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The Role of C/EBP Genes in Adipocyte Differentiation

Journal of Biological Chemistry1998-11-01作者：Gretchen J. Darlington, Sarah E. Ross, Ormond A. MacDougald

uncoupling protein 1 CCAAT/enhancer-binding protein peroxisome proliferator-activated receptor phosphoenolpyruvate carboxykinase untranslated region upstream stimulatory factor insulin-responsive glucose transporter stearoyl-CoA desaturase I adipocyte lipid-binding protein dexamethasone methylisobutylxanthine fatty acid synthase lipoprotein lipase. One of the central problems facing higher animals is that cells require a continuous source of energy; however, it is impractical for organisms to meet this need by supplying a constant external source of calories. Two specialized tissues, brown and white adipose tissues, have evolved to meet the ongoing requirement for energy. White adipose tissue is able to store excess calories in the form of triacylglycerol. When cells require energy, such as during periods of fasting, these needs are largely met by fatty acids and glycerol formed from lipolysis of stored triacylglycerol. Brown adipose tissues use stored triacylglycerols to maintain body temperature. In particular, these cells convert energy from fatty acid metabolism to heat through the action of uncoupling protein 1 (UCP1),1 a mitochondrial protein found only in brown adipose tissue. Brown adipocytes contain less triacylglycerol and many more mitochondria than white adipocytes, resulting in their characteristic color. Humans and rats develop brown adipose tissue depots prenatally, and although these depots largely disappear in humans during childhood, some brown adipocytes likely remain interspersed in white adipose tissue throughout adulthood (1Garruti G. Ricquier D. Int. J. Obes. Relat. Metab. Disord. 1992; 16: 383-390PubMed Google Scholar). In view of the prevalence of obesity and obesity-related diseases, such as type II diabetes, it is important to understand how white and brown adipose tissues develop and how the activities of these tissues are regulated. Many factors are important for normal adipocyte development and function. In this minireview, we explore the role of one family of transcription factors, the CCAAT/enhancer-binding proteins (C/EBPs), in inducing preadipocyte differentiation and in modulating gene expression in the fully differentiated adipocyte. Analyses of cultured cell lines, and more recently, genetically altered mice have contributed significantly to our understanding of the way in which adipose-specific gene expression is directed by C/EBPs. These models have also elucidated some of the molecular mechanisms that regulate the expression of the C/EBP genes themselves. A variety of pluripotent and preadipocyte cell lines that have been developed from mouse embryonic tissue are useful for analysis of the adipocyte differentiation program (reviewed in Ref. 2Cornelius P. MacDougald O.A. Lane M.D. Annu. Rev. Nutr. 1994; 14: 99-129Crossref PubMed Scopus (592) Google Scholar). NIH 3T3 and C3H10T1/2 are two well characterized pluripotent cell lines, which are maintained as fibroblast-like cells, but which are capable of differentiation into multiple cell types (e.g. myocytes, adipocytes, or chondrocytes (2Cornelius P. MacDougald O.A. Lane M.D. Annu. Rev. Nutr. 1994; 14: 99-129Crossref PubMed Scopus (592) Google Scholar)). Two widely studied models, 3T3-L1 and 3T3-F442A, are already committed to the adipocyte lineage and are thus considered preadipocyte cell lines. Analyses of the differentiation program in these cell lines have shown that C/EBP and PPAR transcription factors work sequentially and cooperatively to stimulate the genetic events that result in differentiation. 2A detailed account of the important role of PPARγ in preadipocyte differentiation is outside the purview of this paper; however, it has been reviewed elsewhere (3Mandrup S. Lane M.D. J. Biol. Chem. 1997; 272: 5367-5370Abstract Full Text Full Text PDF PubMed Scopus (416) Google Scholar, 4Spiegelman B.M. Diabetes. 1998; 47: 507-514Crossref PubMed Scopus (1655) Google Scholar). The molecular events associated with preadipocyte differentiation have been most thoroughly studied in 3T3-L1 cells, because they differentiate in a synchronous manner in response to dexamethasone (DEX), methylisobutylxanthine (MIX), insulin, and fetal bovine serum (Fig. 1and see Ref. 5MacDougald O.A. Lane M.D. Annu. Rev. Biochem. 1995; 64: 345-373Crossref PubMed Scopus (947) Google Scholar). This differentiation scheme routinely results in >90% of preadipocytes accumulating triacylglycerol 5 days after differentiation is initiated. Differentiation of brown adipocytes in culture has been investigated using two systems: primary brown preadipocytes (6Yubero P. Manchado C. Cassard-Doulcier A.-M. Mampel T. Vinas O. Iglesias R. Giralt M. Villarroya F. Biochem. Biophys. Res. Commun. 1994; 198: 653-659Crossref PubMed Scopus (63) Google Scholar) and HIB-1B cells, which were derived from SV40-induced brown fat tumors (7Ross S.R. Choy L. Graves R.A. Fox N. Solevjeva V. Klaus S. Ricguier D. Spiegelman B.M. Proc. Natl. Acad. Sci. U. S. A. 1992; 89: 7561-7565Crossref PubMed Scopus (114) Google Scholar) and which express the brown adipocyte marker, UCP1. The roles of C/EBPs in differentiation of brown adipocytes have not been explored. However, it is likely that C/EBPs are involved, becauseC/EBPα and C/EBPβ are expressed in these cell lines and C/EBPs induce UCP1 promoter activity. In addition, analysis of animals with targeted deletions of C/EBP genes suggests that C/EBPs regulate brown adipocyte development in vivo (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar). Role of C/EBPs in the Preadipocyte Differentiation Program—C/EBPs appear to have diverse roles in regulation of preadipocyte differentiation. After treatment of preadipocytes with inducers of differentiation, a rapid and transient increase in transcription and expression of C/EBPβ and C/EBPδ is observed (Fig. 1). Differentiating preadipocytes undergo approximately two rounds of cell division after differentiation is induced; cell proliferation ceases coincident with the transcriptional activation of C/EBPα (Fig. 1). Induction of C/EBPα is followed by transcriptional activation of many genes encoding proteins involved in creating the adipocyte phenotype (Fig. 1). (For a more complete listing of genes induced or repressed during the differentiation process see Refs. 2Cornelius P. MacDougald O.A. Lane M.D. Annu. Rev. Nutr. 1994; 14: 99-129Crossref PubMed Scopus (592) Google Scholar and 5MacDougald O.A. Lane M.D. Annu. Rev. Biochem. 1995; 64: 345-373Crossref PubMed Scopus (947) Google Scholar.)C/EBPζ (CHOP or gadd153) is expressed at relatively low levels in confluent preadipocytes and is suppressed throughout the period of clonal expansion that precedes adipogenesis. On the 4th day of differentiation, C/EBPζ is induced and remains elevated thereafter (Fig. 1). The coordinate activation of C/EBPs and adipocyte markers provides correlative evidence for the hypothesis that induction of C/EBPβ and C/EBPδ increases expression of C/EBPα, which, in turn, activates expression of adipocyte genes and thus stimulates the differentiation process. The positive actions of C/EBPα, C/EBPβ, and C/EBPδ on differentiation may be susceptible to counter-regulation by expression of C/EBPζ, which acts as a dominant-negative for C/EBPs by forming heterodimers that do not bind DNA at the consensus sites for C/EBPα, -β, and -δ. In addition, C/EBPα and C/EBPζ, two factors with antimitotic activity, may regulate preadipocyte cell devision during differentiation because clonal expansion is preceded by repression of C/EBPζ, and clonal arrest is correlated with induction of C/EBPα (reviewed in Ref.5MacDougald O.A. Lane M.D. Annu. Rev. Biochem. 1995; 64: 345-373Crossref PubMed Scopus (947) Google Scholar). C/EBPβ and C/EBPδ are the first transcription factors induced following exposure of preadipocytes to differentiation medium and were thus postulated to be involved in directing the differentiation process. In accord with this notion, expression of either C/EBPβ or C/EBPδ in preadipocytes accelerates the rate of C/EBPα induction and adipogenesis in response to hormonal inducers, indicating that both factors are stimulatory to adipogenesis (9Yeh W.-C. Cao Z. Classon M. McKnight S.L. Genes Dev. 1995; 9: 168-181Crossref PubMed Scopus (825) Google Scholar). In addition, embryonic fibroblasts from mice lacking both C/EBPβ and C/EBPδ expression are unable to differentiate in response to hormonal stimulation (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar). These cells fail to express C/EBPα and PPARγ or adipocyte markers such as 422/aP2 and PEPCK, suggesting that the absence of both C/EBPβ and C/EBPδ blocks adipogenesis. However, ectopic expression of C/EBPβ, but not C/EBPδ, in 3T3-L1 preadipocytes is sufficient to cause differentiation in the absence of DEX and MIX (9Yeh W.-C. Cao Z. Classon M. McKnight S.L. Genes Dev. 1995; 9: 168-181Crossref PubMed Scopus (825) Google Scholar). Taken together, these data suggest that, although C/EBPδ stimulates differentiation, its role may be minor, whereas C/EBPβ is an integral part of the genetic cascade that causes adipogenesis (Table I).Table ISummary of C/EBPs in development of adipocytes in culture and in vivoCell culture models, white preadipocytesKnockout mouse models1-a↓ and ↓↓ indicate decreased expression.White adipose tissueBrown adipose tissueC/EBPα Determination1-bDefined as commitment to the adipocyte lineage in cultured cells and the presence of the tissue type in vivo.Not required (9Yeh W.-C. Cao Z. Classon M. McKnight S.L. Genes Dev. 1995; 9: 168-181Crossref PubMed Scopus (825) Google Scholar, 10Wu Z. Xie Y. Bucher N.L.R. Farmer S.R. Genes Dev. 1995; 9: 2350-2363Crossref PubMed Scopus (486) Google Scholar)UnknownNot required (31Wang N.D. Finegold M.J. Bradley A. Ou C.N. Abdelsayed S.V. Wilde M.D. Taylor L.R. Wilson D.R. Darlington G.J. Science. 1995; 269: 1108-1112Crossref PubMed Scopus (851) Google Scholar) Differentiation1-cDefined as accumulating lipid and expressing adipocyte markers.Necessary and sufficient (12Lin F.-T. Lane M.D. Genes Dev. 1992; 6: 533-544Crossref PubMed Scopus (295) Google Scholar,13Lin F.-T. Lane M.D. Proc. Natl. Acad. Sci. U. S. A. 1994; 91: 8757-8761Crossref PubMed Scopus (394) Google Scholar)Important: ↓↓lipid accumulation (22, 31)Important: ↓lipid accumulation and ↓UCP1 but normal expression of 422/aP2, GLUT4, FAS (22Flodby P. Barlow C. Kylefjord H. Ahrlund-Richter L. Xanthopoulos K.G. J. Biol. Chem. 1996; 271: 24753-24760Abstract Full Text Full Text PDF PubMed Scopus (251) Google Scholar, 31Wang N.D. Finegold M.J. Bradley A. Ou C.N. Abdelsayed S.V. Wilde M.D. Taylor L.R. Wilson D.R. Darlington G.J. Science. 1995; 269: 1108-1112Crossref PubMed Scopus (851) Google Scholar)C/EBPβ DeterminationSufficient (9Yeh W.-C. Cao Z. Classon M. McKnight S.L. Genes Dev. 1995; 9: 168-181Crossref PubMed Scopus (825) Google Scholar, 10Wu Z. Xie Y. Bucher N.L.R. Farmer S.R. Genes Dev. 1995; 9: 2350-2363Crossref PubMed Scopus (486) Google Scholar)Not required (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)Not required (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar) DifferentiationSufficient (9Yeh W.-C. Cao Z. Classon M. McKnight S.L. Genes Dev. 1995; 9: 168-181Crossref PubMed Scopus (825) Google Scholar, 10Wu Z. Xie Y. Bucher N.L.R. Farmer S.R. Genes Dev. 1995; 9: 2350-2363Crossref PubMed Scopus (486) Google Scholar)Not required: normal lipid accumulation and expression of 422/aP2, adipsin, C/EBPα, LPL, PPARγ (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)Involved: ↓lipid accumulation and ↓UCP1 but normal expression of 422/aP2, C/EBPα, PPARγ, LPL (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)C/EBPδ DeterminationNot required (9Yeh W.-C. Cao Z. Classon M. McKnight S.L. Genes Dev. 1995; 9: 168-181Crossref PubMed Scopus (825) Google Scholar, 10Wu Z. Xie Y. Bucher N.L.R. Farmer S.R. Genes Dev. 1995; 9: 2350-2363Crossref PubMed Scopus (486) Google Scholar)Not required (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)Not required (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar) DifferentiationNot sufficient but accelerates (9Yeh W.-C. Cao Z. Classon M. McKnight S.L. Genes Dev. 1995; 9: 168-181Crossref PubMed Scopus (825) Google Scholar)Not required; normal lipid accumulation and expression of 422/aP2, adipsin, C/EBPα, LPL, PPARγ (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)Involved: ↓UCP1 but normal lipid accumulation and expression of 422/aP2, C/EBPα, PPARγ, LPL (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)C/EBPβ and C/EBPδ DeterminationImportant: ↓↓mass (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)Not required (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar) DifferentiationNecessary (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)Not required: normal lipid accumulation and expression of 422/aP2, adipsin, C/EBPα, LPL, PPARγ (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)Important: ↓↓UCP1 and ↓↓lipid accumulation but normal expression of 422/aP2, C/EBPα, PPARγ, LPL (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar)C/EBPζ DifferentiationRepresses (15Batchvarova N. Wang X.-Z. Ron D. EMBO J. 1995; 14: 4654-4661Crossref PubMed Scopus (209) Google Scholar)1-a ↓ and ↓↓ indicate decreased expression.1-b Defined as commitment to the adipocyte lineage in cultured cells and the presence of the tissue type in vivo.1-c Defined as accumulating lipid and expressing adipocyte markers. Open table in a new tab In addition to its involvement in the sequence of genetic events leading to preadipocyte differentiation, C/EBPβ may play a more global role in adipocyte development by causing pluripotent cells to become committed to the adipocyte lineage. Although introduction of C/EBPβ into pluripotent NIH 3T3 cells does not cause spontaneous differentiation, C/EBPβ (but notC/EBPα or C/EBPδ) confers the ability of these cells to be differentiated into adipocytes by hormonal inducers (9Yeh W.-C. Cao Z. Classon M. McKnight S.L. Genes Dev. 1995; 9: 168-181Crossref PubMed Scopus (825) Google Scholar, 10Wu Z. Xie Y. Bucher N.L.R. Farmer S.R. Genes Dev. 1995; 9: 2350-2363Crossref PubMed Scopus (486) Google Scholar). Interestingly, expression of C/EBPβ in these cells causes preadipocyte differentiation without induction of C/EBPα, perhaps indicating that C/EBPβ can functionally replace C/EBPα or that C/EBPα is not required for adipogenesis in these cells. These experiments using cultured pluripotent and preadipocyte cell lines suggest that C/EBPβ plays a dual role as a stimulator of cell determination as well as differentiation (Table I). Work from a number of investigators has solidified the correlative link between expression of C/EBPα and that of adipose-specific genes. For example, promoters from adipocyte genes such as GLUT4, SCD1, leptin (11Hwang C.-S. Mandrup S. MacDougald O.A. Geiman D.E. Lane M.D. Proc. Natl. Acad. Sci. U. S. A. 1996; 93: 873-877Crossref PubMed Scopus (174) Google Scholar), and 422/aP2 are transactivated by C/EBPs, including C/EBPα (reviewed in Ref. 5MacDougald O.A. Lane M.D. Annu. Rev. Biochem. 1995; 64: 345-373Crossref PubMed Scopus (947) Google Scholar). To show that expression of C/EBPα is necessary for preadipocyte differentiation, Lin and Lane (12Lin F.-T. Lane M.D. Genes Dev. 1992; 6: 533-544Crossref PubMed Scopus (295) Google Scholar) blocked its expression through the introduction of antisense RNA into 3T3-L1 preadipocytes. In the absence of C/EBPα, adipose-specific genes were not expressed and triacylglycerol accumulation was not detected. Also, the conditional expression of C/EBPα in stably transfected clones of 3T3-L1 preadipocytes was sufficient to bring about differentiation as measured by the cytoplasmic accumulation of lipid and the expression of 422/aP2, GLUT4, and endogenous C/EBPα (13Lin F.-T. Lane M.D. Proc. Natl. Acad. Sci. U. S. A. 1994; 91: 8757-8761Crossref PubMed Scopus (394) Google Scholar). These studies demonstrate that expression of C/EBPα is both necessary and sufficient for differentiation of 3T3-L1 preadipocytes to adipocytes (Table I). Although it cannot form homodimers, C/EBPζ avidly forms heterodimers with other C/EBP members (14Ron D. Habener J.F. Genes Dev. 1992; 6: 439-453Crossref PubMed Scopus (993) Google Scholar). Because these heterodimers cannot bind traditional C/EBP-binding sites, C/EBPζ acts as a dominant-negative C/EBP (14Ron D. Habener J.F. Genes Dev. 1992; 6: 439-453Crossref PubMed Scopus (993) Google Scholar). Consistent with this role as a sequestrant of C/EBP, enforced expression of C/EBPζ inhibits adipogenesis in 3T3-L1 preadipocytes (Table I (15Batchvarova N. Wang X.-Z. Ron D. EMBO J. 1995; 14: 4654-4661Crossref PubMed Scopus (209) Google Scholar)). It is possible that C/EBPζ also has positive effects on gene expression; C/EBPβ-C/EBPζ heterodimers bind to a novel DNA sequence and thus may redirect C/EBPs from classic C/EBP-binding sites to different elements in other promoters (16Ubeda M. Wang X.-Z. Zinszer H. Wu I. Habener J.F. Ron D. Mol. Cell. Biol. 1996; 16: 1479-1489Crossref PubMed Google Scholar). Consistent with this hypothesis, the N terminus of C/EBPζ is capable of transactivation when tethered to DNA by a heterologous DNA-binding domain (17Wang X.-Z. Ron D. Science. 1996; 272: 1347-1349Crossref PubMed Scopus (753) Google Scholar). However, to date, genes induced by C/EBPζ have not been identified. C/EBPζ causes growth arrest in a variety of cell types when it is induced by stresses such as DNA damage (18Barone M.V. Crozat A. Tabaee A. L. Ron D. Genes Dev. 1994; PubMed Scopus Google Scholar). The role of C/EBPζ in preadipocyte differentiation is not well but when induced by C/EBPζ may differentiation M. Mol. Cell. Biol. PubMed Scopus Google Scholar). its may be required for the clonal expansion of preadipocytes after induction of differentiation. Although the promoters for C/EBPα, and C/EBPζ have been only the regulation of the C/EBPα promoter has been characterized during preadipocyte differentiation. the promoter is a C/EBP consensus that by of C/EBPα as well as activation by other C/EBP family members Geiman D.E. Lane M.D. Proc. Natl. Acad. Sci. U. S. A. PubMed Scopus Google Scholar). In addition, C/EBPα at an thus its expression through an N. Wilson D.R. Taylor L.R. Abdelsayed S. Wilde M. M. Darlington G.J. Mol. Cell. Biol. 1995; PubMed Google Scholar). of C/EBPα may be more in expression is the of When the C/EBPα gene is by of the is expressed at indicating that transcription of C/EBPα is not (22Flodby P. Barlow C. Kylefjord H. Ahrlund-Richter L. Xanthopoulos K.G. J. Biol. Chem. 1996; 271: 24753-24760Abstract Full Text Full Text PDF PubMed Scopus (251) Google Scholar). important of C/EBPα transcription has been J. Geiman D. Lane M.D. Proc. Natl. Acad. Sci. U. S. A. 1998; PubMed Scopus Google Scholar). The that acts as a transcriptional of C/EBPα has elucidated a possible for gene expression of C/EBPα and suggests that is an of adipose differentiation. of regulation that may be important for expression of C/EBPs is the use of C/EBPα and C/EBPβ are from multiple in sites for C/EBPα, proteins of and and for C/EBPβ, proteins of and Although both and to be a more transcription factor and is more capable of inducing adipogenesis and F.-T. MacDougald O.A. Lane M.D. Proc. Natl. Acad. Sci. U. S. A. PubMed Scopus Google Scholar, L.R. Darlington G.J. Res. 1995; PubMed Scopus Google Scholar). In as a dominant-negative of and other C/EBPs. The of to protein to the of adipocyte differentiation, suggesting that may be a process and play a role in the of adipogenesis F.-T. MacDougald O.A. Lane M.D. Proc. Natl. Acad. Sci. U. S. A. PubMed Scopus Google Scholar, M. G. J. Biochem. 1997; PubMed Scopus Google Scholar). In addition, a in the of and their and although not in preadipocytes may for C/EBP gene expression Y. J. Biol. Chem. 1998; Full Text Full Text PDF PubMed Scopus Google Scholar). In fully differentiated adipocytes, regulation of C/EBP may be as important as regulation of of this regulation most of C/EBPs, which has been for C/EBPα N. MacDougald O.A. J. Biol. Chem. 1997; 272: Full Text Full Text PDF PubMed Scopus Google Scholar), C/EBPβ M. Cao Z. Science. 1992; PubMed Scopus Google Scholar, S. J. Biol. Chem. 1995; Full Text Full Text PDF PubMed Scopus Google Scholar), and C/EBPζ (17Wang X.-Z. Ron D. Science. 1996; 272: 1347-1349Crossref PubMed Scopus (753) Google Scholar). C/EBPα is on as many as sites in fully differentiated adipocytes N. MacDougald O.A. J. Biol. Chem. 1997; 272: Full Text Full Text PDF PubMed Scopus Google Scholar). Two of these sites are in response to treatment with or and may be important for the regulation of C/EBPα activity. C/EBPα, C/EBPβ is also in a and this process has been studied in a variety of cell by V. J. Biol. Chem. 1998; Full Text Full Text PDF PubMed Scopus Google Scholar)). its in one that C/EBPβ is in response to increases in S. J. Biol. Chem. 1995; Full Text Full Text PDF PubMed Scopus Google Scholar). This likely at in the increases in transcription of the gene for C/EBPζ has important for adipocyte differentiation. C/EBPζ is by protein at and in the transactivation and this is required for the of C/EBPζ on adipogenesis (17Wang X.-Z. Ron D. Science. 1996; 272: 1347-1349Crossref PubMed Scopus (753) Google Scholar). the sites and of be important for our understanding of C/EBP during preadipocyte differentiation and in fully differentiated studies of cells it has been possible to C/EBP and other proteins as transcriptional of adipocyte differentiation. using cultured fibroblasts and preadipocytes suggest that of C/EBPα or vivo have effects on adipose tissue we this is only Although require adipose tissues to store energy for or the in development at which fully differentiated white and brown adipocytes form In the expression by tissue of genes expressed in adipocytes 422/aP2, or lipid accumulation is observed at the of the characteristic of adipocytes in the first after (31Wang N.D. Finegold M.J. Bradley A. Ou C.N. Abdelsayed S.V. Wilde M.D. Taylor L.R. Wilson D.R. Darlington G.J. Science. 1995; 269: 1108-1112Crossref PubMed Scopus (851) Google Scholar). adipocytes appear in with the expression of adipose-specific genes in and accumulation of triacylglycerol in brown adipocytes to T. A. M. M. Biochem. J. 1995; PubMed Scopus Google Scholar). adipocytes are observed with brown and white adipocytes forming in the of M. J. Full Text PDF PubMed Scopus Google Scholar). of C/EBPs has not been during development of adipose However, of from brown adipose tissue during the days of fetal development of the and mouse indicate are already expressed (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar, T. A. M. M. Biochem. J. 1995; PubMed Scopus Google Scholar), suggesting that C/EBPs may differentiation of as they do in cultured cells. To the of C/EBP the of development in animals in expression of either C/EBPα, C/EBPβ, C/EBPδ, or both C/EBPβ and C/EBPδ have been (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar, P. Barlow C. Kylefjord H. Ahrlund-Richter L. Xanthopoulos K.G. J. Biol. Chem. 1996; 271: 24753-24760Abstract Full Text Full Text PDF PubMed Scopus (251) Google Scholar, 31Wang N.D. Finegold M.J. Bradley A. Ou C.N. Abdelsayed S.V. Wilde M.D. Taylor L.R. Wilson D.R. Darlington G.J. Science. 1995; 269: 1108-1112Crossref PubMed Scopus (851) Google Scholar, I. L. P. A. D. C. S. D. G. F. L. R. A. G. F. V. EMBO J. 1995; 14: PubMed Scopus Google Scholar). Analyses of these models have to the roles of C/EBPs in adipocyte development and function. The phenotype of mice for a in the gene for C/EBPα is with in and to at (22Flodby P. Barlow C. Kylefjord H. Ahrlund-Richter L. Xanthopoulos K.G. J. Biol. Chem. 1996; 271: 24753-24760Abstract Full Text Full Text PDF PubMed Scopus (251) Google Scholar, 31Wang N.D. Finegold M.J. Bradley A. Ou C.N. Abdelsayed S.V. Wilde M.D. Taylor L.R. Wilson D.R. Darlington G.J. Science. 1995; 269: 1108-1112Crossref PubMed Scopus (851) Google Scholar). The because of of a of mice for periods of to (Table I). of these animals the important role of C/EBPα for lipid accumulation (Table I). White adipocytes in type mice have cytoplasmic lipid after In sites in mice do not have cells lipid in the or in the region at this brown adipose tissue is in animals of both However, brown adipocytes mice also show in lipid mice do not lipid in brown adipose tissue normal expression of adipocyte markers GLUT4, and lipid brown adipocytes mice show altered expression of which is at and remains at These evidence is important for the differentiation of adipose tissue. Although C/EBPβ has many including in and and Ref. V. J. Biol. Chem. 1998; Full Text Full Text PDF PubMed Scopus Google Scholar), is on white adipocyte development or function. are normal in and and in their expression of adipocyte markers adipsin, C/EBPα, PPARγ, and The that C/EBPβ is not required for development of white adipose tissue is in view of the important role of C/EBPβ in cultured adipocytes, its expression can cause cell determination and differentiation (Table I). This suggests that although C/EBPβ may be sufficient in cultured cells, it is not necessary for differentiation of white adipose In brown adipose the absence of C/EBPβ to lipid accumulation and a in UCP1 Although brown adipose tissue is commitment to the brown adipose lineage is not other C/EBP family members are expressed (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar). mice are to type in and and show in white or brown adipose (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar). It that the role of C/EBPδ in adipocyte differentiation is minor, because its absence does not the accumulation of lipid or the expression of adipocyte markers PEPCK, C/EBPα, and PPARγ, I). This is with using cultured cells, expression of C/EBPδ is to induce although it in differentiation by induced adipogenesis (Table I). C/EBPδ may in the differentiation of brown adipose tissue. Although brown adipocytes mice fat these cells to have UCP1 with the brown adipocyte may be in mice (Table but C/EBPδ is not required for determination of this tissue Although the absence of C/EBPβ or C/EBPδ in adipose tissues results in an of both has (Table mice have of of these mice their and by less than remain (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar). The of C/EBPβ and C/EBPδ for white adipose tissue was in this of mice by the adipose tissue from type and adipose in the animals was only of that in type fat cells this tissue were normal in and suggesting that the in adipose was because of a in fat cell This that C/EBPβ and C/EBPδ are important in determination of the adipocyte because in their cells become committed to adipocyte development (Table I). cells are to become adipocytes, however, their differentiation does not appear to be by the absence of C/EBPβ and the expression of 422/aP2, adipsin, and LPL is normal in mice (8Tanaka T. Yoshida N. Kishimoto T. Akira S. EMBO J. 1997; 16: 7432-7443Crossref PubMed Scopus (655) Google Scholar). C/EBPβ and C/EBPδ may be more important for differentiation of brown than of white adipose Brown adipocytes mice contain lipid at after and the expression of in these mice is less than of that of type This phenotype suggests that differentiation of brown adipocytes is blocked in mice (Table I). of cultured cell lines has to a in which C/EBPs play integral roles in determination and differentiation of preadipocytes. In this of white adipocyte C/EBPβ cells to the preadipocyte C/EBPβ and C/EBPδ the differentiation C/EBPβ and C/EBPα stimulate and C/EBPζ differentiation (Table I). The of this is largely by from animals for C/EBPs, which suggest that C/EBPβ and C/EBPδ are important for determination to the preadipocyte lineage and that C/EBPα is important for differentiation to the adipocyte these genetically mice evidence for the of C/EBPα, C/EBPβ, and C/EBPδ for normal lipid accumulation and expression of UCP1 in brown adipose tissue. the requirement for C/EBPs in other tissues, analysis of adipose tissues, because most C/EBP mice in from to fat This the of creating models with which to the of C/EBPs in adipocyte For example, animals in which C/EBPs are only in adipose be useful for the of C/EBPs in adipose tissue without the and associated with C/EBP in and other In addition, development of conditional adipose-specific the of gene expression in adipose be development of one C/EBP gene is by such that, for activation of the C/EBPα promoter results in expression of with these animals between in the of C/EBPs and because of the of their The of C/EBP transcription factors and the for these to and functionally with other such as and cell proteins and the of understanding C/EBPs and their mechanisms of In addition, C/EBPs the of other factors, such as PPARγ, that can or with C/EBPs to regulate adipocyte differentiation. The of be to work on C/EBPs and other factors into a of white and brown adipose tissue development that for of obesity and type II

Understanding Adipocyte Differentiation

Physiological Reviews1998-01-07作者：Francine M. Gregoire, Cynthia M. Smas, Hei Sook Sul

The adipocyte plays a critical role in energy balance. Adipose tissue growth involves an increase in adipocyte size and the formation of new adipocytes from precursor cells. For the last 20 years, the cellular and molecular mechanisms of adipocyte differentiation have been extensively studied using preadipocyte culture systems. Committed preadipocytes undergo growth arrest and subsequent terminal differentiation into adipocytes. This is accompanied by a dramatic increase in expression of adipocyte genes including adipocyte fatty acid binding protein and lipid-metabolizing enzymes. Characterization of regulatory regions of adipose-specific genes has led to the identification of the transcription factors peroxisome proliferator-activated receptor-gamma (PPAR-gamma) and CCAAT/enhancer binding protein (C/EBP), which play a key role in the complex transcriptional cascade during adipocyte differentiation. Growth and differentiation of preadipocytes is controlled by communication between individual cells or between cells and the extracellular environment. Various hormones and growth factors that affect adipocyte differentiation in a positive or negative manner have been identified. In addition, components involved in cell-cell or cell-matrix interactions such as preadipocyte factor-1 and extracellular matrix proteins are also pivotal in regulating the differentiation process. Identification of these molecules has yielded clues to the biochemical pathways that ultimately result in transcriptional activation via PPAR-gamma and C/EBP. Studies on the regulation of the these transcription factors and the mode of action of various agents that influence adipocyte differentiation will reveal the physiological and pathophysiological mechanisms underlying adipose tissue development.

Epidemiology Physiology Molecular Biology

Adipocyte Turnover: Relevance to Human Adipose Tissue Morphology

Diabetes2009-10-19作者：Erik Arner, Pål O. Westermark, Kirsty L. Spalding

OBJECTIVE: Adipose tissue may contain few large adipocytes (hypertrophy) or many small adipocytes (hyperplasia). We investigated factors of putative importance for adipose tissue morphology. RESEARCH DESIGN AND METHODS: Subcutaneous adipocyte size and total fat mass were compared in 764 subjects with BMI 18-60 kg/m(2). A morphology value was defined as the difference between the measured adipocyte volume and the expected volume given by a curved-line fit for a given body fat mass and was related to insulin values. In 35 subjects, in vivo adipocyte turnover was measured by exploiting incorporation of atmospheric (14)C into DNA. RESULTS: Occurrence of hyperplasia (negative morphology value) or hypertrophy (positive morphology value) was independent of sex and body weight but correlated with fasting plasma insulin levels and insulin sensitivity, independent of adipocyte volume (beta-coefficient = 0.3, P < 0.0001). Total adipocyte number and morphology were negatively related (r = -0.66); i.e., the total adipocyte number was greatest in pronounced hyperplasia and smallest in pronounced hypertrophy. The absolute number of new adipocytes generated each year was 70% lower (P < 0.001) in hypertrophy than in hyperplasia, and individual values for adipocyte generation and morphology were strongly related (r = 0.7, P < 0.001). The relative death rate (approximately 10% per year) or mean age of adipocytes (approximately 10 years) was not correlated with morphology. CONCLUSIONS: Adipose tissue morphology correlates with insulin measures and is linked to the total adipocyte number independently of sex and body fat level. Low generation rates of adipocytes associate with adipose tissue hypertrophy, whereas high generation rates associate with adipose hyperplasia.

Epidemiology Physiology Cardiology and Cardiovascular Medicine

Cancer-Associated Adipocytes Exhibit an Activated Phenotype and Contribute to Breast Cancer Invasion

Cancer Research2011-03-31作者：Béatrice Dirat, Ludivine Bochet, Marta Dabek

Early local tumor invasion in breast cancer results in a likely encounter between cancer cells and mature adipocytes, but the role of these fat cells in tumor progression remains unclear. We show that murine and human tumor cells cocultivated with mature adipocytes exhibit increased invasive capacities in vitro and in vivo, using an original two-dimensional coculture system. Likewise, adipocytes cultivated with cancer cells also exhibit an altered phenotype in terms of delipidation and decreased adipocyte markers associated with the occurrence of an activated state characterized by overexpression of proteases, including matrix metalloproteinase-11, and proinflammatory cytokines [interleukin (IL)-6, IL-1β]. In the case of IL-6, we show that it plays a key role in the acquired proinvasive effect by tumor cells. Equally important, we confirm the presence of these modified adipocytes in human breast tumors by immunohistochemistry and quantitative PCR. Interestingly, the tumors of larger size and/or with lymph nodes involvement exhibit the higher levels of IL-6 in tumor surrounding adipocytes. Collectively, all our data provide in vitro and in vivo evidence that (i) invasive cancer cells dramatically impact surrounding adipocytes; (ii) peritumoral adipocytes exhibit a modified phenotype and specific biological features sufficient to be named cancer-associated adipocytes (CAA); and (iii) CAAs modify the cancer cell characteristics/phenotype leading to a more aggressive behavior. Our results strongly support the innovative concept that adipocytes participate in a highly complex vicious cycle orchestrated by cancer cells to promote tumor progression that might be amplified in obese patients.

Oncology Epidemiology Genetics

Adipocyte Death, Adipose Tissue Remodeling, and Obesity Complications

Diabetes2007-09-12作者：Katherine J. Strissel, Zlatina S. Stancheva, Hideaki Miyoshi

OBJECTIVE: We sought to determine the role of adipocyte death in obesity-induced adipose tissue (AT) inflammation and obesity complications. RESEARCH DESIGN AND METHODS: Male C57BL/6 mice were fed a high-fat diet for 20 weeks to induce obesity. Every 4 weeks, insulin resistance was assessed by intraperitoneal insulin tolerance tests, and epididymal (eAT) and inguinal subcutaneous AT (iAT) and livers were harvested for histological, immunohistochemical, and gene expression analyses. RESULTS: Frequency of adipocyte death in eAT increased from <0.1% at baseline to 16% at week 12, coincident with increases in 1) depot weight; 2) AT macrophages (ATM Phi s) expressing F4/80 and CD11c; 3) mRNA for tumor necrosis factor (TNF)-alpha, monocyte chemotactic protein (MCP)-1, and interleukin (IL)-10; and 4) insulin resistance. ATM Phi s in crown-like structures surrounding dead adipocytes expressed TNF-alpha and IL-6 proteins. Adipocyte number began to decline at week 12. At week 16, adipocyte death reached approximately 80%, coincident with maximal expression of CD11c and inflammatory genes, loss (40%) of eAT mass, widespread collagen deposition, and accelerated hepatic macrosteatosis. By week 20, adipocyte number was restored with small adipocytes, coincident with reduced adipocyte death (fourfold), CD11c and MCP-1 gene expression (twofold), and insulin resistance (35%). eAT weight did not increase at week 20 and was inversely correlated with liver weight after week 12 (r = -0. 85, P < 0.001). In iAT, adipocyte death was first detected at week 12 and remained <or=3%. CONCLUSIONS: These results implicate depot-selective adipocyte death and M Phi-mediated AT remodeling in inflammatory and metabolic complications of murine obesity.

Epidemiology Physiology Cardiology and Cardiovascular Medicine

The emergence of cold-induced brown adipocytes in mouse white fat depots is determined predominantly by white to brown adipocyte transdifferentiation

American Journal of Physiology-Endocrinology and Metabolism2010-03-30作者：Giorgio Barbatelli, I. Murano, Lise Madsen

The origin of brown adipocytes arising in white adipose tissue (WAT) after cold acclimatization is unclear. Here, we demonstrate that several UCP1-immunoreactive brown adipocytes occurring in WAT after cold acclimatization have a mixed morphology (paucilocular adipocytes). These cells also had a mixed mitochondrioma with classic "brown" and "white" mitochondria, suggesting intermediate steps in the process of direct transformation of white into brown adipocytes (transdifferentiation). Quantitative electron microscopy disclosed that cold exposure (6 degrees C for 10 days) did not induce an increase in WAT preadipocytes. beta(3)-adrenoceptor-knockout mice had a blunted brown adipocyte occurrence upon cold acclimatization. Administration of the beta(3)-adrenoceptor agonist CL316,243 induced the occurrence of brown adipocytes, with the typical morphological features found after cold acclimatization. In contrast, administration of the beta(1)-adrenoceptor agonist xamoterol increased only the number of preadipocytes. These findings indicate that transdifferentiation depends on beta(3)-adrenoceptor activation, whereas preadipocyte recruitment is mediated by beta(1)-adrenoceptor. RT-qPCR experiments disclosed that cold exposure induced enhanced expression of the thermogenic genes and of genes expressed selectively in brown adipose tissue (iBAT) and in both interscapular BAT and WAT. beta(3)-adrenoceptor suppression blunted their expression only in WAT. Furthermore, cold acclimatization induced an increased WAT expression of the gene coding for C/EBPalpha (an antimitotic protein), whereas Ccna1 expression (related to cell proliferation) was unchanged. Overall, our data strongly suggest that the cold-induced emergence of brown adipocytes in WAT predominantly reflects beta(3)-adrenoceptor-mediated transdifferentiation.

Physiology Epidemiology Nutrition and Dietetics

The Fate of Adipocytes after Nonvascularized Fat Grafting

Plastic & Reconstructive Surgery2012-01-19作者：Hitomi Eto, Harunosuke Kato, Hirotaka Suga

BACKGROUND: Clinical outcomes following fat grafting are variable and technique dependent, and it is unknown how the graft is revascularized. The authors recently observed that living and dead adipocytes can be differentiated not with hematoxylin and eosin staining but with immunohistochemistry for perilipin. METHODS: The viability of cellular components (adipocytes, adipose stem/stromal/progenitor cells, vascular endothelial cells, and hematopoietic cells) in human adipose tissue was evaluated using (1) stored lipoaspirates, (2) cultured cells, and (3) organ-cultured adipose tissue. In addition, the groin fat pad (150 to 200 mg) in mice was transplanted under the scalp, and the graft was stained at 0, 1, 2, 3, 5, 7, or 14 days. RESULTS: In vitro studies revealed that adipocytes are most susceptible to death under ischemic conditions, although adipose-derived stromal cells can remain viable for 3 days. The in vivo study indicated that most adipocytes in the graft began to die on day 1, and only some of the adipocytes located within 300 μm of the tissue edge survived. The number of proliferating cells increased from day 3, and an increase in viable adipocyte area was detected from day 7, suggesting that repair/regeneration of the dead tissue had begun. CONCLUSIONS: The authors show convincing evidence of very dynamic remodeling of adipose tissue after nonvascularized grafting. The authors observed three zones from the periphery to the center of the graft: the surviving area (adipocytes survived), the regenerating area (adipocytes died, adipose-derived stromal cells survived, and dead adipocytes were replaced with new ones), and the necrotic area (both adipocytes and adipose-derived stromal cells died).

Genetics Surgery Rehabilitation

Proinflammatory Phenotype of Perivascular Adipocytes

Circulation Research2009-01-03作者：Tapan K. Chatterjee, Lynn L. Stoll, Gerene M. Denning

Adipose tissue depots originate from distinct precursor cells, are functionally diverse, and modulate disease processes in a depot-specific manner. However, the functional properties of perivascular adipocytes, and their influence on disease of the blood vessel wall, remain to be determined. We show that human coronary perivascular adipocytes exhibit a reduced state of adipocytic differentiation as compared with adipocytes derived from subcutaneous and visceral (perirenal) adipose depots. Secretion of antiinflammatory adiponectin is markedly reduced, whereas that of proinflammatory cytokines interleukin-6, interleukin-8, and monocyte chemoattractant protein-1, is markedly increased in perivascular adipocytes. These depot-specific differences in adipocyte function are demonstrable in both freshly isolated adipose tissues and in vitro-differentiated adipocytes. Murine aortic arch perivascular adipose tissues likewise express lower levels of adipocyte-associated genes as compared with subcutaneous and visceral adipose tissues. Moreover, 2 weeks of high-fat feeding caused further reductions in adipocyte-associated gene expression, while upregulating proinflammatory gene expression, in perivascular adipose tissues. These changes were observed in the absence of macrophage recruitment to the perivascular adipose depot. We conclude that perivascular adipocytes exhibit reduced differentiation and a heightened proinflammatory state, properties that are intrinsic to the adipocytes residing in this depot. Dysfunction of perivascular adipose tissue induced by fat feeding suggests that this unique adipose depot is capable of linking metabolic signals to inflammation in the blood vessel wall.

Cardiology and Cardiovascular Medicine Surgery Epidemiology

Adipocyte death defines macrophage localization and function in adipose tissue of obese mice and humans

Journal of Lipid Research2005-09-09作者：Saverio Cinti, Grant A. Mitchell, Giorgio Barbatelli

Macrophage infiltration of white adipose tissue (WAT) is implicated in the metabolic complications of obesity. The precipitating event(s) and function(s) of macrophage infiltration into WAT are unknown. We demonstrate that >90% of all macrophages in WAT of obese mice and humans are localized to dead adipocytes, where they fuse to form syncytia that sequester and scavenge the residual "free" adipocyte lipid droplet and ultimately form multinucleate giant cells, a hallmark of chronic inflammation. Adipocyte death increases in obese (db/db) mice (30-fold) and humans and exhibits ultrastructural features of necrosis (but not apoptosis). These observations identify necrotic-like adipocyte death as a pathologic hallmark of obesity and suggest that scavenging of adipocyte debris is an important function of WAT macrophages in obese individuals. The frequency of adipocyte death is positively correlated with increased adipocyte size in obese mice and humans and in hormone-sensitive lipase-deficient (HSL-/-) mice, a model of adipocyte hypertrophy without increased adipose mass. WAT of HSL-/- mice exhibited a 15-fold increase in necrotic-like adipocyte death and formation of macrophage syncytia, coincident with increased tumor necrosis factor-alpha gene expression. These results provide a novel framework for understanding macrophage recruitment, function, and persistence in WAT of obese individuals.

Epidemiology Physiology Cardiology and Cardiovascular Medicine

<i>FTO</i> Obesity Variant Circuitry and Adipocyte Browning in Humans

New England Journal of Medicine2015-08-19作者：Melina Claussnitzer, Simon N. Dankel, Kyoung-Han Kim

BACKGROUND: Genomewide association studies can be used to identify disease-relevant genomic regions, but interpretation of the data is challenging. The FTO region harbors the strongest genetic association with obesity, yet the mechanistic basis of this association remains elusive. METHODS: We examined epigenomic data, allelic activity, motif conservation, regulator expression, and gene coexpression patterns, with the aim of dissecting the regulatory circuitry and mechanistic basis of the association between the FTO region and obesity. We validated our predictions with the use of directed perturbations in samples from patients and from mice and with endogenous CRISPR-Cas9 genome editing in samples from patients. RESULTS: Our data indicate that the FTO allele associated with obesity represses mitochondrial thermogenesis in adipocyte precursor cells in a tissue-autonomous manner. The rs1421085 T-to-C single-nucleotide variant disrupts a conserved motif for the ARID5B repressor, which leads to derepression of a potent preadipocyte enhancer and a doubling of IRX3 and IRX5 expression during early adipocyte differentiation. This results in a cell-autonomous developmental shift from energy-dissipating beige (brite) adipocytes to energy-storing white adipocytes, with a reduction in mitochondrial thermogenesis by a factor of 5, as well as an increase in lipid storage. Inhibition of Irx3 in adipose tissue in mice reduced body weight and increased energy dissipation without a change in physical activity or appetite. Knockdown of IRX3 or IRX5 in primary adipocytes from participants with the risk allele restored thermogenesis, increasing it by a factor of 7, and overexpression of these genes had the opposite effect in adipocytes from nonrisk-allele carriers. Repair of the ARID5B motif by CRISPR-Cas9 editing of rs1421085 in primary adipocytes from a patient with the risk allele restored IRX3 and IRX5 repression, activated browning expression programs, and restored thermogenesis, increasing it by a factor of 7. CONCLUSIONS: Our results point to a pathway for adipocyte thermogenesis regulation involving ARID5B, rs1421085, IRX3, and IRX5, which, when manipulated, had pronounced pro-obesity and anti-obesity effects. (Funded by the German Research Center for Environmental Health and others.).

Genetics Endocrine and Autonomic Systems Molecular Biology

MicroRNA-143 Regulates Adipocyte Differentiation

Journal of Biological Chemistry2004-10-26作者：Christine Esau, Xiaolin Kang, Eigen Peralta

MicroRNAs (miRNAs) are endogenously expressed 20-24 nucleotide RNAs thought to repress protein translation through binding to a target mRNA (1-3). Only a few of the more than 250 predicted human miRNAs have been assigned any biological function. In an effort to uncover miRNAs important during adipocyte differentiation, antisense oligonucleotides (ASOs) targeting 86 human miRNAs were transfected into cultured human pre-adipocytes, and their ability to modulate adipocyte differentiation was evaluated. Expression of 254 miRNAs in differentiating adipocytes was also examined on a miRNA microarray. Here we report that the combination of expression data and functional assay results identified a role for miR-143 in adipocyte differentiation. miR-143 levels increased in differentiating adipocytes, and inhibition of miR-143 effectively inhibited adipocyte differentiation. In addition, protein levels of the proposed miR-143 target ERK5 (4) were higher in ASO-treated adipocytes. These results demonstrate that miR-143 is involved in adipocyte differentiation and may act through target gene ERK5.

Cancer Research Molecular Biology Cancer Research

Adipogenesis: From Stem Cell to Adipocyte

Annual Review of Biochemistry2012-05-22作者：Qi Qun Tang, M. Daniel Lane

Excessive caloric intake without a rise in energy expenditure promotes adipocyte hyperplasia and adiposity. The rise in adipocyte number is triggered by signaling factors that induce conversion of mesenchymal stem cells (MSCs) to preadipocytes that differentiate into adipocytes. MSCs, which are recruited from the vascular stroma of adipose tissue, provide an unlimited supply of adipocyte precursors. Members of the BMP and Wnt families are key mediators of stem cell commitment to produce preadipocytes. Following commitment, exposure of growth-arrested preadipocytes to differentiation inducers [insulin-like growth factor 1 (IGF1), glucocorticoid, and cyclic AMP (cAMP)] triggers DNA replication and reentry into the cell cycle (mitotic clonal expansion). Mitotic clonal expansion involves a transcription factor cascade, followed by the expression of adipocyte genes. Critical to these events are phosphorylations of the transcription factor CCATT enhancer-binding protein β (C/EBPβ) by MAP kinase and GSK3β to produce a conformational change that gives rise to DNA-binding activity. "Activated" C/EBPβ then triggers transcription of peroxisome proliferator-activated receptor-γ (PPARγ) and C/EBPα, which in turn coordinately activate genes whose expression produces the adipocyte phenotype.

Physiology Molecular Biology Molecular Biology

mPPAR gamma 2: tissue-specific regulator of an adipocyte enhancer.

Genes & Development1994-05-15作者：Peter Tontonoz, E Hu, Reed A. Graves

Previously, we have isolated and characterized an enhancer from the 5'-flanking region of the adipocyte P2 (aP2) gene that directs high-level adipocyte-specific gene expression in both cultured cells and transgenic mice. The key regulator of this enhancer is a cell type-restricted nuclear factor termed ARF6. Target sequences for ARF6 in the aP2 enhancer exhibit homology to a direct repeat of hormone response elements (HREs) spaced by one nucleotide; this motif (DR-1) has been demonstrated previously to be the preferred binding site for heterodimers of the retinoid X receptor (RXR) and the peroxisome proliferator-activated receptor (PPAR). We have cloned a novel member of the peroxisome proliferator-activated receptor family designated mPPAR gamma 2, and we demonstrate that a heterodimeric complex of mPPAR gamma 2 and RXR alpha constitute a functional ARF6 complex. Expression of mPPAR gamma 2 is induced very early during the differentiation of several cultured adipocyte cell lines and is strikingly adipose-specific in vivo. mPPAR gamma 2 and RXR alpha form heterodimers on ARF6-binding sites in vitro, and antiserum to RXR alpha specifically inhibits ARF6 activity in adipocyte nuclear extracts. Moreover, forced expression of mPPAR gamma 2 and RXR alpha activates the adipocyte-specific aP2 enhancer in cultured fibroblasts, and this activation is potentiated by peroxisome proliferators, fatty acids, and 9-cis retinoic acid. These results identify mPPAR gamma 2 as the first adipocyte-specific transcription factor and suggest mechanisms whereby fatty acids, peroxisome proliferators, 9-cis retinoic acid, and other lipids may regulate adipocyte gene expression and differentiation.

Molecular Biology Molecular Biology Cellular and Molecular Neuroscience

Chemerin, a Novel Adipokine That Regulates Adipogenesis and Adipocyte Metabolism

Journal of Biological Chemistry2007-07-18作者：Kerry B. Goralski, Tanya C. McCarthy, Elyisha A. Hanniman

Obesity is an alarming primary health problem and is an independent risk factor for type II diabetes, cardiovascular diseases, and hypertension. Although the pathologic mechanisms linking obesity with these co-morbidities are most likely multifactorial, increasing evidence indicates that altered secretion of adipose-derived signaling molecules (adipokines; e.g. adiponectin, leptin, and tumor necrosis factor alpha) and local inflammatory responses are contributing factors. Chemerin (RARRES2 or TIG2) is a recently discovered chemoattractant protein that serves as a ligand for the G protein-coupled receptor CMKLR1 (ChemR23 or DEZ) and has a role in adaptive and innate immunity. Here we show an unexpected, high level expression of chemerin and its cognate receptor CMKLR1 in mouse and human adipocytes. Cultured 3T3-L1 adipocytes secrete chemerin protein, which triggers CMKLR1 signaling in adipocytes and other cell types and stimulates chemotaxis of CMKLR1-expressing cells. Adenoviral small hairpin RNA targeted knockdown of chemerin or CMKLR1 expression impairs differentiation of 3T3-L1 cells into adipocytes, reduces the expression of adipocyte genes involved in glucose and lipid homeostasis, and alters metabolic functions in mature adipocytes. We conclude that chemerin is a novel adipose-derived signaling molecule that regulates adipogenesis and adipocyte metabolism.

Epidemiology Physiology Pharmacology

Relationship between Adipocyte Size and Adipokine Expression and Secretion

The Journal of Clinical Endocrinology & Metabolism2006-12-13作者：Thomas Skurk, C Alberti-Huber, Christian Herder

CONTEXT: Adipocytes are known to release a variety of factors that may contribute to the proinflammatory state characteristic for obesity. This secretory function is considered to provide the basis for obesity-related complications such as type 2 diabetes and atherosclerosis. OBJECTIVE: To get a better insight into possible underlying mechanisms, we investigated the effect of adipocyte size on adipokine production and secretion. DESIGN, PATIENTS, AND MAIN OUTCOME MEASURES: Protein secretion and mRNA expression in cultured adipocytes separated according to cell size from 30 individuals undergoing elective plastic surgery were investigated. RESULTS: The mean adipocyte volume of the four fractions ranged from 205 +/- 146 to 1.077 +/- 471 pl. There were strong linear correlations for the secretion of adipokines over time. Secretion of leptin, IL-6, IL-8, TNF-alpha, monocyte chemoattractant protein-1, interferon-gamma-inducible protein 10, macrophage inflammatory protein-1beta, granulocyte colony stimulating factor, IL-1ra, and adiponectin was positively correlated with cell size. After correction for cell surface, there was still a significant difference between fraction IV (very large) and fraction I (small cells), for leptin, IL-6, IL-8, monocyte chemoattractant protein-1, and granulocyte colony-stimulating factor. In contrast, antiinflammatory factors such as IL-1ra and adiponectin lost their association after correction for cell surface area comparing fraction I and IV. In addition, there was a decrease of IL-10 secretion with increasing cell size. CONCLUSIONS: The results clearly suggest that adipocyte size is an important determinant of adipokine secretion. There seems to be a differential expression of pro- and antiinflammatory factors with increasing adipocyte size resulting in a shift toward dominance of proinflammatory adipokines largely as a result of a dysregulation of hypertrophic, very large cells.

Epidemiology Endocrine and Autonomic Systems Physiology

Chronic Peroxisome Proliferator-activated Receptor γ (PPARγ) Activation of Epididymally Derived White Adipocyte Cultures Reveals a Population of Thermogenically Competent, UCP1-containing Adipocytes Molecularly Distinct from Classic Brown Adipocytes

Journal of Biological Chemistry2009-12-23作者：Nataša Petrovič, Tomas B. Waldén, Irina G. Shabalina

The recent insight that brown adipocytes and muscle cells share a common origin and in this respect are distinct from white adipocytes has spurred questions concerning the origin and molecular characteristics of the UCP1-expressing cells observed in classic white adipose tissue depots under certain physiological or pharmacological conditions. Examining precursors from the purest white adipose tissue depot (epididymal), we report here that chronic treatment with the peroxisome proliferator-activated receptor gamma agonist rosiglitazone promotes not only the expression of PGC-1alpha and mitochondriogenesis in these cells but also a norepinephrine-augmentable UCP1 gene expression in a significant subset of the cells, providing these cells with a genuine thermogenic capacity. However, although functional thermogenic genes are expressed, the cells are devoid of transcripts for the novel transcription factors now associated with classic brown adipocytes (Zic1, Lhx8, Meox2, and characteristically PRDM16) or for myocyte-associated genes (myogenin and myomirs (muscle-specific microRNAs)) and retain white fat characteristics such as Hoxc9 expression. Co-culture experiments verify that the UCP1-expressing cells are not proliferating classic brown adipocytes (adipomyocytes), and these cells therefore constitute a subset of adipocytes ("brite" adipocytes) with a developmental origin and molecular characteristics distinguishing them as a separate class of cells.

Physiology Epidemiology Rehabilitation

The Perfect Storm: Obesity, Adipocyte Dysfunction, and Metabolic Consequences

Clinical Chemistry2008-04-24作者：Sarah D. de Ferranti, Dariush Mozaffarian

BACKGROUND: As the prevalence of adiposity soars in both developed and developing nations, appreciation of the close links between obesity and disease increases. The strong relationships between excess adipose tissue and poor health outcomes, including cardiovascular disease, diabetes, and cancer, mandate elucidation of the complex cellular, hormonal, and molecular pathophysiology whereby adiposity initiates and maintains adverse health effects. CONTENT: In this report we review adipocyte metabolism and function in the context of energy imbalance and postprandial nutrient excess, including adipocyte hypertrophy and hyperplasia, adipocyte dysfunction, and other systemic consequences. We also discuss implications for laboratory evaluation and clinical care, including the role of lifestyle modifications. Chronic energy imbalance produces adipocyte hypertrophy and hyperplasia, endoplasmic reticulum stress, and mitochondrial dysfunction. These processes lead to increased intracellular and systemic release of adipokines, free fatty acids, and inflammatory mediators that cause adipocyte dysfunction and induce adverse effects in the liver, pancreatic beta-cells, and skeletal muscle as well as the heart and vascular beds. Several specialized laboratory tests can quantify these processes and predict clinical risk, but translation to the clinical setting is premature. Current and future pharmacologic interventions may target these pathways; modest changes in diet, physical activity, weight, and smoking are likely to have the greatest impact. SUMMARY: Adipocyte endoplasmic reticulum and mitochondrial stress, and associated changes in circulating adipokines, free fatty acids, and inflammatory mediators, are central to adverse health effects of adiposity. Future investigation should focus on these pathways and on reversing the adverse lifestyle behaviors that are the fundamental causes of adiposity.

Epidemiology Physiology Cardiology and Cardiovascular Medicine

A Paracrine Loop Between Adipocytes and Macrophages Aggravates Inflammatory Changes

Arteriosclerosis Thrombosis and Vascular Biology2005-08-26作者：Takayoshi Suganami, Junko Nishida, Yoshihiro Ogawa

OBJECTIVE: Weight gain is associated with infiltration of fat by macrophages, suggesting that they are an important source of inflammation in obese adipose tissue. Here we developed an in vitro coculture system composed of adipocytes and macrophages and examined the molecular mechanism whereby these cells communicate. METHODS AND RESULTS: Coculture of differentiated 3T3-L1 adipocytes and macrophage cell line RAW264 results in the marked upregulation of proinflammatory cytokines, such as tumor necrosis factor alpha (TNF-alpha), and the downregulation of the antiinflammatory cytokine adiponectin. Such inflammatory changes are induced by the coculture without direct contact, suggesting the role of soluble factors. A neutralizing antibody to TNF-alpha, which occurs mostly in macrophages, inhibits the inflammatory changes in 3T3-L1, suggesting that TNF-alpha is a major macrophage-derived mediator of inflammation in adipocytes. Conversely, free fatty acids (FFAs) may be important adipocyte-derived mediators of inflammation in macrophages, because the production of TNF-alpha in RAW264 is markedly increased by palmitate, a major FFA released from 3T3-L1. The inflammatory changes in the coculture are augmented by use of either hypertrophied 3T3-L1 or adipose stromal vascular fraction obtained from obese ob/ob mice. CONCLUSIONS: We postulate that a paracrine loop involving FFAs and TNF-alpha between adipocytes and macrophages establishes a vicious cycle that aggravates inflammatory changes in the adipose tissue.

Epidemiology Physiology Cardiology and Cardiovascular Medicine

A Novel Serum Protein Similar to C1q, Produced Exclusively in Adipocytes

Journal of Biological Chemistry1995-11-01作者：Philipp E. Scherer, Suzanne Williams, M Fogliano

We describe a novel 30-kDa secretory protein, Acrp30 (adipocyte complement-related protein of 30 kDa), that is made exclusively in adipocytes and whose mRNA is induced over 100-fold during adipocyte differentiation. Acrp30 is structurally similar to complement factor C1q and to a hibernation-specific protein isolated from the plasma of Siberian chipmunks; it forms large homo-oligomers that undergo a series of post-translational modifications. Like adipsin, secretion of Acrp30 is enhanced by insulin, and Acrp30 is an abundant serum protein. Acrp30 may be a factor that participates in the delicately balanced system of energy homeostasis involving food intake and carbohydrate and lipid catabolism. Our experiments also further corroborate the existence of an insulin-regulated secretory pathway in adipocytes.

Physiology Immunology Immunology

Thematic review series: Adipocyte Biology. Adipocyte stress: the endoplasmic reticulum and metabolic disease

Journal of Lipid Research2007-05-10作者：Margaret F. Gregor, Gökhan S. Hotamışlıgil

In the context of obesity and its related maladies, the adipocyte plays a central role in the balance, or imbalance, of metabolic homeostasis. An obese, hypertrophic adipocyte is challenged by many insults, including surplus energy, inflammation, insulin resistance, and considerable stress to various organelles. The endoplasmic reticulum (ER) is one such vital organelle that demonstrates significant signs of stress and dysfunction in obesity and insulin resistance. Under normal conditions, the ER must function in the unique and trying environment of the adipocyte, adapting to meet the demands of increased protein synthesis and secretion, energy storage in the form of triglyceride droplet formation, and nutrient sensing that are particular to the differentiated fat cell. When nutrients are in pathological excess, the ER is overwhelmed and the unfolded protein response (UPR) is activated. Remarkably, the consequences of UPR activation have been causally linked to the development of insulin resistance through a multitude of possible mechanisms, including c-jun N-terminal kinase activation, inflammation, and oxidative stress. This review will focus on the function of the ER under normal conditions in the adipocyte and the pathological effects of a stressed ER contributing to adipocyte dysfunction and a thwarted metabolic homeostasis.

Cell Biology Physiology Surgery