Abstract
High aldehyde dehydrogenase (ALDH) activity can be used to identify tumor-initiating and metastasis-initiating cells in various human carcinomas, including prostate cancer. To date, the functional importance of ALDH enzymes in prostate carcinogenesis, progression and metastasis has remained elusive. Previously we identified strong expression of ALDH7A1 in human prostate cancer cell lines, primary tumors and matched bone metastases. In this study, we evaluated whether ALDH7A1 is required for the acquisition of a metastatic stem/progenitor cell phenotype in human prostate cancer. Knockdown of ALDH7A1 expression resulted in a decrease of the α2hi/αvhi/CD44+ stem/progenitor cell subpopulation in the human prostate cancer cell line PC-3M-Pro4. In addition, ALDH7A1 knockdown significantly inhibited the clonogenic and migratory ability of human prostate cancer cells in vitro. Furthermore, a number of genes/factors involved in migration, invasion and metastasis were affected including transcription factors (snail, snail2, and twist) and osteopontin, an ECM molecule involved in metastasis. Knockdown of ALDH7A1 resulted in decreased intra-bone growth and inhibited experimentally induced (bone) metastasis, while intra-prostatic growth was not affected. In line with these observations, evidence is presented that TGF-β, a key player in cancer invasiveness and bone metastasis, strongly induced ALDH activity while BMP7 (an antagonist of TGF-β signaling) down-regulated ALDH activity. Our findings show, for the first time, that the ALDH7A1 enzyme is functionally involved in the formation of bone metastases and that the effect appeared dependent on the microenvironment, i.e., bone versus prostate.
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Introduction
Prostate cancer metastatic disease, often occult at time of diagnosis or surgery, is increasingly linked to mortality. Secondary lesions are mostly found in the skeleton, indicating bone as preferred site for the growth of disseminated disease [1]. Understanding the mechanisms of prostate cancer metastasis is essential for the development of novel therapies and detection methods.
Acquisition of an invasive phenotype of cancer cells is a requirement for bone metastasis; transformed epithelial cells can switch to a motile, mesenchymal phenotype by epithelial-to-mesenchymal transition (EMT) [2, 3]. Accumulating evidence suggests that EMT may generate cancer cells with properties of tissue stem cells [4–8]. Prostate cancer cells with a stem/progenitor phenotype are believed to be critically involved in prostate cancer initiation and progression and recent evidence from our group also indicated that this subpopulation of cancer cells is involved in bone metastasis formation [4–8].
An increasing number of studies support the notion that the primary tumor is maintained by a small number of cells, the cancer stem cells (CSCs) or tumor-initiating cells (TICs). It is generally believed that cellular heterogeneity in primary prostate cancers also arises from this subpopulation with stem/progenitor characteristics [4, 7, 9–11].
Because of the heterogeneous nature of solid cancers, the reliability of cell surface markers as the sole way to isolate TICs has remained controversial [4, 11–16]. A complementary strategy for identifying TICs involves measurement of aldehyde dehydrogenase (ALDH) activity. ALDH is a detoxifying enzyme which has important functions in the development of epithelial homeostasis, and as a result, deregulation of this class of enzymes has been implicated in multiple cancers [17]. ALDH activity is involved in detoxification, drug resistance, cell proliferation, differentiation, and response to oxidative stress [18–21]. It is becoming increasingly clear that ALDH activity can be used, either alone or in combination with cell surface markers, to identify TICs [4, 22–26]. In a recent study, we showed that human prostate cancer cells with high ALDH activity are enriched for tumor- and metastasis-initiating cells [4]. This ALDHhi subpopulation showed increased clonogenic and migratory ability in vitro and enhanced tumorigenic and metastatic ability in vivo. At present, it is not clear whether different ALDH isoforms contribute to the high ALDH activity observed in highly tumorigenic and metastatic prostate cancer cells. The reagent ALDEFLUOR™ that is frequently used for viable cell sorting based on ALDH activity has only been validated for ALDH1 and ALDH3 and not for the remaining 17 ALDH enzymes [17]. The prognostic significance of ALDH1 expression has been reported in a number of epithelial tumors, but the role of other ALDH enzymes in prostate cancer has not been addressed to date [22, 23, 26–31].
Previously, we found high levels of ALDH7A1 in various prostate cancer cell lines and primary cultures. Strong ALDH7A1 immunolocalization was also observed in primary prostate cancer tissue and matched bone metastases [4]. The functional involvement of ALDH7A1 in prostate cancer progression and metastasis has not been addressed.
In this paper we investigated the role of ALDH7A1 in prostate cancer initiation, progression, and bone metastasis formation by generating prostate cancer cells with stable knockdown of ALDH7A1. Our findings indicate that ALDH7A1 is involved in bone metastasis formation and that the functional involvement of ALD7A1 is dependent on the tumor microenvironment. Furthermore, the observed differences in the size of prostate cancer stem/progenitor subpopulations reflects the previously found opposite role of TGF-β and BMP7 on experimentally induced metastasis [32].
Results
Generation of prostate cancer cells with stable ALDH7A1 knockdown
A potential strategy for the identification and isolation of cells with a stem cell-like phenotype in hematological and a number of epithelial malignancies involves selection based on ALDH enzyme activity [4, 23, 33] using the ALDEFLUOR® assay. We have previously shown that various ALDH isoforms are expressed in human prostate cancer, all of which can theoretically contribute to the observed ALDEFLUOR activity [4]. One of the ALDH enzymes, ALDH7A1, was strongly expressed in various prostate cancer cell lines, primary cultures and in primary prostate cancer tissue with matched bone metastases [4]. In the present study, we investigated the effects of blocking ALDH7A1 activity on prostate cancer growth and (bone) metastasis by using lentiviral short hairpin RNA interference.
Different shRNAi constructs from the Sigma MISSION library were used to knockdown ALDH7A1 activity and two constructs showed a strong down-regulation of ALDH7A1 compared to the non-targeted control prostate cancer cells (Fig. 1a cell clone #1 and #2). Based on the high level of knockdown, we selected cell clone #1 (ALDH7A1-kd-Pro4luc) for further characterization in vitro and functional analysis in vivo and compared all results to the non-targeted control prostate cancer cells (NT-Pro4luc). Cell viability was confirmed by trypan blue exclusion prior to each experiment, and no differences among experimental groups were observed (data not shown). Potential impact on other ALDH isoforms was investigated by q-PCR analysis (Supplemental Figure S1). The expression levels of the ALDH isoforms 3A2, 5A1, 9A1 and 18A1 were not significantly affected by the ALDH7 knock down, whereas the expression levels of ALDH4A1 and 6A1 displayed a minor increase.
Effects of ALDH7A1 knockdown on clonogenicity, cellular invasion and cancer stem/progenitor characteristics
Selection of cells based on high ALDH activity can be used to enrich for prostate cancer cells with a stem/progenitor cell phenotype, thus linking ALDH activity (ALDEFLUOR) to stem/progenitor phenotypes [4, 23]. ALDH7A1 knock down resulted in a 21% decrease in ALDH activity as measured with the ALDEFLUOR assay (100% ± 1 vs. 79% ± 13 for, respectively the NT-Pro4luc and ALDH7A1-kd-Pro4luc cells). This link is further illustrated by the fact that stable knockdown of ALDH7A1 led to significantly decreased clonogenicity compared to NT-Pro4luc control cells (Fig. 1b). Furthermore, stable knockdown of ALDH7A1 resulted in a strongly impaired migratory response in a Boyden Chamber assays (Fig. 1c). Blocking the activity of ALDH7A1 in PC-3M-Pro4luc cells did not affect their proliferation rates at various time points (Fig. 1d).
Upon stable ALDH7A1 knockdown, a concomitant decrease in previously identified prostate cancer stem/progenitor cell surface markers was observed (Fig. 2a). Furthermore, ALDH7A1 knockdown in prostate cancer cells, led to reduced expression of E-cadherin transcriptional repressors (snail, snail2 and twist) and pro-metastatic factors including N-cadherin, twist, and osteopontin (OPN) (Fig. 2a) [34, 35]. In line with these observations, the E-cadherin/vimentin ratio increased upon ALDH7A1 knockdown, indicating the generation of a more epithelial and less invasive cell phenotype (Fig. 2b).
ALDH7A1 knockdown in prostate cancer cells differentially affects orthotopic and intra-bone growth in preclinical models
Our in vitro data showed that prostate cancer cells with a strongly diminished ALDH7A1 activity are poorly clonogenic and display a more sessile, epithelial phenotype compared with control cells. Subsequently, we analyzed and compared the tumorigenic and metastatic potential of both cell lines in vivo.
When implanted orthotopically in the mouse prostate, no significant differences were observed in tumor growth between both groups (Fig. 3a). Strikingly, we observed marked differences in tumorigenicity and metastatic ability in bone/bone marrow using our preclinical models of intra-bone growth [4, 32, 36]. Tumor take and intra-bone tumor growth were significantly decreased in the ALDH7A1-kd-Pro4luc group versus NT-Pro4luc control cells (Fig. 3b).
Inoculation of cancer cells into the left cardiac ventricle of immunodeficient mice is a widely used animal model of bone metastasis [4, 32, 36]. Significant differences in tumor growth and metastasis formation were observed (Fig. 4). In line with our intra-bone model, the ALDH7A1-kd-Pro4luc cells failed to reproducibly generate bone metastases, although limited growth was observed occasionally (Fig. 4a). Furthermore, metastatic tumor burden was significantly lower in the ALDH7A1-kd-Pro4luc group compared with the NT-Pro4luc control cells (Fig. 4b). Moreover, the total number of (bone) metastases was significantly decreased in the mice injected with the ALDH7A1 knockdown cells (Fig. 4c, d).
Regulation of the size of PC-3M-Pro4luc stem/progenitor subpopulation
The TGF-β superfamily (including TGF-βs and BMPs) plays a key role in EMT (tumor invasiveness), generation of cancer stem cells, and bone metastasis. Our group described previously that TGF-β and BMP7 have opposite roles in oncologic EMT, where BMP7 can counteract TGF-β induced EMT and inhibit bone metastasis [7, 8, 32].
Incubation with different concentrations of TGF-β for 72 h significantly and dose-dependently increased the size of the ALDHhi subpopulation of prostate cancer stem/progenitor cells, whereas incubation with different concentrations of BMP7 significantly and dose-dependently decreased the size of this subpopulation (Fig. 5a). Incubation with BMP2, BMP4, and BMP7 decreased the size of the ALDHhi subpopulation significantly (−56, −62, and −67%, respectively), while the close homolog of BMP7, BMP6, only marginally affected this subpopulation with −25% (Fig. 5b).
Subsequently, we analyzed whether BMPs and TGF-β affected the mRNA expression level of ALDH7A1 in PC-3M-Pro4luc prostate cancer cells. In line with the data shown in Fig. 5a and b we found that incubation with TGF-β for 72 h significantly increased the ALDH7A1 mRNA expression level by 2.5 fold (Fig. 5c). In addition to TGF-β, ALDH7A1 expression was inhibited upon incubation for 72 h with BMP2, 4, 6, and BMP7 (2.3 fold; 3.5 fold; 1.3 fold; and 5.0 fold inhibition, respectively). These q-PCR data were confirmed by Western blot analysis (2.5 fold increase upon TGF-stimulation; Fig. 5d.).
Discussion
Once prostate cancer has spread to the skeleton, treatment options are mainly focused on palliation and the prevention of fractures. Due to the observed heterogeneity in primary tumors and metastases, it has been a major challenge to distinguish and select prostate cancer cells with tumor- and metastasis-initiating ability. The functional identification of metastasis-initiating cells is a prerequisite for properly targeted therapy of metastatic disease in advanced prostate cancer.
It is becoming increasingly clear that ALDH activity (ALDEFLUOR™) can be used, either alone or in combination with other cell surface markers, to identify tumor-initiating cells (TICs) in multiple carcinomas [22–26]. In addition, we have shown recently that high ALDH activity could be used to select for prostate cancer cells with increased metastatic ability [4]. This was confirmed by Yu et al. [37] using subcutaneous implantations of prostate cancer cells. Moreover, we found differential expression of various ALDH isoforms in human prostate cancer, with high expression of ALDH7A1 in several cell lines, primary cultures, and primary prostate tissue with matched bone metastases. This suggests that, besides the ALDH1 enzyme which has been reported to be important in a number of epithelial tumors [22, 23, 26, 27, 30, 31], other ALDH isoforms may contribute to the overall ALDH activity and may be indicative of tumor-initiating and metastasis-initiating cells.
Here we describe, for the first time, the functional involvement of ALDH7A1 in prostate cancer metastasis. The size of this ALDHhi subpopulation, encompassing the cancer cells with tumor-and metastasis-initiating ability, can be regulated by the TGF-β superfamily (TGF-β and BMPs). We used the highly invasive (mesenchymal), osteotropic prostate cancer cell line PC-3M-Pro4luc for functional knockdown studies of ALDH7A1. Knockdown of ALDH7A1 expression resulted in a decrease of the prostate cancer stem/progenitor subpopulation, identified by integrin α2, integrin αv and CD44 [38–41]. In line with the altered expression of these stem/progenitor markers in the ALDH7A1-kd-Pro4luc cells, the clonogenic and migratory ability of the cells was also significantly decreased in vitro. Furthermore, a number of genes/factors involved in migration, invasion (EMT) and metastasis were affected. It is important to note that knockdown of ALDH7A1 in PC-3M-Pro4luc cells significantly diminished bone metastasis and tumor growth in the bone marrow, while intra-prostatic cancer growth was not affected.
Our data suggest that ALDH7A1 is involved in many important processes in prostate cancer and support the notion that ALDH enzyme activity can be used to isolate prostate cancer stem/progenitor cells, although it remains to be established whether this isoform also plays a causal role in other human and mouse prostate cancer cell lines. Both EMT associated genes and stem/progenitor characteristics were negatively affected upon ALDH7A1 knockdown. The data presented in this article further substantiate the previously described association between EMT and cancer stem cells [4–8]. For instance, snail and twist expression were decreased in the ALDH7A1-kd-Pro4luc cells as compared to the NT-Pro4luc control cells. The pro-metastatic transcription factor and E-cadherin repressor twist was recently associated with EMT and the promotion of the tumor-initiating capability in carcinomas [35]. Twist expression was found to be linked to the generation of stem cell properties of cancer cells. The data presented in this article further extend and support this notion for prostate cancer, since ALDH7A1 knockdown decreased twist expression, leading to significant reductions in clonogenic properties and expression of prostate cancer stem cell markers.
Recently other studies have also provided evidence that EMT plays a critical role in the formation of bone metastases and a stem/progenitor cell phenotype [7, 42–44]. In cancer, EMT is fundamental for epithelial cells to become more invasive. We show here that ALDH7A1 is necessary for prostate cancer cells to acquire a metastatic phenotype and form bone metastases, but is not pivotal for growth at the orthotopic site. It appears that the bone microenvironment plays an important role and provides crucial factors for the tumor cells to grow. These data, therefore, provide further evidence for the role of the stroma in the regulation of tumor invasiveness and metastasis as was shown previously for BMP7 [36].
Osteoclasts resorb bone, thereby releasing growth factors like TGF-β that may promote tumor cell proliferation, metastasis and survival, thus perpetuating a vicious cycle of tumor expansion and bone resorption [36, 45]. Strikingly, TGF-β increased the ALDHhi population as well as ALDH7A1 expression. One of the BMPs, BMP7, counteracts the pro-tumorigenic effects of TGF-β [32], and decreased the ALDHhi population and expression of ALDH7A1 in this study. This is in line with the notion that BMP7 induces differentiation towards a more epithelial, sessile tumor phenotype [32, 46–49]. In addition to TGF-β, OPN is prominently expressed at the sites of bone remodeling. Strikingly, TGF-β can induce OPN expression in both bone and tumor cells [50, 51]. Binding of OPN to the tumor cell membrane receptor CD44 can enhance tumor cell motility, migration and invasion in a paracrine and autocrine manner [52–55]. Knockdown of ALDH7A1 resulted in decreased OPN and CD44 expression in prostate cancer cells, which could explain, at least in part, a slowdown in intra-bone tumor growth and inhibition of (bone) metastasis formation.
In conclusion, we show that the ALDH7A1 enzyme may play a role in the formation of distant bone metastases. Downregulation of ALDH7A1 does not impair tumor growth at orthotopic sites but affects bone colonization and intra-osseous growth. This observed effect of ALDH7A1 expression suggests a pivotal role for the microenvironment and may be dependent on the presence of factors such as TGF-β and OPN. Our studies show that stem/progenitor phenotype in human prostate cancer cells can be differentially affected by the ALDH7A1 enzyme and bone-active growth factors like TGF-β and certain BMPs. Modulating and targeting this stem/progenitor subpopulation might be pivotal for the development of therapies for long-term disease-free survival.
Methods
Cell lines and culture conditions
The human prostate cancer cell line stably expressing firefly luciferase PC-3M-Pro4lucA6 (Pro4luc) was maintained in DMEM (GibcoBRL) containing 4.5 g glucose/l supplemented with 10% FCII, 100 units/ml penicillin, 50 μg/ml streptomycin, and 800 μg/ml geneticin/G418 (Invitrogen) [36]. Puromycin in a concentration of 1 μg/ml was added for Pro4lucA6 with stable shRNAi knockdown. HEK293T cells were maintained in DMEM containing 10% FCS. All cell lines were grown in a humidified incubator at 37°C and 5% CO2.
Suppressing ALDH7A1 expression with a shRNA-lentiviral vector
Short hairpin RNAi constructs (ALDH7A1 clone# TRCN0000028463, TRCN0000028408 and TRCN0000028447) were derived from Sigma’s MISSION library. HEK293T cells were transfected with the short hairpin constructs together with the packaging plasmids REV, GAG and VSV in a 1:1:1:1 ratio using Fugene HD (Roche) as transfection reagent. The supernatant of the culture medium containing the lentiviral vector was collected 48 h after transfection.
Pro4lucA6 cells were mixed with 1 ml of shRNA-lentiviral vector and 8 μg Polybrene (Sigma) was added. The mixture was incubated for 1–2 h at room temperature. Scrambled shRNA (clone# TRC1/1.5) was used as control which lack homology with any mammalian mRNA sequence. Cells stably expressing the shRNA were selected using puromycin (1 μg/ml, Sigma).
The ALDH7A1 knockdown cell line will further be referred to as ALDH7A1-kd-Pro4luc cells and the non-targeting control cell line as NT-Pro4luc cells.
Western blot analysis
Cells were washed with PBS and lysed in SDS-sample buffer (Laemmli buffer, Biorad). Proteins were separated on SDS-PAGE and subjected to Western blotting using standard techniques. Antibodies recognizing ALDH7A1 (1:5,000) was from Abcam and anti-β-actin (1:30,000) was from Sigma-Aldrich. Proteins were detected by using a chemiluminescence detection system from Roche.
FACS analysis
Expression of stem/progenitor- and EMT markers was measured by FACS analysis using the Calibur2 flow cytometer (BD Biosciences) and FCS express software (De Novo software USA). The cells (1 × 105 cells) were incubated for 45 min at 4°C in a solution of 90 μl FACS wash buffer containing PBS + 1% FCS + 0.1% natriumazide NaN3 and 10 μl antibody (αv-PE, α2-FITC, CD44-APC, CD44v6-APC, Miltenyi). To determine E-cadherin/vimentin ratios, cells were harvested and labeled with E-cadherin-FITC (BD Biosciences 1:10) in FACS buffer for 30 min at 4°C in the dark. Then cells were washed with 1 ml FACS buffer and fixed with freshly prepared 2% formaldehyde for 15 min. Cells were washed with ice cold PBS and subsequently incubated for 30 min at 4°C in the dark with vimentin rabbit polyclonal antibody (Abcam 1:200 in FACS buffer). Cells were washed twice with 1 ml of FACS buffer and incubated for 30 min at 4°C with goat-anti rabbit IgG-APC antibody (Invitrogen). After the last incubation step, the cells were washed and centrifuged for 5 min followed by adding 250 μl FACS wash buffer.
ALDH activity was measured as described earlier [4].
RNA isolation and real-time qPCR
RNA was extracted using Trizol (Invitrogen) according to manufacturer’s instructions. Real-time qPCR was run and analyzed with a Biorad IQ5 cycler (Biorad). For primer sequences see Supplemental Table 1. Gene expression was measured relative to GAPDH expression using the following formula: Relative transcript abundance (RTA) = 10,000/2(Ctgene−CtGAPDH).
Soft agar colony assay
Cell suspensions of both cell lines were generated (as described previously [4]) and overlayed onto a 60 mm dish containing a solidified bottom layer of 0.6% Noble agarose (Beckton Dickenson) in medium. One ml of medium was placed on top of the solidified cell layer. Plates were incubated for 1–3 weeks until colonies were visible. The colonies on the soft agar plates were counted by using light microscopy (Zeiss Axiovert 200M). Three individual and representative fields of each well were counted. The mean number of colonies/field was calculated.
Colony forming assay
Cells were seeded into a 96-wells plate containing an average of one cell per well. Plates were monitored twice a week and maintained in DMEM/10% FCII medium. After 1–3 weeks colonies were clearly visible and the mean number of positive wells/plate was counted by microscopy (Zeiss Axiovert 200M).
Migration assay
Tumor cell migration was performed in transwell migration chambers (Costar) as described previously [4]. Three random fields were counted for each well, and mean numbers of migrated cells/field were calculated.
Proliferation assay
Cells were seeded at a density of 2,500/cm2 and allowed to grow for, respectively, 24, 48, and 72 h. After the cell incubation, 20 μl MTS was added to the medium and mitochondrial activity was measured at 490 nm after 2 h incubation at 37°C (CellTiter96 Aqueous non-radioactive cell proliferation assay (Promega)).
In vivo animal experiments
Mouse strains: Male nude (Balb/c nu/nu) mice were housed in individual ventilated cages under sterile condition according to the local guidelines for the care and use of laboratory animals (DEC07026 and 09052). Mice were anaesthetized before surgical and analytical procedures were performed.
Intra-osseous inoculation of Pro4luc cells: A single cell suspension of 1 × 105 ALDH7A1-kd-Pro4luc cells or NT-Pro4luc cells/10 μl PBS was injected into the right tibiae as described previously [4, 36, 56]. The progression of cancer cell growth was monitored weekly by BLI (whole body bioluminescent reporter imaging) as described below.
Orthotopic inoculation of Pro4luc into the mouse prostate: A single cell suspension of 1 × 105 ALDH7A1-kd-Pro4luc cells or NT-Pro4luc cells/10 μl PBS was combined with 10 μl growth factor reduced matrigel (BD Biosciences) and surgically inoculated into the prostate of anaesthetized 6-week-old male nude mice [4, 48]. The progression of cancer cell growth was monitored weekly by BLI.
Intracardiac inoculation Pro4luc cells to induce systemic metastases: A single cell suspension of 1 × 105 ALDH7A1-kd-Pro4luc cells or NT-Pro4luc cells per 100 μl PBS was injected into the left cardiac ventricle of anaesthetized 5-week-old male nude mice and cancer cell growth was monitored weekly by BLI [4, 36].
Whole body bioluminescent reporter imaging (BLI) and quantification of the bioluminescent signal:
For all in vivo experiments, the progression of cancer cell growth was monitored weekly by bioluminescent imaging using the IVIS100 Imaging System (Caliper Life Science) as described earlier [36].
Statistical analysis
Statistical analysis was performed using GraphPad Prism 4.0 software© (San Diego, CA) using either t-test (for comparison between two groups) or ANOVA (for comparison between more than two groups). Unless otherwise stated, data is presented as the mean ± SEM. P values of ≤0.05 were regarded as being statistically significant (*P < 0.05, **P < 0.01, ***P < 0.001).
Abbreviations
- ALDH:
-
Aldehyde dehydrogenase
- BLI:
-
Whole body bioluminescent reporter imaging
- BMP:
-
Bone morphogenetic protein
- CSC:
-
Cancer stem cell
- EMT:
-
Epithelial-to-mesenchymal transition
- GAPDH:
-
Glyceraldehyde-3′-phosphate dehydrogenase
- OPN:
-
Osteopontin
- SDS-PAGE:
-
Sodium dodecyl sulphate-polyacrylamide gel electrophoresis
- shRNA:
-
Short hairpin RNA
- TGF-β:
-
Transforming growth factor-β
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Open Access This is an open access article distributed under the terms of the Creative Commons Attribution Noncommercial License (https://creativecommons.org/licenses/by-nc/2.0), which permits any noncommercial use, distribution, and reproduction in any medium, provided the original author(s) and source are credited.
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van den Hoogen, C., van der Horst, G., Cheung, H. et al. The aldehyde dehydrogenase enzyme 7A1 is functionally involved in prostate cancer bone metastasis. Clin Exp Metastasis 28, 615–625 (2011). https://doi.org/10.1007/s10585-011-9395-7
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DOI: https://doi.org/10.1007/s10585-011-9395-7