Article |
2 Department of Urology, New York University School of Medicine, New York, NY 10016
3 Ronald O. Perelman Department of Dermatology and Department of Pharmacology, New York University School of Medicine, New York, NY 10016
4 Kaplan Cancer Center, New York University School of Medicine, New York, NY 10016
5 Department of Urology, Osaka University Medical School, Suita, Osaka 565-0871, Japan
6 Department of Urology, Fukuoka City Medical Center of Sick Children and Infectious Diseases, Fukuoka 810-0063, Japan
Address correspondence to E. Lynette Wilson, Department of Cell Biology, New York University School of Medicine, 550 First Ave., New York, NY 10016. Tel.: (212) 263-7684. Fax: (212) 263-8139. E-mail: wilsoe01{at}endeavor.med.nyu.edu
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Abstract |
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Key Words: prostate; stem cells; slow-cycling cells; branching morphogenesis; prostate regeneration
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Introduction |
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Although the overall organization of the rodent prostate differs from that of the human gland, the rodent prostate provides unique opportunities to study many important features of the prostate, including the involutionregeneration process as well as chemical and hormonal carcinogenesis. Each murine prostatic duct consists of a proximal region attached to the urethra, an intermediate region, and a distal tip (Sugimura et al., 1986a; Cunha et al., 1987; Lee et al., 1990; Hayashi et al., 1991). Proliferating cells are located at the tips of the ducts (Sugimura et al., 1986c; Cunha et al., 1987). Based on this finding, it has been suggested that prostatic stem cells reside in the distal region (Kinbara et al., 1996). However, studies on the stem cells of several other systems have indicated that the rapidly cycling cells are most likely the so-called transit-amplifying cells rather than stem cells. The location of prostatic epithelial stem cells is therefore currently unknown.
A particularly powerful method for identifying epithelial stem cells takes advantage of the slow-cycling nature of such cells (Berardi et al., 1995; Thorgeirsson, 1996; Beauchamp et al., 2000; Lavker and Sun, 2000; Slack, 2000). In this procedure, a tissue is long-term labeled with 3H-thymidine or BrdU so that all cells, including the stem cells, are labeled. This is followed by a "chase" period during which the label is diluted out from all the rapidly dividing (transit amplifying) cells but is retained by the slow-cycling (stem) cells, which can thus be identified as the "label-retaining cells" (Cotsarelis et al., 1989; Tani et al., 2000; Taylor et al., 2000). Using this approach, corneal epithelial stem cells have been shown to reside in the peripheral cornea in the limbal region (Schermer et al., 1986; Cotsarelis et al., 1989) and this region has been used in limbal stem cell transplantation studies to reconstitute the corneal epithelium (Tsubota et al., 1999; Tsai et al., 2000). Using the same label-retaining cell approach, hair follicular epithelial stem cells have been shown to reside in the upper follicle in an area called the bulge (Cotsarelis et al., 1990; Morris and Potten, 1999; Lavker and Sun, 2000; Taylor et al., 2000; Oshima et al., 2001). Another important feature of stem cells is their high proliferative potential as reflected by their ability to yield large colonies in vitro (Barrandon and Green, 1987; Ogawa, 1993), as was shown to be the case for both the limbal zone of the corneal epithelium (Pellegrini et al., 1999) and the bulge area of the hair follicle (Oshima et al., 2001).
We describe here the identification of a subpopulation of mouse prostate epithelial cells, located in the proximal region of prostatic ducts, that are slow cycling and exhibit a high in vitro proliferative potential. Moreover, they are able to reconstitute complex glandular structures in collagen gels. These findings strongly suggest that these proximal cells are the stem cells. Cells located at the distal tips of prostatic ducts are rapidly proliferating, thus representing the transit-amplifying cells. Based on these findings, we propose a model in which the prostatic epithelial stem cells, which are maintained in a dormant state in the proximal region of prostatic ducts, give rise to the proliferating transit-amplifying cells that migrate distally to either maintain the normal prostate gland or repopulate the gland during androgen-induced regeneration.
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Results |
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Heterogeneous distribution of the label-retaining cells
Although few label-retaining cells are present in the intermediate and distal regions of the ducts after a chase period of 39 wk (Fig. 2), ducts that had been chased for an intermediate period (912 cycles of involution and regeneration) revealed clusters of label-retaining cells (Fig. 3). These clustered, label-retaining cells were frequently associated with the "ridges" of epithelial folds projecting into the lumen of the duct, whereas the unlabeled cells were associated mainly with the "valleys" connecting the ridges (Fig. 3 a). Even in areas that were not folded, a similar clustering of the labeled cells was frequently noted (Fig. 3 b). Because most of these label-retaining cells eventually lost their label at the end of a 39-wk chase (16 cycles), they probably represent young transit-amplifying cells that had not yet divided sufficiently to dilute out the BrdU label.
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Discussion |
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Our data indicate that the distal region of the intact gland contains a population of actively proliferating cells (Fig. 4; also see Sugimura et al., 1986c; Cunha et al., 1987). The distal tips of the dorsal and lateral rat prostates undergo significant growth when combined with embryonic urogenital sinus mesenchyme and implanted under the renal capsule (Kinbara et al., 1996). These findings were interpreted to mean that the distal region of prostatic ducts contains the stem cells. However, because the implant studies did not include tissues from the proximal region for comparison, one cannot exclude the possibility that under identical experimental conditions, cells from the proximal region may grow even better than the distal cells (compare Figs. 5 and 6). The observed growth of the distal region may therefore be explained by the presence of some (young) transit-amplifying cells (Fig. 3; also see below). There are many recent examples, including skin (Taylor et al., 2000; Oshima et al., 2001), bone marrow (Williams, 1993; Berardi et al., 1995), and liver (Fausto, 2000; Strain and Crosby, 2000), showing that a post-stem cell population of young transit-amplifying cells can undergo significant growth.
Clusters of young transit-amplifying cells
Another interesting finding we made is that some of the intermediate stage label-retaining cells, which eventually lose their label, form clusters that are interspersed by groups of nonlabeled cells (Fig. 3). A related, earlier observation is that the castration-induced apoptotic cells were also found to form clusters (Rauch et al., 1997). These two observations can be explained if one assumes that the clusters of intermediate stage label-retaining cells (Fig. 3) represent young transit-amplifying cells that have not yet diluted out all their BrdU label via cell division, and that such cells are more resistant to the apoptotic effects of androgen depletion than the older transit-amplifying and terminally differentiated cells. Having groups of young transit-amplifying cells capable of active proliferation placed strategically along the intermediate and distal ducts may allow the gland to respond more rapidly to signals for increased growth or regeneration without having to recruit cells from the distant proximal stem cell region.
Such a dispersion of young transit-amplifying cells may facilitate prostatic gland regeneration, which occurs regularly in some species. For example, male squirrel monkeys, woodchucks, and the vizcacha (a South American rodent) are known to undergo seasonal variations in testosterone levels that are accompanied by pronounced changes in testicular volume (Baldwin et al., 1985; Pasqualini et al., 1986; Fuentes et al., 1993). Although measurements of prostatic size have not been done, it is likely that prostatic involution occurs concomitantly with testicular regression. Thus, the prostate of these animals may undergo physiological involutionregeneration and the strategically located, young, transit-amplifying cells within the ducts may facilitate the rapid regeneration of the gland.
Basal and luminal cells may serve as prostatic epithelial progenitor cells
There are conflicting data on the nature of the epithelial compartment in which prostatic stem cells are located. The existence of a population of cells that possess markers for both the basal (keratins K5 and K14) and luminal cells (K8 and K18) suggests that these represent an intermediate stage between the precursor basal and the mature luminal cells (Bonkhoff et al., 1994a; Bonkhoff and Remberger, 1996; Robinson et al., 1998). In addition, a prostatic epithelial basal cell line has been shown to give rise to luminal cells both in vitro (Danielpour, 1999) and in vivo (Hayward et al., 1999). These data suggest that basal cells are the precursors of luminal cells. On the other hand, kinetic data showing that luminal cells divide before basal cells after an androgen pulse (Evans and Chandler, 1987a,b), and that the luminal cells divide faster than the basal cells in individuals on a long-term androgen block (van der Kwast et al., 1998) have been interpreted to indicate that luminal cells are self-renewing and are thus independent from the basal compartment. However, the more rapid response of luminal cells to androgens could also result from transit-amplifying luminal cells being more responsive to androgens than basal cells.
Our data indicate that label-retaining cells are concentrated in the proximal region of prostatic ducts and, importantly, are present in both the basal and luminal compartments (Figs. 1 and 2). The presence of label-retaining cells in the luminal compartment is unexpected and raises the interesting possibility that luminal cells are self-sustaining. On the other hand, our finding does not exclude the possibility that basal cells can give rise to luminal cells (see below), or that these label-retaining luminal cells represent the youngest transit-amplifying cells, which require a longer period of chase to dilute out their label.
We have also shown that in the distal and intermediate regions of the prostatic ducts, the luminal cells retain the BrdU label for a shorter period of time than the basal cells (Fig. 2). Because we know that the transit-amplifying luminal cells replicate more rapidly than the basal cells (Fig. 4), it is not surprising that the BrdU label is diluted out more efficiently from the luminal cells.
The prostatic stem cell niche and its possible regulation: a hypothesis
Stem cells are usually located in a niche where they are maintained in a quiescent state (Potten and Loeffler, 1990; Lavker and Sun, 2000; Slack, 2000). Because the proximal region of the prostatic ducts is enveloped by a thick band of smooth muscle cells (Nemeth and Lee, 1996) that are known to produce a high level of TGF-ß (Nemeth et al., 1997), it is possible that this smooth muscleproduced TGF-ß plays a role in inhibiting the proliferation of prostatic epithelial stem cells. Consistent with this possibility, it has recently been shown that the expression of a dominant-negative form of the TGF-ß receptor in the prostate induced an excessive proliferation of the prostatic epithelial cells in the proximal region (Kundu et al., 2000). Moreover, there is a gradient of TGF-ß expression in the stroma along the ductal axis; it is highest in the stroma surrounding the proximal epithelium and lowest in the distal region, which is the site of cell proliferation (Nemeth et al., 1997). A similar inhibitory role of TGF-ß is known to be responsible for maintaining hematopoietic stem cells in a quiescent state (Cashman et al., 1990; Hatzfeld et al., 1991; Fortunel et al., 2000).
A model for prostatic epithelial stem cells
Based on the above considerations, we propose a model of prostatic epithelial homeostasis in which the stem cells reside in the proximal region of the ducts and are maintained in a quiescent state by the high local levels of TGF-ß (Fig. 7). During prostatic regeneration, either a reduced level of active TGF-ß or the production of an overriding, positive signal (Fig. 7, GF) stimulates the stem cells to divide, giving rise to a cadre of transit-amplifying cells (TA1 TA2
TA3 ... etc.) that migrate distally. These transit-amplifying cells function as an immediate source of replacement cells along the ductal axis. Upon cell division and distal migration, transit-amplifying cells progressively lose their proliferative potential. During involution, the oldest transit-amplifying cells are preferentially lost through apoptosis; conversely, during regeneration, the surviving (young) transit-amplifying cells, which are clustered at multiple sites along the ducts, serve as the immediate source of cell replication, thus rapidly supplying new cells to form a regenerated gland.
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An alternative interpretation of our results may be that the low numbers of label-retaining cells that we observe in the intermediate and distal regions of ducts may also represent stem cells rather than transit-amplifying cells. These cells would survive involution, resulting in a greater proportion of stem cells in these regions in a regressed gland. During regeneration, these cells may give rise to transit-amplifying cells that migrate in two directions, namely toward the distal as well as the proximal regions. However, our results indicate that even if low numbers of stem cells are located in the intermediate and distal regions, they are concentrated in the proximal region in a regenerated prostate.
Our finding that prostatic stem cells are concentrated in the proximal region of ducts will facilitate their isolation and characterization and help to elucidate the processes involved in prostatic homeostasis and the etiology of prostatic diseases. As both stem cells and androgen-independent prostate cancer cells have extensive self-renewal abilities and do not depend on androgen for their survival, the isolation and characterization of prostatic stem cells will be of major importance for understanding the mechanisms that result in the generation of androgen-independent prostatic carcinoma.
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Materials and methods |
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Detection of quiescent, slow-cycling (label retaining) cells
To locate the cells in the prostatic epithelium that turned over at the slowest rate, we developed a method for labeling the entire epithelial compartment of the prostate with BrdU (Sigma-Aldrich). This was followed by chasing the BrdU from the cells using multiple cycles of androgen withdrawal and replacement as depicted in Fig. 1 e. Young animals (3 wk old) were required to ensure labeling in all prostatic epithelial cells. Mice were castrated and 2 wk later, prostate regeneration and labeling were promoted by the simultaneous subcutaneous implantation of testosterone pellets (Innovative Research of America) and mini-osmotic pumps (model 2002; Alza Corp.) containing 5 mg BrdU in 0.25 ml Ringer's solution (Eldridge et al., 1990; Lehrer et al., 1998). After 2 wk, three mice were killed to ascertain that 9899% of the basal and luminal compartments of the ventral and dorsal prostates were labeled with BrdU. As prostatic epithelium turns over at a slow rate, the process of chasing out the BrdU label was hastened by cycling. The ventral and dorsal prostates were analyzed for BrdU-containing cells at various times up to 39 wk (16 cycles of androgen withdrawal and supplementation) after chasing out the label.
Detection of rapidly cycling cells
To compare the location of slow-cycling cells with that of rapidly cycling cells and to determine the turnover within the epithelial compartment in 5-wk-old mice (the age at the start of the chase) with older animals, we also administered BrdU as a pulse and determined the incidence and location of labeled epithelial cells within the three regions (proximal, intermediate, and distal) of the prostatic ducts. Mice 5, 17, and 34 wk old (the start, midpoint, and end of the long-term labeling experiment) were injected intraperitoneally with BrdU at 50 µg/g body weight, killed 24 h later, and the ventral and dorsal prostates were removed. To identify slow-cycling cells that were stimulated to divide after an androgen pulse, we injected castrated BrdU-labeled animals intraperitoneally with testosterone propionate (4 µg/g body wt) followed 40 h later with 3H-thymidine (8.1 µCi/g body wt). Animals were killed 1 h later and BrdU was detected by immunohistochemistry and 3H-thymidine by autoradiography (Lehrer et al., 1998; Taylor et al., 2000).
Tissue preparation
Animals were killed by cervical dislocation and the urogenital tract was removed en block and transferred into PBS, pH 7.6. The ventral and dorsal prostates were dissected in PBS under a dissecting microscope, using 25-gauge needles (Sugimura et al., 1986a). The tissue was fixed in 70% ethyl alcohol in 50 mM glycine, dehydrated, and embedded in paraffin.
Immunohistochemistry
Tissue sections (3 µm) were deparaffinized and endogenous peroxidase was blocked by immersing sections in 0.3% H2O2 for 20 min. After incubation in 1.5 N HCl for 15 min at 37°C, slides were washed in 0.1 M borax buffer, pH 8.5, for 10 min followed by three washes in PBS. Nonspecific binding sites were blocked by incubation in PBS containing 10% FCS and the slides were then incubated with peroxidase-conjugated anti-BrdU antibody (Boehringer) for 1 h at room temperature. The antibody binding sites were visualized using the substrate DAB (Sigma-Aldrich). Slides were lightly counterstained with hematoxylin. The presence of basal and luminal cells was determined (Salm et al., 2000a) using antibodies to basal keratins 5 and 14 (BL18 and LL001) and luminal keratins 8 and 18 (LE41 and LE61), which were a gift of E.B. Lane (University of Dundee, Dundee, Scotland). The presence of prostatic secretory material was detected using specific antibodies to prostatic secretory products, which were a gift of C. Abate-Shen (Robert Wood Johnson Medical School, Piscataway, NJ; M. Kim, M.M. Shen, and C. Abate-Shen, personal communication), and secondary HRP-conjugated antibodies with DAB as the substrate.
Enumeration of BrdU-labeled cells
The morphology of the rodent prostatic ductal system has been well described (Sugimura et al., 1986a, Cunha et al., 1987; Lee et al., 1990; Rouleau et al., 1990; Hayashi et al., 1991; Sensibar et al., 1991; Kinbara and Cunha, 1996; Nemeth and Lee, 1996). It can be divided into three regions, proximal, intermediate, and distal (Fig. 1 b). At each time point, three mice were killed and two sections from each prostate (ventral and dorsal) were examined immunohistochemically for evidence of labeled basal and luminal cells within each region. At least 1,000 luminal cells and 100200 basal cells were counted in the distal and intermediate regions of each section, making a total of 6,000 luminal and 6001,200 basal cells scored for each time point. Basal cells are less abundant than luminal cells, so fewer basal cells could be enumerated. The proximal region comprises a small area and hence fewer basal and luminal cells could be scored in this region than in the intermediate and distal regions. At least 100200 luminal and 2040 basal cells were counted in the proximal region of each section, making totals of 6001,200 luminal and 120240 basal cells scored for each time point.
Statistical analyses
The percentages of the BrdU-containing cells were determined by dividing the number of labeled cells by the total number of cells scored in each region. Each time point had three animals and two sections were scored from each ventral and dorsal prostate. For the detection of rapidly cycling cells in animals of different age groups, three mice were used per age group and two sections were scored from each ventral and dorsal prostate. The results are depicted as the means and standard deviations at each time point and comparisons between groups were made using the t test.
Cellular proliferation
The ventral and dorsal prostates of 6-wk-old mice were removed and dissected under a dissecting microscope in the presence of collagenase (type II from Clostridium histolyticum; Sigma-Aldrich) (Sugimura et al., 1986a). The proximal and distal regions were excised and incubated in 0.5% collagenase for 30 min at 37°C, followed by digestion in 0.25% trypsin (BD Biosciences) for 5 min at 37°C. Cells were resuspended in a mixture of basal and luminal epithelial growth media (Salm et al., 2000a,b), with conditioned medium from a prostatic smooth muscle cell line, PSMC1 (Salm et al., 2000b) (40:40:20, vol/vol/vol). Cells from both regions were seeded at 2 x 103 cells/well in collagen-coated (Cohesion) 96-well plates. Cells were harvested, counted, and reseeded at 2 x 103 cells/well every 45 d. The total cell output from 2 x 103 cells of each region was determined at the end of the serial culture when their growth capacity was exhausted. The ability of cells from proximal and distal regions of ducts to form colonies was determined by seeding cells at 4 x 103 cells/well in collagen-coated eight-well chamber slides. Colonies were fixed after 5 d in 70% ethanol and stained with hematoxylin and eosin.
Duct formation in collagen gels
Cells isolated from the proximal and distal regions of ducts were suspended in collagen (Elsdale and Bard, 1972) at 8 x 103 cells/100 µl type 1 collagen (BD Biosciences) in 96-well dishes. After gelation, the collagen was overlaid with 100 µl medium comprising a mixture of basal and luminal growth media (Salm et al., 2000a,b) with conditioned medium as described above. Medium was replaced daily. The collagen gels were removed after 6 d, and the numbers of ducts and branch points/duct were scored. Collagen gels were also processed for immunohistochemistry (see above). The area of ducts was measured using an NIH image analysis program (http://rsb.info.nih.gov/nih-image). Clonal analysis was done by seeding cells at limiting dilution in 96-well microtitre dishes and verifying microscopically those wells that contained single cells.
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Footnotes |
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* Abbreviations used in this paper: BPH, benign prostatic hyperplasia; DP, dorsal prostate; LP, lateral prostate; VP, ventral prostate.
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Acknowledgments |
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Submitted: 15 February 2002
Revised: 26 April 2002
Accepted: 7 May 2002
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References |
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