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Cancer Stem Cells Contribute to Cisplatin Resistance in Brca1/p53–Mediated Mouse Mammary Tumors

Departments of ¹ Microbiology and Molecular Genetics and ² Biological Chemistry and Developmental and Cell Biology, College of Medicine, University of California, Irvine, California; and Departments of ³ System Biology and ⁴ Breast Medical Oncology, University of Texas M. D. Anderson Cancer Center, Houston, Texas

Requests for reprints: Eric J. Stanbridge, Department of Microbiology and Molecular Genetics, College of Medicine, University of California, Irvine, CA 92697. Phone: 949-824-7042; Fax: 949-824-2454; E-mail: ejstanbr{at}uci.edu, or Eva Y-H. P. Lee, Departments of Biological Chemistry and Developmental and Cell Biology, College of Medicine, University of California, Irvine, CA 92697. Phone: 949-824-9766; Fax: 949-824-9767; E-mail: elee{at}uci.edu.

	Abstract

Top Abstract Introduction Materials and Methods Results and Discussion Disclosure of Potential... References

 
The majority of BRCA1-associated breast cancers are basal cell–like, which is associated with a poor outcome. Using a spontaneous mouse mammary tumor model, we show that platinum compounds, which generate DNA breaks during the repair process, are more effective than doxorubicin in Brca1/p53–mutated tumors. At 0.5 mg/kg of daily cisplatin treatment, 80% primary tumors (n = 8) show complete pathologic response. At greater dosages, 100% show complete response (n = 19). However, after 2 to 3 months of complete remission following platinum treatment, tumors relapse and become refractory to successive rounds of treatment. Approximately 3.8% to 8.0% (mean, 5.9%) of tumor cells express the normal mammary stem cell markers, CD29^hi24^med, and these cells are tumorigenic, whereas CD29^med24^–/lo and CD29^med24^hi cells have diminished tumorigenicity or are nontumorigenic, respectively. In partially platinum-responsive primary transplants, 6.6% to 11.0% (mean, 8.8%) tumor cells are CD29^hi24^med; these populations significantly increase to 16.5% to 29.2% (mean, 22.8%; P < 0.05) in platinum-refractory secondary tumor transplants. Further, refractory tumor cells have greater colony-forming ability than the primary transplant–derived cells in the presence of cisplatin. Expression of a normal stem cell marker, Nanog, is decreased in the CD29^hi24^med populations in the secondary transplants. Top2A expression is also down-regulated in secondary drug-resistant tumor populations and, in one case, was accompanied by genomic deletion of Top2A. These studies identify distinct cancer cell populations for therapeutic targeting in breast cancer and implicate clonal evolution and expansion of cancer stem-like cells as a potential cause of chemoresistance. [Cancer Res 2008;68(9):3243–50]

	Introduction

Top Abstract Introduction Materials and Methods Results and Discussion Disclosure of Potential... References

 
Mutations in breast cancer susceptibility genes BRCA1 and BRCA2 and several other genes encoding BRCA1/2-interacting proteins are associated with hereditary breast and ovarian cancer syndrome (reviewed in refs. 1, 2). Hereditary breast cancer accounts for 5% to 10% of all breast cancers, and of these, BRCA1 mutations account for approximately half of the cases. In sporadic breast cancer, BRCA1 mutations are rare; however, significant percentages of sporadic cancers show reduced or absent expression of BRCA1 due to promoter hypermethylation (3). BRCA1 encodes a 220-kDa nuclear phosphoprotein that contains multiple functional domains that interact with proteins involved in different cellular processes, including ubiquitously expressed tumor suppressors, oncoproteins, DNA damage repair proteins, cell cycle regulators, and transcriptional activators and repressors (reviewed in refs. 4, 5).

In addition to interacting with ubiquitously expressed proteins, BRCA1 associates and regulates ubiquitination of steroid hormone receptors, estrogen receptor and progesterone receptor (reviewed in ref. 6). Paradoxically, BRCA1-associated breast cancers are frequently high-grade, estrogen receptor /progesterone receptor/Her2 (triple)–negative basal cell–like tumors (7), with frequent mutations of TP53 and PTEN (8). The triple-negative tumors are initially responsive to chemotherapy with a high percentage entering pathologic complete response; however, tumors that recur or do not enter complete remission progress rapidly, resulting in a poor outcome.

Roles of BRCA1 in both homologous recombination and nonhomologous end joining DNA repair have been shown. Therapeutic strategies that explore the DNA repair defect in BRCA mutants have been proposed and are showing promise, in particular with poly(ADP-ribose) polymerase 1 inhibitors (9). BRCA1-mutated cell lines are more sensitive to cisplatin and less responsive to doxorubicin (10, 11). However, the in vivo response and long-term effects of platinum-based therapy in BRCA1-associated tumors have yet to be established.

Mice carrying somatic mutations of Brca1 and/or p53 alleles in mammary epithelial cells using the Cre/loxP system develop mammary tumors with high penetrance (12–15). Tumor latency in Brca1^fp/fpp53^fp/fpWAPCre^c mice, which express exon 11–deleted Brca1 and exon 5– and exon 6–deleted p53, is slightly shorter than that of Brca1^fp/fpp53^fp/fpCK14Cre^c mice, which carry null alleles of Brca1 and p53 (13, 14). On the other hand, MMTVCre^a target a small number of cells in the mammary gland and has much longer tumor latency (12). High tumor penetrance and consistent tumor latency of Brca1^fp/fpp53^fp/fpWAPCre^c and p53^fp/fpWAPCre^c mice allow studies of therapeutic response to single chemotherapeutic agents such as cisplatin [cis-dichlorodiamineplatinum (CDDP)], carboplatin, and doxorubicin, in vivo. CDDP is a member of platinum-based compounds that form various intrastrand and interstrand adducts with DNA (reviewed in ref. 16). Repair of the platinum adduct is mediated by nucleotide excision repair and single-strand and double-strand DNA break repair pathways. The clinical use of this drug is limited due to the emergence of intrinsic and acquired resistance and severe peripheral neurotoxicity. Other platinum derivatives, such as carboplatin and oxaliplatin, have different toxicities and are more commonly used in the clinical setting. Doxorubicin, also known as Adriamycin, is the most widely used anthracycline antibiotic in the treatment of breast cancer. It forms a complex with DNA by intercalation between base pairs, leading to the formation of free radicals and subsequent inhibition of DNA topoisomerase II catalytic activity (17). In clinically aggressive breast cancer, doxorubicin is most lethal to cells that contain high levels of topoisomerase II and are undergoing high rates of DNA replication. Chemotherapy has improved survival rates among cancer patients, but chemoresistance, which results in failure in cancer treatment, remains a major challenge.

There is now much evidence that cancer stem cells, a minority tumor cell population with stem cell properties, are capable of maintaining continuous tumor growth (reviewed in ref. 18). Cancer stem cells were first identified in acute myelogenous leukemia and have recently been shown to be present in many solid tumors, including tumors of the breast, central nervous system, and lung adenocarcinoma (reviewed in ref. 19). In breast cancers, CD44⁺CD24^–/low putative cancer stem cells were identified (20). In glioblastoma, a population of CD133⁺ cancer stem cells showed significant resistance to chemotherapeutic agents including temozolomide, carboplatin, paclitaxel, and etoposide (21). In small-cell lung carcinoma, a small population of stem-like cells showing high clonogenic activity and coexpression of CD44 and multidrug resistance gene, MDR1, showed multidrug resistance (22).

Despite the clinical importance of chemoresistance, to date there have been no reports of chemoresistant stem cell populations in breast cancer. Identification and characterization of such a subpopulation of cells will help develop strategies to target these cells. We show here that spontaneous tumors that developed in the conditional Brca1/p53 knockout mice respond favorably to platinum treatment, but chemoresistance does occur and often emerges over time. Expansion of a subpopulation of cancer stem cells correlates with drug resistance.

	Materials and Methods

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Generation of Brca1^fp/fpp53^fp/fpCre mutant mice and spontaneous mammary tumor formation. Generation of Brca1^fp/fpp53^fp/fpCre and p53^fp/fpCre mice has previously been described (12, 13). Briefly, Brca1 exon 11–floxed (Brca1^fp/fp) mice were obtained from Dr. Chu-Xia Deng (NIH, Bethesda, MD; ref. 15). Brca1^fp/fp mice were bred to p53 exon 5– and exon 6–floxed (p53^fp/fp) mice to obtain Brca1^fp/+p53^fp/+ mice. Brca1^fp/fpp53^fp/fpMMTVCre^a and Brca1^fp/fpp53^fp/fpWAPCre^c mice were generated by crossing the heterozygous floxed mice with MMTVCre^a or WAPrtTACre^c transgenic mice followed by crosses of heterozygous mice. The WAPrtTACre^c transgene expression was detected either before puberty as reported by Lin and colleagues (12) or in doxycycline-treated pregnant mice. Only the former group of mice were analyzed in the current study. PCR reaction was done to confirm exon 11 deletion of Brca1 gene and exon 5 and 6 deletions of p53 gene as previously reported (12, 13). The mice were in a C57BL/6 and 129/Sv mixed background. Mice were monitored for palpable tumors weekly. All animal experiments were in accordance with the guidelines of federal law and Institutional Animal Care and Use Committee at the University of California, Irvine.

Doxorubicin, cisplatin, and carboplatin treatment. Animals were treated with doxorubicin, cisplatin, or carboplatin when tumor diameter reached 0.5 cm. Doxorubicin (Fluka) was prepared at a stock concentration of 58 mg/mL in DMSO and stored at 4°C. Doxorubicin was diluted in 40% polyethylene glycol 400 (PEG-400; Sigma) in saline at the time of treatment. Cisplatin (CDDP; Sigma) was prepared fresh daily in 40% PEG-400 and saline. Stock solution of carboplatin (Sigma) at 10 mg/mL in water was stored at 4°C; dilution in 40% PEG-400 and saline was made at the time of treatment. CDDP was administered i.p. every other day at 0.5, 1.5, 3, or 6 mg/kg daily for 7 d. Carboplatin was administered i.p. once every 3 d for 15 d at 32.5 or 60 mg/kg; doxorubicin was administered i.p. weekly at 1.25 or 5 mg/kg for 21 d. Tumor growth was monitored by daily caliper measurements in two perpendicular dimensions. Tumor volume (mm³) was calculated according to the formula (d² x D) / 2, where d and D represent the shortest and longest diameters, respectively.

Histology and immunohistochemistry. Mice were sacrificed and tissues collected when tumors reached 0.75 to 1 cm³. The tissue was fixed in 4% paraformaldehyde (Sigma-Aldrich) at 4°C overnight followed by paraffin embedding. Paraffin sections were stained with H&E and examined by light microscopy. Immunostaining was done following the protocol described in the Vectastain Elite ABC kit (Vector Laboratories). To retrieve the antigen, slides were heated for 20 min in 10 mmol/L citrate buffer (pH 6.0) in a microwave oven. Caspase-3 (Cell Signaling Technology), phospho-H3 (Upstate), and Rad51 antibodies were used at 1:200, 1:2,000, and 1:50 dilutions, respectively.

Tissue disaggregation and cell preparation. Tumor tissues were processed according to Stingl and colleagues (23) with modifications. Briefly, tumors were minced into 2-mm³ fragments with sterile scalpels and enzymatically disaggregated for 8 h at 37°C in EpiCult-B medium (StemCell Technologies, Inc.) with 5% fetal bovine serum (FBS), 300 units/mL collagenase, and 100 units/mL hyaluronidase. After centrifugation at 450 x g for 5 min, RBC were removed by pipetting in 0.64% NH₄Cl. Single-cell suspensions were obtained by sequential pipetting for 1 to 2 min in 0.25% trypsin, followed by 2 min in 5 mg/mL dispase II plus 0.1 mg/mL DNase I (Sigma). The resulting suspension was then filtered through a 40-µm mesh and subjected to removal of lineage positive cells using anti-CD45, anti-TER119, and anti-CD31 antibodies to eliminate hematopoietic and endothelial cells. Magnetic beads were used to enrich mammary epithelial cells using the Mouse Mammary Stem Cell Enrichment Kit according to the manufacturer's protocol (StemCell Technologies). Following the enrichment step, the resulting cell suspension was kept on ice until use.

Cell labeling, flow cytometry, and sorting. Antibody staining was done in PBS supplemented with 1% bovine serum albumin (BSA). Cells were first incubated with 1% BSA for 20 min at a cell concentration of 1 x 10⁶/mL. Cells were subsequently washed and stained with different conjugated antibodies for 30 min, at dilutions predetermined by titration experiments. Antibodies used in this study were antimouse CD24-phycoerythrin (clone M1/69; BD Biosciences) and antimouse CD29-FITC (clone Ha2/5; BD Biosciences). Following removal of excess unbound antibodies by washing twice in PBS, the cells were resuspended in sorting buffer containing 1% BSA and 1 mmol/L EDTA in PBS. The stained cells were subjected to filtration through a 40-µm mesh and kept on ice until sorted. Flow cytometry analysis and sorting was done with the MoFlo flow cytometer (DakoCytomation). Forward scatter area versus forward scatter width profiles were used to eliminate dead cells and cell doublets. Sorting was done to achieve a final average purity of >95%.

Mammary gland transplantation. The no. 4 inguinal mammary gland outgrowths, between nipple and lymph node, of Rag1^–/– (The Jackson Laboratory) recipient mice were removed at 3 wk of age. Sorted cells were spun down by low-speed centrifugation (850 x g for 5 min) and resuspended in DMEM supplemented with 10% FBS and 2 mmol/L L-glutamine. In all experiments, cell number and viability were confirmed with the trypan blue dye exclusion test. Dilutions were done to achieve the required number of viable cells for appropriate injection doses. Cells were then mixed with BD Matrigel (BD Biosciences) at a 1:1 ratio and injected into cleared mammary fat pads of 6- to 8-wk-old Rag1^–/– recipient mice. To minimize experimental variability due to potential differences in recipient mice, control cell populations sorted by fluorescence-activated cell sorting (FACS) were injected into the opposite flank of each animal.

In vitro epithelial progenitor assays. The colony-forming ability of mammary epithelial progenitors was determined as previously described (23–25). Sorted cells were cultured onto preseeded feeder layers, prepared from irradiated (5 x 10³ cGy) NIH 3T3 cells, at a clonal density of 800/cm², in EpiCult-B medium (StemCell Technologies) supplemented with 5% FBS. After 24 h, the medium was replaced with serum-free EpiCult-B medium. In cases where CDDP was used, a predetermined GI₅₀ value was added to the culture for 48 h. Five to seven days later, cell colonies were fixed with acetone/methanol (1:1), stained with Giemsa, and counted. Colonies were counted from three replicate experiments and tabulated as the average number of colonies per 100 primary cells.

Embryonic stem cell culture. E14 embryonic stem cell line was cultured as described (26). Total RNA was prepared for reverse transcription-PCR (RT-PCR) and used as a positive control for Oct4 expression.

PCR and RT-PCR. Semiquantitative PCR reactions were done with 100 ng of genomic DNA as template in a mixture containing 20 pmol of each gene-specific primer. The PCR cycling conditions were done with an initial denaturation step at 95°C for 1 min, followed by 35 cycles of 40 s at 94°C for denaturation, 40 s at 60°C for annealing, and 1-min extension at 72°C, followed by a final extension at 72°C for 7 min. Semiquantitative RT-PCR analysis of total RNAs was done with the MasterAmp RT-PCR Kit (Epicentre Biotechnologies). Fifty nanograms of total RNA were used as templates for a first strand synthesis at 60°C for 20 min. This single-tube reaction was then subjected to 40 cycles of denaturation at 95°C for 40 s, annealing at 60°C for 40 s, and extension at 71°C for 1 min with a final extension of 7 min at 72°C. Alternatively, 200 ng of total RNA were reverse transcribed into cDNA using Oligo dT primer and the ImProm-II Reverse Transcription System (Promega) according to the manufacturer's protocol. The resulting single-strand cDNAs (1 µL) were either added to 25 µL of PCR reaction or stored at –20°C. Primer sequences are listed in Supplementary Table S1.

Statistical analysis. Results are presented as the mean ± SD for at least three repeated individual experiments for each group. Analyses were done with the SPSS software. The percentages tumor-free mice were generated using Kaplan-Meier survival curves. Analyses were done with GraphPad Prism software, which combines the log-rank (Mantel-Cox) test and the Gehan-Breslow-Wilcoxon method.

	Results and Discussion

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To investigate whether Brca1 mutation alters tumor chemotherapy response in vivo, we established p53- and Brca1/p53–mutant mammary tumor models, respectively, using the Cre/loxP system (12, 13). Nulliparous Brca1^fp/fpp53^fp/fpMMTVCre^a females developed mammary tumors with complete penetrance (11 of 11) between 11.8 and 16.7 months of age, with a median tumor latency of 14.1 months, as compared with nulliparous p53^fp/fpMMTVCre^a females (n = 18), which developed tumors with a median tumor latency of 16.9 months (P < 0.0001; Fig. 1A ). Expression of MMTVCre^a is restricted to a small number of cells in the mammary gland (12). As previously shown, mammary tumor latency varied depending partly on the numbers of targeted cells. In nulliparous Brca1^fp/fpp53^fp/fpWAPCre^c mice, mammary tumors developed between 3.7 and 9.5 months of age, with a median tumor latency of 6.3 months and complete penetrance (39 of 39 mice), as compared with nulliparous p53^fp/fpWAPCre^c mice (n = 18), which have a median tumor latency of 10.6 months (P < 0.0001; Fig. 1A). The median tumor latency in Brca1^fp/fpp53^fp/fpK14Cre^c mice, described by Liu and colleagues (14), is 7.0 months. Thus, double knockout mouse strains harboring WAPCre^c have a slightly shorter median tumor latency compared with K14Cre mice. Whether this is due to the usage of different promoters or the expression of mutant p53 and BRCA1 proteins in our models is unclear. In contrast to MMTVCre^a, the WAPCre^c is expressed in >90% of cells in the adult mammary gland (12). The greater acceleration of tumorigenesis by Brca1 mutation in WAPCre^c mice when compared with MMTVCre^a is likely due to paracrine actions on cell proliferation by the larger number of Brca1/p53–mutated cells.

View larger version (49K): [in this window] [in a new window] [Download PPT slide]   Figure 1. Brca1/p53–mediated mammary tumors are sensitive to cisplatin treatment. A, proportion of tumor-free nulliparous Brca1fp/fpp53fp/fp and p53fp/fp;Cre mice. X axis, age of each mouse when a palpable tumor was first detected. The curves were plotted using the Kaplan-Meier method. n values indicate the number of mice analyzed of each genotype. B, response of p53-mediated (top) and Brca1/p53–mediated (bottom) mammary tumors to doxorubicin or CDDP in vivo. Data were obtained using both WAPCrec and MMTVCrea mice. Tumor growth was monitored by taking daily caliper measurements in two perpendicular dimensions as described in Materials and Methods. C, immunohistochemical staining of activated caspase-3 (Casp-3) and phospho-histone 3 (P-H3) in CDDP- or doxorubicin (DOX)-treated samples at the indicated time points. D, Rad51 foci formation in CDDP- or doxorubicin-treated tumors. Insets, higher magnifications of stained nuclei. A total of 8 Brca1/p53–mediated and 10 p53-mediated tumors were analyzed, and all showed similar results.

Tumor-bearing mice were treated with doxorubicin, CDDP, or carboplatin. p53^fp/fp mouse mammary tumors were refractory to doxorubicin or CDDP treatment at all doses tested (Fig. 1B, top). Conversely, all Brca1^fp/fpp53^fp/fp mammary tumors (n = 19) responded to an initial cycle of four injections of 1.5, 3, or 6 mg/kg CDDP every other day for 7 days (Fig. 1B, bottom). Sensitivity to CDDP treatment was observed in spontaneous tumors developed in WAPCre^c; MMTVCre^a mice, or in tumor transplants in Rag1^–/– mice, indicating that Brca1 mutations render tumor cells sensitive to platinum compounds regardless of which Cre transgenic mice are assessed. Brca1^fp/fpp53^fp/fp mammary tumors were also sensitive to treatment with 32.5 mg/kg (n = 3) or 60 mg/kg (n = 1) carboplatin (data not shown). Taken together, a differential sensitivity of spontaneous Brca1^fp/fpp53^fp/fp mammary tumors to platinum over doxorubicin was found in vivo, consistent with the reported observation in a BRCA1-deficient human breast cancer cell line (11).

Sensitivity to platinum treatment (24–48 hours posttreatment) correlated with increased immunostaining of activated caspase-3, which showed cytoplasmic and perinuclear localization (Fig. 1C). Phospho-histone 3 expression, marker of the mitotic phase of the cell cycle, was decreased in CDDP-treated cells (Fig. 1C). Rad51 foci that formed at DNA double-strand breaks were detected 48 hours after CDDP treatment in p53^fp/fp tumors (Fig. 1D). In contrast, no Rad51 foci were detected in Brca1^fp/fpp53^fp/fp tumors. Thus, lack of homologous recombinational repair correlates with increased cell death and reduced mitotic cells in the favorable response to cisplatin. Recent studies showed that BRCA-deficient cancer cells are profoundly sensitized to inhibitors of poly(ADP-ribose) polymerase 1 in vitro (9). Poly(ADP-ribose) polymerase 1 binds to ssDNA breaks and may lead to persistent DNA lesions, preventing repair by homologous recombination pathways. Indeed, silencing of BRCA1 or BRCA2 network genes in p53-deficient, but not p53-proficient, cells enhances sensitivity to cisplatin (27). Taken together, BRCA1 and p53 deficiency leads to selective sensitivity to specific types of chemotherapeutic drug.

Because with doxorubicin treatment Brca1^fp/fpp53^fp/fp mammary tumors had only a transient slowing down of tumor growth, subsequent studies focused on CDDP-treated mice. Using a lower CDDP dose (0.5 mg/kg; n = 8), 80% of tumors had complete pathologic response to the initial treatment cycle (Fig. 2A ) and 20% had only partial regression for 11 to 12 days followed by rapid growth (data not shown), indicating that there is heterogeneity in the initial cisplatin response at the lower CDDP dosage. Following the initial tumor shrinkage and complete pathologic response, tumors relapsed at the same site 2 to 3 months posttreatment. Relapse also occurred in mice treated with higher dosages of CDDP (data not shown). To address whether recurrent tumors remain sensitive to platinum compounds, a second round of cisplatin treatment was done in three mice (Fig. 2A and data not shown). Tumor shrinkage was observed initially but tumors recurred with a more rapid growth rate than the original relapsed tumor following 1 week of complete regression (Fig. 2A). Rapid recurrence and growth suggest the existence of a subpopulation of cisplatin-resistant cells and selection of the resistant cells during successive platinum treatment.

View larger version (31K): [in this window] [in a new window] [Download PPT slide]   Figure 2. Chemoresistance to CDDP in vivo and the presence of cancer stem cells. A, sensitivity of primary and recurrent mammary tumors to CDDP treatment. CDDP was administered i.p., when tumors reached 0.5 cm3, at 0.5 mg/kg daily for 7 d. Tumor sizes were monitored following detection of palpable tumors before, during, and after CDDP treatment (n = 8). Tumor that recurred in three mice underwent additional cycle of treatments. B, FACS sorting analyses done on cells dissociated from primary tumor. Cells sorted according to the indicated gatings were used for in vivo tumorigenicity assays. C, transplantation using 1,000 cells of the CD29hiCD24med subpopulation resulted in tumor formation (arrows) whereas CD29med24–/lo (arrowhead) or CD29med24hi (asterisk) did not. D, a representative FACS profile of the resulting tumors following CD29hiCD24med cell transplantations.

To systematically investigate the role of CD29^hiCD24^med cells in cisplatin resistance, we investigated whether tumors that developed in Rag1^–/– mice, following transplantation of FACS-sorted tumor cells, respond to platinum treatment. Treatment of first-round primary transplants (n = 10) resulted only in partial regression (Fig. 3A, dotted line ). Importantly, secondary tumor transplants (n = 7) generated from CD29^hiCD24^med cells were completely refractory to CDDP treatment (Fig. 3A, solid line), suggesting an increase in CDDP-resistant cells compared with the primary transplant tumor. Rottenberg and colleagues (29) reported that they were unable to identify resistance to CDDP when they performed transplantations using tumor pieces. They, however, also failed to eliminate the tumors, suggesting the potential existence of CDDP-resistant, tumor-initiating cells. In our study, we showed that these cells are enriched in the CD29^hi24^med subpopulation. To test whether there were expansions of these cancer stem cells, we compared profiles of CD29 and CD24 in tumor cells from the primary and secondary tumor transplants. The frequency of CD29^hiCD24^med cells ranged from 6.6% to 11.0% (mean, 8.8%; n = 10) in the primary transplants and from 16.5% to 29.2% (mean, 22.8%, n = 7) in the secondary tumor transplants (Fig. 3B and data not shown). Thus, there is an 3-fold increase in the frequency of CD29^hiCD24^med cells in the secondary tumor transplants compared with the primary transplants, suggesting that the expansion of the CD29^hiCD24^med population may contribute to platinum resistance. Because frequencies of CD29^hiCD24^med cell populations in primary transplants are comparable to those in recurrent and primary tumors, it is unlikely that expansion of these populations in the secondary tumor transplants is due to transplantation per se. To confirm this, we carried out FACS analysis on primary and secondary transplant tumors that were not treated with CDDP. Results showed that the percentage of CD29^hiCD24^med in these tumors remained low, within the range of 3.5% to 9.8% (mean, 6.6%; n = 5). Importantly, in the CDDP-treated tumors, the CD29^hiCD24^med cells gave rise to heterogeneous cell populations, expressing wide ranges of CD24 and CD29 (Fig. 3B), indicating that the regenerated tumors contained phenotypically diverse populations of cells, as one would expect from cancer stem cells.

View larger version (32K): [in this window] [in a new window] [Download PPT slide]   Figure 3. Chemoresponse, FACS profiling, and colony-forming abilities of the primary and secondary Brca1fp/fpp53fp/fp tumor transplants. A, response to CDDP treatment of the primary and secondary tumor transplants, developed after transplantation with 1,000 CD29hiCD24med cells. The treatment was administered i.p., when tumors reached 0.5 cm3, at 0.5 mg/kg daily for 7 d. Tumor volumes before, during, and after CDDP treatment were shown. Arrows are not drawn to scale. B, FACS analyses of cells dissociated from primary tumor transplant, which showed partial resistance to CDDP (left), and from secondary tumor transplant, which were refractory to CDDP (right). C, colony formation assay of sorted CD29hiCD24med, CD29med24–/lo, and CD29med24hi cells from the primary tumor transplant. D, colony formation of unsorted cells from primary and secondary tumor transplants in the presence or absence of CDDP. C and D, columns, mean number of colonies per 100 primary cells; bars, SD. *, P < 0.05, versus the control group.

To investigate the involvement of key regulators in self-renewal and pluripotency in these CD29^hiCD24^med populations, we carried out semiquantitative RT-PCR for Nanog, Oct4, and Sox2, critical players for the pluripotent embryonic stem cells (reviewed in ref. 30). Sox2 and Oct4 expression was low in all the samples from primary as well as secondary tumor transplants, whereas Oct4 expression was readily detectable in the embryonic stem cells (Fig. 4A and B ). Interestingly, Nanog was readily detectable in these cells, particularly in the primary tumor transplant, whereas Nanog expression was reduced in CD29^hiCD24^med populations of the secondary tumor transplants. Lin and colleagues (31) showed that Nanog expression is suppressed by p53, leading to mouse embryonic stem cell differentiation. In our mouse model, conditional deletion of p53 may contribute to Nanog up-regulation. On the other hand, in contrast to normal stem cells, Nanog may no longer be subject to Sox2-Oct4 transcriptional regulation in cancer stem cells.

View larger version (42K): [in this window] [in a new window] [Download PPT slide]   Figure 4. Selective gene expression profiles in recurrent primary and secondary tumor transplants. A, semiquantitative RT-PCR analyses of CD29hiCD24med, CD29med24–/lo, and CD29med24hi cells from the primary and secondary tumor transplants. B, a positive control for Oct4, using mouse embryonic stem (ES) cells. C, semiquantitative PCR analyses of genomic DNA of CD29hiCD24med cells from the primary and secondary tumor transplants; WT, wild-type. D, model illustrating changes in cancer stem cells during the course of chemotherapy.

Taken together, exposure to CDDP may lead to the emergence of a subpopulation of mouse tumor cells (i.e., CD29^hiCD24^med) that become resistant to CDDP (Fig. 4D). Alternatively, a small population of preexisting cells with inherent CDDP resistance survives CDDP treatment. Following subsequent exposure to CDDP, these resistant cells self-renew as well as differentiate into tumor masses containing cells of various phenotypes. Transplantation of this subpopulation of cells into immunodeficient mice led to its further expansion. Up-regulation of c-Myc was detected in the CD29^hiCD24^med population in the primary, but not secondary, tumor transplant. Whether c-myc and Nanog are involved in the expansion, but not maintenance, of the CD29^hiCD24^med cancer stem cell populations remains to be addressed.

Studies by Rottenberg and colleagues (29) used a model with null alleles of Brca1 and p53, whereas the model described here expressed exon 11–less isoforms of Brca1. The CDDP treatment regimen also differs in the two studies. A 20-day recovery preceded each single injection of CDDP reported by Rottenberg and colleagues (29). Tumors were not eliminated under the regimen, indicating the existence of chemoresistant cells. The spontaneous chemoresistant model described here allows a longitudinal follow-up of putative cancer stem cells that will allow delineation of chemoresistance. Clearly, the platinum-resistant CD29^hiCD24^med cancer stem cells not only expanded but presumably also increased their proliferation rates relative to the total population of tumor cells during the treatment course.

	Disclosure of Potential Conflicts of Interest

Top Abstract Introduction Materials and Methods Results and Discussion Disclosure of Potential... References

 
No potential conflicts of interest were disclosed.

	Acknowledgments

 
Grant support: Avon Foundation-American Association for Cancer Research International Scholar Award in Breast Cancer Research (N. Shafee and E.J. Stanbridge), Department of Defense Breast Cancer Center of Excellence grant DAMD17-02-1-0694, NIH grant CA04964 (E.Y. Lee), and Department of Defense predoctoral fellowship (C.R. Smith). N. Shafee is a Visiting Scholar from Universiti Putra Malaysia. C.R. Smith is inspired by his son Keagen.

The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

	Footnotes

 
Note: Supplementary data for this article are available at Cancer Research Online (http://cancerres.aacrjournals.org/).

Received 9/17/07. Revised 2/28/08. Accepted 3/ 1/08.

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