1-Fc $gamma$ R2 and Fc $gamma$ R2(22). We examined the effect of estrogens on the expressionof both Fc $gamma$ R1-Fc $gamma$ R2 and Fc $gamma$ R2 by isolated splenic macrophages,using flow cytometry with specific MAbs for these receptors (Table2). Treatment with estrogens significantly increased the expressionof both guinea pig macrophage Fc $gamma$ Rs, Fc $gamma$ R1-Fc $gamma$ R2 and Fc $gamma$ R2. Asshown in Table 2, the estrogen-mediated inhibition of macrophageFc $gamma$ R expression was dose dependent. Minimal effective doses areindicated. Et, M, and Ct were more effective than Pm, Ep, or E,and all of them had a greater effect on Fc $gamma$ R1-Fc $gamma$ R2 than on Fc $gamma$ R2.

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TABLE 2. Enhancement of splenic-macrophage Fc $gamma$ R MFI by treatment with estrogens

Immunofluorescence capping experiments were performed to examine the effects of in vivo-administered estrogens on the membranemobilities of Fc $gamma$ R1-Fc $gamma$ R2 and Fc $gamma$ R2. We consider whether the highlylipophilic estrogen molecules might alter the mobilities of surfacemembrane receptors, thus contributing to the stimulatory effectsobserved on Fc $gamma$ R1-Fc $gamma$ R2 and Fc $gamma$ R2 expression. Cells incubatedat 0°C to prevent membrane movement showed a uniform diffuse ringpattern when they were stained for either Fc $gamma$ R1-Fc $gamma$ R2 or Fc $gamma$ R2.When incubated at 37°C, the majority of cells displayed aggregatesor patches of membrane fluorescence, with some cells showing anintense polar distribution of staining for both Fc $gamma$ Rs, similarto that reported for the ligand-induced capping of lymphocytesurface Ig (21). No significant differences were observed betweenresults for sham- and estrogen-treated animals for either Fc $gamma$ R1-Fc $gamma$ R2or Fc $gamma$ R2 staining intensity or distribution (data not shown).Estrogens do not appear to have a major effect on the membranemobilities of thesereceptors.

Our data indicate that treatment with estrogens approved for clinical use enhances the clearance of IgG-sensitized cells byimproving the cell surface expression of splenic-macrophage Fc $gamma$ Rs.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Macrophage Fc $gamma$ Rs play an important role in the regulation of the immune response, in host defense against infection, and inthe pathophysiologies of immune disorders (4, 9, 16).Thus, the modulation of macrophage Fc $gamma$ R expression is a therapeutictarget for immune-mediated diseases (4).

Neuroendocrine mechanisms are relevant to the pathophysiologies of immune-mediated disorders (14). We have been interestedin the modulation of FcRs for IgG by neuroendocrine actions asa new form of Fc $gamma$ R-directed therapy. Our guinea pig animal modelhas been useful in understanding the pathophysiologies of immunecytopenias (17, 18), as well as the effects of glucocorticoids,sex hormones, and dopaminergic drugs on macrophage Fc $gamma$ R expression(6-8, 15, 19).

We have previously observed that estradiol increases the clearance of IgG-sensitized cells by enhancing splenic-macrophageFc $gamma$ R expression (6, 19). The effect of clinically used estrogens,other than estradiol, on the clearance of IgG-containing immunecomplexes has not previously been assessed. Therefore, we studiedthe effect of treatment with estrogens on splenic-macrophage Fc $gamma$ Rexpression. Estrogens increased the clearance of IgG-sensitizedcells by enhancing the expression of splenic-macrophage Fc $gamma$ Rs.Et, M, and Ct were more effective than Pm, Ep, andE.

Two Fc $gamma$ R types, Fc $gamma$ R2 and Fc $gamma$ R1-Fc $gamma$ R2 have been identified in guinea pig macrophages (22). Our data suggest that both receptorsare expressed on essentially all splenic macrophages and participatein the binding of IgG-sensitized erythrocytes (7, 8, 15).Immunofluorescence capping experiments were performed to examineany possible effects of in vivo-administered estrogens on themembrane mobilities of Fc $gamma$ R1-Fc $gamma$ R2 and Fc $gamma$ R2 (21). Estrogensdo not appear to have a major effect on the membrane mobilitiesof these receptors, suggesting that their stimulatory effectsare likely at the level of surface receptorexpression.

The precise homology between guinea pig and human macrophage Fc $gamma$ Rs has not been established. Nevertheless, experimental studiesusing the guinea pig model have contributed to our understandingof the pathophysiologies and therapeutic mechanisms involvingmacrophage Fc $gamma$ Rs in human immunity-mediated disorders (1, 7,8, 15, 17-20). There is substantial similarity between humansand guinea pigs in their responses to steroids. Both species aresteroid resistant and are similar in their steroid metabolisms(23). We have previously measured the circulating levels ofsteroid hormones in guinea pigs and observed that they correlatewith the administered in vivo dose and with the steroid levelsobserved during changes in the hormonal state in humans (7,8, 15, 19). As we have observed with other steroids, likeglucocorticoids, androgens, and progesterones (7, 8, 15),guinea pig macrophage receptor Fc $gamma$ R1-Fc $gamma$ R2 in our experimentsappears to be more responsive to such estrogen-induced modulatorysignals than the other macrophage Fc $gamma$ R, Fc $gamma$ R2.

Our results indicate that treatment with the commonly employed estrogens Et, M, Ct, Ep, and E enhances ithe clearance of IgG-sensitizedcells by increasing the expression of splenic-macrophage Fc $gamma$ Rs.Guinea pig macrophage Fc $gamma$ R1-Fc $gamma$ R2 expression is more responsiveto enhancement than is the other macrophage Fc $gamma$ R, Fc $gamma$ R2.

	ACKNOWLEDGMENTS

This work was supported by grants from the Ministerio de Educación y Ciencia (PM92-0259 and RE90-28515062) and the Consejeriade Educación, Junta Andalucia (Grupo3224).

	FOOTNOTES

^* Corresponding author. Mailing address: Avda. de la Paz, 16 Valdelagrana, 11500 El Puerto de Santa María, Cadiz, Spain. Phoneand fax: 34-956-562714. E-mail: fgomez{at}comcadiz.org.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Atkinson, J. P., A. D. Schreiber, and M. M. Frank. 1973. Effects of corticosteroids and splenectomy on the immune clearance and destruction of erythrocytes. J. Clin. Investig. 52:1509-1517.

2. Blanchette, V., P. Imbach, M. Andrew, et al. 1994. Randomised trial of intravenous immunoglobulin G, intravenous anti-D, and oral prednisone in childhood acute immune thrombocytopenic purpura. Lancet 344:703-707[CrossRef][Medline].

3. Bussel, J. B., R. P. Kimberly, R. D. Inman, et al. 1983. Intravenous gammaglobulin treatment of chronic idiopathic thrombocytopenic purpura. Blood 62:480-486[Abstract/Free Full Text].

4. Deo, Y. M., R. F. Graziano, R. Repp, and J. G. J. van de Winkel. 1997. Clinical significance of IgG Fc receptors and Fc $gamma$ -directed immunotherapies. Immunol. Today 18:127-135[CrossRef][Medline].

5. Fehr, J., V. Hoffman, and U. Kappeler. 1982. Transient reversal of thrombocytopenia in idiopathic thrombocytopenic purpura by high dose intravenous gammaglobulin. N. Engl. J. Med. 306:1254-1258[Abstract].

6. Friedman, D., F. Nettl, and A. D. Schreiber. 1985. Effect of estradiol and steroid analogues on the clearance of immunoglobulin G coated erythrocytes. J. Clin. Investig. 75:162-167.

7. Gomez, F., P. Ruiz, F. Briceño, R. Lopez, and A. Michan. 1998. Treatment with progesterone analogues decreases macrophage Fc $gamma$ receptor expression. Clin. Immunol. Immunopathol. 89:231-239[CrossRef][Medline].

8. Gomez, F., P. Ruiz, F. Briceño, C. Rivera, and R. Lopez. 1999. Macrophage Fc $gamma$ receptor expression is altered by treatment with dopaminergic drugs. Clin. Immunol. 90:375-387[CrossRef][Medline].

9. Gomez, F., P. Ruiz, and A. D. Schreiber. 1994. Impairment of Fc $gamma$ -receptor predisposes to severe infection in alcoholic cirrhosis of the liver. N. Engl. J. Med. 331:1122-1128[Abstract/Free Full Text].

10. Goodhue, P. A., and T. S. Evans. 1962. Idiopathic thrombocytopenic purpura and pregnancy. Obstet. Gynecol. Surg. 18:671.

11. Holdstock, G., B. F. Chastenay, and E. L. Krawitt. 1982. Effects of testosterone, estradiol and progesterone on immune regulation. Clin. Exp. Immunol. 47:162-168[Medline].

12. Kimberly, R. P., J. E. Salmon, J. B. Bussel, et al. 1984. Modulation of mononuclear phagocyte function by intravenous gammaglobulin. J. Immunol. 132:745-750[Abstract].

13. Masi, A. T. 2000. Neuroendocrine immune mechanisms in rheumatic diseases: an overview and future implications. Rheum. Dis. Clin. North Am. 26:1003-1007[CrossRef][Medline].

14. Masi, A. T., J. W. J. Bijlsma, I. C. Chikanza, and M. Cutolo (ed.). 2000. Neuroendocrine mechanisms in rheumatic diseases. Rheum. Dis. Clin. North Am. 26:693-1018[CrossRef][Medline].

15. Ruiz, P., F. Gomez, M. King, R. Lopez, C. Darby, and A. D. Schreiber. 1991. In vivo glucocorticoid modulation of guinea pig splenic macrophage Fc $gamma$ receptors. J. Clin. Investig. 88:149-157.

16. Ruiz, P., F. Gomez, and A. D. Schreiber. 1990. Impaired macrophage Fc $gamma$ receptor function in chronic renal failure. N. Engl. J. Med. 322:717-722[Abstract].

17. Schreiber, A. D., and M. M. Frank. 1972. Role of antibody and complement in the immune clearance and destruction of erythrocytes. I. In vivo effects of IgG and IgM complement-fixing sites. J. Clin. Investig. 81:575-579.

18. Schreiber, A. D., and M. M. Frank. 1972. Role of antibody and complement in the immune clearance and destruction of erythrocytes. II. Molecular nature of IgG and IgM complement-fixing sites and effects of their interaction with serum. J. Clin. Investig. 51:583-587.

19. Schreiber, A. D., F. M. Nettl, M. C. Sanders, M. King, P. Szabolcs, D. Friedman, and F. Gomez. 1988. Effect of endogenous and synthetic sex steroids on the clearance of antibody-coated cells. J. Immunol. 141:2959-2966[Abstract].

20. Schreiber, A. D., J. Parson, P. McDermott, and R. A. Cooper. 1975. Effect of corticosteroids on the human monocyte IgG and complement receptors. J. Clin. Investig. 56:1189-1197.

21. Schreiner, G. F., and E. R. Unanue. 1976. Membrane and cytoplasmic changes in B lymphocytes induced by ligand-surface immunoglobulin alteration. Adv. Immunol. 31:67.

22. Shimamura, T., T. Nakamura, and J. Koyama. 1987. Demonstration of the evidence of two distinct Fc receptors for IgG isotypes on guinea pig macrophages by the use of monoclonal antibodies. Mol. Immunol. 24:67-74[CrossRef][Medline].

23. Sisk, D. 1976. The endocrine system, p. 79-103. In J. E. Wagner, and P. J. Manning (ed.), The biology of the guinea pig. Academic Press, Inc., New York, N.Y.

24. Vernon-Roberts, B. 1969. The effects of steroid hormones on macrophage activity. Int. Rev. Cytol. 25:131-159[Medline].

25. Werb, Z., R. Foley, and A. Nunck. 1978. Interaction of glucocorticoids with macrophages. Identification of glucocorticoid receptors in monocytes and macrophages. J. Exp. Med. 147:1684-1694[Abstract/Free Full Text].

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1.	Atkinson, J. P., A. D. Schreiber, and M. M. Frank. 1973. Effects of corticosteroids and splenectomy on the immune clearance and destruction of erythrocytes. J. Clin. Investig. 52:1509-1517.
2.	Blanchette, V., P. Imbach, M. Andrew, et al. 1994. Randomised trial of intravenous immunoglobulin G, intravenous anti-D, and oral prednisone in childhood acute immune thrombocytopenic purpura. Lancet 344:703-707[CrossRef][Medline].
3.	Bussel, J. B., R. P. Kimberly, R. D. Inman, et al. 1983. Intravenous gammaglobulin treatment of chronic idiopathic thrombocytopenic purpura. Blood 62:480-486[Abstract/Free Full Text].
4.	Deo, Y. M., R. F. Graziano, R. Repp, and J. G. J. van de Winkel. 1997. Clinical significance of IgG Fc receptors and Fc $gamma$ -directed immunotherapies. Immunol. Today 18:127-135[CrossRef][Medline].
5.	Fehr, J., V. Hoffman, and U. Kappeler. 1982. Transient reversal of thrombocytopenia in idiopathic thrombocytopenic purpura by high dose intravenous gammaglobulin. N. Engl. J. Med. 306:1254-1258[Abstract].
6.	Friedman, D., F. Nettl, and A. D. Schreiber. 1985. Effect of estradiol and steroid analogues on the clearance of immunoglobulin G coated erythrocytes. J. Clin. Investig. 75:162-167.
7.	Gomez, F., P. Ruiz, F. Briceño, R. Lopez, and A. Michan. 1998. Treatment with progesterone analogues decreases macrophage Fc $gamma$ receptor expression. Clin. Immunol. Immunopathol. 89:231-239[CrossRef][Medline].
8.	Gomez, F., P. Ruiz, F. Briceño, C. Rivera, and R. Lopez. 1999. Macrophage Fc $gamma$ receptor expression is altered by treatment with dopaminergic drugs. Clin. Immunol. 90:375-387[CrossRef][Medline].
9.	Gomez, F., P. Ruiz, and A. D. Schreiber. 1994. Impairment of Fc $gamma$ -receptor predisposes to severe infection in alcoholic cirrhosis of the liver. N. Engl. J. Med. 331:1122-1128[Abstract/Free Full Text].
10.	Goodhue, P. A., and T. S. Evans. 1962. Idiopathic thrombocytopenic purpura and pregnancy. Obstet. Gynecol. Surg. 18:671.
11.	Holdstock, G., B. F. Chastenay, and E. L. Krawitt. 1982. Effects of testosterone, estradiol and progesterone on immune regulation. Clin. Exp. Immunol. 47:162-168[Medline].
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Enhancement of Splenic-Macrophage Fc Receptor Expression by Treatment with Estrogens

Enhancement of Splenic-Macrophage Fc $gamma$ Receptor Expression by Treatment with Estrogens