Cyclin D3 Maintains Growth-Inhibitory Activity of C/EBP{alpha} by Stabilizing C/EBP{alpha}-cdk2 and C/EBP{alpha}-Brm Complexes

doi:10.1128/MCB.26.7.2570-2582.2006

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Wang, G.-L.
	Articles by Timchenko, N. A.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Wang, G.-L.
	Articles by Timchenko, N. A.

Molecular and Cellular Biology, April 2006, p. 2570-2582, Vol. 26, No. 7
0270-7306/06/$08.00+0 doi:10.1128/MCB.26.7.2570-2582.2006
Copyright © 2006, American Society for Microbiology. All Rights Reserved.

Cyclin D3 Maintains Growth-Inhibitory Activity of C/EBP ${alpha}$ by Stabilizing C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm Complexes

Guo-Li Wang,¹^,2 Xiurong Shi,¹ Elizabeth Salisbury,¹ Yuxiang Sun,¹ Jeffrey H. Albrecht,⁴ Roy G. Smith,¹^,3 and Nikolai A. Timchenko¹^,2^*

Huffington Center on Aging,¹ Departments of Pathology,² Molecular Cellular Biology, Baylor College of Medicine, One Baylor Plaza, Houston, Texas 77030,³ Division of Gastroenterology, Hennepin County Medical Center, Minneapolis, Minnesota 55415⁴

Received 5 December 2005/ Accepted 5 January 2006

ABSTRACT

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

C/EBP ${alpha}$ arrests proliferation of young livers by inhibition ofcdk2. In old mice, C/EBP ${alpha}$ inhibits growth by repression of E2F-dependentpromoters through the C/EBP ${alpha}$ -Brm complex. In this paper, we showthat cyclin D3-cdk4/cdk6 supports the ability of C/EBP ${alpha}$ to inhibitliver proliferation in both age groups. Although cyclin D3-cdk4/cdk6kinases are involved in the promotion of growth, they are expressedin terminally differentiated cells, suggesting that they haveadditional functions in these settings. We demonstrate thatC/EBP ${alpha}$ represents a target for phosphorylation by cyclin D3-cdk4/cdk6complexes in differentiated liver cells and in differentiatedadipocytes. Cyclin D3-cdk4/cdk6 specifically phosphorylate C/EBP ${alpha}$ at Ser193 in vitro and in the liver and support growth-inhibitoryC/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes. We found that cyclin D3is increased in old livers and activates cdk4/cdk6, resultingin stabilization of the C/EBP ${alpha}$ -Brm complex. Old livers fail toreduce the activity of cyclin D3-cdk4/cdk6 after partial hepatectomy,leading to high levels of C/EBP ${alpha}$ -Brm complexes after partialhepatectomy, which correlate with weak proliferation. We examinedthe role of cyclin D3 in the stabilization of C/EBP ${alpha}$ -cdk2 andC/EBP ${alpha}$ -Brm by using 3T3-L1 differentiated cells. In these cells,cyclin D3 is increased during differentiation and phosphorylatesC/EBP ${alpha}$ at Ser193, leading to the formation of growth-inhibitoryC/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes. The inhibition of cyclinD3 blocks the formation of these complexes. Thus, these studiesprovide a new function of cyclin D3, which is to support thegrowth-inhibitory activity of C/EBP ${alpha}$ .

INTRODUCTION

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Quiescence and differentiation of tissues are supported by theRb family proteins and by certain tissue-specific proteins.C/EBP ${alpha}$ is a liver- and adipose-specific protein which maintainsquiescence of these tissues (7, 19) and regulates transcriptionof liver- and adipose-specific genes. Transcriptional and growth-inhibitoryactivities of C/EBP ${alpha}$ are mediated by different mechanisms. Whileactivation of C/EBP ${alpha}$ -dependent promoters requires an intact DNAbinding domain, the inhibition of cell proliferation is mediatedby a direct interaction of C/EBP ${alpha}$ with proteins which regulatecell cycle division (9, 11, 13, 14, 19, 22). Liver is a uniquetissue which is able to regenerate itself after surgical resections.After partial hepatectomy (PH), the initiation of proliferationrequires an orchestrated cascade of alterations of biochemicalpathways (6). These alterations result in activation of cellcycle genes and in the neutralization of a negative controlof liver proliferation. A key event in the activation of cellcycle genes after PH is the induction of D-type cyclins, whichinclude three members, D1, D2, and D3. Although these cyclinshave high levels of homology and might replace each other inknockout mouse models, they seem to play distinct functionsin cell cycle progression and differentiation. Cyclin D1 isnot detectable in quiescent liver, but it is induced after PHand increases liver proliferation. Moreover, overexpressionof cyclin D1 alone is sufficient to initiate proliferation inyoung livers (12). On the contrary, cyclin D3 is expressed ina number of quiescent tissues (including liver) and perhapsdisplays functions that support differentiation status of thetissues (16). Protein levels of cyclin D3 are increased duringdifferentiation of myocytes and are involved in the regulationof the MyoD-mediated program of gene expression (2). Moreover,Reichert and Eick showed that cyclin D3 is increased duringdifferentiation of 3T3-L1 adipocytes (15). However, biologicalfunctions of cyclin D3 in these differentiated cells and downstreamtargets of cyclin D3 have not been described.

A second important event in liver proliferation after PH isthe neutralization of the growth-inhibitory control in the liver.Rb family and C/EBP family proteins are expressed at high levelsin the liver, maintain liver quiescence, and prevent developmentof tumors (9, 12, 22). Although the roles of Rb and C/EBP ${alpha}$ inthe inhibition of liver proliferation have been established,the precise mechanisms by which livers regulate their growth-inhibitoryactivities are not well understood. Recent studies revealedthat the activities of both proteins are regulated by phosphorylationof unique residues of these proteins. The growth-inhibitoryactivity of C/EBP ${alpha}$ is significantly enhanced by phosphorylationof Ser193, while the removal of the phosphate from Ser193 eliminatesthe ability of C/EBP ${alpha}$ to cause growth arrest (22, 23). In livertumors, a PP2A phosphatase accumulates in nuclei and removesa phosphate from Ser193, leading to release of growth-inhibitoryactivity of C/EBP ${alpha}$ (22, 23). We have recently found that partialhepatectomy in young livers also neutralizes growth-inhibitoryactivity of C/EBP ${alpha}$ through activation of the phosphatidyl inositol3-kinase (PI3K)-Akt pathway, which increases the nuclear concentrationof PP2A (22, 23). C/EBP ${alpha}$ inhibits proliferation of young liversby interaction with and inhibition of cdk2. Aging changes thispathway to the repression of E2F transcription via an increasein an age-specific C/EBP ${alpha}$ -Rb-E2F4-Brm complex (further also calledC/EBP ${alpha}$ -Brm), which blocks expression of S-phase genes (9). Sincethis complex represses E2F transcription, the appearance ofthis complex contributes to the reduced proliferative capacitiesof old livers. This model is supported by recent work from Rando'sgroup which showed that cross-circulation of young and old micein parabiotic experiments resulted in decreased C/EBP ${alpha}$ -Brm complexformation and increased hepatocyte proliferation in the liversof old mice (3).

In this paper, we show that cyclin D3 regulates the growth-inhibitoryactivity of C/EBP ${alpha}$ in young and old livers and in differentiated3T3-L1 adipocytes. Cyclin-D3 cdk4/cdk6 specifically phosphorylateC/EBP ${alpha}$ at Ser193 in vitro and in vivo. Experiments with the inhibitionof cyclin D3 by small interfering RNA (siRNA) showed that cyclinD3-dependent phosphorylation of C/EBP ${alpha}$ is required for the formationof growth-inhibitory C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes. Wehave found that cyclin D3 displays this new activity in twobiological processes: during differentiation of 3T3-L1 adipocytesand in maintenance of the quiescent state of young and old livers.We also obtained evidence that aging liver activates cdk4/cdk6via elevation of cyclin D3, leading to the hyperphosphorylationof C/EBP ${alpha}$ at Ser193 and to stabilization of the C/EBP ${alpha}$ -Brm complex.

MATERIALS AND METHODS

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Antibodies. Antibodies (Abs) to cyclin D1, D2, and D3, C/EBP ${alpha}$ (14AA and N19),C/EBPß (C-19), cdk6, cdk4 (C-22), cdk2 (M2), and Brmand Rb (C-15) were purchased from Santa Cruz Biotechnology.Antibodies to peroxisome proliferator-activated receptor ${gamma}$ (PPAR ${gamma}$ )were purchased from Upstate Biotechnology. Antibodies to PP2Awere from Signal Transduction Laboratories. Monoclonal Abs toß-actin were from Sigma. To examine expression ofthe C/EBP ${alpha}$ -Ser193-ph isoform, we generated antibodies which specificallyrecognize C/EBP ${alpha}$ phosphorylated at Ser193. The specificity ofthese antibodies was examined by Western blotting with wild-type(WT) C/EBP ${alpha}$ and with a C/EBP ${alpha}$ -Ser193A mutant. These antibodiesinteract with WT C/EBP ${alpha}$ phosphorylated at Ser193 and do not reactwith the C/EBP ${alpha}$ -S193A mutant (see Fig. 1A, below). These Absspecifically recognize C/EBP ${alpha}$ phosphorylated in 3T3-L1 cells.Examination of phosphorylated isoforms of C/EBP ${alpha}$ in livers wasperformed using two approaches: immunoprecipitation and Westernblotting (IP-Western) and two-dimensional (2D)-Western. Thedirect Western blotting with ph-Ser193 antibodies does not workwith liver nuclear extracts, since these extracts contain immunoreactivebands close to the position of C/EBP ${alpha}$ which interact with Ser193-phantibodies. Therefore, C/EBP ${alpha}$ was first immunoprecipitated fromliver nuclear extracts with antibodies to total protein andthen examined by Western blotting with antibodies to ph-Ser193.To confirm data of the IP-Western with Ser193-ph Abs, we alsoused a 2D-Western assay as described in our previous papers(22, 23).

View larger version (42K):
[in this window]
[in a new window]

FIG. 1. Ser193-phosphorylated isoform of C/EBP ${alpha}$ is abundant in C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes. A. Characterization of antibodies to the phosphorylated Ser193-C/EBP ${alpha}$ isoform. HEK293 cells were transfected with WT and a C/EBP ${alpha}$ -S193A mutant, and nuclear extracts were examined by Western blotting with antibodies to ph-Ser193 of C/EBP ${alpha}$ and with Abs to total C/EBP ${alpha}$ . The filter was reprobed with antibodies to ß-actin. B. Western blotting of C/EBP ${alpha}$ immunoprecipitates with antibodies to Ser193-ph. C/EBP ${alpha}$ was immunoprecipitated from nuclear extracts of young and old livers and examined by Western blotting with Ser193-ph antibodies. The membrane was reprobed with antibodies to total C/EBP ${alpha}$ . Immunoglobulin G detected on the same filter showed an equal addition of antibodies to total C/EBP ${alpha}$ . C. Phosphorylation of C/EBP ${alpha}$ at Ser193 is increased in old livers. Bar graphs show a summary of three experiments with the IP-Western approach. A ratio of signals of ph-Ser193 to total C/EBP ${alpha}$ was determined by densitometry. D and E. Examination of C/EBP ${alpha}$ isoforms in young and old livers by 2D-Western. The upper image shows a 2D analysis of a control sample of C/EBP ${alpha}$ which was overexpressed in cultured cells. Untreated and CIP-treated nuclear proteins were separated by 2D electrophoresis and examined by Western blotting with antibodies to C/EBP ${alpha}$ . The percentage of Ser193 isoforms was calculated by densitometry as a ratio to the total amount of C/EBP ${alpha}$ isoforms (E). F. Isolation of C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes for examination of phosphorylation of C/EBP ${alpha}$ . Upper image: nuclear extracts from young livers were fractionated by size exclusion chromatography on an SEC250 column. Identical fractions of five HPLC runs were combined, and positions of C/EBP ${alpha}$ , Rb, Brm, and cdk2 within fractions were determined by Western blotting. The location of the C/EBP ${alpha}$ -cdk2 complex was determined by co-IP (C/EBP ${alpha}$ IP, cdk2 Western). Bottom image: localization of the C/EBP ${alpha}$ -Brm complex within fractions of the size exclusion chromatography column with nuclear extracts from old livers. Identical fractions of five runs of old livers on the SEC400 column were combined and examined by Western blotting with antibodies to Brm, cdk2, C/EBP ${alpha}$ , and Rb. C/EBP ${alpha}$ was immunoprecipitated from each fraction, and Rb was detected in these IPs (C/EBP ${alpha}$ -IP, Rb-Western; bottom image). G. 2D analysis of C/EBP ${alpha}$ within cdk2 complexes and within the age-specific C/EBP ${alpha}$ -Brm complex. C/EBP ${alpha}$ complexes were immunoprecipitated from fractions containing the complexes and examined by 2D gel electrophoresis. One half of each IP was treated with alkaline phosphatase (CIP) and examined in a parallel run. Positions of Ser193-phosphorylated isoforms are shown by red arrows.

Animals and liver regeneration. In these studies, we used mice ages 3 to 4 months (young) and22 to 24 months (old). Experiments with quiescent livers wereperformed with eight animals of each age group. Data in thepaper summarize multiple experiments. Liver regeneration andexamination of protein expression were performed as describedin our previous paper (9). In this paper, we examined expressionof proteins at earlier time points after PH, which included0, 4, and 8 h after surgery.

Protein isolation and Western blotting. Nuclear extracts were isolated as described in previous papers(9, 24, 25). Proteins (50 to 100 µg) were loaded on gradient(4-to-20% or 8-to-16%) polyacrylamide gels (PAAG), transferredon the membrane, and probed with antibodies to C/EBP ${alpha}$ , C/EBPß,PPAR ${gamma}$ , cdk2, cdk4, cyclins D1 and D3, Rb, E2F4, and Brm. To verifyprotein loading, each filter was reprobed with ß-actinand then stained with Coomassie.

Gel filtration analysis of protein-protein complexes in mouse liver. The detailed procedure for the analysis of protein-protein complexesis described in our previous papers (9, 22). Nuclear extractswere isolated from young and old livers as described elsewhere(20) and fractionated by size exclusion columns SEC-250 or SEC-400(high-performance liquid chromatography [HPLC]; BioLogic HR,Bio-Rad) with monitoring of optical density profiles. Gel filtrationfractions were loaded on denaturing gradient (4-to-20%) PAAG,blotted onto membranes, and probed with antibodies to cdk2,C/EBP ${alpha}$ , Rb, Brm, and E2F4 or with antibodies to cdk4, cdk6, andcyclin D1, D2, and D3. For examination of phosphorylation statusof C/EBP ${alpha}$ within C/EBP ${alpha}$ -cdk2 (young livers) and C/EBP ${alpha}$ -Brm (oldlivers) complexes, five HPLC runs were performed for each agegroup and combined for further studies. The locations of C/EBP ${alpha}$ -cdk2and C/EBP ${alpha}$ -Brm complexes were determined by coimmunoprecipitation(co-IP) as shown in Fig. 1, below. The complexes were precipitatedfrom corresponding fractions using specific Abs. One half ofeach precipitate was treated with alkaline phosphatase (CIP).Untreated and CIP-treated IPs were separated by 2D gel electrophoresisand examined by Western blotting with antibodies to C/EBP ${alpha}$ .

2D gel Western blotting. 2D gel analysis was performed as described in our previous papers(22, 23). Briefly, nuclear lysates from young and old liverswere separated by 2D gel electrophoresis (Protean IEF; Bio-Rad),transferred on the membrane, and probed with antibodies to C/EBP ${alpha}$ .

Coimmunoprecipitation. C/EBP ${alpha}$ was immunoprecipitated from nuclear extracts with polyclonalantibodies (14AA; Santa Cruz), and the presence of Rb, Brm,E2F4, cyclin D3, cdk4, and cdk2 in C/EBP ${alpha}$ IPs was examined byWestern blotting with monoclonal antibodies to the mentionedproteins.

Kinase assay. The conditions for in vitro kinase assays are described in ourprevious publications (24, 25). Briefly, baculovirus-expressedpurified cdk4-cyclin D1 and cdk6-cyclin D3 complexes or cdk4/cdk6/cyclinD3 IPs were incubated with glutathione S-transferase (GST)-Rbor GST-C/EBP ${alpha}$ substrates in the kinase reaction mixtures with[ ${gamma}$ -³²P]ATP. After 30-min incubations, kinase reaction mixtureswere loaded on gradient 8-to-16% PAAG, transferred on a nitrocellulosefilter, and exposed with X-ray film. After exposure, the filterwas stained with Coomassie blue to verify the loading of thesubstrates.

Differentiation of 3T3-L1 adipocytes was initiated as describedin a previous paper (21). Nuclear extracts were isolated at0, 1, 3, 5, and 7 days after initiation and analyzed by Westernblotting with antibodies to cyclin D3, cdk4, and cdk6 as describedabove. The proper differentiation was confirmed by examiningexpression of markers of differentiation, PPAR ${gamma}$ , C/EBPß,and C/EBP ${alpha}$ . In experiments involving the inhibition of cyclinD3 expression, 3T3-L1 cells were transfected with siRNA to cyclinD3 (DHARMACON RNA Tech) or with a control siRNA with randomsequence a day before initiation of differentiation. We havefound that this timing gives a maximum inhibition of cyclinD3 for the whole course of differentiation. Data in the manuscriptpresent a summary of three independent experiments.

RESULTS

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Phosphorylation of C/EBP ${alpha}$ at Ser193 is increased in old livers. C/EBP ${alpha}$ inhibits proliferation of young and old livers throughdifferent mechanisms. In young livers, C/EBP ${alpha}$ interacts withand inhibits cdk2 (24), while in old livers C/EBP ${alpha}$ repressesE2F transcription via the C/EBP ${alpha}$ -Brm complex (3, 9). A recentwork by Rando's group demonstrated that the disruption of theC/EBP ${alpha}$ -Brm complex in a young environment does not change proteinlevels of Brm and C/EBP ${alpha}$ , suggesting that posttranslational modificationsare involved in the formation of the complex (3). Consistentwith this suggestion, our previous investigations in culturedcells showed that phosphorylation of C/EBP ${alpha}$ at Ser193 is requiredfor the interaction of C/EBP ${alpha}$ with cdk2 and with Brm (22). Therefore,we examined if phosphorylation of C/EBP ${alpha}$ is required for theformation of the C/EBP ${alpha}$ -cdk2 (young animals) and the C/EBP ${alpha}$ -Brm(old animals) complexes in the liver. We initially determinedthe phosphorylation status of C/EBP ${alpha}$ in old and young livers.Two approaches were used for these studies. We generated antibodieswhich specifically recognize C/EBP ${alpha}$ phosphorylated at Ser193,as described in Materials and Methods. Figure 1A shows the specificityof these antibodies as determined by Western blotting with WTC/EBP ${alpha}$ and with a C/EBP ${alpha}$ -Ser193A mutant. These studies showedthat the Ser193-ph antibodies interact with WT C/EBP ${alpha}$ phosphorylatedat Ser193 and do not react with the C/EBP ${alpha}$ -S193A mutant. Examinationof these antibodies with nuclear extracts containing endogenousC/EBP ${alpha}$ showed that these Abs recognize a Ser193-ph isoform ofC/EBP ${alpha}$ in 3T3-L1 cells (see Fig. 5, below). In the liver, however,these Abs interact with several cross-reactive proteins locatedclose to the position of C/EBP ${alpha}$ , creating difficulties in interpretingdirect Western blot assays. To solve this problem, we firstimmunoprecipitated C/EBP ${alpha}$ from nuclear extracts of young andold livers with antibodies to total C/EBP ${alpha}$ and then performedWestern blotting with antibodies to Ser193-ph. Figure 1B showsthat the amount of the ph-Ser193 isoform of C/EBP ${alpha}$ is increasedin old livers. After reprobing the filter with antibodies tototal C/EBP ${alpha}$ , calculation of the Ser193-ph isoform to total proteinshowed an approximately 2- to 2.5-fold induction of this isoformin old livers (Fig. 1C).

View larger version (51K):
[in this window]
[in a new window]

FIG. 5. Induction of cyclin D3 in differentiated 3T3-L1 cells is required for the phosphorylation of C/EBP ${alpha}$ at Ser193. A. Protein levels of cyclin D3 are increased in 3T3-L1 after induction of differentiation. Nuclear extracts were isolated from 3T3-L1 cells at different days after initiation of differentiation (shown on the top) and examined by Western blotting with antibodies to the proteins shown on the left. Protein levels of cyclin D3 were calculated as ratios to ß-actin and are shown in the bar graph. B. Expression of markers of 3T3-L1 differentiation, PPAR ${gamma}$ and C/EBPß, and cyclin-dependent kinases. Western blotting was performed with nuclear extracts isolated from 3T3-L1 differentiated cells as described in Materials and Methods. C. Phosphorylation of C/EBP ${alpha}$ during differentiation of 3T3-L1 cells. Nuclear extracts from differentiated 3T3-L1 cells were examined by Western blotting with antibodies to total C/EBP ${alpha}$ and to the ph-S193 isoform of C/EBP ${alpha}$ . D. Examination of activities of kinases associated with cyclin D3. Cyclin D3 was immunoprecipitated from nuclear extracts and added into an in vitro kinase assay mixture with GST-C/EBP ${alpha}$ and GST-Rb substrates. The membranes were stained with Coomassie to visualize substrates. E. Inhibition of cyclin D3 expression by siRNA blocks phosphorylation of C/EBP ${alpha}$ at Ser193. Control siRNA lanes: expression of cyclin D3 in 3T3-L1 cells which were treated with control (random sequence) siRNA. The filter was reprobed with ß-actin to verify protein loading. Cyclin D3 siRNA lanes: siRNA to cyclin D3 was transfected into 3T3-L1 cells 1 day before initiation of differentiation. Proteins extracts were isolated from cyclin D3 siRNA-treated 3T3-Ll cells at different days and examined by Western blotting with antibodies to cyclin D3, cdk4, PPAR ${gamma}$ , total C/EBP ${alpha}$ , and the Ser193-ph isoform of C/EBP ${alpha}$ . Each membrane was reprobed with Abs to ß-actin. The bar graph (bottom) presents levels of cyclin D3 in control 3T3-L1 cells (treated with control siRNA) and in 3T3-L1 cells treated with siRNA to cyclin D3 and is a summary of three independent experiments. Cyclin D3 levels were calculated as ratios to ß-actin and then as ratios to levels at day 0. Cyclin D3-IP kinase lanes: examination of the cdk4/cdk6 activities in cyclin D3 IPs using GST-C/EBP ${alpha}$ as substrate.

Western blotting with ph-Ser193-specific Abs showed the relativeinduction of Ser193 phosphorylation in old livers but couldnot be used for the calculations of the portion of C/EBP ${alpha}$ phosphorylatedon Ser193, since antibodies to total C/EBP ${alpha}$ and to the Ser193-phisoform have different titers. To examine a portion of C/EBP ${alpha}$ phosphorylated on Ser193, we applied the 2D-Western blottingapproach. Untreated nuclear lysates and CIP-treated proteinswere separated by 2D gel electrophoresis and probed with antibodiesto C/EBP ${alpha}$ . We have previously shown that 2D analysis detectedfive major isoforms of C/EBP ${alpha}$ in the liver (a, b, c, d, and e)and that isoforms a and b are not detectable with the Ser193Amutant of C/EBP ${alpha}$ (22, 23). As can be seen in Fig. 1D, Ser193-phosphorylatedisoforms of C/EBP ${alpha}$ (a and b) are observed in both young and oldlivers, and the amounts of these isoforms are higher in oldlivers. The treatment of nuclear extracts with CIP shifted isoformsa, b, and c to the alkali region. Densitometric calculationsrevealed that around 75 to 80% of the C/EBP ${alpha}$ is hyperphosphorylatedat Ser193 in old livers, while in young livers, Ser193-ph isoformsrepresent 35 to 40% of the total amount of C/EBP ${alpha}$ (Fig. 1E).These data are consistent with results obtained by the IP-Westernapproach with ph-Ser193-specific Abs. Taking into account therole of Ser193 in the interactions with cdk2 and Brm (22), wesuggested that the phosphorylation of C/EBP ${alpha}$ might be involvedin the formation of C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes in theliver.

The Ser193-phosphorylated isoform of C/EBP ${alpha}$ is a major isoform within growth-inhibitory C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes in the liver. To examine the phosphorylation status of C/EBP ${alpha}$ within the C/EBP ${alpha}$ -cdk2and C/EBP ${alpha}$ -Brm complexes, we isolated C/EBP ${alpha}$ from these complexesusing an HPLC-based size exclusion-IP procedure as describedin our previous papers (9, 22). cdk2-C/EBP ${alpha}$ and Brm-C/EBP ${alpha}$ complexeswere enriched by size exclusion chromatography of proteins fromyoung and old livers, using SEC-250 and SEC-400 columns, respectively.Examination of C/EBP ${alpha}$ , cdk2, Brm, and Rb in these size exclusionfractions showed that C/EBP ${alpha}$ colocalizes with cdk2 in fractionsof young livers but does not colocalize with cdk2 in fractionsof proteins from old livers. Consistent with previous findings,C/EBP ${alpha}$ colocalizes with Rb and Brm in high-molecular-weight (MW)fractions of the samples from old livers (9). The location ofC/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes in corresponding fractionswas confirmed by Western blotting and by co-IP as shown in Fig.1F. The complexes were isolated from corresponding fractionsby immunoprecipitation with antibodies to cdk2 (young livers)and to C/EBP ${alpha}$ (old livers), and C/EBP ${alpha}$ isoforms were examinedby 2D-Western analysis as described in previous studies (9,22). Half of each IP was treated with an excess of CIP. As canbe seen in Fig. 1G, although C/EBP ${alpha}$ is observed in livers asfive isoforms, only the Ser193-ph isoform of C/EBP ${alpha}$ is detectedin the complexes with cdk2 or in the C/EBP ${alpha}$ -Brm complex. Thepresence of the Ser193-ph isoform in the complexes stronglysuggested that the phosphorylation of Ser193 of C/EBP ${alpha}$ is animportant event in the formation of the growth-inhibitory C/EBP ${alpha}$ complexes in the liver.

cdk4 and cdk6 phosphorylate C/EBP ${alpha}$ at Ser193 in vitro and in liver. We next searched for a liver-specific kinase that might phosphorylateC/EBP ${alpha}$ in young and old livers. Given the interactions of C/EBP ${alpha}$ with cdk4 and cdk2 (22, 24, 25), we examined activities of cdk2,cdk4, and cdk6 in young and old livers. These kinases were immunoprecipitatedfrom liver nuclear extracts, and their activities were measuredin an in vitro kinase assay using as substrates histone H1 (forcdk2) and Rb and C/EBP ${alpha}$ (for cdk4 and cdk6). cdk2 kinase activitywas undetectable in both young and old livers (data not shown),but the activities of cyclin D3, cdk4, and cdk6 were found inyoung and old livers. Figure 2A shows a typical result of thesestudies. In this experiment, cyclin D3, cdk4, and cdk6 wereimmunoprecipitated from liver nuclear extracts of young andold livers, and their abilities to phosphorylate C/EBP ${alpha}$ wereexamined in an in vitro kinase assay. As one can see, theseIPs phosphorylate C/EBP ${alpha}$ . This phosphorylation is specific, sincea mock agarose control showed no phosphorylation of C/EBP ${alpha}$ . Acomparison of the kinase activities of cyclinD3-cdk4/cdk6 reproduciblydemonstrated the induction of cdk4 and cdk6 activities in oldlivers. This induction correlates with a high level of Ser193-phisoform in old livers (Fig. 1). Taken together, these data showthat cyclin D3-cdk4 and cyclin D3-cdk6 are active in liversand that these kinases phosphorylate C/EBP ${alpha}$ .

View larger version (43K):
[in this window]
[in a new window]

FIG. 2. cdk4 and cdk6 phosphorylate Ser193 of C/EBP ${alpha}$ in vitro and in vivo. A. Cyclin D3-cdk4 and cyclin D3-cdk6 phosphorylate C/EBP ${alpha}$ in liver. cdk4, cdk6 and cyclin D3 were immunoprecipitated from young and old livers and examined in a kinase assay with GST-C/EBP ${alpha}$ substrate. Ag, agarose control for absorption. The bottom part shows a Coomassie stain of the filter to verify loading of the GST-C/EBP ${alpha}$ substrate. B. Baculovirus-expressed, purified cdk4-cyclin D1 phosphorylates C/EBP ${alpha}$ . Full-length GST-C/EBP ${alpha}$ or GST-140-200 (growth-inhibitory region of C/EBP ${alpha}$ ) was incubated with the cyclin D1-cdk4 complex in a kinase assay mixture containing [ ${gamma}$ -³²P]ATP. Proteins were transferred on the membrane and exposed. The bottom image shows Western blotting of the same membrane with antibodies to cdk4. C. C/EBP ${alpha}$ forms a stable complex with cyclin D1-cdk4 in the kinase reactions. C/EBP ${alpha}$ was incubated with cdk4-cyclin D1 in a kinase reaction, cyclin D1 was immunoprecipitated, and cdk4 and C/EBP ${alpha}$ in IPs were examined by Western blotting. A control experiment was performed with bovine serum albumin (BSA) instead of C/EBP ${alpha}$ . An aliquot from each reaction mixture was incubated with the GST-Rb substrate in the presence of [ ${gamma}$ -³²P]ATP (bottom part). D. Baculovirus-expressed, purified cdk4-cyclin D1 and cdk6-cyclin D3 phosphorylate Ser193 of C/EBP ${alpha}$ . GST-WT-C/EBP ${alpha}$ (W) and a C/EBP ${alpha}$ -S193A mutant (S193) were incubated with cdk4-cyclin D1 and with cdk6-cyclin D3 in a kinase assay. Positions of C/EBP ${alpha}$ and a nonspecific band (NS for cdk4-cyclin D1) are shown. The filter was reprobed with Abs to C/EBP ${alpha}$ , cdk4, and cdk6 (Western). E. cdk4-cyclin D3 phosphorylates Ser193 of C/EBP ${alpha}$ . WT and S193A mutant GST-C/EBP ${alpha}$ were incubated with cdk4 and cyclin D3 IPs from old livers. The bottom image shows GST-C/EBP ${alpha}$ stained with Coomassie. F. cdk6-cyclin D3 phosphorylates Ser193 of C/EBP ${alpha}$ . WT and S193A mutant GST C/EBP ${alpha}$ were incubated with cdk6 and cyclin D3 IPs from old livers. The bottom image shows GST-C/EBP ${alpha}$ stained with Coomassie. G. Examination of efficiency of phosphorylation of C/EBP ${alpha}$ by cdk4 relative to phosphorylation of Rb. GST-Rb (0.5 µg) and increasing amounts (0.5, 1, and 2 µg) of the growth-inhibitory region of C/EBP ${alpha}$ (GST-C/EBP ${alpha}$ -140-200) were added into kinase reaction mixtures with purified cyclin D1-cdk4 and [ ${gamma}$ -³²P]ATP. The reaction mixtures were loaded on a denaturing PAAG, transferred on membrane, and exposed to X rays. The bottom part shows a Coomassie stain of the gel loaded with the corresponding ratios of the proteins.

We next performed a detailed characterization of these activitiesusing baculovirus-expressed, purified cdk4-cyclin D1 with theC/EBP ${alpha}$ as substrate in an in vitro kinase assay. GST-C/EBP ${alpha}$ wasadded into the kinase reaction mixtures in excess to cyclinD1-cdk4 (1 µg/reaction mixture). A typical picture ofthese experiments is shown in Fig. 2B. As can be seen, GST-C/EBP ${alpha}$ is phosphorylated by cyclin D1-cdk4. Examination of a shortgrowth-inhibitory region of C/EBP ${alpha}$ (amino acids [aa] 140 to 200)as a substrate for cdk4 showed that cdk4 also phosphorylatesthe growth-inhibitory region of C/EBP ${alpha}$ . The region aa 140 to200 contains only one Ser (aa 193) and two tyrosines. Sincecdk4 phosphorylates Ser and Thr residues, these data suggestedthat cdk4 phosphorylates C/EBP ${alpha}$ at Ser193. We next examined ifcyclin D1 and cdk4 are observed in the complex with C/EBP ${alpha}$ inthe kinase reaction mixtures. IP of cyclin D1 from the kinasereactions, following Western blotting with antibodies to cdk4,cyclin D1, and C/EBP ${alpha}$ , revealed that C/EBP ${alpha}$ is in the complexwith cdk4 and cyclin D1 (Fig. 2C). A parallel examination ofthe cdk4 activity in aliquots from these mixtures using Rb assubstrate showed that the kinase activity of cdk4 is only slightlyreduced in mixtures with C/EBP ${alpha}$ , perhaps due to competition forcdk4 with the GST-Rb substrate (see below).

We next determined an amino acid residue of C/EBP ${alpha}$ which is phosphorylatedby cdk4 and cdk6. WT C/EBP ${alpha}$ and the mutant C/EBP ${alpha}$ -Ser193A (23)were incubated with baculovirus-expressed, purified cyclin D1-cdk4and cyclin D3-cdk6 in the presence of [ ${gamma}$ -³²P]ATP. As seen inFig. 2D, both kinases phosphorylate wild-type C/EBP ${alpha}$ ; however,the mutation of S193A abolishes cdk4-mediated phosphorylationof C/EBP ${alpha}$ and significantly reduces cdk6-mediated phosphorylation.To examine if cdk4/cdk6-cyclin D3 complexes from livers specificallyphosphorylate C/EBP ${alpha}$ at Ser193, we performed a similar kinaseassay with these kinases immunoprecipitated from old liversusing WT GST-C/EBP ${alpha}$ and GST-C/EBP ${alpha}$ -S193A as substrates. As seenin Fig. 2E and F, the mutation of Ser193 to Ala abolishes phosphorylationof C/EBP ${alpha}$ by cdk4 IPs, while cdk6 and cyclin D3 IPs show significantlyreduced, but still detectable, phosphorylation of the S193Amutant. Thus, these studies demonstrated that cdk4-cyclin D3and cyclin D3-cdk6 complexes specifically phosphorylate Ser193of C/EBP ${alpha}$ in livers.

Since these experiments identified C/EBP ${alpha}$ as a new substratefor cdk4/cdk6, we asked whether the efficiency in phosphorylationof C/EBP ${alpha}$ by cdk4/cdk6 is comparable to phosphorylation of Rb.To address this question, GST-Rb and GST-C/EBP ${alpha}$ -140-200 (a fragmentof C/EBP ${alpha}$ which interacts with cdk4 and contains Ser193 [24,25]) were simultaneously added in different ratios to an invitro kinase assay mixture with purified cyclinD1-cdk4 complex.The truncated form of C/EBP ${alpha}$ was used in these experiments, becausethe full-length C/EBP ${alpha}$ migrates close to GST-Rb and is not separatedwell from Rb by electrophoresis. At a ratio of Rb and C/EBP ${alpha}$ of 1:1, the levels of phosphorylation of C/EBP ${alpha}$ were identicalto those of Rb (Fig. 2G, lane 1). At ratios of Rb and C/EBP ${alpha}$ of 1:2 and 1:4, the phosphorylation of C/EBP ${alpha}$ was increased,while the phosphorylation of Rb was decreased. These resultsshow that the efficiency of phosphorylation of C/EBP ${alpha}$ by cdk4is comparable with that of Rb and that C/EBP ${alpha}$ might compete withRb for the interaction with cdk4 in the kinase reactions.

Cyclin D3-cdk4/cdk6 are associated with C/EBP ${alpha}$ in young and old livers. Given the induction of cdk4/cdk6 activities in old livers (Fig.2), we next examined mechanisms by which aging increases activitiesof these kinases. Western blotting with antibodies to cyclinsD1, D2, and D3 showed that while cyclins D1 and D2 are not detectablein both young and old livers, cyclin D3 is expressed in quiescentlivers and is dramatically increased in old animals. Figure3A shows examination of young and old animals by Western blottingwith antibodies to cyclin D3. As can be seen, old animals containhigh levels of cyclin D3 compared to those in young livers.Reprobing the membrane with ß-actin and Coomassiestaining the filter revealed equal protein loadings (Fig. 3A).Densitometric calculations of cyclin D3 as a ratio to ß-actinof multiple Western blotting experiments from six animals ofeach age group showed a four- to fivefold increase of proteinlevels of cyclin D3 in old livers (Fig. 3B). Interestingly,real-time PCR analysis with mRNA from young and old livers showedno difference in the levels of cyclin D3 mRNA (data not shown).This observation suggests that aging may increase translationor stability of the cyclin D3 protein.

View larger version (44K):
[in this window]
[in a new window]

FIG. 3. Aging liver increases activities of cdk4 and cdk6 by elevation of cyclin D3. A and B. Protein levels of cyclin D3 are increased in old livers. Nuclear extracts from five livers of young and old animals were examined by Western blotting with antibodies to cyclin D3. The membrane was reprobed with Abs to ß-actin. Coomassie stain shows staining of a parallel gel loaded with the same proteins. Bar graphs (B) represent a summary of multiple experiments. Levels of cyclin D3 were calculated as a ratio to ß-actin. C. C/EBP ${alpha}$ is observed in complexes with cyclin D3 in the liver. Cyclin D3 was immunoprecipitated from young and old livers, and cdk4, cdk6, and C/EBP ${alpha}$ were examined by Western blotting in cyclin D3 IPs. IgG lanes, heavy chains of immunoglobulin G were detected by Coomassie staining of the membrane. An aliquot from each reaction mixture was incubated with GST-C/EBP ${alpha}$ substrate in the presence of [ ${gamma}$ -³²P]ATP (kinase assay, bottom part). D. cdk4-cyclin D3 are associated with the C/EBP ${alpha}$ -Brm complex in old livers. Nuclear extracts from young and old livers were fractionated by size exclusion chromatography on an SEC-400 column as described in the legend to Fig. 1. Positions of molecular mass markers are shown on the top. Western lanes: examination of cdk4, cdk6, cyclin D3, and C/EBP ${alpha}$ in the gel filtration fractions by Western blotting. C/EBP ${alpha}$ -IP lanes, C/EBP ${alpha}$ was immunoprecipitated from fractions and C/EBP ${alpha}$ IPs were probed with antibodies to cyclin D3. Kinase assay lanes: cdk4 and C/EBP ${alpha}$ were immunoprecipitated from each fraction and examined in a kinase assay with GST-Rb and with GST-C/EBP ${alpha}$ substrates. Positions of cyclin D3-cdk4/cdk6 complexes are shown on the bottom.

Since the in vitro kinase assay showed that C/EBP ${alpha}$ is the substratefor phosphorylation by cyclin D3-activated cdk4/cdk6, we askedif cyclin D3 is physically associated with C/EBP ${alpha}$ in the youngand old livers. Cyclin D3 was precipitated from nuclear extractsof young and old livers, and cdk4, cdk6, and C/EBP ${alpha}$ were examinedin these IPs. We observed that cdk4, cdk6, and C/EBP ${alpha}$ are associatedwith cyclin D3 in both young and old livers; however, amountsof these proteins were increased in cyclin D3 IPs from old livers(Fig. 3C). A parallel examination of the cdk4/cdk6 activityin aliquots from these IPs using GST-C/EBP ${alpha}$ as substrate showedthat the kinase activity of cdk's, associated with cyclin D3and C/EBP ${alpha}$ , was also increased in old livers. Thus, cyclin D3-cdk4/cdk6complexes are associated with C/EBP ${alpha}$ in old livers and are ableto phosphorylate C/EBP ${alpha}$ . These findings suggested that C/EBP ${alpha}$ is a substrate for cdk4/cdk6 in quiescent livers.

Cyclin D3-cdk4/cdk6 are observed in high-MW C/EBP ${alpha}$ -Brm complexes in old livers. The presence of C/EBP ${alpha}$ in cyclin D3-cdk4/cdk6 complexes suggestedthat cyclin D3-cdk4/cdk6 might be associated with C/EBP ${alpha}$ and/orRb within a large C/EBP ${alpha}$ -Rb-E2F4-Brm complex. To test this suggestionand to examine kinase activities of cyclin D3-cdk4/cdk6 complexes,we utilized the previously established size exclusion chromatographyapproach (9, 22, 24). Protein extracts from young and old liverswere fractionated by size exclusion chromatography, and thecomposition of cdk4/cdk6-cyclin D3 complexes was examined indifferent fractions of the chromatography column by Westernblotting and co-IP-kinase assays. In young animals, cyclin D3,cdk4, and C/EBP ${alpha}$ colocalized in fractions with molecular massesaround 160 kDa (Fig. 3D). The immunoprecipitation of C/EBP ${alpha}$ fromsize exclusion fractions and examination of cyclin D3 in C/EBP ${alpha}$ IPs revealed that C/EBP ${alpha}$ is present in these 160-kDa cyclin D3-cdk4/cdk6complexes. The size of this complex suggests that the complexconsists of cyclin D3, cdk4, and C/EBP ${alpha}$ . Immunoprecipitationof cdk4 and C/EBP ${alpha}$ , following examination of kinase activity,showed that the 160-kDa cyclin D3-cdk4 complex is active. Theresults of size exclusion chromatography are consistent withdata obtained with a simple coimmunoprecipitation assay (Fig.3C).

Examination of nuclear extracts from old livers by size exclusionchromatography showed different results. Although cdk6- andcdk4-cyclin D3 complexes were observed in extracts from oldlivers in fractions ranging from 44 to 160 kDa, significantportions of cdk4, cdk6, and cyclin D3 were shifted to the positionof high-MW complexes. Western blotting with antibodies to C/EBP ${alpha}$ revealed that this position corresponds to that of the C/EBP ${alpha}$ -Brmcomplex. To examine if cyclin D3-cdk4/cdk6 are associated inthese fractions with the C/EBP ${alpha}$ -Brm complex, the complex wasimmunoprecipitated with antibodies to C/EBP ${alpha}$ and cyclin D3 wasexamined by Western blotting. As one can see, cyclin D3 is detectablewithin the C/EBP ${alpha}$ -Brm complex (Fig. 3D). This result is consistentwith data obtained in the coimmunoprecipitation assay (Fig.3C). We next examined activities of cyclin D3-cdk4/cdk6 complexesin size exclusion fractions from old livers. cdk4 was immunoprecipitatedfrom size exclusion fractions and examined in a kinase assaywith Rb and C/EBP ${alpha}$ substrates. These data showed that old liverscontain two active cyclin D3-cdk4/cdk6 complexes. One activecomplex was observed in the fractions ranging from 160 to 300kDa, while the second active complex colocalized with the C/EBP ${alpha}$ -Brmcomplex. Kinase activity of cdk4 toward both Rb and C/EBP ${alpha}$ wasdramatically increased in these high-MW fractions compared tocorresponding fractions of young livers. To confirm that thehigh-MW active cdk4-cyclin D3 is associated with the C/EBP ${alpha}$ -Brmcomplex, the latter was immunoprecipitated with antibodies toC/EBP ${alpha}$ and kinase activity of these IPs was examined with Rbsubstrate. These experiments clearly demonstrated that the high-MWcyclin D3-cdk4 complex is associated with C/EBP ${alpha}$ -Brm. Takingtogether the direct co-IP studies (Fig. 3C) and examinationof the complexes by size exclusion chromatography, we concludethat the active cdk4/cdk6-cyclin D3 complexes are associatedin quiescent old livers with the age-specific C/EBP ${alpha}$ -Brm complex.Since the ph-193 C/EBP ${alpha}$ isoform is the major one in the complex,the presence of active cyclin D3-cdk4/cdk6 in the C/EBP ${alpha}$ -Brmcomplex might be necessary to keep high levels of phosphorylationof C/EBP ${alpha}$ at Ser193.

High levels of cyclin D3 support the growth-inhibitory C/EBP ${alpha}$ -Brm complex in old livers after PH. The C/EBP ${alpha}$ -Brm complex is not reduced after PH in old mice (9).Our previous work and data in this paper identified a phosphatase,PP2A (22), and cdk4/cdk6 kinases as enzymes that regulate thedephosphorylation-phosphorylation of Ser193 and the formationof the age-specific complex. To elucidate the molecular basisfor the failure of old livers to reduce the complex after PH,we examined the expression of these enzymes after PH in youngand old livers. Since the difference between young and old liversin phosphorylation of C/EBP ${alpha}$ is observed at 4 h after PH (Fig.4B), we focused our studies on the early time period after PH,within 8 h after surgery. Protein levels of cyclin D1 are notdetectable within this time period, since the induction of cyclinD1 is observed at 12 to 24 h after PH (16). Although cyclinD3 expression is not changed in either age group, the relativeamounts of cyclin D3 during this time period remain stably higherin old livers compared to young (Fig. 4A). Examination of kinaseactivity associated with cyclin D3 revealed that the cyclinD3-cdk4/cdk6 complex is more active in old livers at earliertime points after PH (Fig. 4A, cyclin D3 IP kinase assay). Thesedata show that the cdk4/cdk6-cyclin D3 pathway is not altered,but cdk4/cdk6-cyclinD3 complexes remain at high levels in oldlivers at 8 h after PH. Western blotting analysis with antibodiesto catalytic subunit C of PP2A indicated that, although theinduction of PP2A was observed in both age groups, PP2A levelswere 8- to 10-fold increased in young livers at 4 h, while onlya 3- to 4-fold induction of PP2A was observed in old liversat 8 h after PH. To examine if the cyclin D3 is associated withC/EBP ${alpha}$ in young and old livers after PH, C/EBP ${alpha}$ was precipitatedby specific antibodies and cyclin D3 was examined in these IPs.These studies revealed that cyclin D3 is associated with C/EBP ${alpha}$ after PH (Fig. 4A, co-IP). Analysis of these IPs with ph-Ser193-specificantibodies showed that the ph-Ser193 isoform of C/EBP ${alpha}$ is notdetectable after PH in young livers, while amounts of Ser193-phisoforms are abundant in old livers after PH. Examination ofC/EBP ${alpha}$ and C/EBPß in livers showed that patterns oftheir expression were consistent with previously published results:C/EBPß was increased in both age groups, while C/EBP ${alpha}$ was reduced in young livers but not in old livers. We next performeda quantitative examination of C/EBP ${alpha}$ isoforms after PH in youngand old livers using a 2D-Western technique. Figure 4B showsthat, in young livers, PH eliminated growth-inhibitory Ser193-phisoforms of C/EBP ${alpha}$ at 4 h after surgeries. However, the amountsof these isoforms were not altered in old livers after PH. Thelack of dephosphorylation of C/EBP ${alpha}$ in old livers after PH correlateswith a higher activity of cyclin D3-associated kinases and witha weaker induction of PP2A.

View larger version (45K):
[in this window]
[in a new window]

FIG. 4. Old livers fail to dephosphorylate C/EBP ${alpha}$ at Ser193 after partial hepatectomy and contain a high-MW cyclin D3-cdk4-C/EBP ${alpha}$ -Rb-E2F4-Brm complex. A. Expression of cyclin D3 and PP2A in young and old livers at early time points after partial hepatectomy. Nuclear extracts were isolated at 0, 4, and 8 h after PH and examined by Western blotting with antibodies to cyclin D3, cyclin D1, cdk4, cdk6, PP2A, C/EBP ${alpha}$ , and C/EBPß. Each membrane was reprobed with antibodies to ß-actin. ß-Actin controls are shown for cyclin D3 and C/EBP ${alpha}$ membranes. Coomassie stain shows staining of the membrane for cyclin D3. Cyclin D3 IP-kinase assay: examination of cdk4/cdk6 activities in cyclin D3 IPs during early steps of liver proliferation. Cyclin D3 was immunoprecipitated from nuclear extracts isolated at 0, 4, and 8 h after PH. The activities of cdk4 and cdk6 associated with cyclin D3 were examined in a kinase assay with GST-C/EBP ${alpha}$ substrate. C/EBP ${alpha}$ -IP-Western: C/EBP ${alpha}$ was immunoprecipitated from nuclear extracts with antibodies to total C/EBP ${alpha}$ . IPs were probed with Abs to cyclin D3 and with Abs to the Ser193-ph isoform of C/EBP ${alpha}$ . B. The growth-inhibitory Ser193-ph isoform of C/EBP ${alpha}$ is abundant in old livers after PH. C/EBP ${alpha}$ was examined by 2D gel electrophoresis in nuclear extracts from young and old livers at 0 and 4 h after PH. Positions of five major isoforms of C/EBP ${alpha}$ are shown on the top. Ser193-ph isoforms (a and b) are shown in red. C. Examination of C/EBP ${alpha}$ -Brm complex in young and old livers after PH by the co-IP approach. C/EBP ${alpha}$ was immunoprecipitated from nuclear extracts isolated from young and old livers at 4 h after PH, and IPs were examined by Western blotting with antibodies to C/EBP ${alpha}$ , Brm, Rb, cyclin D3, and cdk4. IgG, heavy chains of immunoglobulin G. The composition of the cyclin D3-C/EBP ${alpha}$ -Brm complex is shown on the right. D. Examination of the cyclin D3-C/EBP ${alpha}$ -Brm complex in nuclear extracts isolated 4 h after PH by size exclusion chromatography. Nuclear extracts from young and old livers were examined by HPLC-based gel filtration as described in the legend to Fig. 3. C/EBP ${alpha}$ -IP lanes: C/EBP ${alpha}$ was immunoprecipitated from each fraction, and the presence of cyclin D3 and Brm was examined in these IPs by Western blotting. IgG lanes: heavy chains of immunoglobulin G were determined on the corresponding filters by Coomassie staining.

Cyclin D3 is associated with C/EBP ${alpha}$ -Brm complexes in old livers after PH. HPLC-based examination of C/EBP ${alpha}$ -cyclin D3 complexes in quiescentold livers showed that this complex colocalizes with Brm andRb (Fig. 1 and 3), suggesting that cyclin D3-cdk4/cdk6 mightbe associated with high-MW C/EBP ${alpha}$ -Rb-E2F4-Brm complexes afterPH. To examine this suggestion, we performed coimmunoprecipitationand size exclusion chromatography studies of nuclear extractsisolated from young and old livers at 4 h after PH. Figure 4Cshows that immunoprecipitation of C/EBP ${alpha}$ from young and old liversat 4 h after PH pulled down Brm, Rb, cdk4, and cyclin D3 inold livers, while only Rb was detectable in C/EBP ${alpha}$ IPs from younglivers, suggesting that old livers contain the cyclin D3-cdk4-C/EBP ${alpha}$ -Brmcomplex after PH. To verify this result and to precisely determinethe composition of this complex, protein extracts from youngand old livers isolated at 4 h after PH were fractionated onan SEC-400 column. Size exclusion chromatography fractions wereanalyzed by Western blotting and by co-IP (as described abovefor Fig. 3). Since C/EBP ${alpha}$ levels are reduced in young liversafter PH (Fig. 4A), C/EBP ${alpha}$ signals after fractionation are veryweak or not detectable. In young livers, Rb, E2F4, cyclin D3,and cdk4 were observed in fractions with molecular masses rangingfrom 100 to 300 kDa. Consistent with simple co-IP experiments,cyclin D3 was also not detectable in C/EBP ${alpha}$ complexes by co-IPfrom size exclusion fractions (Fig. 4D). Examination of sizeexclusion fractions from old livers at 4 h after PH showed aquite-different result. While Rb, E2F4, cyclin D3, and cdk4were distributed throughout many fractions, the major amountsof C/EBP ${alpha}$ and Brm were observed in very-high-MW fractions. Precipitationof the C/EBP ${alpha}$ -Brm complex with antibodies to C/EBP ${alpha}$ and examinationof cyclin D3 and Brm in these IPs showed that both cyclin D3and Brm are associated with C/EBP ${alpha}$ in old livers at 4 h afterPH. Thus, co-IP and gel filtration studies demonstrated thatcyclin D3-cdk4 are bound to the C/EBP ${alpha}$ -Brm complex, suggestingthat this association phosphorylates C/EBP ${alpha}$ at Ser193.

Phosphorylation of C/EBP ${alpha}$ at Ser193 by cyclin D3-cdk4/cdk6 is required for the formation of C/EBP ${alpha}$ complexes with cdk2 and Brm. To further examine the role of cyclin D3-cdk4/cdk6 in the regulationof growth-inhibitory C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes, weutilized a tissue culture system involving differentiation of3T3-L1 cells, in which C/EBP ${alpha}$ plays a key role in the inhibitionof proliferation (18). 3T3-L1 cells were selected for thesestudies since endogenous C/EBP ${alpha}$ inhibits proliferation of 3T3-L1by formation of C/EBP ${alpha}$ -cdk2 complexes (24) and, at later stagesof differentiation, C/EBP ${alpha}$ interacts with Brm and forms a C/EBP ${alpha}$ -Brmcomplex (9). Because expression of cyclin D3 is also increasedduring differentiation of 3T3-L1 adipocytes (15), we suggestedthat the formation of the C/EBP ${alpha}$ complexes might be controlledin 3T3-L1 cells by cyclin D3-cd4/cdk6. To examine this possibility,we first determined expression of cyclin D3 in 3T3-L1 cellsafter initiation of differentiation under our conditions. Figure5A shows that protein levels of cyclin D3 were increased afterinitiation of differentiation (day 1) and stayed at high levelsin fully differentiated cells (day 7). Densitometric calculationsof cyclin D3 as a ratio to ß-actin showed that proteinlevels of cyclin D3 were 10- to 12-fold higher at days 5 to7 than those in predifferentiated cells (Fig. 5A, bar graph).Examination of markers of adipocyte differentiation, PPAR ${gamma}$ andC/EBPß, revealed that the genetic program of differentiationwas properly initiated in 3T3-L1 cells (Fig. 5B). Consistentwith previous observations, protein levels of cdk2 and cdk4were not significantly changed during differentiation of 3T3-L1cells (15, 21). Examination of C/EBP ${alpha}$ in differentiated 3T3-L1cells with Abs to total C/EBP ${alpha}$ and to Ser193-ph showed that expressionof C/EBP ${alpha}$ was increased at days 3 to 7 after initiation of differentiationand that C/EBP ${alpha}$ was phosphorylated at Ser193 at days 3, 5, and7 (Fig. 5C). This phosphorylation of Ser193 correlates withthe time of induction of cyclin D3 in differentiated 3T3-L1cells.

We next examined if cyclin D3-cdk4/cdk6 complexes in 3T3-L1cells are able to phosphorylate C/EBP ${alpha}$ . Cyclin D3 was immunoprecipitatedfrom nuclear extracts of differentiated cells and examined inan in vitro kinase assay with C/EBP ${alpha}$ and Rb substrates. Figure5D shows a typical result of these studies. Cyclin D3 activitytoward C/EBP ${alpha}$ and Rb was detectable in predifferentiated cells.At day 1, the ability of cyclin D3 to phosphorylate Rb was increased,while the activity of cyclin D3 toward C/EBP ${alpha}$ was not changed.However, the ability of cyclin D3 to phosphorylate C/EBP ${alpha}$ wasincreased at day 3 and remained high during the later days ofdifferentiation. This timing correlates with the phosphorylationof endogenous C/EBP ${alpha}$ at Ser193. Taken together, these studiessuggested that the induction of cyclin D3 is involved in thephosphorylation of C/EBP ${alpha}$ in differentiated adipocytes.

Inhibition of cyclin D3 blocks the phosphorylation of C/EBP ${alpha}$ at Ser193 and reduces the formation of C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes. To examine if cyclin D3 is required for the phosphorylationof C/EBP ${alpha}$ at Ser193 and for the formation of growth-inhibitorycomplexes of C/EBP ${alpha}$ , the expression of cyclin D3 was inhibitedin 3T3-L1 cells by specific siRNA. In these experiments, weobtained around 70 to 80% efficiencies of transfection. As onecan see in Fig. 5E, cyclin D3 siRNA significantly reduced levelsof cyclin D3 in preadipocytes and blocked the induction of cyclinD3 after initiation of differentiation, while in control cellstreated with siRNA of random sequence, cyclin D3 was increasedduring differentiation. Although we could not inhibit expressionof cyclin D3 completely, we obtained a 15- to 20-fold differencein the levels of cyclin D3 in control and cyclin D3 siRNA-treated3T3-L1 cells at days 3 to 7 of differentiation (Fig. 5E, bargraphs). This inhibition is sufficient to block the phosphorylationof Ser193-ph of C/EBP ${alpha}$ , as was shown by Western blotting withspecific antibodies. Consistent with the lack of phosphorylationof endogenous C/EBP ${alpha}$ on Ser193, phosphorylation of C/EBP ${alpha}$ by cyclinD3 IPs from cells transfected with cyclin D3 siRNA was alsonot detectable in an in vitro kinase assay (Fig. 5E). To examinethe formation of C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes in controlcells and in cells with inhibited expression of cyclin D3, coimmunoprecipitationstudies and HPLC-based size exclusion analyses were performed.Figure 6A shows results of co-IP studies. In control cells,C/EBP ${alpha}$ formed complexes with cdk2 at days 3 and 5, while C/EBP ${alpha}$ -Brmcomplexes were abundant at days 5 and 7 of differentiation.On the contrary, in 3T3-L1 cells in which cyclin D3 was inhibited,C/EBP ${alpha}$ -Brm complexes were not detectable at any stage of differentiation.Although we could detect C/EBP ${alpha}$ -cdk2 complex at day 3, this complexwas very weak at day 3 and was not detectable at day 5 of differentiationof 3T3-L1 cells, while in control 3T3 cells the complex wasstrong and was observed at days 3 and 5 (Fig. 6A). These studiesdemonstrated that the inhibition of cyclin D3 during differentiationof 3T3-L1 cells prevents the formation of C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brmcomplexes.

View larger version (45K):
[in this window]
[in a new window]

FIG. 6. Phosphorylation of C/EBP ${alpha}$ by cyclin D3-cdk4/cdk6 is required for the formation of the C/EBP ${alpha}$ -cdk2 and the C/EBP ${alpha}$ -Brm complexes. A. Examination of C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes during differentiation of 3T3-L1 cells treated with control siRNA (upper) and with siRNA to cyclin D3 (bottom). Input lanes: Western blotting of nuclear extracts with antibodies to Brm and cdk2, showing the levels of these proteins in extracts used for the co-IP. C/EBP ${alpha}$ -IP lanes: C/EBP ${alpha}$ was immunoprecipitated from nuclear extracts, and the IPs were examined by Western blotting with antibodies to cdk2, Brm, and C/EBP ${alpha}$ . Heavy chains of immunoglobulin G (IgG) are shown for each IP. B. Examination of the cyclin D3-C/EBP ${alpha}$ -Brm complex in differentiated 3T3-L1 cells by size exclusion chromatography. Nuclear extracts from differentiated 3T3-L1 cells (day 7) were fractionated with an SEC-400 column. Fractions were analyzed by Western blotting with antibodies to the proteins shown on the right. C/EBP ${alpha}$ -IP Western lanes: examination of cyclin D3 and cdk4 in C/EBP ${alpha}$ IPs from size exclusion fractions was performed with specific antibodies as described in the legends to Fig. 3 and 4. Kinase activity of cyclin D3-cdk4 was examined in C/EBP ${alpha}$ IPs by an in vitro kinase assay with Rb substrate (C/EBP ${alpha}$ -IP kinase). C. Size exclusion chromatography of nuclear extracts isolated from 3T3-L1 cells treated with control siRNA and with cyclin D3 siRNA. Proteins were isolated at day 7 after initiation of differentiation and fractionated on an SEC-400 column. Size exclusion fractions were examined by Western blotting with antibodies to C/EBP ${alpha}$ . Amounts of C/EBP ${alpha}$ were calculated in fractions containing C/EBP ${alpha}$ -Brm complexes relative to total amounts of C/EBP ${alpha}$ throughout the gel filtration.

The cyclin D3-cdk4-C/EBP ${alpha}$ -Rb-E2F4-Brm complex is abundant in differentiated 3T3-L1 cells. In old livers, the elevation of cyclin D3 leads to the formationof a very-high-MW cyclin D3-cdk4/cdk6-C/EBP ${alpha}$ -Rb-E2F4-Brm complex(Fig. 3 and 4). We next asked if this complex is also formedin differentiated 3T3-L1 cells containing high levels of cyclinD3. Protein extracts were isolated from 3T3-L1 cells at day7 of differentiation and examined by size exclusion chromatography.As seen in Fig. 6B, C/EBP ${alpha}$ , Brm, Rb, E2F4, cdk4, and cyclin D3colocalized in high-MW fractions of gel filtrations of differentiated3T3-L1 cells. To examine if cyclin D3 and cdk4 are associatedwith the C/EBP ${alpha}$ -Brm complex in these fractions, C/EBP ${alpha}$ was immunoprecipitatedfrom each fraction of the gel filtration and IPs were analyzedwith antibodies to cyclin D3 and to cdk4. Both cyclin D3 andcdk4 were observed in the C/EBP ${alpha}$ IPs (Fig. 6B). These data showthat differentiated 3T3-L1 cells contain the high-MW cyclinD3-cdk4-C/EBP ${alpha}$ -Rb-E2F4-Brm complex. To examine if cyclin D3-cdk4is active within this complex, aliquots of these IP mixtureswere used in an in vitro kinase assay with GST-Rb substrate.This analysis showed that cyclin D3-cdk4 within the C/EBP ${alpha}$ -Brmcomplex is active and phosphorylates Rb. Using this HPLC technique,we next examined the effects of inhibition of cyclin D3 on theC/EBP ${alpha}$ -Brm complexes in differentiated 3T3-L1 cells. In theseexperiments, we used Western blotting with antibodies to C/EBP ${alpha}$ as a measurement of the C/EBP ${alpha}$ -Brm complex, followed by densitometriccalculations of the portion of C/EBP ${alpha}$ in the position of thecomplex. 3T3-L1 cells transfected with control siRNA containedmore than 90% of C/EBP ${alpha}$ in the position of the C/EBP ${alpha}$ -Brm complex.In 3T3-L1 cells with reduced expression of cyclin D3, the amountsof C/EBP ${alpha}$ in the position of the Brm complexes were reduced to30%. Since efficiencies of transfection in these experimentswere 70 to 80%, the remaining C/EBP ${alpha}$ -Brm complexes perhaps camefrom untransfected cells. Taking together co-IP data and HPLCresults, these studies showed that cyclin D3 is required forthe formation of both C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes andthat cyclin D3-cdk4 is observed in high-MW C/EBP ${alpha}$ -Brm complexes.

DISCUSSION

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

C/EBP ${alpha}$ is a new target for cyclin D3-cdk4/cdk6 in differentiated cells. Searching for a pathway which positively regulates the growth-inhibitoryactivity of C/EBP ${alpha}$ in the liver, we found that cdk4/cdk6 phosphorylatesC/EBP ${alpha}$ at Ser193 and that these kinases are activated in theliver by cyclin D3. Although cyclin D3 clearly promotes cellcycle progression in some models, this protein is expressedin numerous nonproliferating tissues, including quiescent liver(1, 4, 16). Indeed, increased cyclin D3 expression appears toparticipate in cell cycle withdrawal in muscle cells throughinduction of the transcription factor MyoD, and overexpressionof cyclin D3 suppresses reactivation of DNA synthesis in differentiatedmyotubules (2, 5). Although these observations were describedlong ago, molecular targets of cyclin D3 in differentiated settingshave not been found. Data in this paper provide evidence that,in differentiated livers and adipocytes, cyclin D3-cdk4/cdk6phosphorylates C/EBP ${alpha}$ and supports the formation of C/EBP ${alpha}$ -cdk2and C/EBP ${alpha}$ -Brm complexes that inhibit proliferation. We haveshown in our previous studies that C/EBP ${alpha}$ can interact with cdk4;however, this interaction had a minor effect on the kinase activityof cdk4 (24, 25). A slight reduction of the phosphorylationof Rb by cdk4 in the presence of C/EBP ${alpha}$ , rather, reflected acompetition, since under conditions of the in vitro kinase assay,C/EBP ${alpha}$ and Rb were in excess to cdk4. Under conditions of thein vitro kinase assay, both cyclin D1-cdk4 and cyclin D3-cdk4complexes phosphorylated C/EBP ${alpha}$ , suggesting that these complexescan also phosphorylate C/EBP ${alpha}$ in vivo. In quiescent livers, however,cyclin D3 is a major activator of cdk4/cdk6, since the levelsof cyclin D3 are very high while cyclin D1 is not detectable(reference 16 and this study). Although both cdk4 and cdk6 phosphorylateC/EBP ${alpha}$ , cdk4 seems to be more specific for Ser193, since it doesnot phosphorylate the C/EBP ${alpha}$ -S193 mutant, while the phosphorylationof C/EBP ${alpha}$ -S193A by cdk6 is weaker but still detectable (Fig.2).

Cyclin D3 supports growth-inhibitory C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes in differentiated livers and in adipocytes. C/EBP ${alpha}$ is a very strong inhibitor of cell proliferation and isexpressed in highly differentiated tissues such as liver andadipose tissues. On the other hand, there are several biologicalsituations in which cells proliferate and express high levelsof C/EBP ${alpha}$ (22, 23). In these cells, C/EBP ${alpha}$ activity is eliminatedby dephosphorylation of C/EBP ${alpha}$ at Ser193 (22). In this paper,we identified cyclin D3-cdk4/cdk6 as enzymes which phosphorylateSer193, leading to the formation of growth-inhibitory C/EBP ${alpha}$ -cdk2and C/EBP ${alpha}$ -Brm complexes. A hypothetical model for the role ofcyclin D3 in supporting the growth-inhibitory activity of C/EBP ${alpha}$ in adipocytes and quiescent livers is shown in Fig. 7. Boththe liver and differentiated adipocytes express high levelsof C/EBP ${alpha}$ (21, 23, 25) and high levels of cyclin D3 (Fig. 3 and4) (15, 16). Different approaches revealed that, in quiescentlivers, cyclin D3 is associated with C/EBP ${alpha}$ and stabilizes C/EBP ${alpha}$ -cdk2(young liver) and C/EBP ${alpha}$ -Brm (old liver) complexes by phosphorylationof C/EBP ${alpha}$ at Ser193. Additional evidence for the role of cyclinD3-cdk4 in supporting growth-inhibitory activities of C/EBP ${alpha}$ came from experiments with differentiated 3T3-L1 adipocytes.In these cells, C/EBP ${alpha}$ is induced at later stages of differentiationand is required for growth arrest and differentiation (18).We showed that cyclin D3/cdk4 phosphorylates C/EBP ${alpha}$ at Ser193at days 3 to 7 of differentiation, resulting in the formationof C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes. The inhibition of cyclinD3 expression by siRNA leads to failure of C/EBP ${alpha}$ to form growth-inhibitoryC/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes. In agreement with our data,a recent paper by Sarruf et al. showed that the inhibition ofcyclin D3 expression of 3T3-L1 blocks differentiation of 3T3-L1adipocytes (17).

View larger version (21K):
[in this window]
[in a new window]

FIG. 7. Hypothetic model suggesting that cyclin D3 supports quiescence of the liver and differentiated adipocytes by stabilizing growth-inhibitory C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm complexes. Cyclin D3 activates cdk4/cdk6 kinases, which specifically phosphorylate Ser193 of C/EBP ${alpha}$ . The Ser193-ph isoform of C/EBP ${alpha}$ forms complexes with cdk2 (young livers) and with Brm, Rb, and E2F4 (old livers), which inhibit cell proliferation.

Although our data (this paper and reference 16) and those ofothers (1, 2, 5) suggest an antiproliferative role for cyclinD3, data in other systems clearly suggest that this proteincan promote cell cycle progression. For example, ectopic expressionof cyclin D3 promotes progression through the G₁ phase in ratfibroblasts (6). Furthermore, transient overexpression of cyclinD3 in young (2-month) livers promotes a modest proliferativeeffect in hepatocytes (L. Mullany, C. Nelsen, and J. Albrecht,personal communication). These data indicate that cyclin D3can have either a proliferative or inhibitory effect, presumablydepending upon the intracellular environment and levels of cyclinD3 and its downstream targets which mediate inhibition or promotionof proliferation.

Aging liver activates cdk4/cdk6 by increasing cyclin D3 levels and by forming high-MW complexes. Activities of both cdk4 and cdk6 are increased in old liversby the elevation of cyclin D3. Our examination of enzymaticactivities of cyclin D3-cdk4/cdk6 complexes by size exclusionchromatography provided new observations suggesting an additionalpathway for the regulation of cyclin D3-cdk4/cdk6. Previousstudies had shown that in proliferating cultured cells, activecyclin D3/cdk6 complexes are approximately 170 kDa in size (10).Consistent with these observations, in young livers the activecyclin D3-cdk4/cdk6 complexes range from 100 to 160 kDa anda portion of these complexes is associated with C/EBP ${alpha}$ , suggestingthat C/EBP ${alpha}$ is a substrate for cyclin D3-cdk4/cdk6. In aged liver,however, the major cdk4/cdk6 kinase activity was associatedwith higher-MW complexes, one of which is the cyclin D3-C/EBP ${alpha}$ -Brmcomplex. Interestingly, partial hepatectomy in old livers failedto reduce the cyclin D3-C/EBP ${alpha}$ -Brm complex, suggesting that thiscomplex might be involved in the inhibition of liver proliferation.Examination of high-MW complexes in growth-arrested, differentiated3T3-L1 cells presented additional evidence for the role of thecyclin D3-C/EBP ${alpha}$ -Brm complex in the inhibition of cell proliferation.These data suggest that the recruitment of cyclin D3 into higher-MWcomplexes may result in a change in its role in cell cycle control.

In this paper, we identified C/EBP ${alpha}$ as a new target of cyclinD3. Recent publications suggest that there might be more targetsof cyclin D3 which are involved in the differentiation-specificfunctions of cyclin D3. When our manuscript was under review,Sarruf et al. published observations that cyclin D3-mediatedphosphorylation of PPAR ${gamma}$ is also involved in the differentiationof adipocytes (17). In addition to the role of cyclin D3 indifferentiation of 3T3-L1 cells, protein levels of cyclin D3are also elevated in differentiated myocytes at the stage ofgrowth arrest (2, 4), suggesting a putative involvement of cyclinD3 in the inhibition of these cells. Although C/EBP ${alpha}$ is not expressedin myocytes, experimental work from Paterson's group showedthat cdk4 (which is activated by cyclin D3) interacts with themuscle-specific transcription factor MyoD and that this interactionpromotes growth arrest and terminal differentiation (26, 27).It would be interesting to examine if cyclin D3 has a positiveeffect on this interaction and on terminal differentiation ofmyocytes.

ACKNOWLEDGMENTS

This work was supported by National Institutes of Health grantsAG20752, CA10070, and GM55188 (N.A.T.) and DK54921 (J.H.A.).

FOOTNOTES

* Corresponding author. Mailing address: Department of Pathology and Huffington Center on Aging, Baylor College of Medicine, One Baylor Plaza, Houston, TX 77030. Phone: (713) 798-1567. Fax: (713) 798-4161. E-mail: nikolait{at}bcm.tmc.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Bartkova, J., J. Lukas, M. Strauss, and J. Bartek. 1998. Cyclin D3: requirement for G₁/S transition and h

Cyclin D3 Maintains Growth-Inhibitory Activity of C/EBP by Stabilizing C/EBP-cdk2 and C/EBP-Brm Complexes

Cyclin D3 Maintains Growth-Inhibitory Activity of C/EBP ${alpha}$ by Stabilizing C/EBP ${alpha}$ -cdk2 and C/EBP ${alpha}$ -Brm Complexes