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© The Rockefeller University Press, 0021-9525/1999//1049 $5.00
The Journal of Cell Biology, Volume 145, Number 5, , 1999 1049-1061

Functions of c-Jun in Liver and Heart Development

Robert Eferl^*, Maria Sibilia, Frank Hilberg, Andrea Fuchsbichler^*, Iris Kufferath^*, Barbara Guertl^*, Rainer Zenz^*, Erwin F. Wagner, and Kurt Zatloukal^*

^* Department of Pathology, University of Graz, A-8036 Graz, Austria; Research Institute of Molecular Pathology, A-1030 Vienna, Austria; and Boehringer Ingelheim, A-1121 Vienna, Austria

Mice lacking the AP-1 transcription factor c-Jun die around embryonic day E13.0 but little is known about the cell types affected as well as the cause of embryonic lethality. Here we show that a fraction of mutant E13.0 fetal livers exhibits extensive apoptosis of both hematopoietic cells and hepatoblasts, whereas the expression of 15 mRNAs, including those of albumin, keratin 18, hepatocyte nuclear factor 1, β-globin, and erythropoietin, some of which are putative AP-1 target genes, is not affected. Apoptosis of hematopoietic cells in mutant livers is most likely not due to a cell-autonomous defect, since c-jun^–/– fetal liver cells are able to reconstitute all hematopoietic compartments of lethally irradiated recipient mice. A developmental analysis of chimeras showed contribution of c-jun^–/– ES cell derivatives to fetal, but not to adult livers, suggesting a role of c-Jun in hepatocyte turnover. This is in agreement with the reduced mitotic and increased apoptotic rates found in primary liver cell cultures derived from c-jun^–/– fetuses. Furthermore, a novel function for c-Jun was found in heart development. The heart outflow tract of c-jun^–/– fetuses show malformations that resemble the human disease of a truncus arteriosus persistens. Therefore, the lethality of c-jun mutant fetuses is most likely due to pleiotropic defects reflecting the diversity of functions of c-Jun in development, such as a role in neural crest cell function, in the maintenance of hepatic hematopoiesis and in the regulation of apoptosis.

Key Words: apoptosis • neural crest • hematopoiesis • knockout • truncus arteriosus persistens

Abbreviations used in this paper: AP-1, activating protein 1; Cx 43, connexin 43; ES cells, embryonic stem cells; GPI, glucose phosphate isomerase; HGF, hepatocyte growth factor; HNF-1, hepatocyte nuclear factor 1; RT-PCR, reverse transcriptase PCR; TUNEL, TdT-mediated dUTP nick-end labeling.

Address correspondence to Kurt Zatloukal, Department of Pathology, Auenbruggerplatz 25, A-8036 Graz, Austria. Tel.: 43 0316 3804404. Fax: 43 0316 384329. E-mail: kurt.zatloukal{at}kfunigraz.ac.at

THE proto-oncogene c-jun encodes a component of the transcription factor AP-1 (activating protein 1)¹, which has been implicated in the regulation of diverse cellular functions, such as proliferation, differentiation, transformation, and apoptosis. AP-1 is a dimer consisting of different subunits, e.g., proteins of the Jun (c-Jun, JunB, and JunD) and Fos (c-Fos, FosB, Fra1, and Fra2) family as well as CREB/ATF, and Maf proteins. The different AP-1 components are expressed in a development- and tissue-specific manner, implying that AP-1 composed of different subunits may exert different functions in different cell types. Although AP-1 was found to regulate a few genes, such as human metallothionein IIA (Lee et al., 1987), collagenase (Angel et al., 1987), stromelysin (Kerr et al., 1988), and keratin 18 (Oshima et al., 1990), the biological function of the different AP-1 complexes during development is still elusive. The characterization of the role of AP-1 is further impeded by the fact that there are, in addition to the variability in subunit composition, numerous possible interactions between AP-1 and other transcription factors, such as glucocorticoid hormone receptors (Jonat et al., 1990), estrogen receptors (Gaub et al., 1990), retinoic acid and vitamin D3 receptors (Schüle et al., 1990), and MyoD (Bengal et al., 1992) yielding a network of transcriptional regulation.

First clues on tissue-specific functions of AP-1 components came from gene knockout experiments. In c-fos knockout mice the development of bone is impaired because of a block in osteoclast differentiation (Grigoriadis et al., 1994). Moreover, lymphoid cells, germ cells, and neuronal tissues are affected in the absence of c-Fos (Johnson et al., 1992; Wang et al., 1992). In contrast to the inactivation of c-fos, targeted disruption of c-jun and junB is lethal (Hilberg et al., 1993; Johnson et al., 1993; Schorpp-Kistner et al., 1999). Lethality of c-jun^–/– fetuses has been suggested to be due to defective liver development. The livers of some E12.5 animals appeared hypoplastic with rounded, dissociated hepatoblasts showing features of apoptosis and necrosis. Moreover, increased numbers of erythropoietic cells were noted in these livers (Hilberg et al., 1993). A defect in hepatogenesis in c-Jun knockout mice was further indicated by the observation that c-jun^–/– embryonic stem (ES) cells failed to contribute to the liver but not to other tissues of adult chimeric mice (Hilberg et al., 1993). These observations, together with the fact that no morphological alterations were found in organs other than the liver, led to the conclusion that the absence of c-Jun might preferentially affect the development of the liver (Hilberg et al., 1993).

In the mouse, liver development starts at around E9.5 when epithelial cells of the foregut endoderm proliferate and invade the mesenchyme of the septum transversum thus forming the embryonic liver. At around E11 hematopoietic stem and progenitor cells derived from the yolk sac and aorta-gonad-mesonephros region colonize the liver, and the liver becomes the major hematopoietic organ during further fetal development (Dzierzak and Medvinsky, 1995). To allow establishment and maintenance of hematopoiesis, liver cells have to provide the proper microenvironment for hematopoietic cells comparable to stromal cells in the bone marrow during postnatal life. The next major step in mouse liver development occurs at approximately E14.5 when hepatoblasts start to differentiate into the hepatocytic and bile duct epithelial lineage, which is indicated by the formation of the ductal plate, which later differentiates into the intrahepatic bile ducts (Desmet, 1998). It is as yet unclear at which developmental stage c-Jun becomes essential for the liver, and whether the defect is restricted to the hepatocytic lineage or other cell types of the fetal liver, such as bile duct epithelia, endothelial cells, stellate cells (vitamin A–storing cells), Kupffer cells, and hematopoietic cells.

Besides the poorly characterized function in liver development, c-Jun plays a more general role in the regulation of cell proliferation and apoptosis. It has been shown in fibroblasts isolated from E11.5 c-jun^–/– and c-jun^+/– embryos that the absence or diminished expression of c-Jun resulted in greatly reduced growth rates, and that this proliferation defect could not be compensated by addition of purified mitogens (Johnson et al., 1993; Schreiber et al., 1999). Evidence for a role of c-Jun and c-Jun phosphorylation in apoptosis was obtained in neuronal cells where transient overexpression of c-Jun induced apoptosis, and expression of a dominant negative c-jun mutant inhibited apoptosis in vitro (Estus et al., 1994; Ham et al., 1995; Behrens et al., 1999). In vivo, however, c-Jun was regarded not to be essential for apoptosis since in the developing mouse (E11.5 c-jun^–/– fetuses) the physiologically occurring apoptosis appeared unaffected (Roffler-Tarlov et al., 1996).

The different phenotypes observed in the various AP-1 knockout mice point to cell type– and developmental-specific roles of AP-1 complexes. The biological basis for the specific roles is not yet understood. To gain more insight into how the absence of a widely expressed transcription factor like c-Jun affects the liver, and to see whether other tissues are affected, we investigated in detail the morphological and functional alterations in c-jun knockout mice as well as the distribution of c-jun^–/– cells in chimeric mice at various stages during fetal development and postnatal life. A deregulation of apoptosis was found in a variety of cell types lacking c-jun, such as hepatoblasts, erythroid cells, and fibroblasts. In contrast to previous reports that suggested that c-Jun is essential for cells to undergo apoptosis, we observed markedly increased apoptotic rates in the absence of c-Jun. It is possible that an increased susceptibility of cells to apoptosis was responsible for the morphologic alterations seen in the livers of c-jun^–/– mice. Increased apoptotic rates in combination with reduced proliferation rates would result in a disturbance of hepatocyte turnover which could explain the absence of c-jun^–/– hepatocytes in livers of adult chimeric mice. Furthermore, a novel function of c-Jun in heart development was identified, since all c-jun^–/– fetuses had a malformation of the outflow tract of the heart which could be a contributing factor to the fetal lethality.

	Materials and Methods

Top Abstract Materials and Methods Results Discussion References

 
Mice
Heterozygous c-jun^+/– male and female mice of C57BL/129 background (Hilberg et al., 1993) were mated and the appearance of the vaginal plug was taken as E0.5. Pregnant mothers were killed at 11.5–14.5 d of gestation by cervical dislocation and the fetuses were isolated. Genotypes of fetuses were determined by PCR using the primers c-jun 1430 and c-jun 2287 (Table I).

Apoptotic cells were analyzed in paraffin sections by in situ DNA end labeling (TUNEL; Sibilia et al., 1998), and labeled DNA was detected with the ABC procedure (DAKO).

For double-label immunofluorescence analysis fetuses were snap-frozen in isopentane at the temperature of liquid nitrogen, and sections (4 µm thick, fixed in acetone at –20°C for 10 min) were sequentially incubated with the following antibodies: monoclonal mouse antibodies against desmoplakin I and II (Boehringer Mannheim), E-cadherin (ZYMED), connexin 43 (Cx 43; Transduction Laboratories), and monoclonal rat antibodies TER119, CD71, CD11b, and CD34 (PharMingen) against hematopoietic cells or polyclonal rabbit antibodies against desmin (Chemicon) or keratins 8 and 18 (Zatloukal et al., 1990). Primary antibodies were detected with fluorescein isothiocyanate-conjugated or tetramethylrhodamine isothiocyanate-conjugated antibodies directed against mouse and rat or rabbit immunoglobulins, respectively. For negative control, primary antibodies were omitted or replaced by unrelated isotype-matched immunoglobulins. Specimens were analyzed with a MRC600 (Bio Rad Laboratories) laser-scanning confocal device attached to a Zeiss Axiophot microscope. Alternatively, sections of paraffin-embedded liver samples were stained with the antibodies to keratins 8 and 18 or the antibody TER119 after pretreatment with pronase E, and bound antibodies were detected by the APAAP procedure (DAKO).

Reconstitution of Hematopoiesis in Lethally Irradiated Mice and Flow Cytometric Analysis of Blood Cells
Liver cells isolated from C57BL/129 E12.5 c-jun^+/– and c-jun^–/– fetuses were resuspended in PBS, and 10⁶ cells were injected intravenously into adult C57BL/129 wild-type recipient mice that were lethally irradiated (9.5 Gy). All control mice injected with PBS died after 2 wk. After 8 mo, reconstitution of the various hematopoietic lineages was analyzed by FACScan^® with the following cell surface markers: B220, CD43, GR1, MAC1, CD4, CD8, TER119, and HSA as described (Sibilia and Wagner, 1995).

Quantitative RT-PCR
For generation of exogenous artificial RNA standards that served as competitors in quantitative RT-PCR, sequences corresponding to the mRNA or heterologous (unrelated) sequences were cloned into the expression vector pCRII (Invitrogen; Table I). For restriction standards, a cleavage site of a restriction enzyme between the primer binding sites was mutated by filling it with Klenow fragment (Promega Corp.). Standard plasmids with a deletion between the primer binding sites were constructed either by Bal 31 exonuclease digest or by loop out mutagenesis. For heterologous standards, a heterologous sequence, flanked by the specific primer binding sequences, was generated by amplification with hybrid primers and cloned into pCRII. Exogenous artificial RNA transcripts were generated from linearized standard plasmids by in vitro transcription with the corresponding RNA polymerases (T3, T7, and SP6 were obtained from Boehringer Mannheim). First strand cDNA synthesis for quantitative RT-PCR was performed in a 20-µl reaction mixture containing 0.1 µg of total RNA (isolated as described by Krieg et al., 1983), 0.5 units Inhibit-ACE (5' 3' Inc.), 1xAMV reverse transcription buffer (100 mM Tris-HCl, pH 8.3 at 42°C, 40 mM KCl, 10 mM MgCl₂, and 0.5 mM spermidine), 5 mM dNTPs (1.25 mM each), 4 mM sodium pyrophosphate, 5 units AMV reverse transcriptase (Boehringer Mannheim), 0.5 µM lower primer, and a certain number of exogenous artificial RNA molecules. For PCR optimal buffers for each primer pair were selected using the PCR optimizer kit (Invitrogen; Table I). PCR was performed with one-tenth of the cDNA products amplified in a 50-µl reaction containing 1x PCR buffer, 5 µl DMSO, 1 µM of each primer (except 0.5 µM for quantitation of hepatocyte growth factor mRNA), 0.25 µM of each dNTP, and 2.5 units AmpliTaq DNA Polymerase (Perkin Elmer Cetus). The reaction was heated to 94°C, then Taq Polymerase was added, and subsequently cycled for 45 cycles at 94°C, 1 min, 55°C (except 50°C for albumin and transferrin, 52°C for erythropoietin), 1 min, and 72°C, 1 min. At the end of the last cycle a final extension step of 4 min at 72°C was added. PCR products were separated on ethidium bromide-stained agarose gels and band intensities were estimated by video densitometry (Docu Gel V densitometer and Rflp-Scan or ONE-Dscan software; Scanalytics). mRNA copy numbers were calculated from the differences in the band intensities which were corrected by application of standard curves as described (Eferl et al., 1997).

Analysis of Chimeric Mice
c-jun^–/– ES cells (clone D3-2, Hilberg et al., 1993) were injected into C57BL/6 blastocysts. Tissues of chimeric mice were analyzed for glucose phosphate isomerase (GPI) isoenzyme distribution as described (Hilberg et al., 1993). The contribution of c-jun^–/– ES cells to fetal liver tissue was analyzed in short-term cultures of fetal liver cells. Fetal livers were dissected from staged fetuses and after a brief rinse in PBS subjected to 5-min subsequent incubations in solution A (EBSS without Ca²⁺ and Mg²⁺ containing 0.5 mM EGTA), solution B (EBSS containing Ca²⁺, Mg²⁺, and 10 mM Hepes, pH 7.4), and solution C (EBSS containing Ca²⁺, Mg²⁺, 10 mM Hepes, pH 7.4, and 0.3 mg/ml collagenase). Fetal livers were washed once in PBS and liver cells were dispersed by pipetting several times with a 1-ml glass pipette. After centrifugation, cells were cultured in plastic dishes (Falcon Primaria, Becton Dickinson) in DMEM containing 10% fetal calf serum for 2–3 d and nonadherent hematopoietic cells were removed by repeated washings twice daily. GPI analysis was then performed with cultured fetal liver cells and with the residual fetal tissues, which remained after dissection of the liver, to calculate the relative contribution of c-jun^–/– ES cells to the liver in relation to the average chimerism.

The contribution of c-jun^–/– ES cells to the various tissues of chimeric mice at various age after birth was furthermore determined by PCR using the primers c-jun 1430 and c-jun 2287 (Table I). Hepatocytes were isolated from livers of 8-wk-old chimeric mice by collagenase liver perfusion essentially as described by Seglen (1976) except that perfusion was performed via the left ventricle (Edström et al., 1983). This technique yields a hepatocyte preparation with 90% purity (as estimated by immunohistochemical detection of keratin), and, based on trypan blue exclusion, >85% viability. For preparation of bile ducts, sections of snap-frozen livers were stained with methylene blue, and bile ducts were microdissected under a stereo-microscope using a 25-G needle attached to an 1-ml syringe. The microdissected tissue was collected in an Eppendorf tube and DNA was isolated for PCR analysis. PCR products were separated on ethidium bromide–stained agarose gels and band intensities were estimated by video densitometry. Nonlinearity of band intensity ratios was corrected with a standard curve (Eferl et al., 1997).

Simultaneous Detection of S-Phase Cells and Apoptotic Cells in Fetal Liver Cell Cultures
Livers from E12.5 mouse fetuses were mechanically dissociated and plated onto plastic chamber slides (NUNC, Kamstrup, DK) in DME containing 10% FCS. Liver cells were cultured for 2 wk in order to remove hematopoietic cells. Purity of cultured hepatoblasts was controlled by keratin immunostaining using rabbit antibodies to keratins 8 and 18, showing that more than 95% of the cells were keratin positive. Primary fibroblasts from E12.5 fetuses were cultured as described (Robertson, 1987). [³H]thymidine labeling was performed with 300 kBq methyl [³H]thymidine/ml medium (Amersham). Primary hepatocytes were labeled for 2 h, fibroblasts for 1 h at 37°C followed by an incubation step in medium without [³H]thymidine for 30 min. Thereafter cells were rinsed twice with medium and PBS and fixed with 4% paraformaldehyde in PBS, pH 7.4, for 30 min at room temperature. Apoptotic cells were stained with the in situ cell death detection kit (Boehringer Mannheim). After dehydration with increasing concentrations of ethanol [³H]thymidine-labeled cells were visualized with Kodak NTB2 photoemulsion and detected with Kodak D19 developer.

	Results

Top Abstract Materials and Methods Results Discussion References

 
Apoptosis of Hepatoblasts and Erythroid Cells in Fetal Livers Lacking c-jun
Previous studies revealed no readily detectable differences in development or morphology between wild-type and c-jun^–/– fetuses at least up to E11.5 (Johnson et al., 1993; Hilberg et al., 1993). Between E11.5 and E14.5, in some c-jun^–/– fetuses rounded hepatoblasts, which were detached from each other and scattered cells with characteristic features of apoptosis and necrosis, were detected (Hilberg et al., 1993). However, the cell types that are affected primarily in the absence of c-Jun had not been determined yet and the developmental stage at which c-Jun becomes essential for liver development was unclear. To address these questions, detailed histological analyses of fetal livers from E12.5 and E13.0 c-jun^–/– fetuses were performed. At E12.5, no morphologic abnormalities were observed in c-jun^–/– livers. At E13.0, however, 8 out of 19 c-jun^–/– fetuses showed increased apoptosis in the livers when compared with wild-type littermates (Fig. 1, A and B). In two of these c-jun^–/– fetuses, apoptosis was very extensive, affecting up to one-third of all liver cells. Staining by in situ DNA end labeling (TUNEL) revealed fragmented DNA present in the condensed nuclei of cells undergoing apoptosis (Fig. 1, C and D). Characterization of the affected cell type by immunohistochemical staining with antibodies against keratins 8 and 18, which is expressed in hepatoblasts, and the erythroid-specific antibody TER119 confirmed, that condensed and fragmented nuclei typical of early apoptosis were present in hepatoblasts and in erythroid cells (Fig. 1, E and F). However, cells in advanced stages of apoptosis could not be classified by this method. But from the high number and distribution of apoptotic cells it is likely that apoptosis affects hepatoblasts as well as erythroid cells.

View larger version (106K): [in this window] [in a new window] [Download PPT slide]   Figure 1 Apoptosis and distribution of hepato- and erythropoiesis in livers of c-jun–/– mouse fetuses. Liver sections of E13.0 wild-type (+/+, A and C) and homozygous c-jun knockout (–/–, B and D–F) littermates. The HE-stained sections (A and B) show numerous cells with condensed nuclei, typical for apoptotic cells (arrowheads in B) in c-jun–/– livers. These nuclei contain fragmented DNA, as demonstrated by TUNEL staining (C and D, arrowheads in D). The cell types that undergo apoptosis were characterized using rabbit antibodies to keratins 8/18 (E) and the monoclonal rat antibody TER119 (F), respectively. Bound antibodies were detected by the APAAP procedure and sections were counterstained with HE. In E hepatoblasts with fragmented nuclei (filled arrowheads) and hepatoblasts with intact nuclei are visible. Some of the hepatoblasts contain apoptotic bodies (open arrowhead) engulfed by phagocytosis. In F TER119-positive erythroid cells containing fragmented nuclei are shown (arrowheads). Distribution of hepatopoiesis and erythropoiesis in livers of E12.5 wild-type (+/+, G) and c-jun–/– littermates (–/–, H). Liver sections were double-labeled with antibodies to hepatoblasts and erythroid cells using rabbit antibodies to keratins 8 and 18 (green) and the monoclonal rat antibody TER119 (red), respectively. Bars, 20 µm.

At around E11.5, the liver becomes the primary site of hematopoiesis and liver cells are necessary to provide the proper microenvironment to support survival of hematopoietic cells (Dzierzak and Medvinsky, 1995). The apoptosis observed in c-jun^–/– erythroblasts could either be due to a cell-autonomous defect in this particular cell lineage or, alternatively, c-jun^–/– fetal liver cells may be unable to provide the proper microenvironment for hematopoietic cells. To discriminate between these two possibilities and in order to investigate whether c-jun^–/– hematopoietic cells were affected in a cell-autonomous manner, E12.5 c-jun^–/– fetal liver cells were injected intravenously into wild-type lethally irradiated syngeneic adult mice. After six months, mice reconstituted with c-jun^–/– cells were healthy and flow cytometric analysis of spleen, bone marrow, and thymus of two mice showed a similar distribution of myeloid and lymphoid cells as the controls (Fig. 2 A and data not shown). Analysis of peripheral blood showed no significant differences in hematocrits and red blood cell counts (data not shown). PCR analysis of genomic DNA isolated from bone marrow, spleen, and thymus of the reconstituted mice confirmed that these organs had been mostly colonized by c-jun^–/– hematopoietic cells (Fig. 2 B). These results indicate that hematopoietic cells of all lineages are present and functional in c-jun^–/– fetal livers, which excludes an absolute cell-autonomous defect. Therefore, the observed apoptosis in the erythroid lineage might be caused by non–cell-autonomous alterations, such as a disturbance of the microenvironment in c-jun^–/– fetal livers which is essential to sustain hematopoiesis.

View larger version (23K): [in this window] [in a new window] [Download PPT slide]   Figure 2 Reconstitution of hematopoiesis in lethally irradiated mice by c-jun–/– cells. (A) The hematopoietic compartment of a lethally irradiated mouse was reconstituted with c-jun+/– (left column) and c-jun–/– (right column) fetal liver hematopoietic cells and then analyzed by flow cytometry analysis of the spleen cells. The following antibodies to cell surface markers were used: B220 for B cells, CD43 for leukocytes, GR1 for granulocytes, Mac1 for macrophages, CD4 and CD8 for T cells, TER119 for erythroid cells, and heat stable antigen (HSA) for lymphoid precursor cells. (B) PCR analysis of genomic DNA isolated from bone marrow (bm), spleen (sp), and thymus (thy) of mice reconstituted with c-jun+/– and c-jun–/– hematopoietic cells. The genotype of the donor fetal liver cells is indicated above, and the size of the PCR products, derived from mutant and wild-type alleles on the right side. For control, PCR was performed with DNA from c-jun+/+ (+/+) and c-jun–/– (–/–) mice, and without DNA (N).

View larger version (83K): [in this window] [in a new window] [Download PPT slide]   Figure 3 Analysis of mRNA expression in E12.5 wild-type (c-jun+/+), heterozygous (c-jun+/–), and homozygous c-jun–deleted (c-jun–/–) fetal livers by quantitative RT-PCR. (A) Ethidium bromide–stained agarose gels showing quantitative RT-PCR of hepatocyte nuclear factor 1 (HNF-1) mRNA in E12.5 fetal livers. The amount of HNF-1 mRNA was estimated by a titration assay with decreasing copy numbers of RNA standard molecules (indicated at the top of the figure) and a constant amount of liver RNA (0.1 µg). Cleaved PCR products (221 bp, 67 bp) are derived from HNF-1 mRNA; noncleaved PCR products (288 bp) are derived from the RNA standard. (B) Quantitative RT-PCR of mRNAs in E12.5 fetal livers. The bars represent mean values of mRNA copy numbers per 0.1 µg RNA of at least three independent experiments. The standard deviations are indicated. HNF-1, hepatocyte nuclear factor 1; EPO, erythropoietin; HGF, hepatocyte growth factor; GAPDH, glyceraldehyde-3-phosphate dehydrogenase. (C) Expression of c-jun mRNA during liver development. The amount of c-jun mRNA was estimated by quantitative RT-PCR in wild-type mouse livers of different age (E12.5-adult). Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) mRNA was estimated as control.

It is surprising that all mRNAs analyzed, including mRNAs of genes that are known to be regulated by AP-1, such as keratin 18 (Oshima et al., 1990) and β-globin (Ney et al., 1990), showed no significantly deregulated expression levels in E12.5 livers. One explanation is that at E12.5, when these analyses were performed, c-jun is expressed at a very low level (3 x 10⁴ copies per 0.1 µg RNA) in the liver (Fig. 3 C), and there is an up to threefold induction of c-jun in the liver at E13.5-E15.5 (Fig. 3 C), which coincides with the observed apoptosis of hepatoblasts and erythroid cells as well as the death of c-jun^–/– fetuses. This indicates that c-Jun gains significance in the liver around E13.5 possibly by exerting functions that are not essential in earlier phases of fetal development.

ES Cells Lacking c-jun Contribute to the Liver of Young but Not Adult Chimeric Mice
Previous studies of chimeric mice that were generated by injection of ES cells lacking c-jun into wild-type mouse blastocysts showed that the ES cells contributed to all tissues except to the liver (Hilberg et al., 1993), suggesting that in the absence of c-Jun no mature hepatocytes can be generated. However, the morphologic as well as molecular characterization of liver differentiation and function revealed no striking differences between c-jun^+/+ and c-jun^–/– fetuses up to E12.5 (Figs. 1 and 3), which poses the question up to which developmental stage c-jun^–/– hepatoblasts are able to survive and differentiate properly in chimeric mice. Analysis of c-jun^–/– ES cell contribution in E14.5-E17.5 chimeric mouse livers was performed in short-term fetal liver cell cultures. A short culturing period of the fetal livers allowed us to remove most of the hematopoietic cells, which adhere much less efficiently to the culture dishes than hepatoblasts. In these cultures similar amounts of c-jun^+/+ and c-jun^–/– hepatoblasts were detected by GPI assay (Fig. 4 A). ES cell derivatives lacking c-jun were also present in chimeric mouse livers at several weeks after birth (Fig. 4 A). Detailed analysis of the various tissues from an 8-wk-old chimeric mouse by PCR showed substantial contribution of c-jun^–/– cells to the liver cell mass (Fig. 4 B). These c-jun^–/– cells were present among the hepatocyte cell population, which was isolated and enriched by collagenase liver perfusion, ensuring that the c-jun^–/– cells did not reflect nonparenchymal cells, like sinusoidal endothelial or Kupffer cells. Moreover, bile duct epithelial cells were analyzed after enrichment by microdissection. Since we found substantial contribution of c-jun^–/– cells to bile duct epithelia, the absence of c-Jun has no obvious adverse effect on the differentiation of hepatoblasts into the hepatocytic or the bile duct epithelial lineage. There was, however, a tendency of continuous loss of c-jun^–/– hepatocytes in older chimeric mice. c-jun^–/– hepatocytes were detectable up to 8 wk after birth but not in 3-mo-old or older mice. This points to an imbalance in the regulation of hepatocyte cell turnover in adult mice in that c-jun^–/– hepatocytes have either a proliferation or a survival disadvantage over wild-type hepatocytes.

View larger version (27K): [in this window] [in a new window] [Download PPT slide]   Figure 4 Contribution of c-jun–/– ES cells to tissues of chimeric mice. (A) Glucose phosphate isomerase (GPI) analysis of chimeric mice during fetal (E13.5–E15.5) and postnatal development (1–8 wk). The chimerism was determined by densitometric analysis of the GPI-1a (derived from c-jun–/– ES cells) and the GPI-1b isoforms (derived from the wild-type C57BL/6 blastocysts) on a cellugel. Black bars represent the amount (%) of c-jun–/– cells in fetal hepatoblasts and postnatal livers. Gray bars represent the relative contribution of c-jun–/– cells to the fetus or the skin as indicator of average chimerism. Each pair of black and gray bars are data from one chimeric animal (n.d.; no c-jun–/– cells were detectable). Presence of c-jun–/– hepatoblasts during fetal development was analyzed in short-term cultures of fetal liver cells and average chimerism was determined in the residual fetus (after removal of the liver). During postnatal development, GPI analysis was directly performed on liver tissue and coat chimerism was assessed by estimation of the coat colors (agouti versus black fur). (B) PCR analysis of c-jun–/– ES cell contribution to tissues of an 8-wk-old chimeric mouse. c-jun+/+ and c-jun–/– alleles were competitively amplified by PCR from DNA of the indicated tissues (band positions on the right). Hepatocytes were isolated by collagenase perfusion. Bile ducts were microdissected under a stereomicroscope from methylene blue-stained frozen liver sections. Note that at 8 wk of postnatal development c-jun–/– cells are present in the liver and among purified hepatocytes. s. intestine, small intestine; l. intestine, large intestine; sal. glands, salivary glands.

View larger version (71K): [in this window] [in a new window] [Download PPT slide]   Figure 5 Growth of fetal liver cells lacking c-jun. (A and B) Primary liver cultures from E12.5 c-jun+/+ and c-jun–/– littermates. Note the reduced cell number and density in cultures from c-jun–/– livers (B). Bars: 100 µm. (C and D) Simultaneous detection of apoptosis and DNA replication in E12.5 fetal liver cultures. Primary hepatoblasts were stained for apoptotic cells by TUNEL (open arrowheads) and for cells replicating its DNA by [3H]thymidine incorporation (filled arrowheads). The number of apoptotic cells is increased in c-jun–/– cultures (D) whereas the number of [3H]thymidine-labeled cells is reduced. (E) Percentage of [3H]thymidine-labeled cells (dark bars) and apoptotic cells (light bars) in E12.5 primary liver cells and corresponding fibroblast cultures. Note the three- to fourfold increased apoptosis and reduced number of [3H]thymidine-labeled cells in c-jun–/– cultures of primary hepatocytes and fibroblasts. The bars represent mean values of three to six independent experiments using separate fetuses for preparation of liver and fibroblast cultures. The standard deviations are indicated. Bars, 50 µm.

View larger version (122K): [in this window] [in a new window] [Download PPT slide]   Figure 6 Impaired heart development of c-jun–/– fetuses. Corresponding horizontal sections of E12.5 wild-type (A) and c-jun–/– mouse fetuses (B) were stained with HE. At this stage of development, wild-type fetuses show separation of the aorta (ao) and the pulmonary trunk (pt). In c-jun–/– fetuses (B) there is a single outflow vessel (arrow) that arises from the right ventricle. Corresponding horizontal sections through the hearts of E14.5 wild-type (C, E, and G) and c-jun–/– mouse fetuses (D, F, and H). The sections are arranged from cranial to caudal and show three major anomalies: (a) persistence of the right branch of the 4th aortic arch artery (aa in D), (b) persistent truncus arteriosus (pta in F) whereas the wild-type littermate show complete separation of the aorta and pulmonary trunk (arrow in E), and (c) incomplete septation of the ventricles (arrow in H). ao, aorta; pt, pulmonary trunk; rv, right ventricle; lv, left ventricle; ra, right atrium; la, left atrium; aa, aortic arch; tr, trachea; oe, oesophagus; th, thymus; pv, pulmonary valve; pta, persisting truncus arteriosus; av, aortic valve; vs, ventricular septum. Bars, 200 µm.

View larger version (69K): [in this window] [in a new window] [Download PPT slide]   Figure 7 Impaired migration of neural crest cells to the outflow tracts of c-jun–/– fetuses. Corresponding horizontal sections of E12.5 wild-type (A, C, E, and G) and c-jun–/– mouse fetuses (B, D, F, and H) were analyzed for the presence of neural crest cells by double-label immunofluorescence microscopy using a monoclonal mouse antibody against the neural crest cell protein Cx 43 (green) and polyclonal antibodies against desmin (red). The micrographs show corresponding sections of c-jun+/+ (A, C, E, and G) and c-jun–/– (B, D, F, and H) littermates (two c-jun+/+, one c-jun+/–, and four c-jun–/– fetuses were analyzed). Cx 43 positive cells were visible in the outflow tract of wild-type (arrows in A) but not in c-jun–/– fetuses (B). In contrast to the outflow tract, no differences in Cx 43 immunoreactivity were found between wild-type and c-jun–/– fetuses in the peritracheal mesenchyme (arrows in C and D) and the mesenchyme in vicinity of the spinal cord (arrows in E and F). For control, Cx 43 immunoreactivity is shown in the trabeculae carneae of the ventricles (G and H). Note the thinner wall of the ventricles in c-jun–/– hearts (H). pt, pulmonary trunk; ta, truncus arteriosus; vw, ventricle wall; tr, trachea; oe, oesophagus; sc, spinal cord; tc, trabeculae carneae. Bars, 50 µm.

	Discussion

Top Abstract Materials and Methods Results Discussion References

The effect of c-Jun inactivation was not restricted to erythroid cells but also affected other cell types, such as hepatoblasts and fibroblasts. Primary liver cell as well as fibroblast cultures established from E12.5 c-jun^–/– fetuses and their corresponding wild-type littermates showed markedly increased apoptotic rates in the absence of c-Jun. This was surprising, since in contrast to our findings, previous studies reported that overexpression of c-Jun forced fibroblasts into apoptosis, and functional inhibition of c-Jun prevented cell death in some cell types (Estus et al., 1994; Ham et al., 1995; Bossy-Wetzel et al., 1997). These controversial observations indicate that the role of c-Jun in apoptosis depends on the cellular context and mode of treatment. It is interesting that in c-jun^–/– mice no obvious alteration of apoptosis was noted during fetal development until E11.5, whereas primary cell cultures derived from E12.5 c-jun^–/– mice had markedly increased apoptotic rates. One possible explanation for this difference between the in vivo and in vitro situation is that apoptosis is preferentially triggered under enforced stimulation of proliferation as it is the case under cell culture conditions. It is possible that the absence of c-Jun modulates the intracellular signals induced by growth factors so that cells respond with apoptosis instead of mitosis. In addition to the alterations in apoptosis, we noted reduced mitotic rates in primary cultures of c-jun^–/– fibroblasts and hepatoblasts. One mechanism by which lack of c-Jun could result in impaired proliferation was recently shown by Schreiber et al., 1999. The proliferation defect in c-jun^–/– fibroblast cell lines was found to be p53-dependent, indicating that the alterations of proliferation, and probably also the increased propensity of cells to undergo apoptosis may involve p53-dependent pathways.

The altered regulation of cell proliferation and apoptosis in the absence of c-Jun could be an explanation for the occurrence of massive apoptosis of erythroblasts and hepatoblasts in c-jun^–/– E13.0 fetuses. Moreover, the proliferation defect as well as the increase in apoptosis could lead to the loss of c-jun^–/– cells in livers of adult chimeric mice because of a lower capacity of c-jun^–/– hepatocytes to contribute to the cell turnover. However, it is unlikely that the deregulation of proliferation and apoptosis is the only cause of fetal lethality since massive apoptosis was seen in only 2 livers out of 19 c-jun^–/– fetuses, and we have analyzed some c-jun^–/– fetuses that had died in utero without showing severe morphological liver alterations.

It is known from other gene knockout mice, that in addition to the liver, defects in other organ systems, especially the cardiovascular system, have to be considered as causes of mid-gestational lethality (Rossant, 1996). Detailed investigation of hearts of c-jun^–/– fetuses revealed a novel function for c-Jun in fetal heart development. Lack of c-Jun led to several anomalies of the heart outflow tracts. All of the c-jun^–/– fetuses had compared with wild-type littermates anomalies of the aorta ascendens and pulmonary artery in that in mutant mice there was a single outflow vessel arising from the right ventricle resembling a truncus arteriosus persistens. In addition to the outflow tract alteration, some mice showed a right-sided aortic arch. These anomalies are typical for a neural crest cell defect (Kirby and Waldo, 1995). It has been shown that the ectomesenchymal cells of cardiac neural crest, which extends from the midotic placode to the caudal limit of somite 3, migrate into the outflow tract of the heart where they contribute to the aorticopulmonary septum. Moreover, cardiac neural crest cells differentiate into smooth muscle cells of the aortic arch and contribute to the stroma of other derivatives of the pharyngeal arches such as thymus, parathyroid, and thyroid gland (Kirby and Waldo, 1990). Experimental ablation of neural crest cells in chick embryos led to various defects of which a persistent truncus arteriosus was a common denominator. These lesions were always combined with a ventricular septal defect (Nishibatake et al., 1987). Furthermore, a right-sided aortic arch or anomalies of the other great arteries were seen after partial neural crest cell ablation.

The cardiovascular defects observed by us in c-Jun knockout mice were almost identical to those found after neural crest cell ablation in chicken. Similar to the observations in chicken, a variety of gene mutant mice with impaired neural crest cell development showed anomalies of the outflow tract. For instance, the mouse mutant Splotch, which harbors a mutation in the homeobox gene pax3, exhibits conotruncal and aortic arch defects (Conway et al., 1997; for review on mouse mutants with heart defects see Olson and Srivastava, 1996). In contrast to the situation in chicken and in the above-mentioned mouse mutant, where cardiac neural crest cell were either absent or had a general defect, we have observed no difference in neural crest cell distribution in c-jun knockout mice except for a reduced number of Cx 43–expressing cells in the outflow tract of the right ventricle. This observation suggests that the consequences of c-Jun inactivation primarily affects neural crest cell function in the heart and does not result in a general neural crest cell defect. As known from neural crest cell ablation experiments in animals as well as from human diseases with a truncus arteriosus persistens (e.g., DiGeorge syndrome), the malformations are not restricted to the heart but also affect other neural crest cell derivatives, such as the thymus or parathyroid. In c-jun mutant fetuses, however, morphologic analysis provided no evidence for a thymus defect, and thus for a general alteration of the cardiac neural crest (Fig. 6, C and D). Nevertheless, the cardiac malformations observed are highly reminiscent for a disturbance of neural crest function, which may be restricted to the heart and great vessels. Moreover, as shown by neural crest cell transplantation experiments, the mere presence of neural crest cells does not exclude functional deficiencies (Kirby and Waldo, 1990).

The cardiac malformation of a truncus arteriosus persistens may be a major factor contributing to the lethal phenotype. In principle, occurrence of a truncus arteriosus persistens is compatible with survival because of compensation of the hemodynamic imbalance. This compensation may not occur in c-jun mutant fetuses and fetal lethality might be due to pleiotropic defects reflecting the diversity of functions of c-Jun in development, such as a role in neural crest cell function, in the maintenance of hepatic hematopoiesis and in the regulation of apoptosis.

	Acknowledgments

 
This work has been supported by a grant from the Austrian Science Foundation (S7401-MOB) to K. Zatloukal and E.F. Wagner (S07406-MOB). R. Zenz is supported by a scholarship of the Austrian Academy of Sciences.

Submitted: 23 October 1998

Revised: 14 April 1999

The technical assistance of Ms. C. Stumptner is gratefully acknowledged.

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