Adipocyte, Adipose Tissue, and Infectious Disease

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Infection and Immunity, March 2007, p. 1066-1078, Vol. 75, No. 3
0019-9567/07/$08.00+0 doi:10.1128/IAI.01455-06
Copyright © 2007, American Society for Microbiology. All Rights Reserved.

MINIREVIEW

Adipocyte, Adipose Tissue, and Infectious Disease

Mahalia S. Desruisseaux,¹^,2^, Nagajyothi,¹^, Maria E. Trujillo,³^, Herbert B. Tanowitz,¹^,2^* and Philipp E. Scherer²^,3^,4

Departments of Pathology,¹ Medicine,² Cell Biology,³ Diabetes Research and Training Center, Albert Einstein College of Medicine and the Montefiore Medical Center, Bronx, New York⁴

INTRODUCTION

Top
Introduction
References

The adipocyte and its secretory products have been implicatedin a vast array of physiological processes. Work in many laboratoriesis focusing on the specific contributions of the adipocyte inthe areas of metabolism, inflammation, and cancer in order togain a comprehensive understanding of the systemic influenceof the adipocyte under normal and pathophysiological conditions.Until recently, adipose tissue has been considered to be a merestorage compartment of triglycerides. It is now clear that adipocytesare highly active endocrine cells that play a central role inoverall energy homeostasis and are important contributors tosome aspects of the immune system. They do so not only by influencingsystemic lipid homeostasis but also through the production andrelease of a host of adipocyte-specific and adipocyte-enrichedhormonal factors, cytokines, and extracellular matrix components(commonly referred to as "adipokines").

Little attention has been given to the role of adipose tissuein infectious disease. However, the strong proinflammatory potentialof adipose tissue suggests an important role in the systemicinnate immune response. Furthermore, the adipocyte proper servesas an important target for the intracellular parasite Trypanosomacruzi, the cause of Chagas' disease. In chronic Chagas' disease,adipocytes may represent an important long-term reservoir forparasites from which relapse of infection can occur. In othercases, such as with certain subtypes of adenoviruses, infectionwith viral particles leads to long-term hyperplasia and hyperproliferationof adipocytes, associating these adenoviral infections witha high propensity for subsequent obesity.

Here, we discuss briefly the systemic contributions of adiposetissue to the inflammatory response to infection and providea brief overview of infectious agents that have a specific impacton adipose tissue.

Adipose tissue is composed of many different cell types, butadipocytes are among the most predominant cells. Since differentadipose tissue depots show distinct gene expression patternsand vary widely in size and proximity to neighboring organs,individual depots could be viewed as "mini-organs." Despitedifferences between the different pads, the depots share similaritywith respect to their ability to store lipids and secrete adiposetissue-derived hormones. Adipose tissue stores lipid in theform of triglycerides and cholesterol esters within the lipiddroplets that represent specialized organelles inside the adipocyte.Since the lipid droplet is such a large component of the adipocyte(>95% of the mass of the adipocyte), changes in the amountof lipid stored within the adipocyte affect fat cell size (rangingfrom 25 to 250 µm). Due to the enormous size of the lipiddroplet within a normal adipocyte, these cells were viewed originallymerely as lipid storage cells. However, it is now known thatadipose tissue acts as an endocrine organ regulating a varietyof physiological functions, placing the study of adipokines,or adipose tissue-derived secretory products, at the forefrontof research in the field of adipose tissue biology.

ADIPOSE TISSUE AND ADIPOKINES: AN OVERVIEW

Adipose tissue endocrine function was first appreciated in 1989with the report that the serine protease adipsin is secretedby the 3T3-L1 adipocytes (26). Since this initial report severaladditional adipokines have been discovered, including adiponectin(Adn) (115), leptin (141), resistin (121), serum amyloid A3(SAA3) (70), omentin (139), visfatin (39), and RBP4 (138). Theseadipokines contribute to the regulation of energy homeostasisthrough effects on both central and peripheral tissues. Severalof these adipokines also contribute to nonmetabolic processesin the body, emphasizing the fact that adipokines participatein the coordination of multiple physiological functions in avariety of tissues. Adn is the only adipokine produced exclusivelyby the adipocyte. All other known adipokines can also be synthesizedby tissues in addition to adipose tissue and/or by cells otherthan adipocytes.

ADIPOSE TISSUE AND THE INNATE IMMUNE SYSTEM

The cellular composition of adipose tissue is not homogeneous.Indeed, adipose tissue contains many different cell types inaddition to the adipocyte, including pericytes, monocytes, macrophages,and cells of the endothelium (endothelial and vascular smoothmuscle cells). These additional cell types are collectivelyreferred to as the stromal vascular fraction (SVF) of adiposetissue. Since several populations of cells within the SVF ofadipose tissue are cells of the immune system, adipose tissuealso plays a critical role in the immune response.

The mechanisms by which adipose tissue contributes to the immuneresponse may be through direct effects of resident immune cellswithin adipose tissue or through indirect effects whereby adipocytesmodulate immune cell function in an endocrine and/or paracrinefashion. Most likely, adipose tissue contributes to the immuneresponse through both of these modalities. However, more dataare required to determine the importance of either mechanismduring an immune challenge or whether the relative importancevaries with the source and type of the challenge.

Immune cells are functionally active within adipose tissue,where they exert potent effects on adipocyte metabolism andendocrine function. In the obese state, there is an increasein macrophage accumulation in adipose tissue which correlateswith increased expression of cytokines and chemokines includingtumor necrosis factor alpha (TNF- ${alpha}$ ), interleukin-1ß(IL-1ß), IL-6, IL-8, monocyte chemoattractant protein1, and IL-18 (132, 136). The increased expression of inflammatorycytokine in adipose tissue has been implicated in the decreasedinsulin sensitivity (50), increased lipolysis (38), increasedleptin production (125), and decreased Adn secretion by adipocytes(77). The increase in adipose tissue cytokine expression, togetherwith the changes in adipose tissue metabolism and endocrinefunction, contributes significantly to the pathogenesis of themetabolic syndrome associated with obesity. Thus, immune cellswithin adipose tissue and the inflammatory cytokines that theyproduce are active and can significantly alter adipose tissuemetabolism and endocrine function. In addition, increases inadipose tissue inflammatory cytokine levels may affect nonadiposetissues either directly or indirectly. Some adipose tissue-derivedinflammatory cytokines such as TNF- ${alpha}$ are not secreted into thecirculation to any significant extent and are only elevatedlocally; however, increases in adipose tissue expression ofTNF- ${alpha}$ contribute to changes in whole-body metabolism and thein vivo hormonal milieu (127). A likely explanation for thisfinding is that the effects of TNF- ${alpha}$ on nonadipose tissue arelikely mediated by changes in the expression of adipokines suchas leptin and Adn. In contrast, cytokines such as IL-6 are secretedby adipose tissue into the circulation. Interestingly, a highlysignificant fraction of circulating IL-6 is adipose tissue derived(85, 100). Therefore, the production of inflammatory cytokineswithin adipose tissue and the contribution of adipose tissue-derivedcytokines to circulating levels may play a significant rolein host defense mechanisms during immune challenges. These observationsunderscore the potential relationship between adipose tissue-derivedimmune cells and their contribution to an immune response andhow adipocytes contribute to immune cell-stimulated changesin peripheral tissues through the secretion of adipokines. However,the teleological reasons why such a tight connection betweenthe immune system and energy stores exists are unknown. Whyare immune cells within adipose tissue and how does the presenceof adipose tissue modulate immune cell function during an acuteimmune challenge? Several laboratories are starting to explorethese questions. Recent evidence derived from coculture experimentsdemonstrates the relationships between adipocytes and macrophageswhereby secretory products from adipocytes amplify macrophageinflammatory cytokine expression in vitro (13). Similar findingsare reported in vivo, where inducible ablation of adipocytesblunts the lipopolysaccharide (LPS)-stimulated rise in systemiclevels of IL-6 in mice (100). The factors secreted by adipocytescapable of stimulating or amplifying inflammatory cytokine productionby resident macrophages within adipose tissue may include acute-phasereactants such as SAA3 (70). Treatment of monocyte cell linesin addition to cultured SVF cells with SAA3 results in a markedinduction of inflammatory mediators such as IL-6, IL-8, andTNF- ${alpha}$ . It is possible that the acute-phase reactants synthesizedby adipocytes may contribute to the synergy observed betweenadipocytes and the immune cells (70). Additional acute phasereactants are produced by adipocytes that include ${alpha}$ 1 acid glycoprotein,the CRP relative pentraxin-3, and a number of lipocalins suchas 24p3 and retinol-binding protein 4 (Rbp4).

OBESITY AND SEPSIS

It is well established that obesity is associated with increasedrisks of morbidity and mortality (1, 12, 80). Obesity resultsin increased admissions into hospital critical care units. Interestingly,the mortality after blunt trauma is increased eightfold in morbidlyobese patients (80). Intubated patients who are obese have anincreased risk of aspiration pneumonia than nonobese patients.This may be due to several factors, such as higher intra-abdominalpressures and an increased incidence of gastric reflux and highervolumes of gastric fluid with lower pH in obese individuals(80). Moreover, a larger number of skin punctures is often requiredto gain vascular access in obese patients, thus increasing therisks of catheter-related infections and thromboses (18). Postoperatively,the risk of developing a surgical wound infection is greatlyincreased in obese patients, especially with abdominal surgery,which independently carries an increased risk of postoperativeinfections (1, 67).

In view of the role of adipose tissue as an endocrine organand its huge potential to secrete several pro- and anti-inflammatorymediators such as cytokines, hormones, and peptides, it is likelythat under conditions when adipose tissue can contribute between30 and 50% of total body weight, the increase in morbidity andmortality in septic obese patients could be attributed to thisexcess adipose tissue. Adipocytes express many of the knownToll-like receptors (TLRs). In fact, we found that that adipocytesare highly responsive to endotoxin due to the high-level expressionof TLR-4 (69) and respond by inducing high levels of proinflammatorycytokines at concentrations of endotoxin that reflect a sensitivityto these bacterial cell wall components comparable to or higherthan what can be observed in macrophages. In the same study,we reported the induction of TLR-2 in adipocytes, which confersa high degree of sensitivity to fungal cell wall components.

The role of adipose tissue in the pathogenesis of infectionwas underscored by our recent observations when we generatedan inducible "fatless" model system, the FAT-ATTAC (for fatapoptosis through targeted activation of caspase 8) mouse (100).In this model, adipocytes can be inactivated in a triggeredfashion. This allows the assessment of a complete absence offunctional adipocytes prior to the onset of conventionally observedsecondary effects associated with chronic lipodystrophy. Inthe absence of adipocytes, the "septic response" to LPS injectionswas dramatically reduced as judged by a decrease in the systemicIL-6 and SAA3 levels.

Somatostatin, a neuroendocrine secretory product, has been describedin immune cells after activation by the inflammatory processand is induced by administration of IL-1ß and TNF- ${alpha}$ (113, 114). Somatostatin inhibits the secretion of several hormonesin the gastrointestinal tract, including insulin and glucagon(101). Cytokines and LPS induce somatostatin transcription inhuman adipose tissue (116). Increased somatostatin transcriptionalso occurs when adipose tissue is cocultured with Escherichiacoli or activated macrophages. In patients with severe bacterialinfections, the increase in somatostatin mRNA and protein expressionis observed in visceral fat depots but not in subcutaneous fatnor in depots from uninfected patients. This increase is inhibitedin the presence of dexamethasone (116).

Adipose tissue is also an important extrathyroidal source ofinflammation- or sepsis-induced calcitonin and calcitonin precursors.During sepsis there is a thousandfold increase in the expressionof calcitonin and procalcitonin that can be attributed to adiposetissue (71-73). This increase directly correlates with diseaseseverity and mortality and occurs both in subcutaneous and inomental fat depots. The addition of endotoxin to cultured humanadipose tissue, as well as the administration of IL-1ßand TNF- ${alpha}$ , causes an increase in calcitonin and its precursors;the effects of IL-1ß are reversible after treatmentwith IFN- ${gamma}$ (71). These data demonstrate a possible role for calcitoninin the increased morbidity and mortality observed in morbidlyobese patients in the critical care setting. In this regardsupraphysiologic doses of procalcitonin increased mortality(94), and peak levels during infection can serve as early markersof sepsis and an indicator of mortality (120, 133). In addition,procalcitonin has been shown to stimulate inducible nitric oxidesynthase (iNOS) transcription in vascular smooth muscle cells(48). Interestingly, anti-procalcitonin serum reversed the deleteriouseffects and increases survival in sepsis (94). During sepsis,adipose tissue also modulates the increased secretion of adrenomedullinand of the calcitonin gene-related peptide, both of which arepotent vasodilators and modulators of nitric oxide production.Notably, these proteins induce insulin resistance during sepsis(72, 73).

In patients with septic shock due to fulminate cellulitis, therewas a compartmentalization of increased iNOS activity and IL-1ßto inflamed regions of fat, muscle, and arteries that did notoccur in skin, the primary site of infection. Interestingly,the increase in TNF- ${alpha}$ expression was not altered in fat tissuein those cases (5). The expression of iNOS was inversely relatedto mean arterial pressure and to systemic vascular resistance,suggesting a role in cardiovascular failure in septic shock(5).

Sepsis has also been associated with disturbances in lipid metabolismresulting in hypertriglyceridemia and lipid accumulation inthe liver. In animal models, it was demonstrated that E. coli-inducedsepsis resulted in a significant decrease in lipoprotein lipase(LPL), leading to a marked decrease in clearance of triglyceridesand free fatty acids in cardiac tissue, adipose tissue, andmuscle (64, 65). This was associated with an increase in denovo hepatic lipogenesis (65, 131). The administration of LPSand many cytokines to animals rapidly increased serum triglyceridelevels which persisted (65). The alterations in lipoproteinmetabolism differed depending on the amount of endotoxin used(58). At low doses of LPS or cytokines, there was an increasein de novo hepatic fatty acid synthesis, particularly short-chainfatty acids (131), lipolysis of adipose tissue, and suppressionof fatty acid oxidation. Higher doses of LPS induced a decreasein LPL activity in muscle and adipose tissue, thereby decreasingthe clearance of very-low-density lipoproteins. LPS and cytokinescause a decrease in apoE mRNA; apoE is believed to be criticalin the clearance of triglyceride-rich lipoproteins (58). LPSdecreased fatty acid uptake in cardiac and skeletal muscle andadipose tissue (84), and IL-4 reversed some of the actions ofthese cytokines and of LPS. Interestingly, the response to LPSand cytokines was significantly higher in subcutaneous adiposetissue than in visceral adipose tissue.

Bacterial infection induces fatty acid synthesis, increaseslipolysis, generates fatty acids from adipose tissue, and reducesfatty acid oxidation and ketogenesis in the liver. The increasedfatty acids are re-esterified in the liver a process mediatedby liver acyl-coenzyme A synthetase (ACS) activity. ACS is essentialin the regulation of fatty acid metabolism. It allows the catalysisof long-chain fatty acid to acyl-CoA esters, which can be utilizedin the synthesis of cellular lipids or in ß-oxidation(84). ACS is located in the microsomes, mitochondria, and peroxisomesof the liver, as well as in microsomes of adipose tissue andmitochondria of heart and muscle. The administration of LPSand cytokines caused a marked decrease in the transcriptionof ACS in the liver, adipose tissue, and cardiac and skeletalmuscle tissue (84). In the liver, although mitochondrial activitywas reduced, there was an increase in the microsomal activity(84). Mitochondrial ACS regulates activation of fatty acidsfor oxidation and ketone body production as sources of energy,and microsomal ACS is believed to regulate the re-esterificationof fatty acids for triglyceride synthesis (59). Importantly,the administration of insulin reversed the decrease in LPL observedin sepsis. In rats infected with E. coli, isolated adipocytesdemonstrated a sustained decrease in LPL activity. However,after overnight treatment with insulin, there was a significantincrease in LPL synthesis and activity. Hence, the sepsis-induceddecrease in adipose LPL is not a direct consequence of insulinresistance; rather, insulin stimulates LPL synthesis in septicrats (103).

INSULIN RESISTANCE AND GLUCOSE METABOLISM IN SEPSIS

Glucose metabolism is markedly altered during bacterial sepsis,and hyperglycemia in the face of hyperinsulinemia is well documentedin situations of stress such as during systemic infection andshock. The diabetic state worsens during infection, and thisis believed to be due, in part to the increase in certain hormones,such as cortisol, which occur during stress, but the mechanismfor this apparent resistance to insulin is largely unknown.During sepsis, there is an alteration of insulin receptors bothin quantity and in affinity (51). In a study of induced sepsisin rats, no difference was demonstrated in insulin binding inseptic versus control rats despite a significant increase ofplasma glucose levels. This observation suggests no change inquantity or affinity of insulin receptors in that model. Therewas, however, a marked difference in the uptake of glucose byadipocytes in the presence of insulin in a dose-dependent manner,demonstrating a significant decrease in responsiveness to insulin(51). The study by Igarashi et al. (51) demonstrated that inthe rat sepsis model, hyperglycemia in sepsis may be partlydue to postreceptor defects in insulin-mediated glucose transportby adipocytes. High levels of circulating glucose may be proinflammatorysince they can lead to leukocyte rolling and adherence and canbe associated with the production of free oxygen radicals inaortic endothelial cells (91, 92), as well as induce potentproinflammatory responses in adipocytes (68). Importantly, incritically ill patients the administration of exogenous insulinhas a significant effect on survival (129). Thus, the systemicanti-inflammatory effects of insulin during sepsis are increasinglyappreciated and are now used in septic patients. Beyond itseffects contributing to a reversal of sepsis-induced alterationsin lipid metabolism and hyperglycemia, insulin may in additionsuppress the expression of NF- ${kappa}$ B, thereby reducing the productionof cytokines such as TNF- ${alpha}$ (91). A more detailed view of theanti-inflammatory properties of insulin has been discussed byDandona et al. (27).

OBESITY AND ANTIBIOTIC PHARMACOKINETICS

The physiologic changes associated with obesity also influencethe distribution, clearance, and metabolism of drugs. Underlyingsepsis may also complicate the pharmacokinetics of drugs, includingantibiotics (20, 54, 80, 112, 140). The increased levels oflipoproteins, cholesterol, and free fatty acids that competitivelybind serum albumin may inhibit the protein binding of certaindrugs; furthermore, the lipophilicity of drugs largely determinestheir volume of distribution (80). In septic shock, there havebeen several reports of impaired penetration of ß-lactamantibiotics at sites of infection (54, 140). The levels of theseantibiotics in subcutaneous adipose tissue were significantlyless than the levels found in plasma (20, 54, 112). Since infectionsare usually localized to the interstitial fluid of tissues ratherthan in plasma, the decrease in penetration may contribute inpart to therapeutic failures during septic shock in the faceof inhibitory plasma concentrations (54). This phenomenon wasrecently observed with the antibiotic linezolid, where patientswith septic shock had lower concentrations of the drug thanhealthy volunteers (20). The fluoroquinolone levofloxacin wasfound to achieve similar concentrations in inflamed and healthysubcutaneous adipose tissue; thus, not all antibiotics are affectedby inflammation caused by infection (10). In summary, the availabledata indicate a large variability of drug concentration in inflamedtissue from individual to individual during septic conditionsand poses a major challenge in determining the appropriate treatmentdoses.

ADIPOKINES LEPTIN AND ADIPONECTIN: CRITICAL MEDIATORS IN THE INFLAMMATORY RESPONSE DURING INFECTION?

Leptin and Adn are two adipokines important in the modulationof the host response to infection. Leptin, the 16-kDa nonglycosylatedprotein product of the obese (ob) gene (141), is a pleiotropichormone-cytokine synthesized mainly in adipocytes (78). Leptinand leptin receptors have been identified in a variety of tissuesand organs (7, 19, 47, 82). The biological activities of leptinare mediated through the interaction with its specific membranereceptor (Ob-R), which has sequence homology to members of theclass I cytokine receptor (gp130) superfamily (124). Leptinis released into circulation, and its levels correlate withtotal body fat mass (2). During malnutrition or starvation,circulating leptin levels decline and serve as a signal to thehost to conserve energy by reducing energy metabolism (3). Althoughleptin has been more strongly associated with an increase inmetabolic rate and reduction of adipose mass by suppressingappetite and stimulating the sympathetic nervous system (16,17, 22, 23), it is also implicated in negative feedback of thehypothalamic-pituitary-adrenal axis. Leptin receptors are foundin the central nervous system and in peripheral tissues. Accordingly,the physiological role of leptin is not solely restricted tothe regulation of food intake and energy expenditure. Leptinplays a role in hematopoietic differentiation, including lymphoidcells of the immune system, and can be an inducer of the hostinflammatory response (11, 40, 74, 75, 81, 99, 107, 108).

Obese leptin-deficient ob/ob mice and db/db mice display immunedysfunction and lymphoid organ atrophy, and thus they have reducedlevels of T and B cells (75). Missense mutations in humans leadingto leptin deficiency also result in immune system dysfunction(99). Leptin induces the proliferation, differentiation, andfunctional activation of hematopoietic cells. Hence, bone marrowadipocytes may play an important role in this process. Leptinmodulates the proliferation and activation of peripheral T lymphocytesin mice and in humans (75, 81) and can enhance the productionof cytokines (18, 19). In addition, leptin modulates monocyte-macrophagefunction and regulates proinflammatory responses (40, 107).Leptin increases Th1-dependent immunostimulation and autoimmunediseases such as experimental autoimmune encephalomyelitis inSJL mice. The deficiency of leptin signaling decreases bothhumoral and cellular immune responses in arthritis (21). Italso modulates T-cell mediated inflammation, enhances proliferation,and IL-2 production of native T cells and promotes the Th1 phenotypeby increasing IFN- ${gamma}$ and inhibiting IL-4 production from CD4 cells(75). Leptin enhances the synthesis of proinflammatory cytokinesby cultured macrophages after treatment with LPS (74), and similarobservations have been made in vivo in rodents. Therefore, theinvolvement of leptin in the upregulation of the inflammatoryresponse provides a common pathogenic mechanism for severalof the major complications of obesity.

Leptin-deficient mice have an impaired host defense in a bacterialpneumonia model that may be due to a defect in alveolar macrophagephagocytosis and leukotriene synthesis (79). The role of leptinin the host defense against gram-negative pneumonia was studiedby comparing the responses of wild-type and leptin-deficientmice to an intratracheal challenge with Klebsiella pneumoniae.In this model, there was an increase in systemic and pulmonaryleptin levels that was deemed critical for host defense. Theabsence of leptin triggered greater mortality and reduced bacterialclearance from the lungs of the leptin-deficient mice comparedto wild-type mice. Interestingly, no differences were observedbetween wild-type and leptin-deficient mice in lung homogenateswith respect to TNF- ${alpha}$ , IL-12, or macrophage inflammatory protein2 levels after infection; however, there was a reduction inleukotriene production in leptin-deficient mice. These datastrongly suggested that leukotrienes are important mediatorsof leptin effects on macrophage phagocytosis in mice. The absenceof leptin generated marked impairment of polymorphonuclear neutrophilphagocytosis of bacteria (86). This phenomenon was reversibleby leptin replacement in the leptin-deficient mice. Recent studiesalso indicate that leptin has a role in the early immune responseduring pulmonary infection caused by Mycobacterium tuberculosisin mice by mediating an effective IFN- ${gamma}$ -driven Th1 response withadequate lymphocyte trafficking and granuloma formation (135).Bleau et al. (14) reported that an isolate of Lactobacillusacidophilus decreased both leptin production and leptin-mediatedimmunostimulation, leading to a lower Th1 response by SJL adipocytes,and suggested that this was the mechanism by which this strainof Lactobacillus had a protective role in intestinal inflammatorydiseases in their model.

The downstream effects from the leptin receptor in immune cellsare mediated by activation of the JAK-STAT signaling pathwayin peripheral blood mononuclear cells (106). After leptin stimulation,JAK activity was increased and STAT-3 is tyrosine phosphorylated,dimerized, and translocated to the nucleus to activate geneexpression. STAT-3 was also associated with tyrosine-phosphorylatedsrc substrate Sam68 in response to leptin. Martin-Romero etal. (81) demonstrated that leptin stimulation of peripheralblood mononuclear cells promotes the tyrosine phosphorylationof the intracellular domain of the leptin receptor, IRS-1, andSam68 via JAK activation. The substrates IRS-1 and Sam68 associatewith p85, providing a molecular mechanism for phosphatidylinositol3-kinase activation. Leptin also activates various mitogen-activatedprotein kinase pathways (57, 122).

Plasma levels of leptin are elevated during inflammation orinfection (22). Induced peritonitis in rodents leads to an increasein plasma leptin concentrations and in transcription of leptinin adipocytes (17, 22). In patients that had been septic for $≥$ 14 days, there was no correlation between sepsis and serum leptinconcentrations (22). However, during acute bacterial sepsis,there appeared to be a significant increase in plasma leptinlevels associated with a marked increase in cortisol level andIL-6. In these patients there was a complete blunting of thecircadian pattern of leptin release. Interestingly, the patternwas reversed with lower levels of leptin at night and higherlevels during the day (17). These observations suggest thatleptin may contribute to the anorexia observed during sepsis.In addition, leptin can directly suppress adrenal function,thus providing interesting implications for the mechanism ofadrenal insufficiency observed during sepsis. In the presentstudy, patients with higher levels of circulating leptin hada better survival rate compared to nonsurvivors, suggestingthat leptin could serve as a marker for acute stress-mediatedresponse. Although leptin administration in vivo plays a protectiverole in murine pulmonary antibacterial host defense (79), inhumans the role of leptin and microbial infection remains unclear.However, recent developments suggest that studies exploringthe role of leptin as both a diagnostic marker and a therapeuticagent to augment the immune response during sepsis are warranted.

Adn is a secretory protein synthesized exclusively by adipocytes.It serves as an anti-inflammatory cytokine and antagonizes theeffects of TNF- ${alpha}$ . When the plasma levels of Adn were measuredin an animal model of polymicrobial sepsis, there was a gradualdecrease in Adn levels to $~$ 50% at 24 h. Moreover, there was aninverse relationship with levels of circulating TNF- ${alpha}$ (126).Adn was also demonstrated to affect LPS activity in vitro. WhenAdn was incubated with LPS, there was a significant dose-dependentdecrease in the activity of LPS. Western blot analysis demonstratedevidence of binding of Adn to LPS, suggesting that Adn may havea neutralizing effect on LPS, although this has not been provenin vivo. It is not clear whether Adn itself has anti-inflammatoryproperties or whether indirect mechanisms are at work. However,Adn production by adipose tissue can be inhibited by systemicinflammation, at least under some circumstances. Adn productionby cultured adipocytes was demonstrated to be inhibited by inflammatorycytokines (37, 105), and this inhibition may be mediated inpart by NF- ${kappa}$ B signaling. In cultured adipocytes and in obesediabetic mice, inhibition of adipocyte inflammatory NF- ${kappa}$ B signalingby an I ${kappa}$ B kinase inhibitor resulted in a reduction of cytokinelevels and increased plasma levels of Adn (55). Thus, I ${kappa}$ B kinaseinhibition leads to increased plasma Adn levels and an improvementin systemic insulin sensitivity. In contrast, Keller et al.did not observe an effect on Adn levels after LPS administrationto humans (56).

The anti-inflammatory action of Adn may be mediated by one ofits principal signaling targets, the AMP-activated protein kinase(AMPK) (137). There is evidence that the truncated bacterialform of an Adn has anti-inflammatory effects on endotheliumvia AMPK-mediated modulation of NF- ${kappa}$ B and Akt/PKB (95, 97, 98).However, whether such a trimeric globular form exists in vivoin not clear, thus making the interpretation of these resultsfor an in vivo situation difficult. Some of the proven antiatheromatouseffects of Adn may be mediated by anti-inflammatory activitiesacting directly on the vasculature.

Adn has an important role in protecting against cardiac hypertrophyin cardiac overload states such as hypertension, hypertrophiccardiomyopathy, and ischemic heart disease. In mice, this hasbeen supported by data demonstrating that Adn protects againstoverload-induced and adrenergically induced cardiac myocytehypertrophy by inhibiting hypertrophic signals via AMPK (117).Interestingly, Adn may represent the link between obesity (associatedwith decreased Adn levels) and cardiac risk by protecting againstinflammation-induced cardiovascular insufficiency and directmyocardial insults.

HIV INFECTION AND ADIPOCYTES

Patients infected with human immunodeficiency virus (HIV)/AIDSundergo many metabolic abnormalities, including dyslipidemia,insulin resistance, fat loss, or lipoatrophy and fat accumulation.Adipocytes play an important role in HIV infection since significantchanges in adipose tissue morphology and metabolism are observedin HIV-infected individuals. While many authors demonstratethat HIV lipodystrophy is associated with peripheral adiposetissue loss with a concomitant increase in visceral adiposity(43), others have demonstrated that both subcutaneous and centraldepots are affected and undergo reduction (6). The underlyingmechanisms for this phenomenon remain poorly understood. Thislipodystrophy syndrome particularly prevalent in patients onhighly active antiretroviral therapies is associated with othermetabolic complications, including insulin resistance, dyslipidemia,cholesterol, and fat redistribution (90). Most studies havesuggested that the lipodystrophy is associated with the useof two major classes of antiretroviral drugs, nucleoside reversetranscriptase inhibitors (NRTIs) and protease inhibitors (PIs)(45). Subcutaneous fat cell biopsies of HIV-infected patientstreated with PIs demonstrated increased adipocyte cell deathin the subcutaneous fat compartments (34), whereas others havefound little evidence for apoptosis (88).

Adipocytes could be a direct target for HIV infection. Hazanet al. (46) demonstrated the receptors for HIV entry, such asCD4, CXCR4, and CCR5, were expressed in vitro on preadipocytesand adipocytes by reverse transcription-PCR and immunocytochemicalexperiments. In vivo expression of these receptors was alsodemonstrated on sections of human white adipose tissue by immunohistochemistry.However, these authors concluded that in vitro infection ofadipose tissue with the virus was not achievable because thelevel of expression of these HIV receptors did not permit entryinto adipose cells in the biopsies tested (87). Nevertheless,Maurin et al. demonstrated HIV receptor expression in freshlyisolated preadipocytes and in mature adipocytes from subcutaneousfat depots (83). These authors also demonstrated HIV infectionof fat cells by observing HIV-1 transcriptional activity inthe fat cells and provided evidence for adipocyte infectionwith HIV by showing significantly increased Gag p24 antigenexpression upon stimulation of these cells with proinflammatorycytokines, such as TNF- ${alpha}$ or IL-1ß. The results of thatstudy indicate that HIV-1 indeed infects human adipose cellsin vitro and further suggest that the initial infection maybe overcome by treatment with proinflammatory cytokine stimulation.

Altered fat differentiation and morphology has been describedin HIV patients (52), as well as increased levels of collagenfibers and vessel density. Leptin levels were significantlyhigher in HIV-infected patients with lipodystrophy, and theselevels were negatively correlated with insulin resistance (61).Adn levels were reported to be lower in HIV-infected patientswith lipodystrophy and positively correlated with insulin resistance(89). Increased levels of TNF- ${alpha}$ and IL-6 during HIV infectionmay directly affect the insulin signaling pathways and induceinsulin resistance. Moreover, the lipolytic effects of thesecytokines may increase free fatty acids and may also cause insulinresistance through lipotoxic effects in muscle and liver (119).The impact of PIs and NRTIs on adipose cell functions and adipokineproduction in vivo and in vitro has been reviewed elsewhere(62).

Adipocyte differentiation involves the sequential activationof transcription factors which regulate the expression of adipocytespecific markers. CCAAT-enhancer binding protein ß(C/EBPß), peroxisome proliferator activated receptor ${gamma}$ (PPAR ${gamma}$ ), and C/EBP ${alpha}$ are major transcription factors that becomeactivated during the differentiation of adipocytes. Differentiationis enhanced by the transcription factor sterol regulatory elementbinding protein 1 (SREBP1), which activates PPAR ${gamma}$ (36, 104).Bastard et al. demonstrated reduced mRNA expression of the adipogenicdifferentiation factors C/EBPß and C/EBP ${alpha}$ , PPAR ${gamma}$ , aswell as the 1c isoform of SREBP1, in the subcutaneous fat ofindividuals with HIV lipodystrophy treated with PIs comparedto healthy subjects (9). PPAR ${gamma}$ activates C/EBP ${alpha}$ which, in turn,enhances and maintains PPAR ${gamma}$ expression, allowing the expressionof adipocyte specific genes and cell differentiation in centralfat depots, in which SREBP-1 protein levels are also increased(9). PI-induced alterations of SREBP-1 expression may contributeto the changes in fat distribution in HIV-infected individuals,similar to the changes that can be seen in mice with alteredSREBP1c levels (118). PIs (i.e., nelfinavir, ritonavir, andlopinavir) and some NRTIs (i.e., stavudine and zidovudine) inducethe expression and secretion of IL-6 and IL-1ß in3T3-L1 cell lines, suggesting that these drugs can modulatethe complement of secretory proteins regardless of the differentiationstatus (62). This includes altered expression of TNF- ${alpha}$ , IL-6,Adn, and leptin, which has also been observed in the adiposetissue of HIV-infected patients, leading to increased serumlevels of TNF- ${alpha}$ and IL-6 levels in lipodystrophic HIV patients(9, 52, 53, 93).

INFECTIOUS ETIOLOGY OF OBESITY

Although the etiology of obesity is multifactorial, there hasbeen an increasing interest in the fascinating possibility thatinfection with specific pathogens may lead to increased adiposity(28-30, 42). Scrapie, a prion neurodegenerative disease of goatsand sheep with a prolonged incubation, was also reported tocause obesity in mice. The ability of scrapie to cause obesityappears to be strain specific. The observations of Kim et al.(60) suggest that the mechanism is an alteration of the hypothalamic-pituitary-adrenalaxis while others have suggested that alterations in the glucosetransporter (GLUT-1) may be important in the pathogenesis ofobesity in this model (130).

An underlying viral basis was first suggested by Lyons et al.in 1982 (76), who reported that canine distemper virus (CDV)caused obesity in mice. CDV causes respiratory, gastrointestinal,and central nervous system (CNS) diseases in dogs and othermammals. This virus invades the CNS replicating in neurons andglial cells of the white matter and causes an encephalomyelitis.Mice infected with CDV experience an increase in body weight,fat cell size, and fat cell number. The mechanism for this observationwas believed to be the result of virus-induced hypothalamicdamage. However, it has also been suggested that that the virus-induceddownregulation of leptin receptor expression in the hypothalamusof CDV-infected obese mice may be the cause of the obesity.Another virus, Rous-associated virus-7 (RAV-7), an avian retroviruswas reported to cause stunted growth, obesity and hyperlipidemiain chickens. The infected chickens develop fatty enlarged livers,anemia and immunodepression. Carter et al. (24) suggested thata reduction in thyroid hormone level in RAV-7-infected chickenswas the cause of the obesity and hyperlipidemia.

Borna disease virus (BDV) which was also reported to cause obesityinfects many birds and mammals and persists in the nervous system.BDV antibodies were detected in horses in many parts of theworld. Gosztonyi and Ludwig demonstrated that this virus causedobesity in rats and that this was associated with inflammationof the hypothalamus, pancreatic hyperplasia, and elevated levelsof triglycerides and glucose (41). Viral antigen expressionwas noted in several areas of the brain including the hypothalamus.Thus, infection with BDV could result in neuro-endocrine dysregulationleading to obesity. Interestingly, BDV-specific antigens andBDV-RNA have been demonstrated in human brain. This virus hasalso been demonstrated to be associated with a variety of psychiatricdisorders.

The first virus that was reported to be associated with humanobesity was the avian adenovirus SMAM-1. Dhurandhar et al. foundantibodies to this avian adenovirus in obese individuals inIndia (32). However, since this virus was not thought to infecthumans, the observation suggested cross-reactivity to an antigenicallysimilar human virus. The same authors first reported that Ad-36caused obesity in animals (31). In small animal studies, theydemonstrated the presence Ad-36 DNA in adipose tissue of Ad-36-inducedobese animals. Furthermore, these authors demonstrated the potentialof Ad-36 in promoting obesity in nonhuman primates (33).

Human adenoviruses commonly cause infections of the respiratoryand intestinal tract and the eye. Thus, antibody titers to adenovirusesare common in the population. There are 50 adenoviruses thatare placed into six major subgroups (A to F) with specific serotypes.Ad-36, implicated in human obesity is part of group D, serotype36. Ad-36 does not ordinarily cross-react with antibodies toother human adenoviruses. It has an unusual affinity for adiposetissue, and the amount of Ad-36 DNA in visceral adipose tissuecorrelates with the fat depot weight. Approximately 30% of theobese and 11% of the nonobese individuals demonstrated antibodiesto Ad-36 (30). Although the precise mechanism by which thisvirus promotes obesity is unclear, it has been reported thatAd-36 upregulates preadipocyte differentiation in culture. Thedemonstration that adipocyte differentiation, leptin production,and glucose metabolism is modulated by Ad-36 is of interest,but it remains to be conclusively proven that this virus isadipogenic in humans. For example, the recent report by Whighamet al. (134) demonstrated that Ad-31 caused increased differentiationof 3T3-L1 cells, but this did not correlate with obesity inchickens. Furthermore, there was no correlation between thedevelopment of obesity in chickens induced by Ad-37 and humanobesity. The association of adenoviral infection with obesityis highly specific for Ad-36, which is at this time the onlyhuman adenovirus implicated with human obesity.

Finally, recent reports suggest an association of Chlamydiapneumoniae infection with human obesity (30). This is of interestin view of the many reports suggesting that this organism mightbe associated with the pathogenesis of arteriosclerosis andcoronary heart disease. Research into the relationship betweenobesity and infection has only begun to be investigated andmore data are needed to establish definite cause and effectrelationships.

TRYPANOSOMA CRUZI INFECTION AND ADIPOSE TISSUE

Parasitic diseases, caused by both nematodes and protozoa, havebeen reported to be associated with nutritional deficiencies,wasting, and diabetes. Chagas' disease, caused by the parasiteTrypanosoma cruzi is endemic in Latin America. In recent years,the influx of immigrants from these countries into North Americaand Europe has led to an increase in the diagnosis of clinicalChagas' disease in the United States, as well as the recognitionof blood transfusion-induced Chagas' disease in areas wherethis disease is not endemic (66). Reactivation of Chagas' diseasemay present as an opportunistic infection in individuals withAIDS/HIV (128) and in those undergoing immunosuppressive therapyfor malignancies and in organ transplantation (8). When individualswith chronic and/or asymptomatic T. cruzi infection acquireHIV infection the reactivation of this infection (111) may presentas a necrotizing encephalitis and/or acute myocarditis (63,102, 109, 110). Acute chagasic myocarditis may be the sole manifestationof reactivation, or it may accompany encephalitis.

For many years an association between human T. cruzi infectionand obesity and diabetes has been suspected, and there has beengeneral belief that the incidence of diabetes is greater inthe chagasic population. Indeed, in recent years there havebeen several reports indicating that diabetes is more commonin this population (35, 44, 96). One such study demonstrateda significant reduction in insulin among chronically infectedindividuals (44). Interestingly, previous studies from our laboratorydemonstrated that when mice with chemical-induced diabetes ordiabetic db/db mice were infected with T. cruzi, they had ahigher parasitemia and mortality (123). The underlying mechanismsof these observations remain unknown. Interestingly, chemicallyinduced diabetic mice infected with the causative agent of Africantrypanosomiasis, T. brucei developed higher parasitemia andincreased mortality compared to infected nondiabetic mice (4).

As noted above, the adipocyte has been identified as an importantcontributor in the pathogenesis of diabetes, obesity, and themetabolic syndrome, but its relationship to the pathogenesisof T. cruzi infection has only recently been explored. It hasbeen suggested that adipose tissue in Chagas' disease may serveas one of the reservoirs for the parasite from which recrudescencemay occur during immune suppression. However, since no systematicapproach has been undertaken to more precisely define the roleof the adipocyte in the normal and diabetic state during infectionwith T. cruzi, we examined the direct effects of T. cruzi infectionon adipocytes in vitro and in vivo.

Mice were infected with the trypomastigotes of T. cruzi. Todetermine the metabolic consequences of infection, basal glucoselevels as well as insulin sensitivity were monitored by meansof an oral glucose tolerance test prior to infection, duringthe acute phase of infection, as well as during the chronicstage. We observed that acute infection was often associatedwith severe hypoglycemia which correlated with mortality (25),an observation made by others as well (49). As noted above,the metabolic response to bacterial sepsis usually includeshyperglycemia with insulin resistance, profound negative nitrogenbalance, and diversion of protein from skeletal muscle to splanchnictissues. The response to T. cruzi infection, however, differsfrom that observed in most studies of bacterial sepsis. Onepossible mechanism is an effect on glucose metabolism due toinvasion of the liver by the parasite. However, the preciseunderlying reasons for hypoglycemia during acute T. cruzi infectionare not known. Surprisingly, during acute infection, glucoselevels in the infected mice at all stages remained below thelevels measured for the control animals. Even though the baselineglucose levels in the infected animals were lower, the oralglucose tolerance test indicated relatively normal ability toclear the ingested glucose despite the high degree of inflammationassociated with this infection. The fasting glucose levels andsurvival rates of infected mice and uninfected mice were compared,and a strong correlation between the relative reduction in glucoselevels and mortality was observed (25).

The level of Adn, the adipokine that was discussed above, issignificantly decreased during T. cruzi infection in mice. Decreasedlevels of Adn are usually associated with insulin resistance,hyperglycemia, and obesity. In addition, decreased levels ofAdn are observed with increased systemic inflammation associatedwith cardiovascular disease. However, acute inflammation triggeredby endotoxemia does not have an effect on Adn levels (56). Adnlevels were reduced during acute T. cruzi infection, suggestingthat the proinflammatory component of the infection is the maindriving force for the expression of Adn. The hypoglycemia cannotbe readily explained by changes in Adn. This is an example ofa physiologically relevant condition that combines hypoglycemiaand normal glucose tolerance with significantly reduced Adnlevels. It is noteworthy that individuals with malaria infectionhave increased levels of Adn (15).

The decreased insulin levels observed 30 days postinfectionin the mouse model of T. cruzi infection are consistent witha physiological response to the very low glucose levels duringthat time. It is unlikely that this is a reflection of pathologicalchanges at the level of the pancreatic ß cells, sincethe morphology is normal at day 30 postinfection and insulinlevels revert to normal levels at later stages. In addition,leptin levels were significantly reduced in infected mice comparedto controls. Resistin levels, another fat cell-specific secretoryfactor with insulin-desensitizing properties, were not affectedby infection. Levels of plasminogen activator inhibitor 1, whichis also prominently expressed in adipocytes, are completelyunaffected by infection. In contrast, proinflammatory markerssuch as IL-6, MCP-1, and TNF- ${alpha}$ were markedly elevated in infectedmice in response to the high parasite load on day during theacute infection. The significant decrease in leptin levels wasinitially surprising since the infected mice gained more weightthan the control mice. However, magnetic resonance imaging studiesrevealed that there were significantly reduced levels of adiposetissue during the acute phase of the infection. Interestingly,the decrease in adipose tissue persisted even at later stagesduring chronic infection and was primarily caused by a decreasein abdominal adipose tissue. Mice that had marked right ventriculardilation had an even greater loss of fat depots. The weightgain in infected mice appeared to be related to edema, whichmay have been the consequence of right-sided heart failure (25).

Since the plasma levels of Adn were reduced as a result of T.cruzi infection, we wanted to determine whether the parasitehas the potential to actually invade adipocytes in vivo. Real-timePCR data demonstrated that adipose tissue is a relevant targettissue, harboring large numbers of parasites. Particularly noteworthyis that at 300 days postinfection, a comparable number of parasiteswere present in adipose and heart tissue, indicating that adiposetissue is a reservoir tissue for these parasites. We observedthat adipocytes were readily infected in vivo. Since there werenumerous parasites in adipose tissue, we suspected that themassive local parasite count should be responsible for a considerableinflux of macrophages. We wanted to determine whether the highpropensity to harbor and propagate T. cruzi in adipocytes alsohas an effect on macrophage levels. Therefore, white adiposetissue was isolated from two different fat depots of infectedmice. As judged by an immunohistological stain for the macrophage-specificmarker F4/80, there was a marked increase of F4/80-positivecells in white adipose tissue during the acute infection. Evenmore pronounced changes were observed in brown adipose tissue.This persisted even at 300 days postinfection. The parasiteswere located within the adipocytes of brown fat, which is characterizedby multiple smaller intracellular lipid droplets compared tothe densely packed white adipocytes that contain a single largelipid droplet. During the chronic stage of infection, therewas a reduction in the number of macrophages compared to theacute infection (25).

The reduced levels of Adn in plasma in T. cruzi infection (25)suggest that infection of adipocytes may also have consequenceson other proteins synthesized in adipose tissue. Therefore,immunoblot analysis was performed for a number of proteins thatare expressed in adipose tissue. Consistent with the reductionof plasma Adn, the levels of Adn in adipose tissue were alsoreduced during acute infection in a number of fat pads, particularlyin perirenal and visceral adipose pads, both of which are importantsystemic sources of Adn, whereas the levels in brown adiposetissue were not affected. We extended the analysis of proteinexpression on brown and perirenal adipose tissue 30 days postinfectionto a number of additional inflammatory markers. The acute-phasereactants ${alpha}$ -1 acid glycoprotein and SAA3, which are expressedin adipocytes, were upregulated. The expression of TNF- ${alpha}$ , IFN- ${gamma}$ ,and IL-1ß that were also increased acutely, and thesechanges persistent even to 90 days postinfection. The 3T3-L1cells, widely used as a model for primary adipocytes, were infectedwith T. cruzi. Infection triggered a reduction of Adn levels,while the levels of Toll-like receptor 2 (TLR-2), TNF- ${alpha}$ , IFN- ${gamma}$ ,and IL-1-ß were increased. In summary, this parasiteinfects and replicates within adipocytes both in vitro and invivo. Thus, we believe that adipocytes are an important targetof parasite invasion. Chagas' disease is therefore an excellentmodel to study the contributions of adipose tissue in parasiticinfections.

CONCLUDING REMARKS

This has been a targeted review, and clearly we have not performedan exhaustive review of every microorganism. For example, wehave neither dealt with other parasites nor with the fungi norwith HIV/AIDS in detail. This review of the recent contributionsfrom several laboratories, including our own, indicates thatthe adipose tissue and the adipocyte in particular contributesignificantly to the systemic interaction with infectious agents.The adipocyte can be a direct target for a number of infectiousagents and their products. These interactions have the potentialto significantly impact the innate immune response. Adiposetissue plays a major role in inflammation and therefore is amajor player in the pathogenesis of infectious diseases.

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FIG. 1. Schematic overview of the major infectious agents reported to target the adipocyte and the key adipokines release by adipocytes in response to local and systemic infection.

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FIG. 2. Representative electron micrograph of an uninfected 3T3-L1 adipocyte (A) and a cell 48 h after infection with trypomastigotes of T. cruzi. The arrows point to the amastigotes. (Reprinted from Combs et al. [25] with the permission of the publisher.)

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TABLE 1. Pathogens implicated in obesity

	ACKNOWLEDGMENTS

We acknowledge support from National Institutes of Health grantsAI-068538 and AI-052739 (H.B.T.) and DK55758, CA112023, andDK071030 (P.E.S.). P.E.S. is a recipient of an Irma T. HirschlCareer Scientist Award. M.S.D. is supported by the IDSA ERF/NFIDColin L. Powell Minority Postdoctoral Fellowship in TropicalDisease Research sponsored by GlaxoSmithKline and by the NIHTraining Grant in Mechanisms of Cardiovascular Diseases (T32HL-07675). M.S.D. is a Neuroscience Fellow of the Dominick P.Purpura Department of Neuroscience and the Department of Psychiatryand Behavioral Sciences. M.E.T. was supported by a Mentor-BasedPostdoctoral Fellowship Award from the American Diabetes Association(7-05-MI-09).

We thank Todd Schraw, Andrea Nawrocki, and Shankar Mukherjeefor assistance with the graphic designs and Louis M. Weiss forhelpful comments and discussions. In addition, we acknowledgethe technical assistance of Vicki L. Braunstein, Dazhi Zhao,and of Frank Macaluso and Leslie Gunther of the Analytical ImagingFacility.

FOOTNOTES

* Corresponding author. Mailing address: Department of Pathology, Albert Einstein College of Medicine, 1300 Morris Park Ave., Bronx, NY 10461. Phone: (718) 430-3342. Fax: (718) 430-8543. E-mail: tanowitz{at}aecom.yu.edu.

Published ahead of print on 21 November 2006.

Editor: J. B. Kaper

M.S.D., N., and M.E.T. contributed equally to this study.

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