Abstract
PTEN dephosphorylates the 3-position phosphate of phosphatidylinositol 3,4,5 triphosphate (PIP3), thereby inhibiting AKT activation. Although attenuation of PTEN function has a major role in tumourigenesis, the underlying mechanisms remain unclear. Here we show that α-mannosidase 2C1 (MAN2C1) inhibits PTEN function in prostate cancer (PC) cells and is associated with a reduction in PTEN function in primary PC. MAN2C1 activates AKT and promotes the formation of PTEN-positive DU145 cell-derived xenograft tumours by imparing endogenous PTEN function. In 659 PC patients who were examined, ∼60% of tumours were PTEN positive with elevated AKT activation. Of these, 80% display MAN2C1 overexpression that co-localizes with PTEN. Increases in MAN2C1 were detected only in PTEN-positive prostatic intraepithelial neoplasia and carcinomas, and showed a significant association with PC recurrence only in patients with PTEN-positive PCs. Mechanistically, MAN2C1 binds PTEN thereby inhibiting its PIP3 phosphatase activity. These findings show that MAN2C1 function as a PTEN-negative regulator in PC cells.
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Introduction
PTEN is a phosphatase that functions on both protein and lipid substrates1. Accumulating evidence reveals that the lipid phosphatase activity of PTEN, which dephosphorylates the 3-position phosphate from the inositol ring of phosphatidylinositol 3,4,5 triphosphate (PIP3)2,3, can suppress tumour growth and development. As a result, PTEN directly antagonizes a critical oncogenic event mediated by the phosphatidylinositol-3 kinase (PI3K)4,5.
Typical mechanisms responsible for PTEN inactivation in cancers include genetic and epigenetic events. PTEN+/− mice as well as tissue-specific PTEN knockout mice exhibit a variety of tumours, including lymphoma, liver cancer and lung cancer6,7. Consistent with these observations, the PTEN gene is frequently mutated in human cancers8,9,10, including over 50% of glioblastomas and melanomas, 30–50% of endometrial carcinomas and 10% of breast cancers4,11,12. A missense mutation PTEN/G129E, leading to loss of the PIP3 phosphatase activity of the PTEN4,13, is causative for Cowden disease14, a multiple hamartoma syndrome with predisposition to multisystemic malignant tumours15. Hypermethylation of the PTEN promoter in sporadic colorectal cancers and reduction of PTEN protein without mutations in the PTEN gene in prostate cancer (PC) also contribute to tumourigenesis16,17.
Loss of PTEN has a critical role in PC progression13,18. PTEN+/− mice develop prostatic epithelial dysplasia and hyperplasia19,20,21,22,23. Prostate-specific deletion of PTEN in mice elicits PC that mimics the human condition24. This is attributable to the activation of the PI3K/AKT pathway, as loss of AKT1 markedly inhibits the tumourigenesis of prostate and endometrial cancers in PTEN+/− mice22. Loss of the PTEN protein has been reported in PC cell lines, in xenografted PCs and more frequently in metastatic PCs4,8,18,25. Furthermore, inactivation of PTEN and activation of the PI3K/AKT pathway results in androgen independency in prostate carcinogenesis26 and inhibition of AKT activity by Psoralidin can overcome chemoresistance in androgen-independent PCs27. Potential mechanisms resulting in loss of PTEN function in PC include mutations in the PTEN gene and reduction of the PTEN protein in ∼50% of PCs17. However, a large proportion of primary PCs express PTEN at normal levels, suggesting that PTEN can be inactivated during prostate tumourigenesis by mechanisms that are neither genetic nor epigenetic. In support of this concept, PTEN function is impaired when expressed at physiological levels in renal cell carcinoma and T-cell acute lymphobastic leukaemia28,29. These findings strongly suggest that PTEN-mediated tumour suppression can be regulated by additional cellular factors. Consistent with this notion, recent publications show that PTEN is inhibited by binding to Dlg-1 in Schwan cells30, and by interacting with P-REX2a and shank-interacting protein-like 1 (SIPL1) in breast and cervical cancers, respectively31,32.
We report here that α-mannosidase 2C1 (MAN2C1) is a novel PTEN-negative regulator (PTEN-NR) in PC cells. MAN2C1 belongs to the α-mannosidase family33. Consistent with the family being involved in glycoprotein maturation in the endoplasmic reticulum (ER) and Golgi34, MAN2C1 displays mannose-trimming activity33. Although MAN2C1 has been reported to be associated with tumourigenic activity in B cells35 and nasopharyngeal carcinoma36, the underlying mechanisms remain unclear. We demonstrate here that MAN2C1 binds to PTEN both in PC cells and in primary PCs, thereby attenuating the PIP3 phosphatase activity of PTEN and promoting prostate tumourigenesis.
Results
Identification of α-MAN2C1 as a PTEN-NR
We have recently established a screening approach to select for negative regulators (NRs) of PTEN32. Briefly, ectopic PTEN potently inhibited the proliferation of PTEN-deficient LNCaP PC cells, an observation consistent with those reported in glioma, melanoma and breast cancer2,10,37,38, and this inhibition was prevented by specific cDNAs derived from a human prostate cDNA library32. One of four PTEN-NR cDNAs encoded the last carboxy (C)-terminal 236 residues of MAN2C1 (C-MAN236; Supplementary Fig. S1a). Although one candidate elicited moderate PTEN inhibitory activity32, both SIPL132 and MAN2C1 described in this study potently inhibited PTEN function.
To confirm that MAN2C1 attenuates PTEN function, we demonstrated that MAN2C1 enhanced LNCaP cell survival in the presence of ectopic PTEN overexpression in comparison with empty vector (EV; Fig. 1a). To determine the effect of endogenous MAN2C1 on PTEN function, we first raised an anti-MAN2C1 antibody, which specifically recognizes MAN2C1 (Supplementary Fig. S1b–d). By immunoblot analysis using this antibody, we demonstrated knockdown of MAN2C1 using a specific short interfering RNA (siRNA) in PTEN-positive DU145 PC cells (Fig. 1b). Knockdown of MAN2C1 decreased cell survival to 30% of control (Ctrl) siRNA-treated cells, which was increased to 75% when PTEN was also knocked down (Fig. 1c), demonstrating that knockdown of MAN2C1 significantly inhibited DU145 cell survival/proliferation by enhancement of endogenous PTEN function. This is consistent with endogenous PTEN being functional as knockdown of PTEN increased AKT activation (Fig. 1b, see AKT-P in PTEN siRNA versus AKT-P in Ctrl siRNA-treated cells). Similar effects were also obtained following MAN2C1/PTEN knockdown using different siRNA fragments that were delivered into DU145 cells through either oligonucleotide or retrovirus methodologies (Supplementary Table S1). In accordance with PTEN antagonism of PI3K-mediated AKT activation, ectopic MAN2C1 enhanced AKT activation in DU145 cells, which was inhibited by the PI3K inhibitor Wortmannin (Fig. 1d), but was unable to increase AKT activation in PTEN-negative LNCaP and U87 cells (Fig. 1e). These observations suggest that MAN2C1 promotes AKT activation by inhibition of endogenous PTEN function. In further support of this concept, we demonstrated that MAN2C1 siRNA reduced AKT activation in PTEN-positive DU145 (Fig. 1b), as well as in MCF7 breast cancer cells (Supplementary Fig. S2a), but not in DU145 or MCF7 cells in which endogenous PTEN was concomitantly knocked down (Fig. 1b, Supplementary Fig. S2a). Taken together, the above observations demonstrate that MAN2C1 negatively regulates PTEN function.
α-MAN2C1 binds to PTEN
To determine the underlying mechanism whereby MAN2C1 reduces PTEN function, we examined a possible interaction between MAN2C1 and PTEN. C-terminal FLAG-tagged MAN2C1 was expressed with or without PTEN in 293T cells. Immunoprecipitation (IP) of PTEN led to the recovery of MAN2C1 and vice versa, whereas a Ctrl IgG did not precipitate MAN2C1 and PTEN (Fig. 2a). Furthermore, endogenous MAN2C1 and PTEN also coimmunoprecipitated in DU145, MCF7 and NIH3T3 cells (Fig. 2b). Both MCF7 and NIH3T3 cells express higher levels of endogenous PTEN than DU145 cells (Fig. 2b), which likely correlate with the higher efficiencies of co-IP of endogenous PTEN via MAN2C1 (Fig. 2b). To further demonstrate the interaction between MAN2C1 and PTEN, we assessed their intracellular co-localization. Although endogenous MAN2C1 co-localized with endogenous PTEN in DU145 cells (Fig. 2c) and MCF7 cells (Supplementary Fig. S2b), their ectopic counterparts co-localized in LNCaP and 293T cells (Supplementary Fig. S3). In addition, this co-localization was clearly demonstrated by three-dimentional reconstruction of a set of z-stack images (Supplementary Movies 1, 2). Taken together, we provide evidence demonstrating that MAN2C1 binds to and co-localizes with PTEN.
To characterize the putative binding domains in MAN2C1 that associate with PTEN, MAN2C1 truncation mutants were generated (Supplementary Fig. S4a). Both an amino (N)-terminal fragment encompassing the catalytic motif (Cat-MAN) and a C-terminal fragment of MAN2C1 (C-MAN) interacted with PTEN (Fig. 2d). Although the N-terminal 168 residues of C-MAN (C-MAN-N) did not bind to PTEN (Supplementary Fig. S4b), the C-terminal 236 residues of C-MAN (C-MAN236) interacted with PTEN (Fig. 2e). Further deletion of the N-terminal 103 residues from C-MAN236 (C-MAN236-C) greatly reduced its binding affinity to PTEN (Supplementary Fig. S4c). Collectively, these results demonstrate that MAN2C1 binds to PTEN by means of multiple domains, and that C-MAN236 is capable of PTEN interaction, consistent with our initial identification of the C-MAN236 fragment from our screen (Supplementary Fig. S1a).
α-MAN2C1 inhibits the PIP3 phosphatase activity of PTEN
Our observations that MAN2C1 reduces PTEN function (Fig. 1) and binds to PTEN (Fig. 2) prompted us to determine whether MAN2C1 inhibits the PIP3 phosphatase activity of PTEN. Recombinant glutathione S-transferase (GST)-PTEN and GST-MAN2C1 were purified using Escherichia coli (Fig. 3a) and their identities were confirmed by western blot (Fig. 3a). In comparison to GST, GST-MAN2C1 dose-dependently inhibited the PIP3 phosphatase activity of GST-PTEN (Fig. 3b). To examine whether MAN2C1 inhibits cellular PTEN-mediated PIP3 phosphatase activity, we transiently expressed the phosphatase-deficient PTEN(C124S), PTEN, MAN2C1 or PTEN+MAN2C1 in 293T cells (Fig. 3c). Although ectopic PTEN, immunoprecipitated by anti-HA antibody (Y-11), was competent to dephosphorylate PIP3 in vitro, PTEN(C124S) displayed no such activity, as expected (Fig. 3c). MAN2C1 dose-dependently reduced PTEN-mediated PIP3 phosphatase activity (Fig. 3c). At the ratio of 20:5 (MAN2C1:PTEN), MAN2C1 reduced the PIP3 phosphatase activity to a level comparable to PTEN(C124S)-associated background activity (Fig. 3c), showing that MAN2C1 is able to completely inhibit the PIP3 phosphatase activity of PTEN.
As both Cat-MAN and C-MAN236 interact with PTEN (Fig. 2d,e), we transiently expressed PTEN(C124), PTEN, PTEN+Cat-MAN or PTEN+C-MAN236 in 293T cells. IP of PTEN dose-dependently precipitated C-MAN236 and Cat-MAN, respectively (Fig. 3d,e). In comparison with the negative PTEN(C124S) and positive PTEN Ctrls, Cat-MAN (Fig. 3e), but not C-MAN236 (Fig. 3d), dose-dependently inhibited the PIP3 phosphatase activity of PTEN.
To confirm these findings, we directly analysed endogenous PTEN-mediated PIP3 phosphatase activity following knockdown of MAN2C1. In comparison to Ctrl siRNA treatment, MAN2C1 siRNA significantly reduced MAN2C1 protein and enhanced the PIP3 phosphatase activity of PTEN in DU145 cells (Fig. 3f).
To further confirm the physiological relevance of MAN2C1 in inhibiting PTEN activity, we have knocked down MAN2C1 in immortalized but non-transformed human prostate epithelial BPH-1 cells39,40,41 (Fig. 4a). Knockdown of PTEN enhanced AKT activation, as expected (Fig. 4a). Knockdown of MAN2C1 reduced ATK activation (Fig. 4a). This depended on the existence of endogenous PTEN, as concomitant knockdown of PTEN rendered MAN2C1 siRNA ineffective in inhibiting AKT activation (Fig. 4a), indicating that knockdown of MAN2C1 leads to an increase in PTEN-derived PIP3 phosphatase activity. Indeed, knockdown of MAN2C1 increased the PIP3 phosphatase activity of endogenous PTEN (Fig. 4b). Furthermore, knockdown of MAN2C1 also elevated endogenous PTEN-mediated PIP3 phosphatase activity in primary human prostate epithelial cells (Fig. 4c).
α-MAN2C1 promotes tumourigenesis by inhibiting PTEN
Our observations that MAN2C1 inhibits PTEN-dependent PIP3 phosphatase activity and enhances the activities of the PI3K-AKT pathway, strongly suggest that MAN2C1 could promote tumourigenesis. To investigate this possibility, we examined whether MAN2C1 enhances the ability of DU145 cells to form xenograft tumours in immunocompromised mice. By taking advantage of the fact that DU145 cells form xenograft tumours inefficiently in nude mice (He and Tang, unpublished observation), we subcutaneously (s.c.) implanted DU145 EV cells and DU145 MAN2C1 overexpressing cells into these animals. Although DU145 EV cells formed small tumours with low efficiency, DU145 cells expressing MAN2C1 formed significantly larger xenograft tumours (Fig. 5a, Table 1, Supplementary Fig. S5a). These xenografted tumours, as expected, expressed ectopic MAN2C1 and endogenous PTEN with elevated AKT activation (Supplementary Fig. S5b).
We subsequently determined the role of endogenous MAN2C1 in inhibiting endogenous PTEN function during tumourigenesis. As reported previously32,42, we used a transient knockdown system and nonobese diabetes/severe combined immunodeficiency (NOD/SCID) mice were used, as this host produces xenograft tumours with a higher efficiency than nude mice (He and Tang, unpublished observation). DU145 cells were transiently treated with a combination of Ctrl siRNA, MAN2C1 siRNA and/or PTEN siRNA oligonucleotides before being s.c. implanted into NOD/SCID mice. Although knockdown of PTEN seems to facilitate tumour formation at early stages compared with Ctrl siRNA tumours (Table 1, see the tumour volumes for Ctrl siRNA and PTEN siRNA treatments at 21 and 28 days after implantation), both PTEN siRNA-treated cells and Ctrl siRNA-treated cells formed tumours with a comparable efficiency at later stages (Table 1). This might be attributable to the transient nature of siRNA treatment. Knockdown of MAN2C1, however, significantly reduced the rate of tumour formation, which was largely reversed when PTEN was concomitantly knocked down (Table 1, Supplementary Fig. S5c). To confirm these observations and also to overcome the shortcomings associated with the transient knockdown of PTEN and MAN2C1, we stably knocked down PTEN and MAN2C1 individually, and in combination. Xenograft tumours were then generated using these lines. Tumour incidence was 5/5 for all groups except for MAN2C1 knockdown cells, in which 3/5 implantations formed small tumours. As expected, knockdown of PTEN significantly enhanced DU145 cell-derived xenograft tumours (Fig. 5b). Knockdown of MAN2C1 significantly reduced the formation of xenograft tumours, which was reversed by concomitant knockdown of PTEN (Fig. 5b). In addition, knockdown of individual proteins was not only confirmed by immunohistochemistry (IHC) in the respective xenograft tumours, but it was also observed that knockdown of MAN2C1 reduced AKT activation (AKT S473 phosphorylation) in a PTEN-dependent manner (Fig. 5c); that is, knockdown of MAN2C1 was incapable of reducing AKT activation when PTEN was co-knocked down (Fig. 5c). This result, thus, demonstrates that MAN2C1 promotes the formation of DU145 cell-derived xenograft tumours, at least in part, by inhibiting endogenous PTEN function.
α-MAN2C1-mediated tumourigenesis by inhibiting PTEN
Although both Cat-MAN and C-MAN236 bind PTEN (Fig. 2d,e), only Cat-MAN inhibits the PIP3 phosphatase activity of PTEN (Fig. 3d,e). We thus examined how Cat-MAN and C-MAN236 affect tumourigenesis. In comparison with EV, both fragments, when ectopically expressed in DU145 cells, promote xenograft tumour formation (Fig. 5d). Although inhibiting the PIP3 phosphatase activity of PTEN likely contributes to Cat-MAN-mediated tumourigenic activity, C-MAN236 may promote xenograft tumour formation by inhibiting other regulatory events that affect PTEN function, including recruitment of PTEN to the plasma membrane. This concept is supported by the observation that ectopic C-MAN236 co-localizes with endogenous PTEN in DU145 cells (Supplementary Fig. S6a). Consistent with MAN2C1 being an ER protein33, ectopic C-MAN236 largely co-localizes with KDEL (a C-terminal ER retention sequence present in several ER-resident chaperones43) in DU145 cells (Supplementary Fig. S6a). C-MAN236 cofractionated with calnexin-containing ER microsomes (Supplementary Fig. S6b), further supporting its ER localization. More importantly, although ectopic PTEN failed to associate with microsomes, 28% of ectopic PTEN cofractionated with microsomes following C-MAN236 co-transfection (Supplementary Fig. S6b). Furthermore, ∼31% of endogenous PTEN co-localized with the ER-resident chaperone GRP78 in DU145 cells, with C-MAN236 expression increasing this co-localization to 64.7% (determined by analysis of the confocal images using IMARIS software). The concept that Cat-MAN and C-MAN236 may promote tumourigenesis by inhibiting different aspects of PTEN regulation is consistent with the observation that MAN2C1 is more potent than either Cat-MAN or C-MAN236 in promoting the formation of DU145 cell-derived xenograft tumours (Fig. 5d).
α-MAN2C1 associates with reduction of PTEN function
Approximately 50% of PCs display normal PTEN expression17. Given that MAN2C1 inhibits PTEN function and promotes DU145 PC cells forming tumours in mice by suppressing PTEN function, we investigated the possibility that MAN2C1 associates with attenuation of PTEN function in PTEN-positive primary PCs. Consistent with the co-localization of PTEN with MAN2C1 in DU145 PC cells, we were able to detect in our collection of PC tissues (Supplementary Table S2) that PTEN co-localizes with MAN2C1 in PTEN-positive prostate tumour cells (Fig. 6a). Interestingly, in PTEN-negative carcinomas, MAN2C1 expression was also low (Fig. 6a). The differences in PTEN and MAN2C1 staining between PTEN-positive and PTEN-negative carcinomas did not result from variations in immunofluorescent staining, as these carcinomas were from the same specimen (Fig. 6a).
To examine whether this co-localization presaged a reduction in PTEN function, we determined the expression of PTEN, MAN2C1 and AKT activation (AKT-P) by IHC in normal prostate glands, PINs (prostatic intraepithelial neoplasia) and carcinomas within the same primary tissues/slides. Immunodetection of PTEN, MAN2C1 and AKT-P was observed in normal prostate gland, PINs and carcinoma (Fig. 6b). However, the levels of AKT-P in normal prostatic glands were much lower than those present in PINs and carcinomas (Fig. 6b). The staining was specific as Ctrl IgG did not reveal detectable signal, anti-MAN2C1 antibody specifically recognized MAN2C1 by IHC (Supplementary Fig. S7); and in the majority of PTEN-negative carcinomas, anti-MAN2C1 antibody did not produce detectable signals (Fig. 6a,b). Both PTEN-positive and -negative carcinomas showed increased AKT-P, but only PTEN-positive carcinomas displayed intense MAN2C1 staining together with enhanced AKT activation (Fig. 6b). This phenomenon was generally observed in our IHC study, which demonstrates MAN2C1 upregulation in PTEN-positive PCs as well as attenuation of PTEN function in these PCs (see later sections for details).
To confirm this correlation, in addition to our patient cohort (Supplementary Table S2), we examined by IHC two independent patient cohorts, tissue microarrays 2 and 5 (TMA2, TMA5; Supplementary Data 1 and 2). IHC staining of 608 (234+374) (Fig. 6c) patients in the pooled patient cohort (TMA2+5) revealed that 38.5% (234/608) of carcinomas were PTEN negative, in which 42.3% (99(17+82)/234) were MAN2C1 positive (Fig. 6c); 61.5% (374/608) of carcinoma are PTEN positive, in which 79.9% (299(18+281)/374) were MAN2C1 positive (Fig. 6c); 78.6% (184(102+82)/234) of PTEN-negative carcinomas displayed AKT activation (AKT-P), in which 44.6% (82/184(102+82)) were MAN2C1 positive (Fig. 6c); and of the PTEN-positive carcinomas, 93.6% (350(69+281)/374) exhibited intensive AKT-P staining (Fig. 6c), in which 80.3% (281/350(69+281)) showed intensive MAN2C1 staining (Fig. 6c). Similar observations were also obtained in carcinomas and in PINs in the individual patient cohorts (Supplementary Tables S3–S5). MAN2C1 positively correlated with PTEN expression (Pearson Correlation Coefficient: Pearson's ϕ: 0.385, P<0.001 determined by χ2 test) and AKT activation in prostate carcinomas (Pearson's ϕ: 0.142, P<0.001). PTEN also positively correlated with AKT activation in prostate carcinomas (Pearson's ϕ: 0.222, P<0.001). These correlations were also observed in PINs and carcinomas in individual patient cohorts (Supplementary Tables S3–S5) but not in normal prostate glands (Supplementary Tables S3, S5).
Upregulation of α-MAN2C1 in PTEN-positive PC
On the basis of the above observations that MAN2C1 associates with attenuation of PTEN function and that low levels of MAN2C1 were observed in PTEN-negative PCs (Fig. 6), we reasoned that MAN2C1 might be specifically upregulated in PTEN-positive primary PCs. To address this issue, we determined MAN2C1 expression in PTEN-positive versus PTEN-negative primary prostate carcinomas. The results showed that MAN2C1 expression increased significantly only in PTEN-positive PINs and carcinomas in the presence of AKT activation, but not in the PTEN-negative counterparts (Fig. 7a, Supplementary Table S6). In addition, MAN2C1 expression significantly increases only in PTEN-positive PINs and carcinomas of all Gleason scores (except Gleason 5, which might be due to insufficient patient numbers), but not in the PTEN-negative counterparts in TMA2+TMA5 (Supplementary Fig. S8, Supplementary Table S7). There was no difference in MAN2C1 expression between PIN and carcinomas of different Gleason scores.
α-MAN2C1 associates with PC recurrence
Recurrent cancer is the leading cause of cancer-associated deaths. In an effort to address whether MAN2C1 expression associates with PC recurrence, we observed that in TMA5, which was organized according to PC recurrence (see Methods for details), Kaplan–Meier survival analysis revealed that patients with MAN2C1-positive PC were significantly associated with decreased recurrence-free survival (Fig. 7b). Similar observations were also obtained in our patient cohort and TMA2, although with less number of patients (Supplementary Fig. S9). As MAN2C1 was also detected in a small proportion of PTEN-negative carcinomas (Fig. 6c), we further determined the groups of patients (PTEN-positive versus PTEN-negative) in which MAN2C1 associates with PC recurrence. Interestingly, MAN2C1 associates with decreased recurrence-free survival only in patients displaying PTEN-positive PC (Fig. 7b,c). Taken together, these observations support the concept that MAN2C1 mediates PTEN inactivation in PC cells.
Discussion
Genetic alternations in the PTEN gene are frequently detected in a variety of human cancers4. Although PTEN is infrequently mutated in sporadic colorectal cancers, ∼19% of those cancers with high levels of microsatellite instability have the PTEN promoter hypermethylated16. Reduction of the PTEN protein without mutations in the PTEN gene has been observed in PC17. Besides these genetic and/or epigenetic events that lead to loss of PTEN function, putative PTEN-NRs may also attenuate PTEN function during the process of tumourigenesis. This possibility is supported by recent reports that PTEN is expressed normally but with impaired function in human cancers28,29. Although the function PTEN can be indirectly inhibited by factors including DJ-1 and Surivin44,45, P-REX2a and SIPL1 have been reported to inhibit PTEN by binding to PTEN during breast and cervical tumourigenesis31,32. It is therefore possible that different NRs of PTEN may inhibit PTEN by binding to PTEN in different types of human cancers.
In this study, we identified MAN2C1 as a NR of PTEN in PC cells. The α-mannosidase family is involved in glycoprotein maturation in the ER and Golgi34. Although MAN2C1 has been suggested to have a role in the aforementioned process, it remains to be determined whether the catalytic activity of MAN2C1 contributes to PTEN inactivation. Our observation that MAN2C1 associates with prostate tumourigenesis is consistent with reports that overexpression of MAN2C1 transforms human B cells35 and that reduction in MAN2C1 suppresses the metastasis of nasopharyngeal carcinoma36. Interestingly, MAN2C1 transgenic mice that have recently been developed are prone to enhanced tumour growth, invasion and metastasis46. These investigators speculated that the mechanism might be through impaired antibody response to tumour antigens, but this was not specifically studied.
Mechanistically, MAN2C1 promotes the formation of DU145 cell-derived xenograft tumours at least in part by inhibiting the PIP3 phosphatase activity of PTEN by binding to PTEN. However, this may not be the only mechanism responsible for MAN2C1 to inhibit PTEN function, as C-MAN236 also attenuates PTEN function without inhibiting the PIP3 phosphatase activity of PTEN. Although C-MAN236 does not inhibit PTEN-derived PIP3 phosphatase activity, it may impair PTEN function by reducing the plasma membrane recruitment of PTEN by binding to PTEN (Supplementary Fig. S6). This concept is consistent with MAN2C1 being an ER protein33. In addition, both MAN2C1 and C-MAN236 are exclusively ER proteins when overexpressed in DU145 and other cells. This possibility is also in line with the observation that ectopic PTEN associates with the ER in C-MAN236 overexpressing cells (Supplementary Fig. S6). In addition, a similar mechanism was reported, in which caspase 7 was recruited to ER through interaction with GRP78, leading to prevention of its apoptotic activity in response to etoposide47. It is also possible that the catalytic activity of MAN2C1 may also contribute to the inactivation of PTEN at the ER. This may be achieved by MAN2C1-mediated alteration of glycosylation on specific components of the MAN2C1/PTEN complex, which may result in reduction of PTEN function.
On the other hand, it remains an intriguing possibility that PTEN may in turn affect the mannose-trimming activity of MAN2C1 towards its substrates. As changes in the patterns of protein glycosylation are well known to associate with oncogenesis48, PTEN may regulate this aspect of tumourigenesis by potentially regulating MAN2C1 function. As MAN2C1 has been demonstrated to hydrolyse p-nitrophenyl-α-D-mannopyranoside33, the notion whether PTEN may influence the enzymatic activity of MAN2C1 can thus be readily tested.
The PI3K pathway has essential roles in tumourigenesis by coordination of cell cycle progression, survival and cytoskeletal organization5. PTEN is the major mechanism that suppresses the PI3K pathway, as loss of PTEN activates the PI3K-AKT pathway in mice and in cells19,49,50,51. Therefore, attenuation of PTEN function represents a major step during tumourigenesis. Although the PTEN gene is frequently mutated in human cancers4,12, a large population of breast and PCs express PTEN at physiological levels with elevated AKT activation52 and high levels of PTEN and AKT activation were observed in renal cell carcinomas28. These observations suggest that PTEN is inactivated during tumourigenesis by its negative regulatory mechanisms in addition to the observed genetic and epigenetic events. We provide evidence that MAN2C1 is a novel PTEN-NR in PC cells. The possibility that MAN2C1 may also have a role in attenuation of PTEN function during the tumourigenesis of other types of PTEN-positive human cancers remains to be explored.
Methods
Cell lines and retrovirus infection
DU145, PC3, LNCaP, 293T, MCF7 and NIH3T3 lines were obtained from American Type Culture Collection and cultured according to the conditions specified. Immortalized human prostate epithelial BPH-1 cells were kindly provided by Dr Simon Hayward at Vanderbilt University Medical Center, Nashville, Tennessee, USA. Human primary prostate epithelial cells were purchased from Sciencell Research labs. At passage 2, human primary prostate epithelial cells were infected with a Ctrl or MAN2C1 siRNA lentivirus (Santa Cruz), selected in puromycin at 1 μg ml−1 for 36 h, and then analysed for protein expression and assayed for PTEN-derived PIP3 phosphatase activity. Retrovirus infection was performed as described previously53.
Collecting primary prostate cancer tissue
Prostate tissue was collected at St Joseph's Hospital in Hamilton, Ontario, Canada under the approval from the local Ethics Board and consent from patients. Cancers were examined and graded by pathologists of the Hospital.
Immunofluorescence and confocal microscopy
Double immunofluorescence staining was carried out using the following antibodies: monoclonal anti-PTEN (A2B1, Santa Cruz, 1 μg ml−1) or a polyclonal anti-PTEN (1:100; Upstate Technologies), and polyclonal anti-FLAG or a monoclonal anti-FLAG (M2, 1:500; Sigma). FITC-Donkey anti-mouse IgG (1:200; Jackson Immuno Research), Rhodamine-Donkey anti-rabbit IgG (1:200; Jackson Immuno Research) and FITC-Goat anti-mouse IgM (1:200; Jackson Immuno Research) were used as secondary antibodies.
For dual immunofluorescence staining, tissues were deparaffinized, rehydrated and subjected to antigen retrieval and endogenous peroxidase quenching as indicated for IHC. Tissue sections were blocked for 1 h at room temperature in 3% donkey serum and 3% BSA in TBST. Dual immunofluorescent staining was carried out using a TSA Plus kit (PerkinElmer) according to the manufacturer's protocol. Sections were counterstained with 4,6-diamidino-2-phenylindole. Images, including confocal, were captured using a MP Leica TCS SP5 confocal microscope (Leica). Images were analysed using IMARIS 6.2 and processed using CorelDraw 12 and Adobe Photoshop 7.
Xenograft tumour formation
The designed DU145 cells were resuspended in Minimum Essential Medium (MEM)/Matrigel mixture (1:1 volume), followed by implantation of 0.1 ml of this mixture s.c. into flanks of 8-week-old male nude or NOD/SCID mice (The Jackson Laboratory). Tumour volume was determined using the standard formula: L×W2×0.52, where L and W are the longest and shortest diameters, respectively. The presence of each tumour nodule was confirmed by necropsy. All animal work was carried out according to experimental protocols approved by the McMaster University Animal Research Ethics Board.
Western blot and immunoprecipitation
Frozen PC tissue and the corresponding normal tissue from nine patients were crushed under liquid nitrogen and suspended on ice in lysis buffer containing 20 mM Tris (pH 7.4), 150 mM NaCl, 1 mM EDTA, 1 mM EGTA, 1% Triton X-100, 25 mM sodium pyrophosphate, 1 mM NaF, 1 mM β-glycerophosphate, 0.1 mM sodium orthovanadate, 1 mM PMSF, 2 μg ml−1 leupeptin and 10 μg ml−1 aprotinin. Cell lysates were prepared and western blot was performed according to our published procedure53. Cell lysates containing 200 μg of protein were incubated with specific antibodies plus Protein G agarose (Invitrogen) at 4 °C overnight and were then washed six times in a buffer containing 50 mM Tris (PH 7.5), 100 mM NaCl, 1.5 mM EGTA and 0.1% Triton X-100. Antibodies used for IP were monoclonal anti-PTEN (A2B1, Santa Cruz, 1 μg), monoclonal anti-HA (12CA5, Y-11, Santa Cruz, 1 μg), monoclonal anti-FLAG (M2, Sigma, 1 μg) for MAN2C1 and mouse IgG (Sigma, 1 μg) as a negative Ctrl. The IP was analysed by western blot using polyclonal anti-PTEN (Upstate, 1:100) and anti-FLAG (Sigma, 1:500).
RNA interference
PTEN siRNA was expressed by a retroviral-based H1 promoter-driven shRNA vector (pRIH). The PTEN targeting sequence was previously described in ref. 54. PTEN was also knocked down by oligonucleotide PTEN siRNA (see Supplementary Table S1 for targeting sequences). The oligonucleotide MAN2C1 siRNA (Invitrogen) target sequence was as follows: 5′-ATAGCTGGTCTTCTCACCCTCTTTC-3′. MAN2C1 siRNA was transfected into cells, using Lipofectamine 2000 (Invitrogen) according to the manufacturer's protocol. We also performed a large-scale knockdown of MAN2C1 using a lentivirus system in DU145 PC cells, immortalized human prostate epithelial BPH-1 cells and human primary prostate epithelial cells to assay its effect on the PIP3 phosphatase activity of PTEN. Briefly, a MAN2C1 siRNA lentiviral vector (MAN2C1 shRNA; a TAT-independent lentiviral vector) was purchased from Santa Cruz. This vector expresses a pool of MAN2C1 siRNA. Packaging plasmids were gifts from Dr Bryan E. Strauss (University of Sao Paulo School of Medicine, Brazil). MAN2C1 siRNA lentivirus was packaged according to a published methodology55. The PTEN siRNA retrovirus (PTEN shRNA) has been described in ref. 32.
PTEN lipid phosphatase assay
PTEN with MAN2C1 was co-transfected into 293T cells. Ectopic PTEN was immunoprecipitated with an anti-PTEN antibody (A2B1, Santa Cruz, 1 μg) and subsequently assessed for phosphatase activity. Phosphatase assay was performed by the addition of 50-nM water-soluble DiC8-PtdIns(3,4,5)P3 (Echelon) as a substrate to assay for immunoprecipitated PTEN and recombinant PTEN-derived PIP3 phosphatase activity at 37 °C for 40 min. Released free phosphates were measured with BIOMOL Green reagent (BIOMOL) and were normalized against a reaction containing PIP3 substrate only56.
Immunohistochemistry
Paraffin-embedded sections of PC specimens were deparaffinized and heat-treated for 20 min in a 10 mM sodium citrate buffer (pH 6.0) in a food steamer. The following primary antibodies were incubated with the sections overnight at 4 °C: anti-MAN2C1 (1:500), anti-PTEN (1:100, A2B1, Santa Cruz) and anti-Ser473 phosphorylated AKT (1:200, Cell Signalling). Biotinylated goat anti-rabbit IgG (1:200) and avidin–biotin complex (ABC) were then added (Vectastain ABC kit, Vector Laboratories). Chromogen reaction was carried out with diaminobenzidine, and counterstaining was done with hematoxylin. An average staining score was given to representative sections from each sample. The intensity of staining was graded on a scale of 1–3, where 1 (low)=less than 20% of cells stained, 2 (medium)= 20–60% of the cells were stained and 3 (high)= >60% of cells were stained. For statistical analysis, scores 0–1 and 2–3 were grouped as 0 and 1, respectively, which were analysed using SPSS 10.0 software. Pearson's ϕ coefficient (Pearson's r computed on two dichotomous variables) was used to test for correlation between MAN2C1 and PTEN, and MAN2C1 and AKT pSer473 in normal, PIN and carcinoma. All tests were two tailed. A P-value <0.05 was considered statistically significant.
Recurrence-free survival analysis
Kaplan–Meier survival analysis was performed for a subset of 20 patients, obtained from the patients in our hospital, who had follow-up data following radical prostatectomy of at least 5 years (mean age±s.d.=62.3±7.0 years, range=50–72 years; mean Gleason score±s.d.=6.8±0.8, range=6–8; mean preoperative prostate-specific antigen (PSA)±s.d.=11.3±9.9 ng ml−1; range=2.6–40.5 ng ml−1). Median follow-up time was 69.5 months. Biochemical recurrence (first documented increase in serum PSA levels >0.2 ng ml−1 after radical prostatectomy) was used as the endpoint for analysis for patients in our cohort. Censored data (all censored data in patient subset showed no biochemical recurrence) are for the last documented follow-up. Log-rank test was performed to assess statistical significance between survival curves. A P-value <0.05 was considered statistically significant.
Kaplan–Meier survival analysis was also carried out for two independent patient cohorts, TMA2 and TMA5 (Supplementary Data 1 and 2). TMA2 and TMA5 were obtained from New York University and University of Chicago, respectively, through Cooperative Prostate Cancer Tissue Resource. TMA5 is a large patient cohort that was organized according to the biochemical recurrence of PC. Biochemical recurrence in Cooperative Prostate Cancer Tissue Resource was defined as an increase in serum PSA levels >0.6 ng ml−1 (single value) or consecutive rise in serum PSA levels between 0.4 and 0.6 ng ml−1 after radical prostatectomy57.
Tissue microarray staining and analysis
TMA2 was organized according to Gleason score and consisted of 1,128 PC tissue cores that were derived from 250 patients (Supplementary Data 1). TMA5 contained 1,616 PC tissue cores that were derived from 404 patients based on their PC biochemical recurrence (Supplementary Data 2). IHC staining of TMA was performed according the procedure described above. TMA slides were scanned using a ScanScope (University of Toronto) and analysed using the ImageScope software. All spots (stained cores) were also manually examined to exclude those spots that were either scratched or contained no prostate glands (only stromal tissue). All spots were also manually scored. The scores obtained using the ImageScope software are identical with the scores obtained manually. Statistical analysis was performed as described below.
Statistical analysis
Statistical analysis was performed using SPSS 10.0 for Windows software. For immunohistochemical analysis, Pearson's ϕ coefficient (Pearson's r computed on two dichotomous variables) was used to test for correlations between MAN2C1 and PTEN, and between MAN2C1 and AKT pSer473 (AKT-P) in normal, PIN and carcinoma. For Kaplan–Meier survival analysis, log-rank test was performed to assess statistical significance between survival curves. All tests were two tailed. For multiple comparisons between normal, PINs and different PC Gleason scores, a one-way ANOVA was performed. A P-value <0.05 was considered statistically significant for all tests.
Additional information
How to cite this article: He, L. et al. α-Mannosidase 2C1 attenuates PTEN function in prostate cancer cells. Nat. Commun. 2:307 doi: 10.1038/1309 (2011).
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Acknowledgements
We thank Dr Tak Mak at University of Toronto for providing HA-tagged PTEN and Dr Simon Hayward at Vanderbilt University Medical Center for providing immortalized BPH-1 human prostate epithelial cells. We also thank Dr Biao Chen for his work in detecting the co-localization between PTEN and MAN2C1, Mr Aubrey Gillis for his work in collecting primary prostate cancer tissues and Lieqi Liu for her superb technical assistance. L.H. is supported by a postdoctoral fellowship from the Father Sean O'Sullivan Research Center (FSORC) at St Joseph's Healthcare Hamilton. C.F. is supported by studentships from CIHR and FSORC. Supported by grants from Prostate Cancer Canada and CFI to D.T. and the Canadian Institutes of Health Research to R.C.A. Research funding from St Joseph's Healthcare Hamilton is also gratefully acknowledged. R.C.A. is a Career Investigator of the Heart and Stroke Foundation of Ontario and holds the Amgen Canada Research Chair in the Division of Nephrology at St Joseph's Healthcare and McMaster University.
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Contributions
L.H. identified MAN2C1, performed all biochemical characterization of MAN2C1-mediated PTEN inhibition and generation of xenograft tumours. C.F. conducted all experiments using primary prostate cancer tissues to examine the expression and co-localization of PTEN, MAN2C1 and AKT activation, as well as performing the statistical analysis. A.P.R. contributed to the generation of xenograft tumours. A.K., A.J.I. and J.S. were responsible for radical prostatectomy and the collection of primary prostate cancer tissues. J.-C.C. performed the pathological examination of all primary prostate cancer tissues. R.C.A. and J.D. performed the ER-stress experiments. D.T. designed and supervised the project. D.T., L.H., C.F., R.C.A. and A.J.I. prepared the manuscript.
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Supplementary information
Supplementary Figures, Tables and Methods.
Supplementary Figures S1-S9, Supplementary Tables S1-S7 and Supplementary Methods. (PDF 2782 kb)
Supplementary Data 1
Clinical information for tissue microarray 2 (XLS 88 kb)
Supplementary Data 2.
Clinical information for tissue microarray 5 (XLS 107 kb)
Supplementary Movie 1.
Co-localization of ectopic PTEN (red) with ectopic MAN2C1 (green) in 293T cells. Nuclei were counterstained with DAPI (blue). (AVI 3486 kb)
Supplementary Movie 2.
Co-localization of endogenous PTEN (red) with endogenous MAN2C1 (green) in DU145 cells. Nuclei were counterstained with DAPI (blue). (AVI 3699 kb)
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He, L., Fan, C., Kapoor, A. et al. α-Mannosidase 2C1 attenuates PTEN function in prostate cancer cells. Nat Commun 2, 307 (2011). https://doi.org/10.1038/ncomms1309
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DOI: https://doi.org/10.1038/ncomms1309
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