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Anti-Mitochondrial Antibodies and Primary Biliary Cirrhosis in TGF- Receptor II Dominant-Negative Mice¹

Sabine Oertelt^2,*,, Zhe-Xiong Lian^2,*, Chun-Mei Cheng^*, Ya-Hui Chuang^*, Kerstien A. Padgett^*, Xiao-Song He^*, William M. Ridgway, Aftab A. Ansari, Ross L. Coppel^¶, Ming O. Li^||, Richard A. Flavell^||, Mitchell Kronenberg^#, Ian R. Mackay^** and M. Eric Gershwin^3,*

^* Division of Rheumatology, Allergy and Clinical Immunology, University of California School of Medicine, Davis, CA 95616; Division of Internal Medicine, Department of Medicine, Surgery and Dentistry, San Paolo School of Medicine, University of Milan, Milan, Italy; Division of Rheumatology and Immunology, University of Pittsburgh School of Medicine, Pittsburgh, PA 15261; Department of Pathology, Emory University School of Medicine, Atlanta, GA 30322; ^¶ Department of Microbiology, Monash University, Melbourne, Australia; ^|| Section of Immunobiology, Howard Hughes Medical Institute, Yale University School of Medicine, New Haven, CT 06520; ^# La Jolla Institute of Allergy and Immunology, San Diego, CA 92121; and ^** Department of Biochemistry and Molecular Biology, Monash University, Clayton, Victoria, Australia

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
Primary biliary cirrhosis (PBC) is an autoimmune disease of the liver, characterized by lymphocytic infiltrates in portal tracts, selective destruction of biliary epithelial cells, and anti-mitochondrial Abs (AMAs). The elucidation of early events in the induction of tissue inflammation and autoimmunity in PBC has been hampered by the cryptic onset of the disease, the practical limitations in accessing the target tissue, and the lack of a suitable animal model. We demonstrate in this study that a mouse transgenic for directed expression of a dominant-negative form of TGF- receptor type II (dnTGFRII), under the direction of the CD4 promoter, mimics several key phenotypic features of human PBC, including spontaneous production of AMAs directed to the same mitochondrial autoantigens, namely PDC-E2, BCOADC-E2, and OGDC-E2. The murine AMAs also inhibit PDC-E2 activity. Moreover, there is lymphocytic liver infiltration with periportal inflammation analogous to the histological profile in human PBC. Additionally, the serum cytokine profile of affected mice mimics data in human PBC. The concomitant presence of these immunopathological features in the transgenic mice suggests that the TGF-RII pathway is implicated in the pathogenesis of PBC. Finally, these data point away from initiation of autoimmunity by mechanisms such as molecular mimicry and more toward activation of an intrinsically self-reactive T cell repertoire in which necessary regulatory T cell influences are lacking.

	Introduction

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Primary biliary cirrhosis (PBC) is a progressive autoimmune liver disease characterized by portal inflammation and immune-mediated destruction of the intrahepatic bile ducts. The damage of bile ducts is associated with cholestasis and progressive development of hepatic lesions which include fibrosis, cirrhosis, and eventually lead to liver failure. Serologically, PBC is characterized by the presence of anti-mitochondrial Abs (AMAs) in 90–95% of patients preceding the occurrence of symptoms by many years (1). AMAs react with an epitope on the E2 subunit of the pyruvate dehydrogenase enzyme complex (PDC-E2) and, in a smaller proportion of cases, with the E2 subunit of functionally related 2-oxo-acid dehydrogenase complexes, branched chain 2-oxo-acid dehydrogenase (BCOADC-E2), and 2-oxo-glutarate dehydrogenase (OGDC-E2) (2). All of these enzymes contain two sites (the inner and outer domains) at which lipoic acid is attached to a lysine residue and acts as a swinging arm to transfer chemical groups between other members of the respective enzyme complexes. The major epitope for both autoantibodies and for reactive CD4 and CD8 T cells (3, 4) resides in the inner lipoyl domain of these enzyme complexes (5).

We report in this study that mice transgenic for directed expression of a dominant negative form of TGF receptor type II (TGFRII), under the CD4 promoter lacking the CD8 silencer (6), spontaneously develop features characteristic of PBC. These features include the development of significant titers of autoantibodies with specificity against PDC-E2, BCOADC-E2, and OGDC-E2 that, as in PBC, inhibit enzyme function in vitro and react with the inner lipoyl domain epitope of the respective E2 subunits. Histologically there is extensive CD4⁺ and CD8⁺ lymphocytic infiltration in portal tracts, associated with biliary destruction. Moreover, mice manifest increased serum IFN- and elevated TNF-, as seen in PBC (7, 8). The fact that TGFRII-transgenic mice have specific impairment of TGF signaling, exclusively in T lymphocytes, provides the unique opportunity to identify a mechanism for the development of autoimmune biliary disease that could be applicable to human PBC. A previous report indicating the involvement of the TGFRII pathway in the development of liver fibrosis (9) combined with the data presented herein suggest that lack or aberrant activity of TGF- signaling contributes to a loss of self tolerance to autoantigenic proteins in the liver, which in turn leads to autoimmunity. Moreover, it points away from initiation of autoimmunity by mechanisms such as molecular mimicry and more toward activation of an intrinsically self-reactive T cell repertoire in which necessary regulatory T cell (T reg) influences are lacking.

	Materials and Methods

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Dominant-negative (dn) TGFRII mice

dnTGFRII mice were originally developed by R. A. Flavell (6). The dnTGFRII mice were bred onto the C57BL/6 background (The Jackson Laboratory) at the University of California animal facility (Davis, CA). Nineteen dnTGFRII mice and 17 control littermates were used for the described experiments. dnTGFRII and wild-type littermates were fed with the sterile rodent Helicobacter Medicated Dosing System (three-drug combination) diets (Bio-Serv) and maintained in individually ventilated cages under specific pathogen-free condition. dnTGFRIIRag1^–/– mice were generated by backcrossing female B6 Rag1^–/– with male dnTGFRII mice. The resulting F₂ generation was genotyped and selected for dnTGFRIIRag1^–/– mice. All studies were performed with approval from the University of California Animal Care and Use Committee.

Production of recombinant mouse mitochondrial proteins

cDNA encoding the full-length protein of mouse OGDC-E2 and BCOADC-E2, as well as amino acids 1–391 of PDC-E2, which includes the inner lipoyl domain on this protein, were generated with standard reverse transcription and PCR, using total RNA isolated from mouse liver. The PDC-E2 cDNA was engineered into the Escherichia coli expression vector pCAL-n-Flag (Stratagene) with a 6x His purification tag on the C terminus of the partial protein. The OGDC-E2 and BCOADC-E2 cDNA were engineered into the E. coli expression vector pET32a. The recombinant proteins were expressed in E. coli Rosetta-gami 2(DE3) (Novagen). The expressed His-tagged fusion proteins were purified with Ni-NTA affinity chromatography (Qiagen) under denaturing conditions.

ELISA and immunoblotting for AMA

Ninety-six-well ELISA plates (Nunc) were coated overnight with 100 µl of rAMA Ags (PDC-E2, BCOADC-E2, OGDC-E2) at a concentration of 10 µg/ml. A reference standard was composed of pooled AMA-positive mouse sera, used to construct a standard curve by serial dilutions of the reference serum and an ELISA performed as described (10). Plates were read at 450 nm. Threshold values are set by mean + 2 SD of values for B6 controls. For immunoblotting, 20 µg of the purified mouse rPDC-E2 protein was loaded on a 4–20% Novex mini protein gel (Invitrogen Life Technologies) and fractionated at 170 V for 1 h and probed as described with known positive and negative sera (10). The signal was detected with a FluorTech 8900 gel doc system (Alpha Innotech) equipped with a chemiluminescent filter.

Inhibition of pyruvate dehydrogenase (PDC) enzyme activity

A predetermined serum dilution (1/100) was incubated with PDC (Sigma-Aldrich) for 10 min at room temperature. The solution was then added to a PDC reaction mixture containing 5 mM sodium pyruvate, 2.5 mM NAD+, 0.2 mM thiamine pyrophosphate, 0.1 mM coenzyme A, 0.3 mM DTT, 1 mM magnesium chloride, 50 mM potassium phosphate buffer (pH 8.0). UV absorbance change per minute at 340 nm was monitored for 5 min. Enzyme activity measurements without addition of serum were run in parallel to define 100% activity. Enzyme inhibition activity was assayed in parallel on sera from dnTGFbRII mice, B6 mice, patients with PBC and negative human controls.

Liver tissue preparation

dnTGFbRII and control mice were sacrificed at age 24–28 wk. Whole liver tissue was explanted and immediately fixed with a 1:1 solution of formalin (18.75%) and methanol (100%) for 1 to 2 h at room temperature. Paraffin-embedded tissue sections were then cut into 5-µm slices for routine hematoxylin (DakoCytomation) and eosin (American Master Tech Scientific) staining.

Immunohistochemistry

Abs against cell markers, including CD4 (1/200 dilution), CD8 (1/200), CD19 (1/50; all obtained from eBioscience), pDCA1 (1/200; Miltenyi Biotec), DX5 (1/50; Biolegend), and myeloperoxidase (MPO; 1/10; Cell Sciences) were used for immunohistochemical staining of the portal tract infiltrates. Anti-cytokeratin 7 (1/10; Research Diagnostics) was used as a biliary cell marker. Briefly, after deparaffinization sections were incubated in a Decloaking Chamber (Biocare Medical; set point (SP)1 123°C for 2 min, SP2 85°C for 10 s, SP limit 10°C) soaked in 3% H₂O₂ methanol solution for 5 min, then 15 min in 1x Universal blocking solution (BioGenex) and 20 min in 10% goat serum to prevent nonspecific staining. Primary Abs were applied for 1 h at room temperature in a moist chamber. After three washes with 0.1% Tween 20 in PBS (PBST) for 5 min, HRP-conjugated polyclonal rabbit anti-rat Ig (DakoCytomation; 1/100) or polyvalent anti-mouse Ig (DakoCytomation, ready to use) or goat anti-hamster IgG (GeneTex; 1/100 dilution) was applied as secondary Ab for 1 h at room temperature in a moist chamber. After three washes with PBST, the sections were developed with 3,3'-diaminobenzidine (DAB; DakoCytomation) and counterstained with Mayer’s hematoxylin (DakoCytomation).

For phenotypic definition of the MPO-positive cells, double enzyme immunohistochemical staining was performed. Briefly, anti-F4/80 (Caltag Laboratories; 1/25) was applied as a primary Ab as described above, and polyclonal HRP-conjugated rabbit anti-rat Ig (DakoCytomation) was used as the secondary Ab. After development with DAB, sections were boiled in water for 10 min to denature excess Ab. Anti-MPO (Cell Sciences; 1/10) was then applied for 1 h at room temperature in a moist chamber. After washing with PBST, alkaline phosphatase-conjugated polyvalent anti-mouse Ig (DakoCytomation) was used for development and Mayer’s hematoxylin for counterstaining.

Flow cytometry

Lymphoid cells from PBS-perfused liver were separated by centrifugation with Histopaque-1077 (Sigma-Aldrich). FcR were blocked by incubation with 2.4G2 mAb (eBioscience) and cells were stained with fluorochrome-conjugated Abs specific for CD3, CD4, CD8, NK1.1 (eBioscience), and -GalCer-loaded CD1d tetramers at 4°C in PBS/0.2% BSA for 30 min. The stained cells were analyzed on a five-color FACScan flow cytometer (BD Immunocytometry Systems). Acquired data were analyzed with CellQuest (BD Biosciences) and FlowJo software (Tree Star).

Measurement of serum cytokines

Serum samples were collected at different ages and kept at –70°C until assayed. Thawed serum samples were diluted 1/2 (for IFN-, TNF-, and IL-6) or 1/5 (for IL-12p40) with PBS. Concentrations of IFN-, TNF-, and IL-6 were measured with a cytometric bead assay using the mouse inflammation cytokine kit, a cytometric bead assay (BD Biosciences). Concentrations of IL-12p40 were measured using the mouse IL-12p40 ELISA kit, respectively (R&D Systems).

	Results

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dnTGFRII-transgenic mice (dnTGFRII) were first developed for studies aimed at dissection of the role of this receptor in T lymphocyte function (6). During the characterization of these dnTGFRII mice, histological studies revealed mononuclear cell infiltration of various tissues and specifically clusters of macrophages and lymphocytes in the parenchyma and portal tracts of the liver. Analysis of these histological features indicated that the pathological findings in the dnTGFRII mice appeared very similar to those seen in human PBC and prompted us to examine the sera of these mice for PBC-like serologic reactivity. Positive results for Abs to recombinant human PDC-E2 specifically directed against the inner lipoyl domain of the molecule provided the impetus to carry out the studies described herein.

dnTGFRII mice develop species-specific AMAs

Although the murine orthologs of the human PBC autoantigen show a high degree (> 99%) of similarity with the human protein, we needed to ensure that the detected reactivity was a true autoimmune response, directed also against the rodent enzymes as well as to recombinant human PDC-E2, BCOADC-E2, and OGDC-E2. Hence, all three murine genes were cloned and expressed as recombinant proteins. The cloned proteins encompassed the entire length of the native protein for BCOADC-E2 and OGDC-E2. For PDC-E2 a partial protein was produced that included the major epitope sequence of the inner lipoyl domain. AMA reactivity in mice was demonstrated by ELISA (Fig. 1A), immunoblot and immunofluorescence (data not shown) at all time points examined starting at 4 wk of age. Transgenic mice displayed an increase in reactivity toward all tested Ags over time. By weeks 22–24, 100, 95, and 68% of the mice sera samples were positive for Abs against PDC-E2, OGDC, and BCOADC, respectively. The mean titers for anti-PDC-E2, anti-OGDC-E2, and anti- BCOADC-E2 were all significantly higher for weeks 22–24 than weeks 4–10 (p < 0.0005, Mann-Whitney U test). Comparable autoantibody reactivity in the control littermate mice was not detected. This time sequence resembles that of the natural history of PBC in humans where the disease is not observed in childhood and typically presents in the fourth or fifth decade of life.

View larger version (18K): [in this window] [in a new window]   FIGURE 1. dnTGF-RII mice produce Abs to mitochondrial Ags. A, ELISA for sera from dnTGFbRII mice and control B6 littermates. Wells were coated with recombinant proteins PDC-E2, OGDC-E2, or BCOADC-E2. Serum samples were diluted 1/500. Sera from 4- to 10-wk-old mice (dnTGFRII n = 11, B6 n = 10), 12- to 16-wk-old mice (dnTGFRII n = 10, B6 n = 9), and 22- to 39-wk-old mice (dnTGFRII n = 19, B6 n = 10) were tested. Threshold values are set by mean + 2 SD of values for B6 controls. B, PDC enzyme inhibition assay. PDC was preincubated with 1/100 diluted sera from 20-wk-old dnTGFbRII mice (n = 7) and control B6 mice (n = 4), along with sera from patients with PBC (n = 6) and normal human control, followed by enzyme activity assay. *, p < 0.001. Tg+, dnTGFRII transgenic mice; Tg-, littermate controls.

Lymphocytic liver infiltrate and selective biliary ductular cell destruction in dnTGFRII mice

The liver histology of human PBC is characterized by the presence of lymphocytic infiltration associated with selective small bile duct destruction, eventually leading to cirrhosis (11). The severity and temporal progression vary widely among patients and do not correlate with AMA titers (12). The liver of 6- to 7-mo-old dnTGFRII mice was examined and compared with livers of normal B6 littermates. Moderate to severe lymphoid cell infiltration was detected within the portal tracts in association with bile duct damage (Fig. 2, A–C), occurring only in the dnTGFRII mice, and mirroring what is characteristically seen in PBC. Direct bile duct destruction was determined by the detection of scattered cytokeratin 7-positive cells in the portal infiltrates (Fig. 2D). Moreover, in liver tissues from some of the mice, biliary cell destruction was sufficiently advanced that identification of an intact bile duct structure was impossible; yet another feature similar to that seen in advanced human PBC (Fig. 2B).

View larger version (142K): [in this window] [in a new window]   FIGURE 2. Histological features of the 24–28 wk liver. A–C, Different degrees of lymphocytic infiltration (red arrows) surrounding the small bile ducts were detected within the portal tracts (H&E staining); D-L, individual cells (red arrows) of cell types composing the portal tract infiltrates were stained with Abs against cell markers: D, biliary cells identified by cytokeratin 7; E, CD4+ lymphocytes; F, CD8+ lymphocytes; G, CD19+ B cells; H, pDCA1+ plasmacytoid dendritic cells; I, DX5+ NK cells; J, MPO+ macrophages; K, macrophages stained with MPO, confirmed by costaining with F4/80 (black arrows, MPO+ cells; red arrows, MPO+F4/80+ cells).

Lymphocytic infiltrates in the liver are represented by CD4⁺ and CD8⁺ lymphocytes

The lymphocytic infiltrate detected in the liver of patients with PBC comprises both CD4⁺ and CD8⁺ lymphocytes (13) and, additionally, there is a relative increase in the resident NKT cell population compared with healthy controls (14). We analyzed the composition of the intrahepatic lymphoid cell population within the liver of transgenic mice and control littermates to establish quantitative and qualitative differences. In the liver, both the total number of CD3⁺ lymphocytes (Table I) and the percentage of CD3⁺ cells among the total lymphoid cell infiltrate (Fig. 3A) were significantly increased in the transgenic mice. Although the total number of intrahepatic CD4⁺ lymphocytes was enlarged (Table I), the percentage of CD4⁺ cells in the CD3⁺ population did not increase (Fig. 3C). In contrast, the CD8⁺ population was significantly amplified (p < 0.05) in total number (Table I) as well as percentage in the CD3⁺ population compared with controls (Fig. 3C). These features resulted in a change in the ratio of CD4 to CD8 T cells biased toward the CD8⁺ population (Table I). This finding is particularly interesting, considering previous reports of an increase in precursors of CTLs in the blood of patients in the early stages of PBC vs advanced stages and the 10-fold increase of autoantigen-specific CTLs within the liver as compared with the circulating pool, reported in the same study (4). In addition, the transgenic mice showed a marked increase in the number of intrahepatic NKT cell population, resembling the increase described in human PBC (14); although the percentage of NKT cells in intrahepatic lymphocytes did not increase in the mouse model (Fig. 3E). Interestingly, this increase was associated with a decrease of the NKT cell population within the spleen of the transgenic mice (Fig. 3F, Table I).

View larger version (47K): [in this window] [in a new window]   FIGURE 3. Lymphoid cells isolated from liver and spleen were stained with fluorochrome-conjugated mAbs and analyzed by flow cytometry. A and B, Frequency of CD3+ lymphocytes in total lymphocyte population. C and D, The percentage of CD4+ and CD8+ cells in total CD3+ population. E and F, The percentage of CD1d tetramer+ NKT cells in total lymphocyte population.

Cytokine profiles of dnTGFRII mice

A transcriptional up-regulation of IFN-, TNF-, and IL-6 within biliary epithelial cells, associated with up-regulation of their cognate receptors, has been demonstrated in PBC (7, 8). We thus analyzed the serum levels of these and various other cytokines in dnTGFRII mice and B6 littermates of different ages. The levels of IFN-, TNF-, IL-6, and IL-12p40 at ages of 14–16, 22–26, and 28–32 wk were all significantly increased in dnTGFRII mice compared with B6 littermates (p < 0.001) (Fig. 4). Of note, the levels of IFN- and TNF- in the older transgenic mice were lower than those in younger mice, while those of IL-6 and IL-12p40 did not decline with age.

View larger version (14K): [in this window] [in a new window]   FIGURE 4. Serum cytokine profiles of dnTGFRII mice. Concentrations of IFN-, TNF-, IL-6, and IL-12p40 in sera of dnTGFRII transgenic mice (Tg+) and B6 control littermates (Tg–) of different ages were determined by ELISA (*, p < 0.05 compared with 14–16 wk).

Absence of disease in dnTGFRIIRag1^–/– mice

dnTGFRIIRag1^–/– mice were observed for 6 mo. No AMAs could be detected in the serum and, more importantly, the liver histology appeared normal and similar to wild-type B6 controls without evidence of hepatic or biliary-specific pathology (data not shown).

	Discussion

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The murine model of PBC described herein, based on a deficiency in a pathway involved in peripheral tolerance, generates a new pathogenetic scenario for autoimmunity that differs from the loss of tolerance resulting from molecular mimicry or chemical modifications of a native epitope. The selective deficiency of the TGF-R-signaling pathway exclusively in T lymphocytes accounts for the impairment of a system essential to peripheral tolerance. Circulating Treg cells depend on TGF- for their regulatory activity, thus allowing the emergence of tissue-specific autoreactive effector T cells if impaired. To assess whether the liver pathology in dnTGFRII mice was due to an immune response or a TGF--mediated lesion in the biliary target tissue, we generated dnTGFRIIRag1^–/– mice. As discussed above, there was no evidence of liver pathology in these mice. This new colony represents a valuable tool for use in adoptive transfer and consequent focus on effector mechanisms. Such experiments are ongoing and are preferable to the use of anti-CD4- or anti-CD8-treated animals due to the pleiotropic sites of action of these depleting Abs. Cell transfer will allow not only dissection of the effector mechanism, but also the critical question of specific donor cell age requirements. Additional future work will also be directed at the role of bacterial flora. A number of T cell-depleted animal models of inflammatory bowel disease demonstrate reduction in their bowel pathology in a germfree environment (15). Therefore, the specific contribution of bacterial flora to disease development in this model should be addressed because PBC is frequently used as an example of molecular mimicry (16).

At a systemic level, TGF- appears as an essential modulator of Foxp3 expression by Treg cells (17), conditioning their suppressive ability in the periphery. Recent studies from our group have identified selective defects in the circulating Treg population of patients with PBC as compared with healthy controls (18). In addition, it is reported that the population of CD4⁺CD25⁺ lymphocytes that coexpress Foxp3 and TGF- decreases with age, specifically in female NOD mice, modifying both the degree of lymph node localization and target tissue infiltration (19). These results, unique to females, are of specific interest to PBC, considering also that the primary activation site of CD8⁺ T cells, whether in the regional lymph nodes or liver, appears to be fundamental for the predominance of immunity over tolerance (20). Interestingly, TGF- selectively targets circulating Treg cells and not thymic precursors. Nonetheless, the expression of CD4 by dendritic cells within the murine thymus (21) could modify the responsiveness of these cells to TGF-, altering their maturation and potentially accounting for a defect in negative selection of the intrathymic T cells. These features appear of particular importance given the recent description of autoimmune cholangitis in a congenic strain of NOD mice, with features very similar to those of human PBC (22). The most interesting connection between the two models concerns the role of TGF-. The genetic locus of autoimmune biliary disease in the NOD.c3c4 model appears within the abd locus. A candidate molecule within that region is Cdkn2b, which is induced by TGF- and is a possible mediator of TGF- cell cycle arrest (23). If the B6 variant of Cdkn2b mediates a decreased TGF- response in NOD.c3c4 mice, it might provide a mechanistic connection between the NOD.c3c4 and dnTGFRII models of PBC.

Considering the striking similarities of the murine cholangitis model described herein to human PBC, and its potential contribution to the analysis of novel pathways involved in pathogenesis, we need to annotate that this model does have some clear differences from human PBC. First, we could not detect the female bias characteristic of PBC within our population of affected animals; second, the consistent increase of circulating IgM is not shared by affected mice, which, on the contrary, develop an increase in IgA (6). However, these differences could well be secondary to species-specific differences in response to equivalent perturbations in the signaling cascade within the two species, similarly to the previously mentioned decrease of TGF-/FoxP3-positive Tregs in NOD mice. Moreover, we cannot rule out that selected factors involved in human PBC might be absent or not consistently mimicked in the murine model, such as hormonal influences (24).

Another essential difference detected in the mouse model is the absence of eosinophilic infiltration and granuloma formation. These features are reported in a number of cases of human PBC, but due to the cryptic onset of the human disease, it has not been possible to effectively define the temporal relation of eosinophilia and granuloma formation with serological positivity (25). At present, we are unable to define whether the absence of these histological characteristics is due to not sufficiently advanced disease or to consistent lack of these features in the mouse model.

In conclusion, we describe herein a murine model in which immunoregulatory defects within the lymphocytic and phagocytic components of the immune system, potentially in association with a particular vulnerability of the biliary ductular target tissue, initiate an autoimmune response resembling that seen in PBC. This model, and the newly described NOD.c3c4 model, both facilitate analysis of causal events and help define the essential steps necessary to biliary disease.

	Acknowledgments

 
We thank Dr. Patrick S. Leung for performing enzyme inhibition assays, Dr. Guo-Xiang Yang for taking care of the animal colony, and Dr. Yuki Moritoki and Thomas P. Kenny for conducting ELISA. Moreover, we thank Cynthia He for performing Western blots.

	Disclosures

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The authors have no financial conflict of interest.

	Footnotes

 
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

¹ This work was supported in part by National Institutes of Health Grant DK39588.

² S.O. and Z.-X.L. contributed equally to the results described in this report.

³ Address correspondence and reprint requests to Dr. M. Eric Gershwin, Division of Rheumatology, Allergy and Clinical Immunology, University of California School of Medicine, Genome and Biomedical Sciences Facility, 451 East Health Sciences Drive, Suite 6510, Davis, CA 95616. E-mail address: megershwin{at}ucdavis.edu

⁴ Abbreviations used in this paper: PBC, primary biliary cirrhosis; AMA, anti-mitochondrial Ab; Treg, regulatory T cell; dn, dominant negative; MPO, myeloperoxidase; SP, set point.

Received for publication March 16, 2006. Accepted for publication May 11, 2006.

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Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 

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