Amino-terminal enhancer of split gene AES encodes a tumor and metastasis suppressor of prostate cancer

Characteristics of PCa patients

Formalin-fixed, paraffin-embedded (FFPE) sections of primary tumors were obtained from 82 men who underwent prostate needle biopsy with informed consents signed as approved by the Kyoto University Ethics Committee (G52), and consequently were diagnosed to have PCa at Kyoto University Hospital. Patient characteristics are shown in Table 1. Decalcified FFPE sections of bone metastasis lesions were obtained from nine PCa patients who underwent a palliative surgery (mostly decompression laminectomy) for vertebral bone metastasis. All nine patients were on androgen deprivation therapy (ADT) and had developed castration-resistant disease at the time of surgery.

Mouse strains

Mice with the following genotypes were used: a conditional allele for Pten (Pten^f/f in C57Bl/6 background) with loxP sites flanking exon 5,21 a conditional allele for Aes with loxP sites flanking Exon2 of Aes,16 a Probasin-Cre allele (TgPbsn Cre in C57Bl/6 background) having Cre recombinase gene placed under the control of Probasin promoter,22 obtained from NCI.

Histological, immunohistochemical and immunofluorescent analyses

Tissues were fixed in 4% paraformaldehyde, embedded and sectioned at a thickness of 4 μm for histological, immunohistochemical (IHC), and immunofluorescent analyses. These sections were stained with hematoxylin and eosin (H&E) or processed further for immunostaining as described previously.23 For immunofluorescence staining, Alexa Fluor 594-conjugated goat anti-mouse IgG or 488-conjugated goat anti-rabbit IgG (Molecular Probes, Invitrogen, Carlsbad, CA) was used as the secondary antibody. Bright-field and fluorescence images were captured with Olympus DP73 (Olympus, Tokyo, Japan) or Leica CTR6000 fluorescent microscope (Leica, Wetzler, Germany) and analyzed using Adobe Photoshop software (Adobe, San Jose, CA, USA).

Microinvasion of the mouse prostate tumor cells were defined as broken basement membrane by tumor cells infiltrated into the interstitial space. Microinvasion was counted in three randomly selected light microscopy fields at 100× magnification for each section. Cells positive for nuclear Ki67 immunostaining were counted, and the proportion of Ki67-positive cells in at least 200 cells was determined for the positive cell frequency. The extent of AES immunohistochemical staining was validated using the intestinal polyp tissue from Apc^Δ716 polyposis mice16 as positive control, whereas the prostate tumor tissue from TgPbsnCre;Pten^f/f;Aes^f/f mice as negative control. It was scored as none (negative control), weak (positive but weaker than positive control), moderate (as strong as positive control) or strong (stronger than positive control) as shown in the representative images (Fig. S1).

Cell culture, and proliferation and invasion assays

PCa cell lines LNCaP, PC3, and DU145 were purchased from American Type Culture Collection (ATCC, Manassas, VA, USA) and cultured in RPMI 1640 with 10% fetal bovine serum (FBS). Cell proliferation in culture was evaluated using Cell Counting Kit-8 (Dojindo, Kumamoto, Japan).

For Matrigel invasion assays, cells were serum starved for 6 h and suspended in serum-free RPMI 1680. The cell suspension (5 × 10⁴ cells) was then added to the Matrigel-coated 8.0-μm pore polyethylene terephthalate filter insert of a 24-well cell culture chamber (BD Falcon, Franklin Lakes, NJ, USA) and was incubated for 24 h with the medium containing 10% FBS in the bottom chamber. Residual cells on the upper side of chambers were removed by scraping with cotton swabs and the cells that attached to the lower side of the membrane were fixed with 70% ethanol and stained with H&E. Invaded cells were counted under light microscopy.

Animal experiments

All experiments using animals were performed according to the protocols approved by Animal Research Committee of Kyoto University. Mice were housed in a specific pathogen-free room.

To assess the influence of Aes on prostate tumor development, male TgPbsn^Cre Pten^+/+ Aes^+/+ (wild-type), TgPbsn^Cre Pten^f/f Aes^+/+ (Pten), TgPbsn^Cre Pten^f/f Aes^f/f (Aes/Pten) mice (n = 5 for each) were sacrificed at 3, 6, 12, and 18 months of age and the genitourinary complex (bladder, urethra, prostate glands, and seminal vesicles) was excised and photographed. Then, each prostatic lobe was dissected, weighed, and subjected to further experiments. Samples were snap-frozen in liquid nitrogen for western blot analyses and isolation of RNA or genomic DNA. At dissection, the intraperitoneal cavity was also carefully inspected for any metastatic lesions. The lungs and liver were excised and subjected to histopathological examinations.

For in vivo transplantation models, we generated PCa cells that stably expressed firefly luciferase, and Aes or none (control). Cells were collected by trypsinization and centrifugation at 1000 g, resuspended in PBS and kept on ice until injection. In the cardiac injection model, 6-week-old male nude mice (Clea, Japan) were anesthetized and 5 × 10⁵ cells/mouse were injected into the left ventricle as described previously.24 Correct injection into the systemic circulation was confirmed by the lack of photon flux from the injection site detected by an in vivo imaging system (IVIS, Xenogen, Alameda, CA, USA) 2 min after each injection. In the orthotopic inoculation model, 6-week-old male NOD/SCID mice (Clea, Japan) were anesthetized and 1 × 10⁶ cells were injected into the anterior prostate as described previously.25

In the femur implantation model, 6-week-old male nude mice (Clea, Japan) were anesthetized and 1 × 10⁶ cells were injected into the left femur body as described previously.26 Following injections, mice were monitored daily for their general condition, and the extent of bone metastasis was determined on post-injection days 14, 28, and 42 by injecting luciferin intraperitoneally followed by photon flux determination using IVIS. The mice were euthanized, and bones, prostates and other organs with tumor involvement detected by IVIS were collected, fixed in formalin, and embedded in paraffin. Metastatic tumors were identified in sections under a light microscope.

Western blotting

For Western blots, tissues or cells were lysed in the NP-40 lysis buffer containing 20 mM Tris-HCl (pH 7.5), 150 mM NaCl, 10% glycerol, 1% Nonidet P-40, 10 mM sodium fluoride, 1 mM sodium pyrophosphate, 1 mM sodium orthovanadate, and Cømplete protease inhibitor (Roche Applied Science). Lysates containing 20 or 40 μg of protein were separated by SDS/PAGE and transferred to Immobilon P membranes (Millipore, Billerica, MA, USA). Membranes were blocked with 5% nonfat dry milk (in Tris-buffered saline, 0.05% Tween-20) for 1 h at room temperature. They were then probed with the primary antibodies for at 4°C 8 h. After incubation with horseradish peroxidase-conjugated secondary antibodies (anti-mouse IgG, Pierce, Rockford, IL; anti-rabbit IgG, GE Healthcare Amersham, Buckinghamshire, UK), bound proteins were detected by incubation with Immobilon chemiluminescent substrate (Millipore).

Antibodies

Anti-Aes antibody was described previously.16 Goat polyclonal anti-prostate-specific antigen (PSA) was purchased from Santa Cruz Biochemistry (Santa Cruz, CA, USA), mouse polyclonal β-actin from SIGMA (A5316), mouse polyclonal Cyclyn D1 from BD (556470), mouse monoclonal anti-Cyclyn E1 from Santa Cruz (sc-248), goat polyclonal anti-Probasin from Santa Cruz (sc-17126), rat monoclonal anti-Hes1 from MBL (D134-3), rabbit monoclonal anti-Snail from CST (C15D3), rabbit polyclonal anti-EZH2 from CST (4905S), and rabbit polyclonal anti-MMP9 from Abcam (ab38898).

Quantitative RT-PCR (q-RT-PCR)

q-RT-PCR was performed using an ABI StepOnePlus (Applied Biosystems, Foster City, CA, USA). We used the following primer sets and probes: human AES primers (F, forward, 5′- TCCCTTTTCTTTGACAGATGGG -3′; and R, reverse, 5′- AGGAGTCCGAGGTGGTGAATT -3′) and probe (5′- CTCCTCGCACCTACCCCAGCAACTC -3′), mouse Aes primers (F, 5′- GGCGGAAATTGTGAAGAGGCT -3′; R, 5′- CTTGGCTCTCTCGATGGCTC -3′) and probe (5′- TTTGCGCCCAGGTTCTGCCC -3′).

Levels of human ribosomal S18 RNA, human ACTB, and mouse Gapdh were determined using Taqman Ribosomal RNA, human β-actin and rodent GAPDH Control Reagents (Applied Biosystems). Reactions were prepared using Taqman Universal PCR Master Mix (Applied Biosystems). Relative transcript levels were calculated by the comparative C_T method (ABI User Bulletin #2). Primers used were as follows, HES1 (111 bp); F, 5′- TCAACACGACACCGGATAAA -3′ and R, 5′- TCAGCTGGCTCAGACTTTCA -3′, PSA (74 bp); F, 5′- GGAAATGACCAGGCCAAGAC -3′ and R, 5′- CAACCCTGGACCTCACACCTA -3′.

Reporter activity assays

Notch1 transcription activity was evaluated using Notch reporter assay. Cultured cells were transfected with pGa981-6 luciferase reporter27 simultaneously with Aes or control (Mock) expression vector with or without RAMIC.16 Twenty-four hours after transfection, luciferase activities were determined using Dual-Luciferase Reporter Assay System (Promega) according to the manufacturer's protocol with a MITHORAS LB 940 luminometer (Berthold Biolumat, Bad Wildbad, Germany). Firefly luciferase activities were normalized against those of Renilla luciferase.

Statistical analyses

Each experimental series was performed at least in triplicate, and the results are presented as means ±SEM. Student's t-test, Fisher's exact test and a logistic regression test were employed using commercially available software (SPSSII, SPSS, Tokyo, Japan Inc.). All tests were two-sided and P-values <0.05 were considered statistically significant.

AES levels in primary PCa are inversely correlated with extents of progression and metastasis

We have recently found that AES suppresses colon cancer metastasis through inhibition of Notch signaling.16 PCa data extracted from a gene expression database show that AES expression is down-regulated in PCa in a stage-dependent manner (Fig. S2),19 suggesting that AES is a candidate tumor and/or metastasis suppressor in PCa.

To test the possibility, we examined human PCa tissues for AES expression by IHC, and asked whether its expression is associated with clinical aggressiveness of PCa. We analyzed needle biopsy specimens of the prostate obtained from 82 untreated PCa patients, and found that AES expression levels were inversely correlated with lymph node involvement and clinical stage of PCa (Table 1). In this patient population, AES-negative PCa had twice higher frequency of lymph node involvement, which was statistically significant (44% vs 22%, P = 0.042). Additionally, AES-negative PCa was more likely to have bone metastasis than AES-expressing PCa, although the difference was not statistically significant (52% vs 33%, P = 0.097). Overall, 67% of patients with PCa lacking AES expression had metastasis, whereas only 42% of those expressing AES did (P = 0.03). On the other hand, AES expression was not significantly associated with the PSA level or Gleason grade (data not shown) suggesting that AES expression is an independent biomarker that predicts metastatic spread of PCa. Indeed, after adjusting to the Gleason score, expression of AES was still significantly associated with lymph node involvement (odds ratio (OR) 2.79, 95% confidence interval (CI) 1.079–7.191, P = 0.0343, logistic regression test) as well as to metastasis (OR 2.87, 95% CI: 1.037–7.918, P = 0.0423), except bone metastasis (OR 2.26, 95% CI: 0.894–5.723, P = 0.0848).

Furthermore, AES expression was abrogated in 78% (n = 7) of nine bone metastatic lesions (Fig. S3), whereas it was negative only in 44% (n = 14) of primary prostatic lesions of PCa with bone metastasis.

AES suppresses prostate tumor growth in culture and in vivo through androgen receptor inhibition

To investigate the effects of AES expression on androgen activity, we first studied the relationship between tumor growth and AES expression using human PCa cells in culture. Exogenous expression of Aes inhibited the proliferation by approximately 50% in androgen-dependent LNCaP cells (Fig. 1a), whereas it did not affect the proliferation of AR-independent PC3 (Fig. 1b) or DU145 (Fig. 1c) cells. Consistently, silencing of AES by shRNA promoted the proliferation rate twice in LNCaP cells (Fig. 1d). These data suggest that AES reduces the proliferation of PCa cells through inhibition of AR activity.

Because it was reported that AES could inhibit the AR transcriptional activity,17, 18 we next tested whether AES blocked the AR activity by determining the expression levels of an AR target gene PSA upon androgen stimulation. As anticipated, q-RT-PCR (Fig. 1e) and Western blotting (Fig. 1f) demonstrated significant reductions in both mRNA and protein levels of PSA upon AES expression.

To investigate the inhibitory function of AES on prostate tumor growth in vivo, we crossed mice carrying a floxed allele of Aes16 (Aes^f/f) with PIN model mice with prostate-specific deletion of a tumor suppressor Pten under the control of probasin promoter (TgPbsn^Cre Pten^f/f). The latter model develops PIN in an androgen-dependent manner.20, 28 The weight of the prostate gland was 1.5–2 times heavier in Aes/Pten compound knock-out mice than that in Pten single knock-out mice (Fig. 1g,h) (P < 0.05).

The enlarged prostate size in Aes/Pten mice was attributable to an increased growth of prostate epithelium as shown by larger area of PIN lesion in histology, and as evident by approximately twice higher density of Ki67-expressing cells in the prostatic epithelium of Aes/Pten mice compared with that of Pten littermates (Fig. 1i,j), suggesting accelerated proliferation of prostatic epithelial cells in Aes/Pten mice.

It has been reported that AR transcriptional activity is reduced by Pten loss-of-function mutation in the prostatic epithelial cells.29 Consistently, we found that probasin was scarcely expressed in the prostatic epithelium of Pten mice by immunofluorescence analysis (Fig. 1k, left). Notably, expression of probasin was remarkably restored in that of Aes/Pten mice (Fig. 1k, right), suggesting that Aes suppressed AR transcriptional activity in the Pten-deficient prostatic epithelium. It is known that activation of the AR promotes cell-cycle progression in the prostate epithelium and cancer cells.7 Consistent with the AR activation by Aes loss-of-function mutation, cyclin family proteins were expressed more abundantly in the prostate of Aes/Pten mice than that of Pten mice (Fig. 1l). Taken together, these results suggest that AES inhibits the proliferation of prostate tumor cells through AR inhibition.

AES blocks PCa cell invasion through Notch signaling inhibition

We previously reported that AES inhibits Notch signaling, and subsequently suppresses the invasion and metastasis of mouse colorectal cancer cells.16 Western blotting revealed that the AES expression levels were inversely correlated with the metastatic ability30 among three PCa cell lines (Fig. 2a,b). We also confirmed that all of PC3, DU145, and LNCaP cell lines express Notch1 and Notch2 receptors, and their ligands Jagged1 (data not shown) as reported previously.31 We then assessed the effects of Aes overexpression on Matrigel invasion activity. Exogenous expression of Aes decreased the number of invading cells by 50%–70% in both PC3 (Fig. 2c) and DU145 (Fig. 2d) cell lines without affecting proliferation. In LNCaP cells, reduced invasion may be partly attributable to the inhibition of proliferation, which was reduced by ~50% upon exogenous expression of Aes (Fig. 1a).

We next determined the effects of Aes expression on Notch signaling transcription using a luciferase-reporter assay. Forced expression of Aes suppressed the Notch reporter activity by 70%–90% in all three PCa cell lines either in the absence or presence of RAMIC, a recombinant form of activated Notch receptor (Fig. 2e–g). Moreover, exogenous expression of Aes caused approximately 70% reduction in the mRNA levels for HES1, one of the representative transcriptional targets of Notch signaling (Fig. 2h). Collectively, these results suggest that AES reduces Notch signaling transcription and cellular invasion also in PCa cells as in CRC cells.

AES suppresses metastatic spread of human PCa cell grafts in mice

To further investigate the role of AES in PCa metastasis in vivo, we next evaluated the effect of AES expression using two transplantation-metastasis mouse models. When injected into the cardiac left ventricle, PC3 and MDA-PCa2b cells can metastasize to bones such as the mandible, humerus and femur of nude mice. Notably, expression of Aes in PC3 cells significantly reduced (by ~50 times) the metastatic spread to the bone after cardiac injection when assessed with an in vivo photon-count imaging system (Fig. 3a–c).

Next we injected PC3 cells with or without exogenous Aes expression directly into the mouse femur to interrogate tumor growth between Aes-expressing and -nonexpressing PC3 cells in the bone. Notably, we found no significant difference between PC3 cells with and without exogenous Aes expression by this experimental design (Fig. 3d,e), suggesting that the less metastatic spread with Aes-expressing cells is attributable to other features of PCa cells than the proliferative properties at the metastatic sites, and that Aes expression is critical for the processes before metastatic colonization.

Taken together, these results with the in vivo transplantation and metastasis models suggest that Aes suppresses the ability of PCa cells to progress through the metastatic steps such as invasion, intravasation and extravasation without affecting tumor growth at the primary or metastatic sites.

Loss of Aes accelerates local microinvasion and lymph node metastasis of Pten-deficient mouse PCa

Next we investigated whether loss of Aes affects local invasion and distant metastasis of PCa in mutant knock-out mice along the course of progression. At 3 and 6 months of age, we found neither local microinvasion from the primary PIN or cancer to mesenchymal stroma, nor distant metastasis in Pten or Aes/Pten mice. However, at 12 months, local microinvasion was detectable and it was more frequent in Aes/Pten than in Pten mice (Fig. 4a,b). Notably, at 18 months of age, we observed lymph node metastasis in 70% (7/10) of Aes/Pten mice whereas such metastasis was detected only in 14% (1/7) of Pten simple mutant mice of the same age (P < 0.05, Fig. 4c,d).

As our cell culture analysis showed that AES inhibited Notch signaling, we analyzed Hes1 expression in mouse prostates by IHC. Nuclear Hes1 expression was more prevalent in Aes/Pten than in Pten mice (Fig. 4e), indicating that Aes deletion in Pten mice activated Notch signaling.

Snail, EZH2 and MMP9 were reported to be involved in PCa invasion through epithelial-mesenchymal transition (EMT) 32. Expression levels of these proteins were increased in Aes/Pten mouse prostates compared with those in Pten prostates (Fig. 4f). Additionally, we observed more abundant expression of MMP9 in the prostate of Aes/Pten than that of Pten mice (Fig. 4g), suggesting more active invasive phenotype of the former mice.