Mouse Husbandry

The mice used in this study were housed under standard animal housing conditions. All protocols involving animal experimentation were approved by the Institutional Animal Care and Use Committee at Massachusetts General Hospital. Mice were maintained on C57BL/6;129/SvEv mixed genetic background. Amhr2^tm3(cre)Bhr (Amhr2-Cre) mice [17] (Dr. Richard Behringer, M.D. Anderson, Houston, TX) were mated with Ctnnb1^{tm1Mmt/tm1Mmt} [16] to generate Amhr2^tm3(cre)Bhr/+;Ctnnb1^tm1Mmt/+ mice. The DNA from tail biopsies was used to genotype mice using the standard PCR protocols. The uterus collected from Amhr2^tm3(cre)Bhr/+;Ctnnb1^tm1Mmt/+ and control mice were photographed by using a Nikon SMZ1500 microscope with an attached Spot camera (Diagnostic Instruments, Sterling Heights, MI).

Oocyte and Blastocyst Collection and Assessment

The 6- to 7-wk-old mutant and control mice were superovulated with i.p. injections of 7.5 IU equine chorionic gonadotropin (eCG; Sigma Chemical Co., St. Louis, MO) followed by 7.5 IU human chorionic gonadotropin (hCG; Sigma) after 48 h. Fourteen hours after hCG injection, females were euthanized, and their oviducts were removed. The cumulus-oocyte complexes were released from the ampullary region of each oviduct by puncturing the oviduct. Cumulus cells were removed by exposure to 80 IU/ml hyaluronidase (Irvine Scientific, Santa Ana, CA) in Hepes buffer and washed out with human tubal fluid (HTF; Irvine Scientific) with 10% fetal bovine serum (FBS). Isolated oocytes were transferred into HTF media with 10% FBS and assessed by morphology. Oocytes were classified into four groups as mature, germinal vesicle break down, immature, and atretic. For blastocysts, the 6- to 7-wk-old mutant and control mice were superovulated with 7.5 IU eCG and 7.5 IU hCG as above then mated with wild-type males. Mice were euthanized at 3.5 days after mating, and uteri were removed. Blastocysts were flushed from the uteri and transferred into HTF media with 10% FBS and assessed by morphology. Blastocysts were classified as 4-cell to morula, expanded blastocyst, and early blastocyst.

Histology

Human myometrial and fibroid samples were collected using Institutional Review Board approved protocols. Murine uteri and human samples were fixed by immersion in 4% paraformaldehyde for 10–12 h and then transferred to 70% ethanol until processing. The fixed tissues were dehydrated in a graded ethanol series, cleared in xylene, and embedded in paraffin wax. Embedded tissue samples were sectioned at 5-μm thickness and mounted on slides. Hematoxylin and eosin (H&E) staining was performed using standard histological techniques. Photomicrographs of nontumorous myometria (n = 3 mice for each group) were measured to determine the ratio of the width of myometria to total uterine width.

In Situ Hybridization

Analyses for Amhr2 mRNA are described in a detail in a previous study [14, 15]. Briefly, urogenital ridges were collected from timed pregnant dams and at Embryonic Day 13.5 (E13.5) and fixed overnight at 4°C in 4% paraformaldehyde. Tissues were pretreated with protease prior to overnight hybridization with either Amhr2 full-length [18] digoxigenin-labeled antisense riboprobes in 50% formamide hybridization solution at 70°C. The resultant hybrids were detected with alkaline phosphatase-conjugated antidigoxigenin antibodies and BM purple colorimetric solution (Roche Molecular Biochemicals, Indianapolis, IN).

Immunofluorescence

Serial sections of tissues were deparaffinized with xylene and rehydrated with graded series of ethanol (absolute, 95%, 80%, and 50%, respectively, and distilled water), followed by two washes of 5 min each in PBS containing 0.05% Tween 20 (PBS-T). After a wash with PBS-T, antigen retrieval was performed by boiling the tissue sections in 0.01 M citrate buffer (pH 6) for 20 min. Sections were then washed for 5 min in PBS-T and blocked at room temperature for 1 h by using 2% normal donkey or goat serum, 2% bovine serum albumin, and 0.1% triton-X in PBS. Tissue sections were then incubated in a humidified chamber overnight at 4°C with primary antibody. Sections were subsequently washed with PBS-T, incubated at room temperature for 1 h with secondary antibody, then counterstained with 4′,6′-diamidino-2-phenylindole (DAPI). Images were photographed using a microscope (Nikon Eclipse TE 2000-S; Micro Video Instruments, Avon, MA) equipped with a Spot digital camera. DAPI-stained nuclei and phospho-histone H3 (pH3)-positive cells from sections of three different lesions were counted with the nucleus-counting analysis plugin of Image J software (v1.37; NIH, Bethesda, MD) after setting a black and white threshold at 27–30 in Photoshop (v10; Adobe Systems Inc., San Jose, CA).

Antibodies

Following are the primary and secondary antibodies used in this study: anti-β-catenin (1:250; BD Transduction Laboratories, San Jose, CA); anti-KIT (1:200; R&D Systems, Minneapolis, MN); anti-TGFB3 (1:200; Abcam, Cambridge, MA); anti-HMGA2 and anti-PECAM1 (1:200; Santa Cruz Biotechnology, Santa Cruz, CA); anti-vimentin (1:200; Santa Cruz Biotechnology); anti-Ecadherin (1:100; Santa Cruz Biotechnology); anti-pH3 (1:200; BD Transduction Laboratories); anti-CD11B (1:100; eBiosciences, San Diego, CA); anti-CD140B (1:200; Ebiosciences); anti-ACTA2, CY3-conjugated (Sigma); anti- PCNA (ready to use; Zymed, San Francisco, CA); anti-FRAP1 (1:200; Cell Signaling, Danvers, MA); AlexaFluor secondary antibodies (1:500; Invitrogen, Carlsbad, CA); and biotinylated donkey anti-mouse or anti-rabbit antibody F(ab)₂ (1:1000; Jackson ImmunoResearch Laboratories, West Grove, PA).

Leiomyoma-Like Lesions

Amhr2^tm3(cre)Bhr/+;Ctnnb1^tm1Mmt/+ mutant and Amhr2^tm3(cre)Bhr/+ or Ctnnb1^tm1Mmt/+ control mice were examined for phenotypic analysis. Initial gross examination of adult nulliparous mutant uteri occasionally showed hemorrhagic areas (data not shown) along both horns and an extraneous layer of tissue with protruding nodules at the anti-mesometrial side of the uteri (Fig. 1A). Examination of mutant uteri from multiparous mice revealed the presence of large tumorous growths and consistent multiple hemorrhagic sites on the surface of the uteri (Fig. 1B). No abnormalities were detected in the uteri collected from control mice (Fig. 1C). Histological examination of noncycling 4-wk-old uteri showed that the nodules observed on the surface of uteri appear to originate from the longitudinal myometrial layer of the uterus (shown with a red arrowhead in Fig. 1D). We also observed a small area of dysplasia (shown with a black arrowhead and outlined in white) in the mutant uteri, which otherwise appear similar to controls (Fig. 1E), suggesting that tumorigenesis starts before the mice begin estrous cycling. Staining of the mutant and control uteri for α-smooth muscle actin (ACTA2) shows that the polyps are derived from the myometrium and that there was expansion of the myometrium in the mutants (Fig. 1, F and G). The ratio of the width of ACTA2-positive myometrium to total uterine width in the mutant (0.45 ± 0.04, n = 3) was significantly higher (P = 0.009) than that of control uteri (0.22 ± 0.03, n = 3) suggesting smooth muscle hyperplasia. Normal WNT signaling is highly active at the coelomic epithelium of the Müllerian duct [20]. The nodules we observe in the mutant mice may be the result of constitutively activated β-catenin on the coelomic epithelium and adjacent mesenchyme of the presumptive anti-mesometrial side of the E13.5 urogenital ridge where Amhr2 is highly expressed (Fig. 1H).

In mutant mouse uteri, we observed dysplastic lesions in myometria with 100% penetrance that appeared to increase in size and number with age and parity (Fig. 2, A and B, and Table 2). The mutant murine tumors were composed of plump spindle cells surrounded by an extracellular matrix that formed fascicles (Fig. 2C) that are remarkably similar to those typically found in human uterine leiomyomas [2] (Fig. 2D). The largest tumors were often necrotic with hemorrhagia and fibrosis (data not shown). The murine smooth muscle tumors are ACTA2-positive (Fig. 2, E–G), which is also characteristic of human uterine leiomyomas (Fig. 2H). Typically, human uterine leiomyomas are very slow-dividing tumors and are usually present with a low proliferative index (0–2 mitoses per 10 high power field) [21]. We analyzed proliferation in the uterine smooth muscle tumors observed in mutant mice by performing pH3 expression analysis and found few pH3-positive cells (5–6 per high-powered filed or 2.4 ± 0.2/1000 cells) in these tumors, whereas pH3 expression was high in luminal epithelium (LE; Fig. 2, I and J). Proliferating cell nuclear antigen (PCNA) expression was also analyzed with similar results (data not shown). These data suggest that, similar to human uterine leiomyomas and unlike most other more aggressive tumors, these mouse uterine smooth muscle tumors also have a low mitotic activity. Another characteristic of many human uterine leiomyomas is that leiomyomas express higher levels of TGFB, particularly TGFB3, than the surrounding myometrium [22–26]. Analysis of TGFB3 in the uteri of mutant mice showed much higher levels of expression by immunohistochemistry in the epithelium and endometrial stroma, as well as in the central areas of the leiomyoma-like lesions, than in surrounding areas and the remaining myometrium and at levels consistent with those observed in human leiomyoma (Fig. 2, K and L). Together with the appearance of polyps shown above, these results suggest that constitutively activated β-catenin induces smooth muscle hyperplasia, which can then lead to smooth muscle tumor development.

The oncogenic serine/threonine kinase, mammalian Target of Rapamycin (FRAP1), which lies downstream of the PI3K signaling pathway and is a master regulator of cell proliferation [27], is up-regulated in the Eker rat leiomyoma model because of a mutation in tuberous sclerosis 2 (Tsc2) [28]. We assayed whether FRAP1 is also induced in these tumors by constitutively activated β-catenin using immunohistochemistry (Fig. 3). In the mutant with CA β-catenin, FRAP1 appears highly expressed in the central portion of the leiomyoma-like lesion, with little expression observed in the surrounding hypocellular areas (Fig. 3A). Relatively strong FRAP1 expression was also observed in both the circular and longitudinal myometrial layers (Fig. 3B). In the normal myometrium of control mice, FRAP1 expression appears to be limited to the endothelial cells or pericytes (Fig. 3, C and D).

ESS-Like Lesions

In addition to uterine smooth muscle tumors, Amhr2^tm3(cre)Bhr/+;Ctnnb1^tm1Mmt/+ mutants also developed ESS-like neoplastic lesions that were restricted to the endometrial stroma (ES; Fig. 4A). These lesions were ACTA2-negative (Fig. 4B), which we used as a marker to distinguish between ESS and ACTA2-positive leiomyomas. These tumors expressed high levels of nuclear β-catenin, indicating their origin from Amhr2-Cre-expressing mesenchymal cells (Fig. 4C). As expected, only membranous β-catenin is detected in LE and endometrial glands (EG) of both mutant (Fig. 4C) and control uterus (Fig. 4D), since Amhr2 is not expressed in these cells [15]. Some cells at the junction of the longitudinal and circular smooth muscle layers also expressed nuclear β-catenin (Fig. 4D). The ESS-like tumors expressed vimentin, a mesenchymal marker, suggesting the mesenchymal origin of these tumors (Fig. 4E). Consistent with a previous study [29], vimentin is also expressed in ES and blood vessels of both the mutant and control uteri (Fig. 4F).

Further analysis of the ESS-like neoplastic lesions with various markers used in the diagnosis of human tumors was performed to determine how well the murine tumors compare. The ESS-like neoplastic growths observed in mutant uterus are strongly estrogen receptor alpha (ESR1) positive (Fig. 5A), suggesting that these tumors can be responsive to changes in the levels of estrogen. KIT (CD117) is the tyrosine kinase receptor for the stem cell factor that has been shown to be expressed at relatively high levels in uterine sarcomas and mesenchyme-derived tumors of the uterus [30, 31]. We also find high levels of KIT expression in the ESS-like tumors (Fig. 5B). Co-staining with ITGAM (CD11B), a monocyte/macrophage cell marker, was performed to ensure that the KIT⁺ cells were not hematopoietic cells that had infiltrated the lesion. In the rest of the endometrial stroma, KIT is only expressed in a few cells, probably of hematopoietic origin. In addition, these tumorous lesions do not express PECAM1, an endothelial cell marker, except for the endothelial cells of blood vessels present inside the tumorous area (Fig. 5C). HMGA2 is a member of the high mobility group (HMG) of proteins. The disruption and misexpression of HMGA2 has been reported in various benign mesenchymal tumors such as lipomas, uterine leiomyomas, endometrial polyps, and salivary gland adenomas [32, 33]. In mutant uteri, we detected very high expression of HMGA2 in ESS-like tumor lesions compared with the normal adjacent tissue (Fig. 5D). Although E-cadherin, an epithelial cell marker, and PDGFRB (CD140B), a fibroblast marker, were expressed in normal LE and a few scattered cells of ES and myometrium, respectively, they were not expressed in ESS-like tumors of mutant uteri (Fig. 5, E and F). These results suggest that the ESS-like tumors in Amhr2^tm3(cre)Bhr/+;Ctnnb1^tm1Mmt/+ mice strongly resemble ESS tumors found in human uteri both by histology and by marker profile.

Adenomyosis

The mutations in phosphorylation sites on exon 3 of the β-catenin gene have been shown to occur in various tumors [34, 35]. In humans, 38% of cases of endometrial carcinoma show nuclear and/or cytoplasmic accumulation of β-catenin, suggesting that β-catenin plays an important role in the development of this disease [36]. In the present study, we observed hyperplasia and pseudostratification of epithelia of EGs in 14% of the mutant uteri (Table 2). We also observed aberrant EGs in the myometrium of the mutant uteri (Fig. 6A). The colocalization of ACTA2 and E-cadherin further confirms the presence of EGs in the myometrial layer of the mutant uteri (Fig. 6B). These phenotypic changes observed in EGs were surprising because Amhr2-Cre is only expressed in the stromal and myometrial compartments of the uterus [15], and the activation of β-catenin only occurred in these two compartments (Fig. 2). However, correctly functioning uterine stroma is required for normal adenogenesis [10], and our previous study has shown that conditional deletion of β-catenin from ES and the myometrium leads to fewer EGs [15]. Collectively, our findings suggest that tight regulation of the β-catenin signaling in ES and possibly myometrium is essential for the maintenance of normal EGs.