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Imaging, Diagnosis, Prognosis

Prognostic Value of Preoperative Serum Cell-Free Circulating DNA in Men with Prostate Cancer Undergoing Radical Prostatectomy

Patrick J. Bastian, Ganesh S. Palapattu, Srinivasan Yegnasubramanian, Xiaohui Lin, Craig G. Rogers, Leslie A. Mangold, Bruce Trock, Mario Eisenberger, Alan W. Partin and William G. Nelson
Patrick J. Bastian
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Ganesh S. Palapattu
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Srinivasan Yegnasubramanian
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Xiaohui Lin
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Craig G. Rogers
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Leslie A. Mangold
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Bruce Trock
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Mario Eisenberger
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Alan W. Partin
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William G. Nelson
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DOI: 10.1158/1078-0432.CCR-06-2781 Published September 2007
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Abstract

Purpose: We evaluated the association of preoperative serum cell-free circulating DNA concentration in men with clinically localized prostate cancer who underwent radical prostatectomy with prostate-specific antigen (PSA) recurrence.

Experimental Design: One hundred and ninety-two men with clinically localized prostate cancer, who underwent radical prostatectomy at the Johns Hopkins Hospital and had preoperative serum available for analyses constituted our study population. All serum samples were collected before prostate biopsy or at least 4 months after prostate biopsy. The total amount of serum cell-free circulating DNA from each sample was calculated using a standard curve generated via quantitative real-time PCR. PSA recurrence was defined as a single postoperative PSA level of ≥0.2. The natural logarithm (ln) of the DNA concentration was used for statistical analyses.

Results: Of the 192 men in our study, 56 (29%) experienced PSA recurrence within the study period (median time to PSA recurrence 2 years). The median follow-up time for men free of disease at last follow-up was 3 years. The median serum cell-free DNA concentration of all men in the study was 5.3 ng/mL (mean 18.05 ng/mL; range 0.2-320 ng/mL). The mean serum DNA concentration for men who recurred and for those who did not was 3.8 ± 34.1 and 13.7 ± 33.6 ng/mL, respectively (P = 0.001). In a univariate analysis, ln DNA concentration was significantly associated with PSA recurrence (hazard ratio, 1.49; 95% confidence interval, 1.3-1.8; P < 0.001). In the multivariate model, ln DNA concentration was significantly associated with PSA recurrence (hazard ratio, 2.56; 95% confidence interval, 1.1-1.6; P = 0.003). Using bootstrap analyses, serum cell-free DNA concentrations ≥5.75 ng/mL were associated with an increased risk of PSA recurrence within 2 years of radical prostatectomy.

Conclusion: Our study suggests that preoperative serum cell-free DNA concentration may be a useful prognostic biomarker for men with clinically localized prostate cancer treated with radical prostatectomy.

  • prostate cancer
  • cell free DNA
  • biomarker
  • hypermethylation
  • serum
  • PSA recurrence

Prostate cancer is the most commonly diagnosed solid organ malignancy among men in the United States, with an estimated 244,000 new cases that will be diagnosed in 2006 alone (1). Primary therapy in the form of radical prostatectomy is one of the principal treatment modalities available for men with clinically localized disease. Approximately two thirds of patients treated with curative intent by surgery will remain disease free 15 years after radical prostatectomy (2). Men who experience early prostate-specific antigen (PSA) recurrence, particularly within the first 2 years of surgery, are likely to develop metastatic lesions and are prone to die because of prostate cancer (3, 4). Besides the commonly accepted risk factors for high-risk disease (i.e., biopsy Gleason sum 8-10, positive lymph nodes, and preoperative PSA >20 ng/mL; ref. 5), no established pretreatment laboratory test exists to identify men at risk for early disease progression after radical prostatectomy. A preoperative test that potentially identifies patients at risk for early PSA relapse postsurgery would be an important tool in the process of treatment planning.

The development of traditional tumor markers has been accelerated by the recent introduction of novel technologies that can quantify small amounts of circulating proteins that are relatively specific for a certain type of cancer. The shortcomings of these methods, such as limited sensitivity and specificity, are well established (6). PCR-based methods have the ability to detect extremely minute amounts of nucleic acids and offer new molecular targets for the development of cancer biomarkers.

The presence of cell-free DNA and RNA in plasma/serum of cancer patients was described as early as the late 1970s (7, 8), but it was not until 1989 that the characteristics of plasma/serum DNA in cancer patients was recognized (9). In addition to quantitative changes, qualitative changes such as microsatellite alterations, decreased strand stability, and mutations have been shown in plasma or serum DNA in the cancer state (9–11). Although the clinical relevance of circulating cell-free DNA has not been completely elucidated, tumor-derived changes in circulatory nucleic acids may offer promising alternatives for cancer screening, detection, and treatment monitoring (12).

Despite the high prevalence of prostate cancer, there is little information on cell-free circulating DNA in the serum or plasma of prostate cancer patients. A recent analysis revealed limited use for cell-free circulating DNA derived from plasma in patients with metastatic prostate cancer as a biomarker of metastatic disease compared with serum PSA level (13). In addition, a recent report established reference ranges of cell-free circulating DNA in various types of cancer, but no correlation of cell-free circulating DNA in nonmalignant prostatic diseases as well as with clinical outcome was done (14).

Using a standard quantitative PCR, we sought to further characterize total cell-free circulating DNA, not specifically cancer nor specific gene DNA, in the preoperative serum of men with prostate cancer and to determine its association with PSA progression in men with clinically localized disease after radical prostatectomy.

Materials and Methods

Sample collection and DNA isolation. All serum samples were collected before or at least 4 months after prostate biopsy and stored at −80°C. All serum samples were stored on ice between the blood draw and further processing, which was done immediately afterward. Clotting of serum samples was allowed for 30 min on ice before centrifugation (1,800 × g, for 10 min). The study cohort consisted of 192 men who underwent radical prostatectomy at The Johns Hopkins Hospital for localized prostate cancer between 1990 and 2004 (Table 1 ). DNA was extracted from 600 μL of archived serum from each patient using the Qiagen Blood Mini Kit and diluted in a total volume of 25 μL. Thirty-five men without evidence of cancer on prostate biopsy served as a control population. Sera from 18 men with metastatic prostate cancer were also examined.

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Table 1.

Patient characteristics of 192 men with clinically localized prostate cancer treated with radical prostatectomy

The primary end point of the study was PSA recurrence, which was defined as a single postprostatectomy PSA level of ≥0.2 ng/mL. Routine PSA follow-up consisted of assessment at 3 months postoperatively and annually thereafter. All of the men studied had an undetectable serum PSA level 3 months after radical prostatectomy. All studies were conducted with the approval of the Institutional Review Board and Health Insurance Portability and Accountability Act compliance.

Quantitative real-time PCR. Quantitative real-time PCR was done with primers flanking the promotor regions of three separate genes: GSTP1, MDR1, and EBNRB. All PCR reactions were carried out in an iCycler real-time thermal cycler (Bio-Rad) using specific primer sets [GSTP1: 5′ primer: ACTCACTGGTGGCGAAGACT; 3′ primer: GACCTGGGAAAGAGGGAAAG (15); MDR1: 5′ primer: AAACCGTAGTGGCACTGGACCAT; 3′ primer: AGCATCTCCACGAAGGCAGAGTT; EDNRB: 5′ primer: ATTCTCGCAGCGTTTCGT; 3′ primer: CGCGATTGAACTCGAAAGAC]. PCR conditions were set as follows: 95°C for 15 min followed by 45 cycles of 94°C for 30 s, 60°C for 30 s, and 72°C for 45 s. The within-run and between-run imprecisions for a DNA template were 2.9% and 6.8%, respectively. Calibration curve analysis was done after each PCR. PCR was accomplished using a 25 μL reaction mixture, consisting of 4 μL template DNA, 100 nmol/L of forward and reverse primer, and 12.5 μL of a 2× Sybr Green PCR Master Mix (Qiagen). In each reaction set, WBC DNA, the standard DNA (human male genomic DNA, Novagen), commercially available and not self-prepared (Novagen), served as a positive control; water served as negative controls. Each reaction was done in triplicate. A 10-fold dilution series of known DNA concentrations was used to generate a standard curve (100-0.001 ng). The total amount of DNA from each sample was calculated using this standard curve. All three assayed genes (i.e., GSTP1, MDR1, and EBNRB) are present in the genome of all cells.

All samples were tested for GSTP1 CpG island hypermethylation and the total amount of cell-free circulating serum DNA using the three mentioned primer sets. The GSTP1 CpG island hypermethylation was studied previously and the results of this analysis were included into the statistical analyses (categorical; ref. 16). We used the previously described restriction enzyme–quantitative PCR method to detect GSTP1 CpG island hypermethylation (17). This method allows the quantification of the amount of total DNA and methylated DNA in each sample and is able to detect as few as one methylated GSTP1 allele. Briefly, DNAs extracted from serum samples were subjected to restriction enzyme digestion with HpaII (NEB). HpaII cuts the sequence CCGG, but does not cut the methylated form of this sequence, C5mCGG. If the CpG island does not contain C5mCGG, the DNA is cut and no product can be detected after PCR amplification. Typically, 4 μL of DNA were incubated at 37°C for 5 h with 60 units of restriction enzyme, 2 μL of 10× restriction enzyme buffer (NEB), and the appropriate amount of DNase-free water to give a final reaction volume of 20 μL. To ensure complete digestion, an additional 30 units of restriction enzyme, 1 μL of restriction enzyme buffer, and 6 μL of DNase-free water were added to each reaction and incubated at 37°C overnight. As individual sample controls, PCR amplification was done on undigested DNA and DNA digested with the restriction enzyme MspI (NEB) using the above protocol. MspI cuts both the unmethylated and methylated sequence; thus, no PCR product should be detected. All PCR reactions were carried out in an iCycler real-time thermal cycler (Bio-Rad) using a specific primer set (5′ primer: ACTCACTGGTGGCGAAGACT; 3′ primer: GACCTGGGAAAGAGGGAAAG) that brackets six HpaII/MspI recognition sites (15). PCR conditions were set as follows: 95°C for 15 min followed by 45 cycles of 94°C for 30 s, 60°C for 30 s, and 72°C for 45 s. Calibration curve analysis was done after each PCR. PCR was accomplished using a 25 μL reaction mixture, consisting of 4 μL template DNA, 100 nmol/L of forward and reverse primer, and 12.5 μL of a 2× Sybr Green PCR Master Mix (Qiagen). In each reaction set, restriction enzyme–treated universally methylated DNA (Chemicon) served as a positive control and restriction enzyme–treated WBC DNA and a water blank served as negative controls. Each reaction was done in duplicate.

Statistical analysis. The natural logarithm (ln) of the DNA concentration was used for statistical analyses. Univariate comparisons between recurrent and nonrecurrent patients consisted of χ2 or Fisher's exact tests for categorical variables, and t tests for continuous variables. Hazard ratios and 95% confidence intervals were adjusted for multiple prognostic factors using the Cox proportional hazards model. Models were developed in a manual hierarchical approach, based on the likelihood ratio test and changes in the magnitude of hazard ratios. The effect of the ln of total DNA concentration on recurrence-free survival was evaluated using the proportional hazards model. The serum GSTP1 hypermethylation status was coded as a categorical variable in this analysis. The optimal cut point for total DNA in the multivariable model was chosen using the minimum P value method with bootstrap resampling to correct for overfitting (18). For the multivariate analysis, we used the significant variables from the univariate model: total DNA level, surgical margin status, and lymph node status. A variable “DATA” was included into the multivariate model to correct for the fact that the cohort consisted of 55 matched pairs (110 patients) that have a much higher “recurrence rate” compared with the remaining 85 patients (consecutive patients) because recurrent patients were matched to nonrecurrent patients (based on pathologic Gleason score). Three patients were part of both cohorts, so the total cohort consisted of 192 patients. The concordance index was estimated using the modification for censored data, and was calibrated using bootstrap resampling (19). ANOVA was used to compare mean ln(DNA) levels among the four disease progression groups. Results are expressed as geometric means of DNA levels.

Results

Detection of cell-free circulating DNA and association with established prognostic features. The median serum cell-free DNA concentration of all men in the study was 5.3 ng/mL (mean 18.05 ng/mL; range 0.2-320 ng/mL). Table 2 shows the concentrations of cell-free circulating DNA detected with the GSTP1 primer set. Mean levels of cell-free circulating DNA were similar for the three different primer sets (i.e., GSTP1, MDR1, and EDNRB; Figs. 1 and 2 ). Therefore, the calculated total DNA concentration based on the primer set for GSTP1 PCR was used for statistical analysis. Total DNA levels were higher in association with each adverse prognostic feature (Table 2). Significant associations were observed for biopsy Gleason score, prostatectomy Gleason score, surgical margin status, organ-confined status, and extraprostatic extension in relation to total serum cell-free DNA concentration.

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Table 2.

Association cell-free circulating cancer DNA and established pathologic factors (GSTP1 primer set)

Fig. 1.
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Fig. 1.

Cell-free circulating serum DNA levels were determined as described in Materials and Methods by quantitative real-time PCR using primer sets for GSTP1 (A), MDR1 (B), and EDNRB (C). Mean levels of cell-free circulating DNA were similar for the three different primer sets. PCA, prostate cancer.

Fig. 2.
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Fig. 2.

Correlation plot revealing the degree of correlation in DNA levels in serum measured with GSTP1, MDR1, and EDNRB.

Of the 192 men in our study, 56 (29%) experienced PSA recurrence within the study period (median time to PSA recurrence 2 years, mean 4 years, range 1-14 years). The median follow-up time for men free of disease at last follow-up was 3 years (mean 3 years, range 1-7 years).

Association of cell-free circulating DNA levels with disease progression. The mean concentration of cell-free circulating DNA in patients without PSA recurrence (n = 136) and in patients with PSA recurrence (n = 56) was 3.8 ± 33.6 and 13.7 ± 34.1 ng/mL (P = 0.001), respectively. Univariate analysis with respect to PSA progression after radical prostatectomy revealed a hazard ratio of 1.49 (95% confidence interval, 1.3-1.8; P < 0.001; Table 3 ). The optimal calculated cut point for total preoperative cell-free circulating cancer DNA content with regard to PSA recurrence after radical prostatectomy was 5.75 ng/mL (ln 1.75 ng/mL) with a concordance index of 0.762 (also see Fig. 3 ).

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Table 3.

Univariate model with respect to PSA progression

Fig. 3.
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Fig. 3.

Kaplan-Meier analysis cell-free circulating DNA in association with early PSA recurrence after radical retropubic prostatectomy for prostate cancer. The optimal calculated cutpoint for total preoperative cell-free circulating cancer DNA content with regard to PSA recurrence after radical prostatectomy was 5.75 ng/mL (ln 1.75 ng/mL) with a concordance index of 0.762.

Multivariable analysis incorporating the most powerful predictors of PSA recurrence. The multivariate model of the study cohort (n = 192) accounted for lymph node status, surgical margin status, biopsy and pathologic Gleason score, and pathologic stage. Because the univariate analyses revealed similar results for all three primer sets, only the GSTP1 primer set was used in the analyses. In the multivariate Cox proportional hazard model, the total amount of cell-free circulating DNA was almost as predictive for PSA recurrence as positive lymph node status at the time of the operation (Table 4 ). The comparison of GSTP1 hypermethylation status and level of cell-free circulating DNA did not reveal a statistically significant relationship (P = 0.21).

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Table 4.

Multivariable model incorporating optimal predictors of PSA recurrence

Comparison of total DNA concentration among disease progression groups.Table 5 shows the concentrations of total cell-free circulating DNA detected for the GSTP1 primer set among disease progression groups. Disease progression groups consisted of patients undergoing prostate biopsies without histologic evidence of disease, patients with localized prostate cancer with or without biochemical recurrence, and patients with known metastatic prostate cancer. The amount of cell-free circulating DNA increased between disease progression groups to a significant extent (P < 0.0001).

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Table 5.

Cell-free circulating DNA (GSTP1) levels among disease progression groups

Discussion

In the present study, we have shown that the content of cell-free circulating DNA, not cancer DNA, is higher in patients with prostate cancer than those with a negative prostate biopsy and that adverse pathologic findings in the surgical specimen are associated with elevated levels of circulating cell-free DNA. Significant associations were observed for biopsy Gleason score, prostatectomy Gleason score, surgical margin status, organ-confined status, and extraprostatic extension. In a multivariate model, the content of cell-free circulating DNA was an independent predictor of early PSA recurrence in patients undergoing radical prostatectomy alone or in combination with other prognostic markers.

These results suggest that the content of cell-free circulating DNA before diagnosis may be a promising independent DNA-based prognostic serum biomarker for prostate cancer.

Presently, the true origin of cell-free circulating DNA is not fully understood. In addition to cell lysis, apoptosis, and necrosis, active DNA release has been advanced as possible sources of cell-free circulating DNA (20–22). Sozzi et al. (23) investigated the source of cell-free circulating DNA in lung cancer patients and concluded that the release of cell-free circulating DNA is not related to tumor necrotic rate or malignant cell proliferation. Active DNA release from fragile cells during the clotting process after blood sampling may be an additional source of serum cell-free circulating DNA (24) although a study by Jahr et al. (21) found this contribution to be negligible. Others, however, have shown that the amount of cell-free circulating DNA can be affected by blood sampling and processing (25, 26). For instance, Lee et al. (25) found that the amount of cell-free circulating DNA in serum significantly increased during longer storage at 4°C. A meticulous study by Jung et al. (27) also showed that preanalytic factors of blood sampling and processing may affect DNA concentrations in serum samples. They compared the influence of time delay in blood processing for plasma and serum samples at room temperature and at 4°C (27). From their analyses, it is obvious that there is a significant difference in the amount of serum DNA due to time delay and storage temperature. Also, Lui et al. (28) showed that the use of different centrifugation speeds (400 × g–16,000 × g) did not significantly alter the median total plasma DNA level in plasma samples. They feared that the use of high-speed centrifugation may destroy blood cells and thus lead to ex vivo release of DNA (28). How that may translate into serum samples remains unclear at this point. However, it is important to notice that not all serum samples can be compared with each other without acknowledging these major issues during the preanalytic sample collecting and preparation. Different DNA extraction protocols may also contribute to the in vitro release of cell-free circulating DNA (29, 30). Interestingly, a recent study by Umetani et al. (31) showed that the higher amount of cell-free circulating DNA in serum compared with plasma is not caused by contaminated extraneous DNA released from leukocytes or other sources during extraction and seems negligible and concluded that serum is the better specimen source for circulating DNA as a biomarker. Their possible explanation for this phenomenon was unequal distribution of DNA during separation from whole blood samples. They measured 6.1-fold more DNA in serum samples compared with plasma samples, which may result from electrostatic forces between DNA that is anionic and platelets that may also be anionic existing only in plasma (31). It is obvious that future studies have to be done to increase our understanding of these complex interactions.

The clearance of blood-borne DNA is also poorly understood. Plasma nucleases as well as hepatic and renal clearance mechanisms may play an important role in clearing the blood of free nucleic acids (32, 33). The half-life of circulating cell-free DNA is reported to be in the order of hours (34, 35).

Circulating DNA-based biomarkers have certain advantages over those using RNA or protein. DNA is more stable experimentally than RNA and is easier than protein to manipulate in the laboratory to identify changes. Multiple studies have shown that the amount of cell-free circulating DNA in the serum differs among normal and cancer patients. In healthy patients, the total amount of cell-free circulating DNA has been shown to be up to 50 ng/mL (14, 36, 37), compared with ∼1,200 ng/mL in samples of patients with different types of cancer (21). Elevated levels of free nucleic acids in cancer patients are thought to originate, in part, from tumor cells. Evidence for this is based on cell-free circulating DNA having similar genetic and epigenetic properties as tumor DNA (16, 38–41). In a recent report by Jung et al. (13), patients with localized prostate cancer were observed to have similar amounts of cell-free circulating DNA in plasma compared with a healthy control group (∼20 ng/mL). Higher levels of cell-free circulating DNA were found in patients with benign prostatic hyperplasia (28.1 ng/mL) as well as in patients with positive lymph nodes (25.8 ng/mL) and distant metastases (41.6 ng/mL; ref. 13). Chun et al. (42) reported on a total of 161 plasma samples from benign prostatic hyperplasia and prostate cancer patients (benign prostatic hyperplasia, n = 19; prostate cancer, n = 142) and found that DNA plasma level is an informative and highly accurate predictor for presence of prostate cancer. However, they do not provide specific information on the sample collection and processing as discussed above. Interestingly, those data are in contrast to the data by Boddy et al. (43), revealing a significantly higher level of plasma DNA in benign prostatic hyperplasia than in prostate cancer patients. However, Boddy et al. used different preanalytic techniques (i.e., centrifugation) that may contribute to their results.

In our study, we found that the total cell-free circulating DNA concentration of patients with localized prostate cancer was 3.8 and 13.7 ng/mL for men without and with PSA recurrence, respectively, after radical prostatectomy. We also noted that the ideal value of total DNA concentration that predicted which men who were destined to biochemically recur post surgery was 5.75 ng/mL.

In men with metastatic prostate cancer, serum PSA level and the amount of plasma DNA have been similarly associated with survival (13). Unfortunately, we were not able to correlate the amount of cell-free circulating DNA in serum with clinical or pathologic information for the subgroup of patients with metastatic disease. However, the amount of cell-free circulating DNA in patients with metastatic prostate cancer was significantly higher compared with men with localized prostate cancer with or without biochemical recurrence. This finding supports the finding by Wu et al. (14) of increased serum tumor markers (PSA in prostate cancer and CA 15-3 in colorectal cancer) in combination with the amount of cell-free circulating DNA in prostate cancer and colorectal cancer patients. Only a low serum tumor marker concentration correlated with the amount of cell-free circulating DNA (14). In our study, we were not able to show correlations of the amount of cell-free circulating DNA with the preoperative serum PSA value (binary or categorical; Table 2).

The group of Allen et al. (44) showed that the total amount of cell-free circulating plasma DNA in patients before and after prostate biopsy was significantly higher in prostate cancer and in benign prostatic hyperplasia 60 min postbiopsy. Interestingly, this increase in cell-free circulating DNA was not detected in PIN cases. They attributed this increase of cell-free circulating DNA to direct cell disruption during biopsy as has been described in a greater scale in trauma patients (45). As mentioned, the serum samples of our cohort were drawn before digital rectal examination or prostatic biopsy and are therefore not subject to these potential confounders.

Interestingly, Sozzi et al. (23) reported that the amount of cell-free circulating DNA in plasma rapidly decreased in patients undergoing lung resection for lung cancer. Furthermore, no increasing level of cell-free circulating plasma DNA in patients with recurrent disease was detected. The authors suggested that the simple quantification of cell-free circulating DNA may serve to monitor patients undergoing surgery or to assess treatment efficacy in lung cancer patients (23). No study on this topic exists for prostate cancer, but we are awaiting results in the very future.

One limitation of our study warrants further discussion. Because sufficient follow-up time has not yet elapsed for the majority of men in the entire cohort, we chose time to PSA recurrence as the end point and not time to metastasis or death. Regardless, PSA recurrence within the first 2 or 3 years of surgery has been associated with a higher probability of developing distant metastasis, a short PSA doubling time, and prostate cancer–specific mortality (4, 46, 47). Also, at this point, it remains unclear whether the amount of cell-free circulating DNA varies between samples drawn from the same patient at different times. Future studies are warranted to further evaluate this issue.

Furthermore, the role of GSTP1 hypermethylation in serum samples of prostate cancer patients warrants discussion. As shown in our previous work, GSTP1 hypermethylation was the strongest predictor of early PSA recurrence after surgical monotherapy. In this study, we compared the results of the GSTP1 hypermethylation with the level of cell-free circulating DNA as a predictor and found that the level of cell-free circulating DNA is almost as predictive as the pathologic lymph node status for PSA recurrence (hazard ratios, 2.56 and 2.85, respectively). Because the true nature of cell-free circulating DNA and cell-free circulating cancer DNA (detected by GSTP1 hypermethylation) remains unknown, future studies are necessary to address these uncertainties. Additionally, we do not know whether any of these markers may predict prostate cancer–specific mortality and need to wait longer follow-up periods. Other studies looking into the detection of tumor-specific DNA in blood from prostate cancer patients have been published and this will be an emerging field with an interesting future (48).

Conclusion

In our study, preoperative serum cell-free DNA concentration was a powerful predictor of PSA progression after radical prostatectomy for localized prostate cancer. Men who experienced biochemical recurrence after prostatectomy had a significantly greater preoperative serum cell-free DNA concentration than those men who were free of disease at last follow-up. If corroborated by other prospective studies, DNA-based biomarkers, such as total DNA amount, may be helpful in identifying men who are most likely to fail after surgery and thus most likely to benefit from adjuvant therapy.

Footnotes

  • Grant support: NIH/National Cancer Institute grant R01 CA70196, NIH/National Cancer Institute Specialized Programs of Research Excellence grant P50 CA58236 and the Early Detection Research Network, a division of the National Cancer Institute (CA86323). ” Work by G.S. Palapattu was supported by the American Foundation for Urologic Disease/American Urological Association Education and Research program.

  • 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.

  • Note: W.G. Nelson has a patent (U.S. patent 5.552.277) titled “Genetic diagnosis of prostate cancer.” Parts of this study were presented at the Annual Meeting of the American Urological Association in Atlanta, May 2006.

  • Received November 27, 2006.
  • Revision received June 17, 2007.
  • Accepted July 11, 2007.

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Clinical Cancer Research: 13 (18)
September 2007
Volume 13, Issue 18
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Prognostic Value of Preoperative Serum Cell-Free Circulating DNA in Men with Prostate Cancer Undergoing Radical Prostatectomy
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Prognostic Value of Preoperative Serum Cell-Free Circulating DNA in Men with Prostate Cancer Undergoing Radical Prostatectomy
Patrick J. Bastian, Ganesh S. Palapattu, Srinivasan Yegnasubramanian, Xiaohui Lin, Craig G. Rogers, Leslie A. Mangold, Bruce Trock, Mario Eisenberger, Alan W. Partin and William G. Nelson
Clin Cancer Res September 15 2007 (13) (18) 5361-5367; DOI: 10.1158/1078-0432.CCR-06-2781

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Prognostic Value of Preoperative Serum Cell-Free Circulating DNA in Men with Prostate Cancer Undergoing Radical Prostatectomy
Patrick J. Bastian, Ganesh S. Palapattu, Srinivasan Yegnasubramanian, Xiaohui Lin, Craig G. Rogers, Leslie A. Mangold, Bruce Trock, Mario Eisenberger, Alan W. Partin and William G. Nelson
Clin Cancer Res September 15 2007 (13) (18) 5361-5367; DOI: 10.1158/1078-0432.CCR-06-2781
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