Tumor necrosis factor (TNF)-alpha  induces leptin production through the p55 TNF receptor

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Tumor necrosis factor (TNF)- $alpha$ induces leptin production through the p55 TNF receptor

Brian N. Finck and Rodney W. Johnson

Laboratory of Integrative Biology, Department of Animal Sciences, University of Illinois, Urbana, Illinois 61801

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Tumor necrosis factor (TNF)- $alpha$ acts directly on adipocytes to increase production of the lipostatic factor, leptin. However,which TNF receptor (TNFR) mediates this response is not known.To answer this question, leptin was measured in plasma of wild-type(WT), p55, and p75 TNFR knockout (KO) mice injected intraperitoneallywith murine TNF- $alpha$ and in supernatants from cultured WT, p55, andp75 TNFR KO adipocytes incubated with TNF- $alpha$ . Leptin also was measuredin supernatants from C3H/HeOuJ mouse adipocytes cultured withblocking antibodies to each TNFR and TNF- $alpha$ as well as in supernatantsfrom adipocytes incubated with either human or murine TNF- $alpha$ , whichactivate either one or both TNFR, respectively. The results usingall four strategies show that the induction of leptin productionby TNF- $alpha$ requires activation of the p55 TNFR and that althoughactivation of the p75 TNFR alone cannot cause leptin production,its presence affects the capability of TNF- $alpha$ to induce leptinproduction through the p55 TNFR. These results provide new informationon the interplay between cells of the immune system andadipocytes.

tumor necrosis factor receptor; ob gene; cytokine; adipocytes

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

TUMOR NECROSIS FACTOR (TNF)- $alpha$ induces adipocytes to secrete the lipostatic hormone leptin (11, 14, 17, 26). Becauseleptin reduces food intake (4, 15, 21) and increases energyexpenditure (21), the increased production of leptin in responseto TNF- $alpha$ may be involved in the negative energy balance that iscommon to infectious, autoimmune, and neoplastic diseases. However,the induction of leptin by cytokines may also serve some otherpurpose. For example, mice lacking the secreted form of leptin(ob/ob), in addition to being obese, have severe deficits in Tlymphocyte maturation and cytotoxicity (6). These deficienciesmay be the result of the absence of leptin, because culturingT cells from ob/ob mice with recombinant leptin induced memoryT cell proliferation and cytokine production (19). Recent findingsalso suggest that low plasma leptin levels explain the immunoinsufficienciesof malnourished individuals, because leptin administration correctedstarvation-induced deficits in the immune response in mice (19).Thus the induction of leptin by TNF- $alpha$ may be an important immunologicalresponse. Despite the potential significance of this immune-endocrineinteraction, the cellular signaling pathways involved in the inductionof leptin by TNF- $alpha$ are not yetknown.

Two distinct receptors in the TNF/nerve growth factor receptor superfamily mediate the diverse biological actions of TNF- $alpha$ (7). These two receptors, the murine p55 and p75 TNFR, sharesequence homology in their ligand-binding domains, but their intracellulardomains are dissimilar and thus discrete intracellular signalingpathways are activated by each (7). Accordingly, activationof the p55 receptor elicits biological responses that are distinctfrom those induced by activation of the p75 TNFR (2, 3).Unfortunately, the TNFR on adipocytes that stimulates leptin geneexpression has not yet been defined, which is a necessary firststep to understanding the alliance between TNFR signaling andleptin gene transcription. Therefore, to determine the TNFR activatedby TNF- $alpha$ to induce leptin production, TNFR knockout (KO) mice,antagonistic antibodies to each of the TNFR, and human TNF- $alpha$ ,which binds only the murine p55 TNFR, were employed in a seriesof in vivo and in vitro experiments. The results of this studysuggest that the p55 TNFR is critical for the induction of leptinby TNF- $alpha$ .

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Experimental Animals

Adult female C57BL/6-TNFR1^tm1Mak (p55 TNFR KO), C57BL/6-TNFR2^tm1Mwm (p75 TNFR KO), and C57BL/6J (WT) mice (22-25 g) were purchased fromJackson Laboratories. Adult male C3H/HeOuJ (OuJ) mice (26-32 g)were obtained from a breeding colony maintained at the Universityof Illinois. All mice were housed in groups of three or four inpolypropylene cages under a reverse 12:12-h light-dark cycle (lightson at 2100) with ad libitum access to water and rodent chow. Allhousing conditions and procedures were approved by the Universityof Illinois Laboratory Animal Care AdvisoryCommittee.

Reagents

Recombinant murine and human TNF- $alpha$ were purchased from Pharmingen (San Diego, CA). Whereas murine TNF- $alpha$ had a biological activityof 1 × 10⁸, human TNF- $alpha$ had a biological activity of 1 × 10⁷as measured by the murine L929 cell bioassay. The fact that humanTNF- $alpha$ binds only to the murine p55 receptor (31) may explainthe difference in the activity of these two species of TNF- $alpha$ inthe murine bioassay. Each species of TNF- $alpha$ was certified by Pharmingento contain <0.1 ng endotoxin/1 µg TNF- $alpha$ as assessed by Limulusamoebocyte assay. Bovine insulin was purchased from Sigma Chemical(St. Louis, MO). For injection, murine TNF- $alpha$ was dissolved insterile PBS (Sigma) containing 0.2% BSA. Insulin, murine, andhuman TNF- $alpha$ were dissolved in sterile Krebs-Ringer phosphate (KRP)for use in cell cultureexperiments.

Antagonistic hamster anti-mouse antibodies specific for the p55 or p75 receptor (30) were purchased from Genzyme (Cambridge,MA). Each was certified by the manufacturer to bind specificallyto either the p55 or p75 TNFR, and no cross-reactivity betweenTNFRs or TNF- $alpha$ was reported. An isotype matched control antibodyraised against Schistosoma japonicum glutathione S-transferasewas also purchased from the same source. Antibodies were providedin preservative-free solutions, which were diluted in sterileKRP for use in cell culturesystems.

Measurements

Leptin. Cell supernatant leptin concentration was measured using a commercially available RIA specific for murine leptin (LincoResearch, St. Charles, MO). The assay was conducted as specifiedby the manufacturer except that all reagents were used at one-halfrecommended volume as previously described (11). The sensitivityof the assay was <0.2 ng/ml. The intrassay variation was 5.7%and interassay variation <6.0%.

RNase protection assay. Total cellular RNA was isolated by the TRI-REAGENT (Sigma) method, except an additional centrifugationstep was necessary to remove excessive lipid. RNA integrity wasconfirmed by denaturing agarose gel electrophoresis and RNA concentrationdetermined by spectrophometric absorbency at twodilutions.

Radiolabeled RNA probes were generated by in vitro transcription using the MAXIscript protocol (Ambion, Austin, TX). The cDNAsfor the murine leptin gene (the generous gift of Amgen, ThousandOaks, CA) or 18S rRNA (Ambion) were used as templates to produceUTP- $alpha$ -³²P-labeled anti-sense probes. The full-length leptin and 18S probeswere 560 and 155 bp in length, and protected fragments were 515and 80 bp,respectively.

RNase protection assays (RPA) were performed using the RPA III (Ambion) protocol with minor modification. After gel purification,~1 × 10⁴ counts/min of each probe were hybridized to 15 µg of total cellularRNA from ovarian fat pads in an overnight incubation at 42°C.RNase digestion was performed at 37°C for 30 min and fragmentsprecipitated using RNase inactivation/precipitation solution (Ambion).Protected fragments were then separated using an 8 M urea-5% acrylamidegel. Gels were exposed to Kodak Biomax MR film at $-$ 80°C usingan intensifyingscreen.

Adipocyte Isolation

Adipocytes were isolated as previously described (11). Briefly, mice were euthanized by CO₂ gas asphyxiation at the onsetof the dark phase, when leptin production was anticipated to beat its nadir (12, 26). Gonadal fat pads were excised and mincedinto small pieces, and adipocytes were dissociated by a 35-mincollagenase (1 mg/ml; Sigma) digestion in a 37°C shaking waterbath. The resulting cell suspension was filtered through a 140-µmmesh screen to remove any remaining tissue. Cells were then washedfour times by centrifugation (500 g) in KRP containing 2 mg/mldextrose (Sigma) and 33 mg/ml BSA (Fraction V; cell culture grade;Sigma) to remove contaminating cells. Adipocytes were counted,adjusted to 2 × 10⁶ cells/ml, and then plated in 0.5 ml of KRP in 24-wellplates.

Experimental Procedure

Effect of murine TNF- $alpha$ on leptin in TNFR KO mice. At the onset of the dark phase, after fasting 12 h to reduce circulatingleptin levels, adult WT, p55, and p75 KO mice were injected intraperitoneallywith 0.25 ml vehicle (PBS with 0.2% BSA) or vehicle containing500 ng recombinant murine TNF- $alpha$ . At 8 h postinjection, mice wereeuthanized by CO₂ gas asphyxiation, and ovarian fat pads wereremoved and quickly frozen in liquid nitrogen for later measurementof leptin mRNA. A blood sample from the inferior vena cava ofeach mouse was collected into an EDTA-coated syringe, and plasmaleptin content was later determined by RIA. A total of 36 micewas used in two separate but identical trials (n =6).

Effect of TNF- $alpha$ on leptin production by adipocytes from TNFR KO mice. Adipocytes isolated from WT, p55, or p75 receptor KOmice were cultured in the presence of insulin (300 ng/ml) or murineTNF- $alpha$ (0, 1, 10, 100 ng/ml; n = 8). After 8 h of culture in thepresence of TNF- $alpha$ or insulin, cell-free supernatants were removedand stored frozen ( $-$ 80°C) until assayed for leptinconcentration.

Effect of antagonistic anti-TNFR antibodies on TNF- $alpha$ -induced leptin production. Adipocytes were isolated from OuJ mice asabove. The OuJ mouse strain was used in this study because theypossess large fat stores at maturity and have previously beenused to determine the effects of TNF- $alpha$ on leptin production (11).Adipocytes were cultured in KRP alone or in KRP containing anti-p55antibody (10 µg/ml), anti-p75 antibody (10 µg/ml), or isotypiccontrol antibody (10 µg/ml) in the presence or absence of murineTNF- $alpha$ (100 ng/ml; n = 6) for 8 h. In a separate experiment, insulin(300 ng/ml; n = 6) was used in place of TNF- $alpha$ . Supernatants wereremoved after 8 h and assayed for leptin concentration. The doseof antibody employed in this study was in accordance to Genzyme'srecommended concentration for inhibition of ligandbinding.

Comparison of murine and human TNF- $alpha$ . Adipocytes isolated from OuJ mice were cultured in the presence of murine or human TNF- $alpha$ (0, 1, 10, 100 ng/ml; n = 12). As assessed by Pharmingen usingthe murine L929 cell-line bioassay, there was a 10-fold differencein the activity of these two species of cytokine. Because therelative difference in activity of these two species of TNF- $alpha$ could be explained by the use of the murine bioassay to determinebioactivity, they were employed in equimolar concentrations forcomparison of effect on leptin production. Supernatants were collectedafter 8 h of culture and stored at $-$ 80°C until assayed for leptincontent.

Statistical Analysis

All data were analyzed using general linear model procedures (27). Data were subjected to one- or two-way ANOVA to determinethe significance of main factors and main factor interactions.When ANOVA revealed a significant effect of a main factor or aninteraction between main factors, differences between treatmentmeans were tested using least squares difference. All data arepresented as means ±SE.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

TNF- $alpha$ induces leptin production in p75 but not p55 TNFR KO mice. Intraperitoneal injection of TNF- $alpha$ in WT mice has been shownto increase leptin mRNA in adipose tissue (14, 26) and increasecirculating leptin levels (11, 14, 17, 26). To determinewhich TNFR is involved, following an overnight fast, WT, p55,and p75 KO mice were injected with vehicle or 500 ng of recombinantmurine TNF- $alpha$ . Eight hours later, fat pads and blood plasma werecollected for determination of leptin mRNA and protein, respectively.As expected, TNF- $alpha$ significantly increased plasma leptin and leptinmRNA levels in WT mice (Fig. 1). However, p55 KO mice were completelyresistant to this effect of TNF- $alpha$ , suggesting that TNF- $alpha$ inducesleptin by activating the p55 receptor. Consistent with this hypothesis,TNF- $alpha$ significantly increased plasma leptin and leptin mRNA levelsin p75 KO mice. In fact, mice that lacked the p75 receptor werehypersensitive to the induction of leptin by TNF- $alpha$ , possibly becausethey had less circulating soluble TNFR (22) to neutralize TNF- $alpha$ .

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Fig. 1. Effect tumor necrosis factor (TNF)- $alpha$ on plasma leptin protein concentration and fat pad mRNA expression in TNF receptor (TNFR) knockout (KO) mice. After an overnight fast, wild-type (WT), p55, and p75 KO mice were injected with vehicle or recombinant murine TNF- $alpha$ (500 ng/mouse; n = 6). Eight hours later, blood and ovarian fat pads were collected. Values are means ± SE. Groups denoted with different letters are significantly different at P < 0.05. A: plasma leptin concentrations as determined by RIA. B: ovarian fad pad leptin mRNA levels expressed as a percentage of 18S rRNA as determined by RNase protection assay (n = 3). C: representative RNase protection assay for leptin and 18S RNA. Leptin and 18S rRNA protected fragments are 515 and 80 bp, respectively.

Adipocytes from p55 TNFR KO mice do not secrete leptin in response to TNF- $alpha$ . The previous experiment suggested that TNF- $alpha$ activated the p55 receptor to induce leptin production. To morecarefully evaluate this, adipocytes from WT, p55, or p75 KO micewere isolated and cultured in the presence of increasing concentrationsof murine TNF- $alpha$ . Consistent with a previous report (11), TNF- $alpha$ increased supernatant leptin content in a dose-dependent fashionin cultures of adipocytes from WT mice (Fig. 2). Conversely, adipocytesfrom p55 KO mice did not secrete higher amounts of leptin in responseto TNF- $alpha$ . Murine TNF- $alpha$ increased supernatant leptin levels incultures from p75 KO mice, but the magnitude of increase was lessthan that of cultures from WT mice.

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Fig. 2. Effect of TNF- $alpha$ on leptin production by adipocytes from WT, p55, and p75 TNFR KO mice in vitro. Adipocytes from WT, p55, or p75 KO mice were cultured for 8 h in presence insulin (300 ng/ml) or TNF- $alpha$ (0, 1, 10, 100 ng/ml; n = 8). Values are means ± SE. Groups denoted with different letters are significantly different at P < 0.05.

As a positive control, adipocytes of each genotype were also cultured in the presence of insulin (300 ng/ml). A twofold increasein supernatant leptin concentration was induced by insulin inall three strains of adipocytes (Fig. 2). The fact that the absenceof either TNFR did not affect insulin-induced leptin productionindicates that adipocytes from KO mice have retained the abilityto synthesize and secrete leptin and that the lack of sensitivityto TNF- $alpha$ is more likely due to the absence of the TNFR, not anonspecific cellulardefect.

Antagonistic antibodies to either TNFR attenuate TNF- $alpha$ -induced leptin production. Adipocytes from OuJ mice were cultured inmedium alone, medium containing anti-p55 antibody, anti-p75 antibody,or an isotypic control antibody in the presence or absence ofmurine TNF- $alpha$ or insulin for 8 h. Supernatants were then removedand assayed for leptin concentration. As expected, TNF- $alpha$ alonedramatically increased supernatant leptin concentration. However,culturing adipocytes with antagonistic anti-p55 TNFR antibodiescompletely prevented this effect of TNF- $alpha$ (Fig. 3). Treatmentwith the isotype control antibody had no effect on TNF- $alpha$ -inducedleptin production. Furthermore, the p55 antibody did not bluntproduction of leptin in response to insulin (Table 1).

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Fig. 3. Effect of antagonistic antibodies to p55 TNFR on induction of leptin by TNF- $alpha$ in vitro. Adipocytes from OuJ mice were cultured in medium alone, medium containing anti-p55 antibody (p55), or an isotypic (Iso) control antibody in presence or absence of murine TNF- $alpha$ (100 ng/ml) for 8 h (n = 6). Values are means ± SE. Groups denoted with different letters are significantly different at P < 0.05.

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Table 1. Antibodies to the p55 and p75 TNFR do not block insulin-induced leptin production by C3H/HeOuJ mouse adipocytes

As evident in Fig. 4, culture with p75 antibody partially blocked the induction of leptin by TNF- $alpha$ . Supernatant leptin concentrationsin cultures exposed to p75 antibody and TNF- $alpha$ , though higher thanlevels in control cultures, were lower than those subjected toTNF- $alpha$ alone. Culturing cells in the presence of the isotype controlantibody again did not inhibit TNF- $alpha$ -induced leptin production.In addition, the use of p75 antibodies did not interfere withinsulin-induced leptin production (Table 1).

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Fig. 4. Effect of antagonistic antibodies to p75 TNFR on induction of leptin by TNF- $alpha$ in vitro. Adipocytes from OuJ mice were cultured in medium alone, medium containing anti-p75 antibody (p75), or an isotypic control antibody in presence or absence of murine TNF- $alpha$ (100 ng/ml) for 8 h (n = 6). Values are means ± SE. Groups denoted with different letters are significantly different at P < 0.05.

Murine TNF- $alpha$ is more potent at inducing leptin production than human TNF- $alpha$ . To evaluate further the role of each TNFR in theinduction of leptin by TNF- $alpha$ , primary adipocytes from OuJ micewere cultured in the presence of human TNF- $alpha$ , which selectivelybinds the p55 TNFR (31), and murine TNF- $alpha$ , which binds bothreceptors. Although both species of TNF- $alpha$ increased supernatantleptin content in a dose-dependent manner, murine TNF- $alpha$ was significantlymore potent at inducing leptin production (Table 2). This againis consistent with the idea that the p55 receptor is criticalto the induction of leptin by TNF- $alpha$ , but also that p75 costimulationsomehow enhances this effect.

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Table 2. Human and murine TNF- $alpha$ differentially affect leptin production by C3H/HeOuJ mouse adipocytes

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

TNF- $alpha$ has been shown to act directly on adipocytes to induce the production of leptin (11, 14, 17, 26), but untilnow the TNFR that mediates this response was not known. In thepresent study, we measured leptin in 1) plasma of WT, p55, andp75 TNFR KO mice after intraperitoneal injection of murine TNF- $alpha$ ;2) supernatants from cultured WT, p55, and p75 TNFR KO adipocytesthat had been incubated with TNF- $alpha$ ; 3) supernatants from culturedOuJ mouse adipocytes that had been incubated with blocking antibodiesto the p55 and p75 TNFR and with TNF- $alpha$ ; and 4) supernatants fromcultured OuJ adipocytes incubated with either human or murineTNF- $alpha$ that bind either one or both TNFR, respectively. The resultsusing all four strategies show that the induction of leptin geneexpression and production by TNF- $alpha$ requires activation of thep55 receptor and that although activation of the p75 TNFR alonecannot cause leptin production, its presence affects the capabilityof TNF- $alpha$ to induce leptin production through the p55receptor.

The fact that the p55 TNFR was essential for TNF- $alpha$ to stimulate leptin production was evident in the first study where WT,p55, and p75 KO mice were injected intraperitoneally with TNF- $alpha$ .Whereas WT mice showed a marked elevation in plasma leptin andleptin mRNA accumulation after injection of TNF- $alpha$ , mice lackingthe p55 TNFR were entirely refractory to these effects of TNF- $alpha$ .It should be noted that in the present study, leptin was measuredat 8 h only. This point in time was chosen because previous workof this lab found that plasma leptin was still maximally elevated8 h after inflammatory challenge (11). Nonetheless, it is possiblein the present study that the absence of the p55 TNFR alteredthe kinetics of leptin production. Because leptin was only measured8 h postinjection, it may be that leptin production was elevatedearly on, but had already declined. However, adipocytes from p55KO were completely refractory to TNF- $alpha$ -induced increases in theaccumulation of leptin in the culture medium, arguing againstthatpossibility.

In contrast to p55 TNF KO mice, mice lacking p75 TNFR were hyperresponsive to the effects of TNF- $alpha$ on leptin production andleptin mRNA expression compared with WT controls. The findingthat p75 KO mice exhibited an exacerbated response to TNF- $alpha$ iscomparable with other studies (22) and may be explained by theabsence of soluble p75 TNFR (sTNFR). On TNF- $alpha$ treatment, a significantnumber of p55 and p75 TNFR are shed from the cell membrane ofleukocytes to become soluble receptors that compete with membrane-boundTNFR for available ligand (1). Although both types of solubleTNFR can inhibit the effects of TNF- $alpha$ , p75 sTNFR appears to bethe major form of this receptor in circulation (1, 23). BecauseTNF- $alpha$ levels had most likely returned to baseline by 8 h postinjection(22), plasma cytokine concentration was not assessed in thecurrent study. However, there is at least one previous reportthat lipopolysaccharide (LPS)-stimulated plasma TNF- $alpha$ levels aresignificantly greater in TNFR KO mice than in WT controls (22).Thus in the present study, the hypersensitivity of p75 KO miceto the induction of leptin could be due to high levels of bioactiveTNF- $alpha$ that act through intact p55 receptors found onadipocytes.

To eliminate potentially confounding factors such as the presence or absence of sTNFR, which are reportedly liberated fromleukocytes (1, 23), an adipocyte primary culture system wasused in subsequent studies. Consistent with what was observedin vivo, studies employing blocking antibodies or primary culturesof adipocytes from p55 TNFR KO mice showed that the p55 TNFR isnecessary for the increased leptin production induced by TNF- $alpha$ .However, whereas the absence of the p75 TNFR resulted in hypersensitivityto this effect of TNF- $alpha$ in vivo, all three in vitro approaches(i.e., blocking antibodies, adipocytes from KO mice, and humanTNF- $alpha$ ) revealed that the induction of leptin by TNF- $alpha$ was partiallyabrogated by the absence or blockade of the p75 receptor. Thissuggests that the p75 TNFR somehow cooperates with the p55 TNFRto enhance TNF- $alpha$ -induced leptin production. This concept of TNFRcooperativity has been reported for several other biological effectsof TNF- $alpha$ . For instance, whereas p55 TNFR KOs failed to produceIL-6 in response to TNF- $alpha$ (2, 20), the absence of p75 receptorcostimulation markedly reduced the production of IL-6. Likewise,concomitant stimulation of the p75 receptor enhanced p55-mediatedcytotoxicity (3, 32), apoptosis (8), and nitric oxideproduction (24).

It is not yet clear how TNF receptors interact to enhance the actions of TNF- $alpha$ . In some cases, a putative ligand passing mechanismbetween the two receptors may exist. In that model, the p75 receptorbinds circulating TNF- $alpha$ and acts as a sink to prevent extracellulardegradation (30). Subsequently, soluble TNF- $alpha$ bound to the p75receptor cross-links or is passed over to the p55 receptor, throughwhich the cytokine induces itseffects.

In other cases, because the p75 receptor possesses signaling capabilities (16, 25), cross-talk between certain intracellularlylocated TNFR-associated elements seems to be responsible for theamplification of p55 TNFR-mediated responses (32). This is possiblebecause the p55 and p75 TNFRs share several receptor-associatedproteins (7). The results of the current study could be explainedby either the ligand passing or receptor cross-talkmodel.

Grunfeld and colleagues (14) were the first to report that endotoxin or cytokines could increase leptin mRNA expression.It was proposed that leptin contributed to anorexia and cachexiain sick people and animals, because, like the proinflammatorycytokines, leptin is a potent anorectic agent. However, ob/obmice, which fail to secrete leptin, are hypersensitive to theanorectic properties of LPS (10). Furthermore, plasma leptinlevels in cachectic tumor-bearing rats (5) and acquired immunedeficiency syndrome patients (13) were not inappropriately increasedas would be expected if leptin were a key mediator of cachexia.Long-term exposure to TNF- $alpha$ , which occurs in cachexia, may actuallydecrease leptin production by a p55 TNFR-mediated mechanism (33).In fact, in a study by Yamaguchi and colleagues (33), it wasfound that culturing parametrial adipocytes from pregnant micewith TNF- $alpha$ for >48 h significantly reduced leptin production.Collectively, this suggests that the induction of leptin secretionby TNF- $alpha$ may serve some otherpurpose.

For example, several lines of evidence suggest that leptin is necessary for complete immunocompetence. In accordance withthe idea that leptin improves immunocompetency, protein/energymalnutrition not only depletes body fat stores and reduces leptinlevels, but also leaves the individual severely immunocompromisedand prone to opportunistic infections (28). More importantly,leptin administration reversed starvation-induced suppressionof the immune response in mice (19). This may be mediated byleptin acting directly on functional receptors found on cellsof the immune system, because leptin also enhanced T cell proliferation,macrophage phagocytosis, and cytokine production in vitro (18,19). Collectively, there is now sufficient evidence to concludethat leptin is itself a cytokine and an important regulator ofthe immunesystem.

More recent evidence suggests that leptin is also a necessary negative feedback signal that prevents cytokine toxicity. Twostudies have shown that ob/ob mice are significantly more sensitiveto TNF- $alpha$ - and LPS-induced lethality (9, 29) and that theheightened sensitivity can be alleviated by the administrationof exogenous leptin. The mechanism by which leptin exerts itsanti-inflammatory effects is still unclear, but further demonstratesthe importance for a better understanding of the induction ofthis hormone by cytokines such as TNF- $alpha$ .

Implications

Seemingly disparate systems of the body are actually closely linked by commonality of the communication pathways that theyuse. For instance, interplay between cells of the immune systemand adipocytes such as that demonstrated in this study is potentiallyimportant when the ability of leptin to modulate immune functionis considered. What is known hints that the induction of leptinby cytokines such as TNF- $alpha$ is an adaptive response that aids theclearance of invading pathogenic microorganisms and is importantto the anti-inflammatory response to potentially toxic stimuli.The studies presented here provide an important first step tobetter understanding the TNFR signaling pathways involved in thisimmune-endocrineinteraction.

	ACKNOWLEDGEMENTS

This research was supported by National Institute of Diabetes and Digestive and Kidney Diseases Grants DK-51576 and DK-49311and the Illinois Council on Food and Agricultural Research. B.N. Finck is supported by a National Institute of General MedicalSciences fellowship (GM-007143).

	FOOTNOTES

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate thisfact.

Address for reprint requests and other correspondence: R. W. Johnson, Univ. of Illinois, Urbana/Champaign, 390 Animal Sciences Laboratory, 1207 W. Gregory Dr., Urbana, IL 61801.

Received 2 June 1999; accepted in final form 17 September 1999.

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Tumor necrosis factor (TNF)- induces leptin production through the p55 TNF receptor

Tumor necrosis factor (TNF)- $alpha$ induces leptin production through the p55 TNF receptor