The therapeutic efficacy of I¹³¹-PSCA-mAb in orthotopic mouse models of prostate cancer

Prostate cancer is one of the most frequently diagnosed malignancies worldwide and has become one of the leading causes of cancer-related death in men, only behind lung cancer [1, 2]. Some patients with metastatic disease die within 2–3 years of diagnosis, whereas others with organ-confined disease can live for 10–20 years, which indicates that prostate tumors might have tremendous genomic diversity [3].

Androgens could contribute to the initial growth of prostate cancer [4]. In 1941, Huggins and Hodges successfully applied androgen deprivation therapy (ADT) by the injection of estrogens in metastatic prostate cancer patients in the form of surgical castration [5, 6]. Within 1–2 years after initial response, progression of prostate cancer typically occurs; ADT could be considered as the treatment of choice for patients with advanced metastatic prostate cancer [7, 8]. However, most prostate tumors ultimately progress to hormone-resistant prostate cancer (HRPC), which is androgen-independent growth, and resistance inevitably occurs within a few years, while antiandrogen therapy is initially effective [9]. Though early detection and treatment have improved significantly, biochemical recurrence might happen to almost 40% of men after radical retropubic prostatectomy [10]. The clinical manifestations of HRPC include increased concentrations of prostate serum antigen (PSA), bone metastases, soft-tissue/lymph node metastases and substantive pain [11].

Prostate stem cell antigen (PSCA) belongs to the Thy-1/Ly-6 family of the glycosylphosphatidylinositol-anchored cell membrane glycoprotein, which can overexpress in prostate cancer tissues [12]. Although PSCA expression has been detected in all stages of prostate cancer, the increased expression level of PSCA is positively correlated with biochemical recurrence, advanced stage, transition to the castration-resistant state and metastatic progression [13‐16]. Ahmad et al. reported that a plasmid-based vaccine against PSCA may have the potential to be used in multimodal treatment programs for prostate cancer [17]. Saffran et al. found that administration of anti-PSCA mAbs could inhibit metastasis to distant sites and restrain the growth of established orthotopic tumor, which could significantly prolong the survival time of tumor-bearing mice [18]. However, the therapeutic outcomes using anti-PSCA mAbs for prostate cancer patients are very poor and limited. There are few studies on radioimmunotherapy guided by anti-PSCA mAbs for prostate cancer. The interesting area indicating the region of interest has been used in many surveillance systems, such as medical image processing [19].

In this study, anti-PSCA mAbs labeled with I¹³¹ (I¹³¹-PSCA-mAb) were made to investigate the potential therapeutic efficacy of I¹³¹-PSCA-mAb for prostate cancer. The proliferation abilities, apoptosis and invasion abilities of PC-3 and LNCaP cells treated with I¹³¹-PSCA-mAb in vitro were measured by methyl thiazolyl tetrazolium (MTT) assay, flow cytometry and transwell culture, respectively. Furthermore, human prostate cancer xenograft nude mice models were established by injection of androgen-dependent LNCaP cells and androgen-independent PC-3 cells. The distribution and variation of I¹³¹-PSCA-mAb in the tumor-bearing nude mice over time were measured by single-photon emission computerized tomography (SPECT) and the ROI method. Tumor cell apoptosis was detected by the terminal-deoxynucleotidyl transferase-mediated nick end labeling (TUNEL) technique.

PSCA is an ideal candidate for the detection or immunotherapy of prostate cancer because it has increased expression specificity for prostate cancer and has a specific cell surface location [12, 20, 21]. Radioimmunotherapy (RIT) uses monoclonal antibodies against tumor-specific antigens in conjunction with a particle-emitting radioisotope to deliver cytocidal ionizing radiation directly to the tumor [22]. In our study, the potential therapeutic efficacy of anti-PSCA mAbs in conjunction with I¹³¹ for prostate cancer was evaluated. We found that I¹³¹-PSCA-mAb showed great advantages in radioimmunotherapy and stronger positive anti-prostate tumor activity compared with I¹³¹-IgG and PSCA-mAb. Therefore, I¹³¹-based elimination of PSCA-producing cells seems to be a more efficient therapeutic method.

The immunotherapeutic efficacy of PSCA-mAb has been investigated by many studies considering PSCA as a putative target in a prostate cancer model, and the results of these studies have indicated that anti-PSCA antibodies have potential therapeutic roles for the treatment of prostate cancer [21, 23]. In our study, we found that PSCA-mAb could inhibit the growth, apoptosis and migration of PC-3 and LNCaP cells to some extent. Therefore, these results are consistent with previous reports on anti-PSCA-based immunotherapy. RIT, which can target the corresponding antigens via binding radionuclides to antibodies, has a promising role in the treatment of metastatic melanoma, ovarian cancer and metastatic colorectal cancer [24‐26]. The characteristic and complex interactions among the tumor, host, antigen-antibody complex and radionuclide determine the effectiveness of RIT [27]. In this study, the inhibitory and apoptosis rates of PC-3 and LNCaP cells treated with I¹³¹-PSCA-mAb reached up to the maximum of 84%, 80% and 50%, 46%, respectively, which were obviously higher than in the cells treated with I¹³¹-IgG or PSCA-mAb. Therefore, I¹³¹-PSCA-mAb could effectively inhibit the proliferation of cancer cells and promote the apoptosis of cancer cells. Compared with the control group, the number of invaded PC-3 and LNCaP cells treated with I¹³¹-PSCA-mAb was significantly reduced, which indicated that the invasion abilities of tumor cells were significantly reduced by I¹³¹-PSCA-mAb.

Furthermore, the ratios of I¹³¹-PSCA-mAb in tumor to intramuscular I¹³¹-PSCA-mAb (T/NT) in androgen-independent and -dependent tumor-bearing nude mice increased with time, which demonstrated that I¹³¹-PSCA-mAb-targeted radioimmunotherapy may have few or minimal undesired toxic effects on the other tissues. The T/NT stayed above 3.0 after 12 h, and the tumor could still be observed after 24 h. Therefore, guided treatment for prostate cancer could be precisely conducted. What is more, the number of apoptotic cells in androgen-independent or -dependent nude mice treated with I¹³¹-PSCA-mAb was larger than that in the control group. That is to say, I¹³¹-PSCA-mAb-targeted radioimmunotherapy could effectively promote cancer cell apoptosis in tumor-bearing nude mice. However, PSCA-mAb might not be able to specifically target non-PSCA-expressing tumor cells. Therefore, the applicability of I¹³¹-PSCA-mAb treatment in humans needs to be further explored.

In conclusion, I¹³¹-PSCA-mAb has the potential to become a new targeted therapy drug for the radioimmunotherapeutic treatment of prostate cancer because it exhibited good targeting ability and efficacy and few side effects in nude mice models of human prostate cancer. We optimistically anticipate that I¹³¹-PSCA-mAb can be applied in clinical therapy.

Shengqiang Yu and Fan Feng, the first two authors, should be regarded as joint first authors.