Significance of Fatty Acids in Pregnancy-Induced Immunosuppression

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Clinical and Diagnostic Laboratory Immunology, July 1999, p. 587-593, Vol. 6, No. 4
1071-412X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Significance of Fatty Acids in Pregnancy-Induced Immunosuppression

Ian Crocker,¹^,^* Nigel Lawson,² Ian Daniels,¹ Philip Baker,³ and John Fletcher¹

Medical Research Centre,¹ Department of Clinical Chemistry,² and School of Human Development, University of Nottingham,³ Nottingham City Hospital NHS Trust, Nottingham NG5 1PB, United Kingdom

Received 14 September 1998/Returned for modification 6 January 1999/Accepted 19 April 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Pregnancy can exert suppressive effects on chronic inflammatory conditions. We have previously demonstrated a depression inpolymorphonuclear leukocyte (PMN) respiratory burst during pregnancywhich could explain this amelioration. To elucidate the biochemicalmechanism, we have examined PMN phospholipase A₂ (PLA₂) activityand its relationship to cellular and circulating fatty acids inpregnant women (30 to 34 weeks) and nonpregnant controls. PMNPLA₂ activity was determined by arachidonic acid (AA) and leukotrieneB₄ (LTB₄) release, respiratory burst activity was determined bylucigenin-enhanced chemiluminescence, and total serum and PMNfatty acid levels were determined by gas-liquid chromatography.AA release was significantly reduced for pregnancy PMNs in responseto N-formyl-met-leu-phe (fMLP) under unprimed and tumor necrosisfactor alpha (TNF- $alpha$ )- or interleukin 8-primed conditions. Similarly,LTB₄ liberation was significantly reduced in response to fMLPand phorbol myristate acetate in unprimed and TNF- $alpha$ -primed pregnancyPMNs. All major fatty acid classes were altered in the pregnantstate. Of these differences in PMNs, oleic acid and $alpha$ -linolenicacid showed a significant increase (13 and 26%, respectively)and stearic acid and AA showed a significant decrease (8 and 30%,respectively). The stearic acid, oleic acid, and AA compositionsof all cells analyzed correlated with their corresponding changesin serum fatty acid levels. Crossover serum incubations modifiedboth fatty acid profiles and the PMN respiratory burst accordingly,while individual fatty acid incorporation studies highlightedthe importance of polyunsaturated fatty acids for NADPH oxidaseefficiency. These findings indicate that the attenuation of PMNfunction in pregnancy may originate from a reduction in the availablepool of cellular fatty acids. Furthermore, this reduction arisesas a direct result of a pregnancy-induced shift in circulatingfatty acids from polyunsaturated to monounsaturatedforms.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

For more than a century, clinical observations have highlighted the ameliorating effect of pregnancy on certain inflammatorydisorders. Since the first detailed account of this phenomenonpublished by Hench in 1938 (21), the beneficial effect of pregnancyon rheumatoid arthritis (RA) has been continually reaffirmed.Most authors agree that the activity of RA is significantly alteredduring pregnancy, with approximately 70% of patients experiencinga substantial resolution of pain, swelling, and stiffness (fora review, see reference 39). This symptomatic relief becomesapparent from the first trimester and then progresses throughoutgestation, often enabling patients to reduce or completely interruptthe use of medication (13). Unfortunately, this remission isshort-lived; more than 90% of the improved patients will relapsewithin 8 to 9 months postpartum, and the majority will relapsewithin 6 weeks of delivery (31).

A steadily increasing number of theories have been proposed to explain this dramatic gestational improvement in RA. The majorityof these proposals invoke one or more mechanisms of pregnancy-inducedimmunosuppression. Although humoral immunity during pregnancyremains unchanged (7), a marked depression in cell-mediatedimmunity is suggested by a diminished skin reaction to tuberculin(17), by prolonged skin graft survival (1), and by an increasedsusceptibility to specific intracellular infections (27, 36).Polymorphonuclear leukocytes (PMN) are thought to be of centralimportance in the eradication of invasive pathogens and in thetissue damage associated with connective-tissue disorders. Previousstudies of functional differences during pregnancy have emphasizeda reduction in PMN chemotaxis (24), adherence (5), and microbialkilling (15). Pregnancy sera have been shown to suppress bacterialkilling (34) and to diminish PMN phagocytosis (33) and enzymerelease (20). Recently, we have reported a depression in PMNfunction in pregnancy characterized by a reduction in receptor-mediatedrespiratory burst activity (11). A significant decline in NADPHoxidase activity, as measured by superoxide anion release, wasobserved for pregnancy PMN in response to formyl-peptide and tozymosan-activated serum. A longitudinal study showed that thiseffect begins in the first trimester and gradually progressesto term before returning to preconception and control levels within6 weeks of delivery (11).

According to the current knowledge of PMN regulation, a conceivable and relevant mechanism explaining these variations inoxidative metabolism could be differences in cell membrane composition.Modulating agents which can affect lipid composition, order, andmobility, such as cholesterol, cholesterol esters, and certainsaturated and unsaturated fatty acids, have been shown to modifythe neutrophil superoxide anion response (10, 16, 25, 35).In addition, certain unsaturated fatty acids, most notably arachidonicacid (AA), can have a direct effect on the assembly and activationof the NADPH oxidase system (12). The mobilization and liberationof free AA from membrane phospholipids by phospholipase A₂ (PLA₂)is one of the earliest events in PMN activation. Once liberated,AA can be further metabolized by 5-lipoxygenase or by cyclooxygenaseto yield the inflammatory metabolites leukotriene B₄ (LTB₄) andprostaglandin E₂. To investigate the relationships among PMN activity,cell lipid composition, and the oxidative metabolic response inpregnancy, we have examined the PLA₂ activity of PMN from pregnantand nonpregnant subjects. PLA₂was measured by the release of AAand the formation of LTB₄ following either direct stimulationor priming, an induced condition of increased readiness whichcan enhance cell activation upon stimulation. In addition, inresponse to the suggestion that the levels of plasma free fattyacids are considerably altered during pregnancy (37), we haveexamined their relative amounts in the sera and isolated PMN ofpatients from both study groups and have confirmed a relationshipbetween PMN fatty acid composition and cell function. Finally,by incubating normal PMN in pregnancy serum, we have producedchanges in both cellular fatty acids and cell responses equivalentto those observed for pregnancyPMN.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Reagents. Ficoll-Hypaque was purchased from Flow Laboratories, Hertfordshire, United Kingdom. Gentran 70 (6% dextran 70 in 0.9% NaCl)was supplied by Baxter Healthcare Ltd., Norfolk, United Kingdom.EDTA (analytical grade) and 2,6-di-ter-p-cresol were obtainedfrom BDH, Dorset, United Kingdom. [³H]AA was purchased from Amersham Plc, Buckingham, United Kingdom.Tumor necrosis factor alpha (TNF- $alpha$ ), interleukin 1 $beta$ (IL-1 $beta$ ), andIL-8 were obtained from Genzyme Corporation, Kent, United Kingdom.All other reagents used were supplied by Sigma Chemical CompanyLtd., Poole, UnitedKingdom.

Study subjects. Venous blood was obtained from healthy pregnant women during the third trimester of pregnancy (30 to 34 weeks of gestation)and placed into EDTA-dipotassium at a final concentration of 3mM. Subjects with any preexisting medical disorders or takingany medication apart from vitamin or iron supplementation wereexcluded from the study. Blood was simultaneously obtained fromhealthy nonpregnant women of comparable age and who were not takinga contraceptive pill or any other form of medication. The agerange of the pregnancy group was 18 to 37 years, with a mean of28 years; that of the control group was 19 to 39 years, with amean of 27 years. There were no demographic differences betweenthe two groups. Informed consent was obtained from all subjectsbefore inclusion in the study, which was approved by the localethicalcommittee.

Preparation of human PMN. Human peripheral blood PMN were prepared by standard methods (6). Erythrocytes were sedimented on dextran, and the leukocyte-richplasma was further purified by centrifugation over Histopaque1077. The contaminating erythrocytes were lysed with 0.2% (wt/vol)NaCl, and the osmolality was restored with an equal volume of1.6% (wt/vol) NaCl. Once isolated, cells were washed twice inphosphate-buffered saline (pH 7.2) (PBS), and their viabilitywas assessed by trypan blue dye exclusion. PMN were regularlyobtained with a purity greater than 97% and a viability greaterthan 99%. Cells were resuspended in PBS and usedimmediately.

Cytokine priming. Prior to stimulation, PMN were preincubated with priming agents for the following times and concentrations: TNF- $alpha$ 250 pg/ml,30 min; IL-1 $beta$ , 1 ng/ml, 60 min; IL-8, 20 ng/ml, 30 min; and cytochalasinB, 5 µg/ml, 30 min. When necessary, initial dilutions were madewith dimethyl sulfoxide. All priming agents were further dilutedin PBS containing 1 mM CaCl₂, 0.7 mM MgCl₂, and 0.1% (wt/vol)endotoxin-free bovine serum albumin (BSA) (PBS/Ca/Mg/BSA). Finalconcentrations of dimethyl sulfoxide did not exceed 0.01%, andsolvent controls were included for all experiments. Preincubationswere conducted at 37°C with end-over-endrotation.

Respiratory burst activity. Extracellular PMN superoxide anion production was measured by lucigenin-enhanced chemiluminescence with a Labsystems (Basingstoke,United Kingdom) Luminoskan plate-reading luminometer. Briefly,140 µl of PBS/Ca/Mg/BSA, 20 µl of 250 µM lucigenin (bis-N-methylacridiniumnitrate), and 20 µl of PMN suspension (10⁷/ml) were added to triplicate wells of a 96-well Immunofluor microtiterplate (Dynatech, Billinghurst, United Kingdom). The plate waswarmed in the luminometer to 37°C before the addition of 10 µMN-formyl-met-leu-phe (fMLP). Chemiluminescence light output wasmonitored every 60 s for 30 min, and the integral over this periodwas expressed as relative lightunits.

Measurement of PLA₂ activity. [³H]AA release from PMN was determined by a modification of a previous method (9). PMN at 10⁷/ml were incubated with 1 µCi of [³H]AA per ml at 37°C for 1 h in PBS containing 0.1% (wt/vol) fatty-acid-freeBSA. Cells were washed three times and resuspended in PBS containing1 mM CaCl₂, 0.7 mM MgCl₂, and 0.1% (wt/vol) fatty acid-free BSAat a concentration of 3 × 10⁷/ml. Cell suspensions were primed as outlined above, and 100-µlaliquots were stimulated with 1 µM fMLP at 37°C. The reactionswere stopped by the addition of 0.5 ml of ice-cold 0.9% (wt/vol)NaCl at time zero, immediately after stimulation, and at 20 min.PMN were sedimented by centrifugation, and the [³H]AA release in the supernatant and pellet was determined by liquidscintillationcounting.

Determination of LTB₄ generation. The generation of LTB₄ was determined with a commercially available enzyme-linked immunosorbent assay (R&D Systems, Oxon,United Kingdom). The reaction mixture, containing PBS/Ca/Mg/BSA(250 µl) and primed or unprimed PMN (10⁷/ml), was preincubated at 37°C for 10 min before the additionof the stimulus. The final concentration of the stimulus was 1µM fMLP or 10 ng of phorbol myristate acetate (PMA) per ml. Thereaction was terminated by the addition of 13 µl of ice-cold citricacid (0.035 M) to reduce the pH to 5.5. PMN were sedimented bycentrifugation, and the supernatants were removed and stored at $-$ 80°C before beingassayed.

Fatty acid composition determination. Analysis of fatty acids was performed with serum samples (200 µl) and aliquots of PMN preparations (3 × 10⁷ cells) by extraction of total lipids with methanol-benzene (4:1[vol/vol]) plus 0.5 mM 2,6-di-ter-p-cresol as an antioxidant.Fatty acids were methylated by a direct transesterification technique(26), and the resulting fatty acid methyl esters were separatedby a gas-liquid chromatographic method (40) with a Cpsil 8850-m capillary column (Chrompak; Millharbour, London, United Kingdom)on a 5890 Series II gas chromatograph (Hewlett-Packard, Amsterdam,The Netherlands). Peak identifications were made with commerciallyavailable reference fatty acids, and heptanoic acid (C17:0) wasused as an internal standard. Fatty acid composition data wereexpressed as relative molar percentages of fatty acid methyl estersbased on peakareas.

Fatty acid incorporation. Individual fatty acids were complexed with fatty-acid-free BSA in 1:1 molar ratios according to the method of Mahoney et al.(28). The resulting fatty acid-BSA solutions were added to isolatedPMN (10⁷/ml) in PBS to give a final fatty acid concentration of 33 µM.Cells were incubated for 5 h at 37°C with continuous end-over-endrotation, washed three times with PBS, and then resuspended inPBS to their originalconcentration.

Statistical analysis. Statistical significance of differences was determined by use of the nonparametric Mann-Whitney U test for independent samplesand the Wilcoxon rank sum test for paired samples. The relationshipbetween different parameters was investigated with the nonparametricSpearman's rho correlation coefficient test. The results are presentedas the means ± the standard errors of the means (SEM); data wereconsidered significant at a P value of <0.05 (twotailed).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

PMN PLA₂ activity. PLA₂ catalyzes the hydrolysis of the ester bond between a fatty acid and the hydroxyl group at the sn-2 position of the glycerolbackbone of a phospholipid to generate a lysophospholipid anda fatty acid (usually AA). By labelling the phospholipid poolwith [³H]AA and measuring its subsequent stimulated release into theextracellular medium (against total incorporation), we were ableto determine the general activity of cellular PLA₂. Figure 1 showsthe contrast between the release of AA from [³H]AA-loaded pregnancy PMN and that from nonpregnancy PMN. In responseto fMLP, PLA₂ activation was significantly reduced in pregnancyPMN compared to nonpregnancy PMN. Similarly, cells primed witheither TNF- $alpha$ or IL-8 prior to activation showed a marked reductionin responses. Both cytochalasin B, the most potent priming agentused, and IL-1 $beta$ , the least effective, gave the same alterationsin pregnancy PMN activation, although these changes did not appearto reach significance over the experimental time period.

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FIG. 1. Comparison of AA liberation from PMN of women in their third trimester of pregnancy (n = 6) and nonpregnant age-matched women (n = 6). The results represent the extracellular release of [³H]AA from radioisotope-loaded, fMLP-stimulated PMN under primed (TNF- $alpha$ , IL-1 $beta$ , IL-8, and cytochalasin B [cyto b]) and unprimed conditions. The data are expressed as mean ± SEM and are significantly different (P values) at the following levels: *, <0.05; **, <0.02. Significance was determined with the Mann-Whitney U test.

LTB₄ production. Once AA has been liberated from membrane phospholipids, it can be further metabolized by 5-lipoxygenase to yield LTB₄. LTB₄is recognized as a potent inflammatory mediator and is capableof priming PMN (38) and further activating the NADPH oxidasesystem (14). Figure 2 illustrates LTB₄ production over a 15-minperiod from fMLP-stimulated, TNF- $alpha$ -primed and unprimed cells.No differences were evident in resting-cell responses betweenthe two study groups. However, under both primed and unprimedconditions, pregnancy PMN did show a marked reduction in LTB₄production following stimulation.

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FIG. 2. Comparison of LTB₄ release by PMN of pregnant women (30 to 34 weeks of gestation) and nonpregnant women following fMLP and PMA activation under TNF- $alpha$ -primed and unprimed conditions. The data are expressed as mean ± SEM and are significantly different at a P value of <0.05 (Mann-Whitney U test) (asterisks).

Serum and PMN fatty acids. The fatty acid compositions of sera and PMN from pregnant and nonpregnant subjects were determined by gas-liquid chromatography.The mean fatty acid compositions of PMN from both study groups,expressed as relative molar percentages, are given in Table 1.Almost all major fatty acid classes, including saturated, monounsaturated,and polyunsaturated species, were altered in pregnancy. Of thesedifferences in PMN, oleic acid and $alpha$ -linolenic acid showed significantincreases of 13 and 26%, respectively, while stearic acid andAA showed significant decreases of 8 and 30%, respectively. Serumvariations in total fatty acids included significant increasesfor palmitic acid (13%) and oleic acid (11%) and significant decreasesfor stearic acid (27%), linoleic acid (9.9%), and AA (18%) inpregnancy. Interestingly, the stearic acid, oleic acid, and AAcompositions of all the PMN analyzed correlated with correspondingchanges in the serum levels of these fatty acids. Figure 3 showsthe ratios of unsaturated fatty acids, monounsaturated fatty acids(MUFA), and polyunsaturated fatty acids (PUFA) for the study groups.In pregnancy, a more general pattern of fatty acid abnormalitiesemerges. For serum and PMN, an increase in PUFA (11.4 and 11.2%,respectively) and a decrease in MUFA (10.5 and 12.7%, respectively)would indicate an overall shift in fatty acid species in pregnancy.

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TABLE 1. Total fatty acid content of serum and PMN for pregnant women (30 to 34 weeks of gestation) and nonpregnant women

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FIG. 3. Ratios of mean fatty acids in PMN and serum for pregnant women (30 to 34 weeks of gestation) and nonpregnant women. SFA, saturated fatty acids. The degree of statistical significance is indicated by asterisks (P, <0.05) (Mann-Whitney U test).

Respiratory burst activity. Lucigenin is a cell-impermeable probe that amplifies photoemissions from oxygenation events. It is considered to be highlyselective for the extracellular generation of superoxide anionsand thus provides a convenient measure of PMN NADPH oxidase activity(19). In response to fMLP, PMN isolated from pregnant subjectsgenerated fewer superoxide anions than those from age-matchedcontrols (2,825 ± 384 versus 1,379 ± 225; P, <0.01, Mann-WhitneyU test). Taken together, the cellular concentrations of AA fromboth groups correlated positively with the NADPH oxidase activity(Fig. 4). In nonpregnancy cells, a more intimate relationshipwas recorded. This observation may suggest the influence of othercellular fatty acids or even additional regulatory factors inpregnancy, where AA concentrations are limited.

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FIG. 4. Linear regression plot of AA content and fMLP-stimulated superoxide anion release for PMN of pregnant women (30 to 34 weeks of gestation) and nonpregnant age-matched women. The relationship between parameters was significant at a P value of <0.05 (r, Spearman's rho correlation coefficient). RLU, relative light units.

Fatty acid incorporation. Individual fatty acids, incorporated as complexes with BSA, were successfully taken up by isolated PMN over a 5-h incubationperiod. This procedure produced a range of cells enriched in saturatedfatty acids, MUFA, and PUFA (Fig. 5). PMN with enhanced saturatedfatty acids and MUFA levels showed no difference in their respiratoryburst response to fMLP; however, cells with increased PUFA levelsall showed exaggerated responses (Fig. 5). Adhesion molecule markersof PMN, including CD18, CD11b, and CD62L, indicated that prioractivation or priming of the cells did not occur as a result ofthe incubation procedure (data not shown). Incubations were limitedto 5 h, as longer times were associated with a loss of cell viabilityand responsiveness.

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FIG. 5. Incubation of PMN in environments enriched for saturated fatty acids (FA), MUFA, and PUFA. Isolated PMN were incubated for 5 h at 37°C in a 1:1 molar ratio of individual fatty acids complexed with BSA. The final concentrations of fatty acids was 33 µM, and control samples were incubated in BSA alone. Cellular fatty acid profiles and chemiluminescence responses to fMLP were recorded for the washed cells. The data are expressed as mean ± SEM for six different PMN donors. The results were significantly different (P values) at the following levels: *, <0.05; **, <0.01. Significance was determined with the Wilcoxon rank sum test.

Serum incubations. To further investigate the relationship between both cellular and circulating fatty acid levels and PMN NADPH oxidase activity,PMN isolated from pregnant or nonpregnant subjects were incubated(5 h, 37°C) in either heat-inactivated (56°C, 30 min) autologousserum or heat-inactivated pooled heterologous serum. Figure 6demonstrates how incubation with 50% (vol/vol) pregnancy serummodifies the cellular fatty acid profile of normal nonpregnancyPMN to one comparable to that of pregnancy PMN. Similarly, thefMLP-stimulated NADPH oxidase activity of these cells is reducedto a level comparable to that of pregnancy PMN. Figure 7 showsthe reverse experiment. Incubation with 50% (vol/vol) nonpregnancyserum appears to redress the changes to the cellular fatty acidsof pregnancy PMN as well as to increase the total respiratoryburst output.

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FIG. 6. Serum incubation study for nonpregnancy PMN. The effect of pregnancy serum (50% [vol/vol]) on the fatty acid content and fMLP-stimulated superoxide anion release of normal nonpregnancy PMN was examined. Isolated peripheral blood PMN from nonpregnant subjects were incubated (5 h, 37°C) in either heat-inactivated (56°C, 30 min) autologous serum or heat-inactivated pooled pregnancy sera (n = 6). The data are expressed as mean ± SEM for eight different PMN donors. The results were significantly different (P values) at the following levels: *, <0.05; **, <0.01. Significance was determined with the Wilcoxon rank sum test. RLU, relative light units.

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FIG. 7. Serum incubation study for pregnancy PMN. The effect of nonpregnancy serum (50% [vol/vol]) on the fatty acid content and fMLP-stimulated superoxide anion release of pregnancy PMN was examined. Isolated peripheral blood PMN from pregnant subjects were incubated (5 h, 37°C) in either heat-inactivated (56°C, 30 min) autologous serum or heat-inactivated pooled nonpregnancy sera (n = 6). The data are expressed as mean ± SEM for seven different PMN donors. The results were significantly different (P values) at the following levels: *, <0.05; **, <0.03. Significance was determined with the Wilcoxon rank sum test. RLU, relative light units.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

PMN play an important role in host defense against infectious agents; paradoxically, however, their "unrestricted" activationhas also been implicated in the pathology of a variety of inflammatoryconditions, such as RA. Activated PMN generate superoxide anions,an initial step leading to the formation of a variety of reactiveoxygen species that have both microbicidal and proinflammatoryproperties. The formation of reactive oxygen species requiresthe correct assembly of a membrane-associated, multicomponentNADPH oxidase system. We have previously investigated the activityof this enzyme complex in PMN isolated from pregnant subjectsand have shown a reduction in its activity compared to that innonpregnant controls; furthermore, we have shown that this reductionparallels the symptomatic relief seen in pregnant RA patients(11). To further investigate the biochemical mechanisms underlyingthis observation, we have examined the effect of pregnancy uponthe activation of PLA₂ in humanPMN.

PLA₂ catalyzes the hydrolysis of the ester bond between a fatty acid and the hydroxyl group at the sn-2 position of the glycerolbackbone of a phospholipid. Although other pathways have beensuggested to cause the release of AA from intact cells, PLA₂ isstill considered to be the dominant, rate-limiting step in theformation of AA from membrane phospholipids. In human PMN, exogenouslyadded AA has been shown to induce Ca²⁺ influx (23), degranulation (2), leukotriene synthesis (29),and NADPH oxidase activation (12). AA formed as a result ofPLA₂ activation also serves as the substrate for both lipoxygenaseand cyclooxygenase enzymes, whose action leads to the generationof a group of proinflammatory lipids termed the eicosanoids. InPMN, the main products of this "AA cascade" are LTB₄, the 5-lipoxygenaseproduct of AA, and platelet-activating factor (PAF), resultingfrom the liberation of AA from phosphotidylcholine. Both PAF andLTB₄ can act in an autocrine manner to activate or prime the PMNNADPH oxidase system (14).

We have demonstrated a reduction in the activity of PLA₂ in PMN isolated from pregnant subjects. This attenuated responseis seen following direct stimulation of cells with fMLP and inPMN that have first been primed with TNF- $alpha$ or IL-8. To supportthe concept of reduced AA liberation by these cells, we have alsomeasured their ability to generate LTB₄ and have found that theproduction of this eicosanoid in pregnant subjects is likewisereduced. These two observations, which coincided with a previouslyreported reduction in PMN PAF production (3), may partiallyexplain the parallel reduction in NADPH oxidase activity in pregnancycells. However, whether this decrease in oxidase activity resultsfrom a reduction in LTB₄ generation or more directly from an attenuationof AA release is notknown.

Several lines of investigation have suggested that changes in the phospholipid and fatty acid compositions of PMN plasma membranescan modulate the function of NADPH oxidase (10, 25). Withthis in mind, we have examined the relative amounts of major fattyacids in the sera and PMN of both nonpregnant and pregnant subjects.The variations in the amounts of all forms of fatty acids betweenthe groups would suggest that profound changes in cellular phospholipidmetabolism occur during pregnancy. Of the observed differences,the most important with respect to NADPH oxidase activity appearsto be a decrease in the levels of PUFA, more specifically, AA(4). Flesch and Ferber (18) have shown that the incorporationof PUFA into the phospholipids of macrophages is accompanied byan increase in PLA₂ activity and superoxide anion generation.Conversely, it can be envisaged that a reduction in PUFA wouldreduce NADPH oxidase activity in PMN. Indeed, the PMN in thisstudy showed a strong relationship between modified PUFA levelsand NADPH oxidase activity both through individual fatty acidincorporations and through crossover serumincubations.

Although there is little doubt as to the importance of PUFA in both the activation and the maintenance of NADPH oxidase inhuman PMN, the possibility that changes in the fatty acid contentmay have more far-reaching effects upon PMN function cannot bedisregarded. It has recently been established that compounds thatreadily affect membrane fluidity in PMN also affect oxidase activity(16, 25). Furthermore, since the fluidity of membranes isknown to be influenced by the degree of saturation or unsaturationand/or hydrocarbon chain length of fatty acids, it seems reasonableto assume that the pregnancy-induced fatty acid changes that wehave reported will alter PMN membrane fluidity. The fluidity ofthe plasma membrane may affect oxidase activity in a number ofways: (i) by the manner in which the multicomponent NADPH oxidaseis arranged within the lipid bilayer or (ii) by the extent ofexpression and affinity of membrane-bound receptors. This latterexplanation seems unlikely, since LTB₄ generation was reducedin PMN from pregnant subjects not only in response to fMLP butalso in response to PMA, an agent that bypasses receptor-mediatedsignalling events by directly activating protein kinaseC.

The results of this study indicate a strong relationship between serum fatty acid levels and cellular fatty acid content.To put these observations into perspective and to establish arationale for changes in pregnancy, a closer examination of thebiosynthetic pathways of fatty acids is necessary. In human PMN,a deficiency exists in the stepwise elongation of short-chainfatty acids. In vivo and in vitro studies suggest that althoughelongase activity in PMN is normal, the cells specifically lackthe $Delta$ 5-desaturase enzyme necessary for long-chain PUFA biosynthesis(8). Given this information, serum levels of fatty acids mayhave a direct influence on cellular fatty acids which lie upstreamof those involved in this reaction. The findings of this study,showing an association between serum and cellular AA, would supportthis proposal, while further changes in pregnancy would causean exaggeration of this effect. For AA, a deficiency in $Delta$ 5-desaturasewould promote the cellular accumulation of its precursor, linoleicacid. This suggestion directly corresponds with our observationsfor cellular fatty acid content in pregnancy and accounts forthe discrepancy between PMN increases and serum decreases in linoleicacid.

The correlation between the relative amounts of the individual essential fatty acids (EFA) in maternal and umbilical plasmaphospholipids highlights a dependence of the growing fetus onmaternal sources of EFA (22). This relationship is particularlytrue with respect to AA and docasahexanoic acid, the major structuraland functional fatty acids involved in the development of thehuman brain and vascular and central nervous systems. In thisstudy we have demonstrated a decline in serum maternal EFA (linoleicacid, AA) levels in the latter stages of pregnancy. Others haveshown a progressive loss of these particular fatty acids throughoutpregnancy, with a more pronounced reduction in the third trimester,when fetal brain development is maximal (37). This pattern ofincreased burden on the essential PUFA from maternal sources wouldfit with our progressive reduction in PMN activity in pregnancyand would also parallel the progressive improvement in the symptomsof pregnant RApatients.

Extensive studies in the late 1970s and 1980s have strongly suggested the presence in the circulation of pregnant women ofan immunomodulating factor(s) which is capable of modifying PMNfunction. Pregnancy PMN have been shown to exhibit reduced chemotaxis(24), microbial killing (15), and adherence to nylon wool(5), while pregnancy serum has been demonstrated to suppressPMN phagocytosis and killing of Staphylococcus aureus (34) andEscherichia coli (33). A number of factors produced by boththe placenta and maternal tissues, including cortisol (32),progesterone, and pregnancy-associated $alpha$ ₂-glycoprotein (30),have been suggested to explain these effects. However, to dateno single factor can satisfactorily explain the pattern of improvementand relapse in inflammatory diseases during pregnancy. We believethat while efforts in the past have concentrated on the identificationof a particular factor during pregnancy, one important mechanismof cell modulation has been neglected. This study has fosteredthe idea that an alteration in the fatty acid metabolism of PMNand perhaps other cells of the immune system allows pregnancy-inducedchanges in the circulating levels of fatty acids to have a directbearing on their inflammatoryresponsiveness.

	FOOTNOTES

^* Corresponding author. Mailing address: Medical Research Centre, Nottingham City Hospital NHS Trust, Hucknall Rd., NottinghamNG5 1PB, United Kingdom. Phone: 44 (0) 115 9858354, ext. 46509.Fax: 44 (0) 115 9858864. E-mail: Ian.Crocker{at}pmfmrc.nottingham.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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6. Boyum, A. 1968. Isolation of mononuclear cells and granulocytes from human blood. Scand. J. Clin. Lab. Investig. 21:77-89[Medline].

7. Brabin, B. J. 1985. Epidemiology of infection in pregnancy. Rev. Infect. Dis. 7:579-603[Medline].

8. Chilton-Lopez, T., M. E. Surette, D. D. Swan, A. N. Fonteh, M. M. Johnson, and F. H. Chilton. 1996. Metabolism of gammalinolenic acid in human neutrophils. J. Immunol. 156:2941-2947[Abstract].

9. Cockcroft, S., and J. Stutchfield. 1989. The receptors for ATP and f-MetLeuPhe are independently coupled to phospholipase C and A₂ via G-proteins. Biochem. J. 263:715-723[Medline].

10. Corey, S. J., and P. M. Rossoff. 1991. Unsaturated fatty acids and lipoxygenase products regulate phagocytic NADPH oxidase activity by a non-detergent mechanism. J. Lab. Clin. Med. 118:343-351[Medline].

11. Crouch, S. P. M., I. P. Crocker, and J. Fletcher. 1995. The effect of pregnancy on polymorphonuclear leukocyte function. J. Immunol. 155:5436-5443[Abstract].

12. Dana, R., H. L. Malech, and R. Levy. 1994. The requirement for phospholipase A₂ for activation of the assembled NADPH oxidase in human neutrophils. Biochem. J. 297:217-233.

13. Da Silva, J. A. P., and T. D. Spector. 1992. The role of pregnancy in the course and etiology of rheumatoid arthritis. Clin. Rheumatol. 11:189-194[Medline].

14. Dewald, B., and M. Baggiolini. 1985. Activation of NADPH oxidase in human neutrophils. Synergism between fMLP and the neutrophil products PAF and LTB₄. Biochem. Biophys. Res. Commun. 128:297-304[Medline].

15. El-Maallem, H., and J. Fletcher. 1980. Impaired neutrophil function and myeloperoxidase deficiency in pregnancy. Br. J. Haematol. 44:375-381[Medline].

16. Ferrante, A., K. Carman, M. Nandoskar, A. McPhee, and A. Poulos. 1996. Cord-blood neutrophil responses to polyunsaturated fatty-acids $---$ effects on degranulation and oxidative respiratory burst. Biol. Neonate 69:368-375[Medline].

17. Finn, R., C. A. St. Hill, and A. J. Govan. 1972. Immunologic response in pregnancy and survival of the fetal homograft. Br. Med. J. 3:150-152.

18. Flesch, I., and E. Ferber. 1986. Effect of cellular fatty acid composition on the phospholipase A₂ activity of bone-marrow derived macrophages and their ability to induce lucigenin-dependent chemiluminescence. Biochim. Biophys. Acta 889:6-14[Medline].

19. Gyllenhammer, H. 1987. Lucigenin chemiluminescence in the assessment of neutrophil superoxide anion production. J. Immunol. Methods 97:209-213[Medline].

20. Hempel, K. H., L. A. Fernandez, and R. H. Persellin. 1970. Effect of pregnancy sera on isolated lysosomes. Nature 225:955-957[Medline].

21. Hench, P. S. 1938. The ameliorating effect of pregnancy on chronic atrophic (infectious rheumatoid) arthritis, fibrositis, and intermittent hydrarthrosis. Proc. Staff Meet. Mayo Clin. 13:161-167.

22. Hornstra, G. 1995. Essential fatty acids in pregnancy and early human development. Eur. J. Obstet. Gynecol. Reprod. Biol. 61:57-62[Medline].

23. Jacobson, P. B., and D. J. Schier. 1993. Regulation of CD11b/CD18 expression in human neutrophils by PLA₂. J. Immunol. 151:5639-5652[Abstract].

24. Krause, P. J., C. J. Ingardia, L. T. Pontius, H. L. Malech, T. M. Lobello, and E. G. Maderazo. 1987. Host defense during pregnancy: neutrophil chemotaxis and adherence. Am. J. Obstet. Gynecol. 157:274-280[Medline].

25. Kusner, D. J., J. N. Aucott, D. Franceshi, M. M. Sarasua, P. J. Spagnuolo, and C. H. King. 1991. Protease priming of neutrophil superoxide production. J. Biol. Chem. 266:16465-16471[Abstract/Free Full Text].

26. Lepage, G., and C. C. Roy. 1986. Direct transesterification of all classes of lipids in a one-step reaction. Lipid Res. 27:114-120[Abstract].

27. Luft, B. J., and J. S. Remington. 1982. Effect of pregnancy on resistance to Listeria monocytogenes and Toxoplasma gondii infections in mice. Infect. Immun. 38:1164-1171[Abstract/Free Full Text].

28. Mahoney, E. M., A. L. Hamill, W. A. Scott, and Z. A. Cohn. 1977. Response of endocytosis to altered fatty acyl composition of macrophage phospholipids. Proc. Natl. Acad. Sci. USA 74:4895-4899[Abstract/Free Full Text].

29. Marshal, L. A., J. D. Winkler, D. E. Grinswold, B. Bolognese, A. Rishar, C.-M. Sung, E. F. Webb, and R. Jacobs. 1994. Effects of Scalaradial, a type II phospholipase A₂ inhibitor on human neutrophil AA mobilisation and lipid mediator formation. J. Pharmacol. Exp. Ther. 268:709-717[Abstract/Free Full Text].

30. Nolten, W. E., and P. A. Rueckert. 1981. Elevated free cortisol index in pregnancy; possible regulatory mechanisms. Am. J. Obstet. Gynecol. 139:492-498[Medline].

31. Persellin, R. H. 1977. The effect of pregnancy on rheumatoid arthritis. Bull. Rheum. Dis. 27:922-927.

32. Persellin, R. H. 1981. Inhibitors of inflammatory and immune responses in pregnancy serum. Clin. Rheum. Dis. 7:769-780.

33. Persellin, R. H., and J. K. Leibfarth. 1978. Studies of the effects of pregnancy serum on polymorphonuclear leukocyte functions. Arthritis Rheum. 21:316-325[Medline].

34. Persellin, R. H., and L. L. Thoi. 1979. Human polymorphonuclear leukocyte phagocytosis in pregnancy: development of inhibition during gestation and recovery in the post partum period. Am. J. Obstet. Gynecol. 134:250-255[Medline].

35. Qian, M. W., and J. W. Eaton. 1994. Free fatty-acids enhance hypochlorous acid production by activated neutrophils. J. Lab. Clin. Med. 124:86-95[Medline].

36. Reinhardt, M. C. 1980. Effects of parasitic infections in pregnant women. Ciba Found. Symp. 77:149-159.

37. Sanjurjo, P., R. Matorras, N. Ingunza, M. Alonso, J. Rodriguez-Alarcon, and L. Perteagudo. 1993. Cross sectional study of percentual changes in total plasmatic fatty acids during pregnancy. Horm. Metab. Res. 25:590-592[Medline].

38. Serhan, C. N., A. Radin, J. E. Smolen, H. Korchak, B. Samuelson, and G. Weissmann. 1982. LTB₄ is a complete secretagogue in human neutrophils: a kinetic analysis. Biochem. Biophys. Res. Commun. 107:1006-1012[Medline].

39. Spector, T. D., and J. A. P. Da Silva. 1992. Pregnancy and rheumatoid arthritis: an overview. Am. J. Reprod. Immunol. 28:222-225.

40. Taylor, A. J., H. Pandov, and N. Lawson. 1998. Determination of erythrocyte fatty acids by capillary gas liquid chromatography. Ann. Clin. Biochem. 24:293-296.

This article has been cited by other articles:

Crocker, I, Lawson, N, Fletcher, J (2002). Effect of pregnancy and obstructive jaundice on inflammatory diseases: the work of P S Hench revisited. Ann Rheum Dis 61: 307-310 [Abstract] [Full Text]
Crocker, I.P., Lawson, N., Baker, P.N., Fletcher, J. (2001). The anti-inflammatory effects of circulating fatty acids in obstructive jaundice: similarities with pregnancy-induced immunosuppression. QJM 94: 475-484 [Abstract] [Full Text]

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Antimicrob. Agents Chemother.	Clin. Microbiol. Rev.	Infect. Immun.
J. Clin. Microbiol.	J. Virol.	ALL ASM JOURNALS

1.	Andresen, R. H., and G. W. Monroe. 1962. Experimental study of the behavior of adult human skin homografts during pregnancy. Am. J. Obstet. Gynecol. 84:1096-1103.
2.	Barnette, M. S., J. Rush, L. A. Marshall, J. J. Foley, D. B. Schmidt, and H. M. Sarau. 1994. Effects of Scalaradial, a novel inhibitor of 14KDa phospholipase A₂ on human neutrophil function. Biochem. Pharmacol. 47:1661-1668[Medline].
3.	Beilin, L. J., K. D. Croft, C. A. Michael, J. Ritchie, L. Schmidt, R. Vandongen, and B. N. J. Walter. 1993. Neutrophil platelet activating factor in normal and hypertensive pregnancy and in pregnancy-induced hypertension. Clin. Sci. 85:63-70[Medline].
4.	Bellavite, P., P. Guarini, D. Biasi, A. Carletto, M. T. Trevisan, P. Caramaschi, L. M. Bambara, and R. Corrocher. 1995. Correlations between the intensity of fMLP-dependent respiratory burst and cellular fatty acid composition in human neutrophils. Br. J. Haematol. 89:271-276[Medline].
5.	Bjorksten, B., T. Soderstrom, M.-G. Damber, B. Von Schoultz, and T. Stigbrand. 1978. Polymorphonuclear leucocyte function during pregnancy. Scand. J. Immunol. 8:257-262[Medline].
6.	Boyum, A. 1968. Isolation of mononuclear cells and granulocytes from human blood. Scand. J. Clin. Lab. Investig. 21:77-89[Medline].
7.	Brabin, B. J. 1985. Epidemiology of infection in pregnancy. Rev. Infect. Dis. 7:579-603[Medline].
8.	Chilton-Lopez, T., M. E. Surette, D. D. Swan, A. N. Fonteh, M. M. Johnson, and F. H. Chilton. 1996. Metabolism of gammalinolenic acid in human neutrophils. J. Immunol. 156:2941-2947[Abstract].
9.	Cockcroft, S., and J. Stutchfield. 1989. The receptors for ATP and f-MetLeuPhe are independently coupled to phospholipase C and A₂ via G-proteins. Biochem. J. 263:715-723[Medline].
10.	Corey, S. J., and P. M. Rossoff. 1991. Unsaturated fatty acids and lipoxygenase products regulate phagocytic NADPH oxidase activity by a non-detergent mechanism. J. Lab. Clin. Med. 118:343-351[Medline].
11.	Crouch, S. P. M., I. P. Crocker, and J. Fletcher. 1995. The effect of pregnancy on polymorphonuclear leukocyte function. J. Immunol. 155:5436-5443[Abstract].
12.	Dana, R., H. L. Malech, and R. Levy. 1994. The requirement for phospholipase A₂ for activation of the assembled NADPH oxidase in human neutrophils. Biochem. J. 297:217-233.
13.	Da Silva, J. A. P., and T. D. Spector. 1992. The role of pregnancy in the course and etiology of rheumatoid arthritis. Clin. Rheumatol. 11:189-194[Medline].
14.	Dewald, B., and M. Baggiolini. 1985. Activation of NADPH oxidase in human neutrophils. Synergism between fMLP and the neutrophil products PAF and LTB₄. Biochem. Biophys. Res. Commun. 128:297-304[Medline].
15.	El-Maallem, H., and J. Fletcher. 1980. Impaired neutrophil function and myeloperoxidase deficiency in pregnancy. Br. J. Haematol. 44:375-381[Medline].
16.	Ferrante, A., K. Carman, M. Nandoskar, A. McPhee, and A. Poulos. 1996. Cord-blood neutrophil responses to polyunsaturated fatty-acids $---$ effects on degranulation and oxidative respiratory burst. Biol. Neonate 69:368-375[Medline].
17.	Finn, R., C. A. St. Hill, and A. J. Govan. 1972. Immunologic response in pregnancy and survival of the fetal homograft. Br. Med. J. 3:150-152.
18.	Flesch, I., and E. Ferber. 1986. Effect of cellular fatty acid composition on the phospholipase A₂ activity of bone-marrow derived macrophages and their ability to induce lucigenin-dependent chemiluminescence. Biochim. Biophys. Acta 889:6-14[Medline].
19.	Gyllenhammer, H. 1987. Lucigenin chemiluminescence in the assessment of neutrophil superoxide anion production. J. Immunol. Methods 97:209-213[Medline].
20.	Hempel, K. H., L. A. Fernandez, and R. H. Persellin. 1970. Effect of pregnancy sera on isolated lysosomes. Nature 225:955-957[Medline].
21.	Hench, P. S. 1938. The ameliorating effect of pregnancy on chronic atrophic (infectious rheumatoid) arthritis, fibrositis, and intermittent hydrarthrosis. Proc. Staff Meet. Mayo Clin. 13:161-167.
22.	Hornstra, G. 1995. Essential fatty acids in pregnancy and early human development. Eur. J. Obstet. Gynecol. Reprod. Biol. 61:57-62[Medline].
23.	Jacobson, P. B., and D. J. Schier. 1993. Regulation of CD11b/CD18 expression in human neutrophils by PLA₂. J. Immunol. 151:5639-5652[Abstract].
24.	Krause, P. J., C. J. Ingardia, L. T. Pontius, H. L. Malech, T. M. Lobello, and E. G. Maderazo. 1987. Host defense during pregnancy: neutrophil chemotaxis and adherence. Am. J. Obstet. Gynecol. 157:274-280[Medline].
25.	Kusner, D. J., J. N. Aucott, D. Franceshi, M. M. Sarasua, P. J. Spagnuolo, and C. H. King. 1991. Protease priming of neutrophil superoxide production. J. Biol. Chem. 266:16465-16471[Abstract/Free Full Text].
26.	Lepage, G., and C. C. Roy. 1986. Direct transesterification of all classes of lipids in a one-step reaction. Lipid Res. 27:114-120[Abstract].
27.	Luft, B. J., and J. S. Remington. 1982. Effect of pregnancy on resistance to Listeria monocytogenes and Toxoplasma gondii infections in mice. Infect. Immun. 38:1164-1171[Abstract/Free Full Text].
28.	Mahoney, E. M., A. L. Hamill, W. A. Scott, and Z. A. Cohn. 1977. Response of endocytosis to altered fatty acyl composition of macrophage phospholipids. Proc. Natl. Acad. Sci. USA 74:4895-4899[Abstract/Free Full Text].
29.	Marshal, L. A., J. D. Winkler, D. E. Grinswold, B. Bolognese, A. Rishar, C.-M. Sung, E. F. Webb, and R. Jacobs. 1994. Effects of Scalaradial, a type II phospholipase A₂ inhibitor on human neutrophil AA mobilisation and lipid mediator formation. J. Pharmacol. Exp. Ther. 268:709-717[Abstract/Free Full Text].
30.	Nolten, W. E., and P. A. Rueckert. 1981. Elevated free cortisol index in pregnancy; possible regulatory mechanisms. Am. J. Obstet. Gynecol. 139:492-498[Medline].
31.	Persellin, R. H. 1977. The effect of pregnancy on rheumatoid arthritis. Bull. Rheum. Dis. 27:922-927.
32.	Persellin, R. H. 1981. Inhibitors of inflammatory and immune responses in pregnancy serum. Clin. Rheum. Dis. 7:769-780.
33.	Persellin, R. H., and J. K. Leibfarth. 1978. Studies of the effects of pregnancy serum on polymorphonuclear leukocyte functions. Arthritis Rheum. 21:316-325[Medline].
34.	Persellin, R. H., and L. L. Thoi. 1979. Human polymorphonuclear leukocyte phagocytosis in pregnancy: development of inhibition during gestation and recovery in the post partum period. Am. J. Obstet. Gynecol. 134:250-255[Medline].
35.	Qian, M. W., and J. W. Eaton. 1994. Free fatty-acids enhance hypochlorous acid production by activated neutrophils. J. Lab. Clin. Med. 124:86-95[Medline].
36.	Reinhardt, M. C. 1980. Effects of parasitic infections in pregnant women. Ciba Found. Symp. 77:149-159.
37.	Sanjurjo, P., R. Matorras, N. Ingunza, M. Alonso, J. Rodriguez-Alarcon, and L. Perteagudo. 1993. Cross sectional study of percentual changes in total plasmatic fatty acids during pregnancy. Horm. Metab. Res. 25:590-592[Medline].
38.	Serhan, C. N., A. Radin, J. E. Smolen, H. Korchak, B. Samuelson, and G. Weissmann. 1982. LTB₄ is a complete secretagogue in human neutrophils: a kinetic analysis. Biochem. Biophys. Res. Commun. 107:1006-1012[Medline].
39.	Spector, T. D., and J. A. P. Da Silva. 1992. Pregnancy and rheumatoid arthritis: an overview. Am. J. Reprod. Immunol. 28:222-225.
40.	Taylor, A. J., H. Pandov, and N. Lawson. 1998. Determination of erythrocyte fatty acids by capillary gas liquid chromatography. Ann. Clin. Biochem. 24:293-296.