Background
Nowadays breast cancer is becoming the second leading cause of cancer deaths in females, almost 10% women have the risk of developing breast cancer [
1]. Although great improvements have been made in curing breast cancer, the overall five-year survival rate remains < 50% and many patients relapse after surgical resection because of the dispersion of undetectable cancer cells [
2,
3]. Therefore, it is necessary to establish sensitive and specific techniques for the detection of occult tumor cells. A better method for early diagnosis may help in predicting recurrence and planning appropriate therapies to improve survival [
4,
5].
Many investigations have indicated that epithelial cells from the initial tumor can be recognized in peripheral blood or bone marrow aspirates of patients with breast cancer [
6,
7]. The detection of circulating tumor cells (CTCs) in the peripheral blood of cancer patients has been associated with recurrence and metastasis of breast cancer [
8‐
10]. Cytokeratins (CKs), characteristic intermediate filament of epithelial cells, especially CK19, are widely used to detect tumor cells derived from epithelial tissues [
11,
12]. CK19 has been shown to correlate with poor clinical outcome for patients with breast cancer [
13].
Flow cytometry is a technology which can not only give information of high statistical precision and subpopulation quantification but also analyze cells individually and rapidly, compared with immunocytochemistry [
14,
15] and reverse transcriptase polymerase chain reaction (RT-PCR) [
16,
17]. In this study, flow cytometry was used to detect occult tumor cells in peripheral blood of patients with breast cancer. The detection of CTCs in peripheral blood of 48 patients was intended to find the relationship of CK19
+ cell percentage with disease progress. CK19 was positive in the peripheral white blood cells of breast cancer patients at stages II to IV, but not the patients at stage I and healthy controls. The percentage of CK19
+ cells was increased following the severity of the disease and decreased after lumpectomy and chemotherapy.
Methods
Cell line
The A431 (human epithelial carcinoma) cell line obtained from the American Type Culture Collection was grown in Dulbecco's modified Eagle's medium (DMEM) supplemented with 15% fetal calf serum (both from GIBCO), 100 U/ml penicillin, and 100 μg/ml streptomycin at 37°C in a humidified incubator with 5% CO2. Subculture was performed when confluence reached 70%.
Patients
Breast cancer patients were treated at the Affiliated Hospital of Anhui Medical University. The cohort included 7 patients with benign tumor, 34 patients with primary breast cancer and 7 patients with metastatic breast cancer from October 2006 to April 2008. The patients underwent lumpectomy except those with distant metastases. And we detected CK19 expression of 15 patients with primary breast cancer during three month chemotherapy. Blood samples were obtained with informed consent after approval of the protocol by the Ethics Committee of the University of Science and Technology of China. Control blood samples were collected from 25 healthy female volunteers.
Blood sample preparation
The first 8 ml of blood was discarded to avoid epithelial contamination before the collection of 5 ml blood sample. Human white blood cells were isolated from adult peripheral blood using RBC lysis buffer (RX-2-1-2 U-gene China). Briefly, 3 ml blood and 15 ml RBC lysis buffer were mixed with vortex and kept on ice for 15 min until pellucid, then were centrifuged at 450 g for 10 min. Cells were suspended with 5 ml RBC lysis buffer and centrifuged at 450 g for 10 min again followed by twice rinse with PBS.
Immunofluorescence staining
A431 cells were counted onto glass slides at a concentration of 5 × 105 cells per spot. Subsequently, the cells were fixed with 4% paraformaldehyde in PBS for 15 min at room temperature, rinsed in PBS, and incubated with FITC-conjugated mouse anti-human CK19. Laser scanning confocal microscopy was performed and the data were processed with MetaMorph program.
Flow cytometric analysis
After fixation with 1% paraformaldehyde for 1 hour at room temperature, A431 cells or leukocytes were permeabilized with 0.01% Triton X-100 for 1 h at room temperature followed by mouse serum block (30 min, room temperature). Then the cells were incubated with FITC-conjugated CK19 antibody or FITC-mouse IgG1 isotype antibody (both from BD PharMingen) as negative control overnight. After washed twice with permeabilization buffer, samples were analyzed by FACSCalibur (Becton Dickinson).
Statistical analysis
K Related Samples Test was used for the analysis of CK19 expression in peripheral blood of patients before and after clinical treatment. Mann-Whitney U test was used to compare CK19 expression levels in peripheral blood between patients at stage III and stage IV. The statistical significance was defined as values of p < 0.05.
Discussion
The dispersion of tumor cells is one of the primary causes of recrudescence at distant sites and of death from cancer. So the detection of occult metastatic cells is important to predict recurrence and improve survival. In this study, we applied flow cytometry to examine the expression of CK19 in the peripheral blood of breast cancer patients to monitor CTCs.
Immunocytochemistry gives morphological detail of tumor cells but is not sensitive and lack of methodological standardization [
18]. Although RT-PCR is able to find 1 cancer cell among 10
6 irrelevant cells [
19], it cannot exactly quantify the number of tumor cells according to mRNA levels. Furthermore, its utility was limited for its low specificity because of the false positive results which may be explained by the phenomenon of "illegitimate expression" [
20,
21].
In the present study, flow cytometry is utilized to examine the expression of CK19 to test CTCs in 48 breast cancer patients because most breast cancer cells but not blood cells express CK19. Although the sensitivity of our method is 1 cancer cell among 10
4 irrelevant cells, its specificity is very high. No CK19 expression was detected in healthy volunteers and patients with benign tumor. We consider high specificity is more important than high degree of sensitivity for clinical diagnoses because a wrong positive test will result in unnecessary treatments that may cause injury. Our data demonstrated that 86% of stage IV patients and 70% of stage III patients were detected CK19
+ cells in the peripheral blood, which were a little higher than that reported by Aerts J [
22]; but the percentage of patients at stages I and II was lower. This may be explained by that the detection of protein level is more precise than RNA level because of the false positive result of RT-PCR also reported by others [
23]. In our study the percentages of CK19
+ cells in the peripheral blood samples of patients were increased as the illness grew worse. This result was similar with that of Ivy Wong and his group that positive expression level of CK19 correlates strongly with disease stage in colorectal cancer [
24]. Moreover, most patients positive for CK19 had a tumor size of more than 2 cm. It was also mentioned by Weihrauch that CK19 detection rate increased with tumor size [
25]. However, Xenidis N and his colleagues found the presence of CK19 positive cells had nothing to do with clinicopathological prognostic factors [
26].
After a follow-up period of three month-chemotherapy, the number of occult tumor cells in most metastatic patients was decreased rapidly, convincing the effect of adjuvant chemotherapy. In another hand, this can also be considered that most CTCs are apoptotic [
27] so they vanished automatically. However, 2 patients with no metastasis before operation had CK19 positive cells after chemotherapy. It may be explained by that chemotherapy may evoke the exudation of proinflammatory cytokines which can regulate gene expression [
28]. The tumor cells of one patient vanished after durative chemotherapy, but for the other patient they increased during this treatment. This phenomenon indicates that some tumor cells are sensitive to chemotherapy but others are resistant to it.
In conclusion, we have established a simple method for the test of CTCs in peripheral blood. Despite its sensitivity seems not as high as PCR, the specification and quantification accuracy is encouraging. Our technique can also be applied for bone marrow metastasis investigation. Many groups have reported the relationship of CK19+ cells with reduced overall survival and risk of distant relapse. The detection of CTCs by flow cytometry in breast cancer may monitor disease progression and be helpful in the selection of patients who have the risk of relapse after adjuvant treatment.
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
LW performed the laboratory assays and drafted the manuscript. YW carried out the statistical analysis and revised the manuscript. MC conceived of the study and participated in its coordination. YL contributed to cell culture, image treatment and manuscript revision. XW participated in the use of LSCM. HW was the principal investigator of the study. All authors read and approved the final manuscript.