Characterization of single disseminated prostate cancer cells reveals tumor cell heterogeneity and identifies dormancy associated pathways

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Discussion

We identified and characterized a definitive set of DTC in patients with a high prostate epithelial score and a low erythroid progenitor-like score. The majority of the PCa DTC had an EpCAM score of 3+ or 4+, with only a few cells displaying an EpCAM score of 2+. We profiled individual cells instead of pools of cells to avoid the inclusion of any contaminating cell types in our signatures, which would confound data analyses for definitive PCa DTC. Until further evidence is available to suggest that the predominantly EpCAM 2+ cells with a low prostate epithelial score and a high erythroid-progenitor-like score are associated with PCa, we determined that based on the extensive cellular plasticity present in these cells that they should be removed from our analysis. Of note, it is unlikely that these erythroid progenitor-like cells are present in the blood contaminating the analysis of CTC as erythropoiesis usually occurs in the BM, however the possibility should not be ruled out, e.g. extrameduallary erythropoiesis can occur in myelofibrosis [27].

DTC from most patients (except one patient) unsurprisingly were heterogeneous between and within patient samples at the transcriptional level, regardless of disease type (i.e. NED or ADV) [28, 29]. One could speculate that DTC obtained from one patient may all arise from a single micrometastasis (e.g. patient 2613), providing some clonality and a similar microenvironment for each of these cells. However, in the other patients, cells may have been isolated from different micrometastases or individual cells present in the BM and this would explain why some but not all cells from patients cluster together. Similar reasoning/hypothesis may explain why ADV_2 clusters with NED, with ADV_2 and NED cells being present as individual cells and ADV_1 cells being isolated from groups of cells. Of note, when we clustered individual DTC based on the expression of the top and bottom 50 differentially expressed genes in NED and ADV_1, we observed a greater degree of patient-associated clustering of the individual DTC [Figure 4]. This suggests the level of heterogeneity observed will depend on the number of genes, or more specifically the biological process assessed in the signature.

DTC in ADV patients could be clustered into two groups: ADV_1 and ADV_2. Of note, we observed no difference between biochemical and radiographic disease states in ADV patient samples when compared to NED patient samples (data not shown). Among the patients in the ADV category, 4 of 6 had DTC in both the ADV_1 and ADV_2 clusters. This indicates that the DTC in the patients with clinically advanced disease harbor cells in different biological states. For the top 50 and bottom 50 genes differentially expressed between NED and ADV_1 categories, surprisingly the ADV_2 DTC were similar to the NED DTC. This does not necessarily mean the ADV_2 DTC were also in a state of dormancy, but the similarity in the gene expression pattern suggests potential concordance in their behavior. This is of clinical importance, as the current therapies for treatment of advanced PCa targets cells that are actively replicating. Cells in a state of dormancy/quiescence would not be affected by these treatment strategies, and they could potentially exit dormancy and become active metastases after treatment has concluded. If the ADV_2 DTC possess some of the hallmarks of the DTC from the NED patients, it could be hypothesized that a subpopulation of PCa cells in the BM of the ADV patients are in a dormant/quiescent state. Further, the challenge for cure in these patients would rely on treating both the active and dormant PCa DTC.

The identification of clinically-relevant pathways involved in PCa dormancy in patients is needed to develop dormancy models, identify robust markers and design effective treatment strategies. The activation of the p38 pathway has been identified to promote and maintain tumor dormancy [10, 16, 18, 25, 26]. A recent report demonstrated that PCa stem-like cells in the BM enter a p38-dependent dormancy state in an animal model, however the clinical relevance of the p38 pathway in PCa dormancy is yet to be established [18]. In our study, genes associated with the p38 stress response pathway were shown to be altered when we compared DTC from NED patients to a group of DTC from ADV patients. In addition to the genes identified in the IPA analysis, both KIAA1804 (MLK4β) and MTRR were downregulated in the NED DTC [Supplemental Table 2]. The mitogen-activated protein kinase family and specifically MLK4β has been shown to inhibit the p38 pathway [19]. MTRR is an electron transferase involved in methionine synthesis and has also been shown to inhibit the p38 pathway [21]. Thus, loss of these genes may be more permissive for persistent p38 activation in DTC in PCa patients.

NUAK1 is a protein kinase that has been linked to the activation of the p38 pathway and cell proliferation [20]. NUAK1 was found to be upregulated in the ADV_1 DTC population. PIN4 was also upregulated in the ADV_1 DTC group compared to the NED DTC. PIN4 function is linked to cell proliferation [30]. MALT1, which showed upregulation in the NED DTC, is a cysteine protease whose function has been linked to activation of the p38 pathway [23]. MALT1 regulates p38 and CDC25B is a downstream target of p38 [24]. CDC25B, a phosphatase that activates the cyclin-dependent kinase CDC2, was upregulated in NED DTC. p38 phosphorylates CDC25B, which results in an inhibition of entry into the M phase of the cell cycle [24]. Elevated mRNA levels for CDC25B might be a compensatory mechanism for p38-induced growth arrest. While extrapolating from gene expression to function is not completely reliable, the elevated expression of these 6 genes discussed above suggests a role for the p38 stress-response pathway in the DTC isolated from the BM of the NED patients.

We developed a p38-associated dormancy signature based on the top 50 and bottom 50 differentially expressed genes between NED DTC and ADV_1 DTC. This signature, while biased, could clearly differentiate between NED DTC and ADV DTC. To further validate our findings we interrogated the DTC expression profiles for a dormancy signature previously developed from a HNSCC model [16, 25, 31] and a PCa model [18]. Dormancy upregulated genes were enriched in the NED DTC, suggesting that the dormancy signature could consistently identify dormant PCa cells present in the patient BM. Among the dormancy-up genes in NED DTC, TGFβ2 and BMP7 have been implicated specifically in dormancy of DTC in the BM [16, 18]. However, the dormancy downregulated genes could not distinguish between the NED, ADV_1 and ADV_2 DTC. One possible explanation for this is that solitary PCa DTC may be slow cycling or non-proliferative in nature, therefore the dormancy-down genes that are linked to proliferation may not be changing sufficiently. Furthermore, dormancy initiation and maintenance may require an induction of the p38 stress response pathway, which results in the activation of different downstream cell cycle effectors among different tumor types.

The lack of clinically-relevant models in the dormancy field is a challenge that needs to be overcome. New model systems involving TGF-beta and the perivascular niche are emerging and may be relevant for PCa DTC study if proven clinically relevant [16, 32]. Despite the clinical relevance, our study is restricted in its interpretation due to the limited number of EpCAM+ cells that can be isolated from NED patient BM and the fact that we were unable to further interrogate individual cells at the protein level or functionally to validate our findings. Nonetheless, our study provides the first clinical evidence supporting a role for the p38 pathway in dormancy in PCa DTC in patients, which supports further functional validation in vitro and in vivo.

In summary, this study illustrates a first-in-field transcriptomic signature from individual DTC in cancer patients. We established a gene signature to definitively identify PCa DTC from other EpCAM+/CD45- cells that do not demonstrate typical prostate epithelial markers in the BM. We further demonstrated that patients with advanced disease may harbor at least two populations of DTC, in which one group of DTC is similar to those isolated from patients with NED for up to 18 years. We also validated our signature using a mechanistically modeled dormancy-associated signature from head and neck cancer supporting the hypothesis that the p38 pathway is associated with the dormant nature of these DTC in NED patients. Ultimately, in the clinical setting, the intent is to maintain DTC in a dormant state or to better understand dormancy such that active disseminated cells can be shifted to a state of dormancy, and hence delay the onset of symptomatic and lethal metastatic disease. Our results suggest that the p38 pathway may serve as a potential biomarker to monitor early recurrence and identifies the p38 axis as an attractive target for therapeutic intervention to regulate dormancy in PCa patients.

Methods

Selection criteria for patients

Patients from 2 clinical categories were selected. Patients who had a diagnosis of adenocarcinoma of the prostate, had undergone a radical prostatectomy (RP), had not received neoadjuvant or adjuvant treatment and had a PSA that was undetectable (less than 0.1 ng/mL) for a minimum of 7 years (range 7-18 years) after RP, were considered to have no evidence of disease (NED). Patients with advanced disease (ADV) were defined as either having radiographic evidence of metastatic disease at the time of diagnosis of adenocarcinoma of the prostate or having biochemical recurrence (defined as two consecutive rises in PSA > 0.2 ng/mL in a patient who previously had a RP and an undetectable PSA), after primary curative therapies for adenocarcinoma of the prostate.

Enrichment of DTC from the BM of PCa patients

All materials were acquired and used conforming to IRB-approved protocols at the University of Washington. DTC were isolated from BM samples of PCa patients as previously reported [13]. Briefly, ten ml of BM was aspirated from the posterior iliac crest into a 30 ml syringe containing 10 ml of 6% sodium citrate under local anesthesia. Processing of samples commenced within 1–2 hours and was completed within 5 hours. BM aspirates were separated using 15 ml of Ficoll-Isopaque (1.077 g/ml) (Accurate Chemical, Westbury, NY). Centrifugation yielded a mononuclear cell layer containing DTC, which underwent immunomagnetic selection with the MACS system (Miltenyi Biotec, Auburn, CA). Anti-CD45 and anti-CD61 antibodies were used first for negative selection to eliminate leukocytes, megakaryocytes, and platelets. Positive selection was then performed with immunomagnetic beads coated with anti-human epithelial antigen (HEA) antibodies to target epithelial cells.

Isolation of individual DTC

For identification and isolation of DTC, the enriched population was subjected to immunostaining with fluorescein isothiocyanate labeled anti-BerEP4/EpCAM antibodies (Dako, Carpinteria, CA), which bind a different epitope on HEA than the anti-HEA antibody used for positive selection. A phycoerythrin conjugated anti-CD45 antibody was also added for identification of leukocytes. EpCAM+/CD45- cells were kept on ice, viewed under fluorescent light, and intact cells with a clearly defined EpCAM labelled membrane were isolated using a micromanipulator. Based on historic testing of this method using the trypan blue exclusion assay, DTC picked at this stage of isolation are viable. Individual cells were lysed with 2 µl of WT-Ovation™ One-Direct Amplification System (NuGEN) lysis buffer and stored at −80oC for gene expression profiling.

Amplification of total RNA from individual DTC

Total RNA was amplified from each sample using the WT-Ovation™ One-Direct Amplification System (NuGEN) according to the manufacturer’s directions. The use of an aluminum cooling block on ice facilitated the handling of the reaction tubes. The amplified cDNA products passed the purity test of showing Abs260/Abs280 ratios between 1.9 to 2.0, and a subset was analyzed on an Agilent Bioanalyzer using the RNA 6000 Pico LabChip with the mRNA Pico program to assess size distribution as previously described [13]. Post-SPIA modification and post-amplification work was performed in a separate workspace.

Labeling and hybridization of amplified material on Agilent chips

Amplified cDNA from each sample were labeled using the BioPrime® Total Genomic Labeling System (Invitrogen™). Hybridization probes were prepared by combining 6 mg of Alexa Fluor® 3 labeled sample and 1 mg Alexa Fluor® 5 labeled reference and denatured at 95°C and hybridized at 63°C on Agilent Human 4x44K microarrays and processed following the manufacturer’s specifications. Arrays were scanned on an Agilent DNA Microarray Scanner [13].

DTC Selection

We analyzed DTC from 5/9 NED patients. The remaining 4 patients all had DTC, but had too few to move forward and analyze. These samples were not processed as our goal was to obtain approximately 10 cells/patient to analyze tumor cell heterogeneity, whereas these patients only had 1-4 cells. We analyzed DTC from 6/8 ADV sampled patients. The DTC isolated from one patient were of poor quality, the other patient had no DTC observed in the bone marrow sample.

Gene expression analysis

Data were loess normalized within arrays and quantile normalized among arrays in R using the Limma Bioconductor package. Samples with poor microarray hybridization signals were removed. Data were filtered to remove probes with mean signal intensities below 300. The Statistical Analysis of Microarray (SAM) program (http://www-stat.stanford.edu/~tibs/SAM/) was used to analyze expression differences between groups. Unpaired, two-sample t-tests were calculated for 11202 unique genes passing filters and controlled for multiple testing by estimation of q-values using the false discovery rate (FDR) method. Microarray data are deposited in the Gene Expression Omnibus database under the accession number GSE48995. To determine whether transcriptomic differences observed in ADV versus NED groups were enriched for genes within canonical pathways and Gene Ontology gene sets, the t-test results were subjected to Gene Set Enrichment Analysis (GSEA) using preranked mode with permutation testing of the gene sets to adjust for multiple hypothesis testing, generating an FDR. Global unsupervised, hierarchical clustering analysis was performed with the top 5000 most variable genes among all samples as determined by inter-quartile range (IQR). Unsupervised, hierarchical clustering of the top and bottom 50 most differentially expressed between NED and ADV groups based on SAM score identified subgroups ADV_1 and ADV_2. Erythroid progenitor-like and prostate enrichment scores were calculated using the Gene Set Variation Analysis (GSVA) Bioconductor package in R [33].

Ingenuity Pathway Analysis

The top and bottom 50 most differentially expressed genes (total 100 genes) between NED, ADV, ADV_1 and ADV_2 groups were imported into Ingenuity Pathway Analysis (IPA, Ingenuity Systems; https://www.ingenuity.com) to identify biological pathways involved in different groups of DTC. IPA is a repository of biological interactions and functional annotations to demonstrate relationships between proteins, genes, complexes, metabolites, and drugs. The IPA knowledge library includes information from NCBI databases (EntrezGene, RefSeq, OMIM disease associations), microRNA-mRNA target databases, GWAS (Genome Wide Analysis Study) databases, and Kyoto Encyclopedia of Genes and Genomes (KEGG).

Analysis of DTC expression profiles for the presence of a p38α/β-regulated dormancy signature

For the p38α/β dormancy-associated signature identified in the IPA, the enrichment for dormancy upregulated or downregulated genes for each DTC was calculated. Specifically, the percent of dormancy upregulated genes that were also upregulated in the DTC was scored as the percent coverage of dormancy UP genes induced for each individual DTC. The same was applied to the downregulated genes in the above-mentioned signature. Cutoffs were the same as those used for all normalization analysis. In all cases, differences in means were estimated using a linear regression model and statistical significance was evaluated using t-tests of appropriate model coefficients. For the previously identified tumor dormancy-associated signature, expression profiles of the NED, ADV, ADV_1 or ADV_2 subgroups of DTC were parsed for the genes upregulated and downregulated in a previously published tumor dormancy gene signature of 19 upregulated and 21 downregulated genes linked to p38α/β activation in a head and neck squamous cell carcinoma (HNSCC) model [16, 25, 31] or to BMP7 signaling in a PCa model [18]. The latter signature only added BMP7. This signature was expanded to incorporate an additional 7 genes that have been linked to in vivo quiescence of dormant HNSCC cells (Aguirre-Ghiso et al., unpublished). The percent of upregulated genes in the signatures that were also upregulated in the DTC was scored as the percent coverage of dormancy UP genes induced for each individual DTC. The same was applied to the downregulated genes in the above-mentioned signatures. Cutoffs were the same used for all normalization analysis. For example, when 26 of the genes upregulated in the expanded signature (19+7 genes induced in the HNSCC and PCa model) were all upregulated in an individual DTC, that DTC was scored as having 100% of coverage of the dormancy UP genes. The same was applied for downregulated genes. In all cases, differences in means were estimated using a linear regression model and statistical significance was evaluated using t-tests of appropriate model coefficients.

Acknowledgements

We would like to thank the patients who donated BM aspirates that made this work possible. These studies were supported by resources from NIH RC1 CA144825 ARRA Challenge, Janssen Research and Development LLC, NIH PO1 CA85859, U01 CA164188, the PNW Prostate Cancer SPORE NIH P50 CA097186 to P.S.N., and Samuel Waxman Cancer Research Foundation Tumor Dormancy Program NIH CA109182 and NIH CA163131 to J.A.A-G. H.M.L. is a recipient of a Young Investigator Award from Prostate Cancer Foundation and a Career Development Award from NIH Pacific Northwest Prostate Cancer SPORE. This material is also the result of work supported by resources from the VA Puget Sound Health Care System, Seattle, Washington (R.L.V is a research career scientist, P.H.L is a staff physician).

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