Mita Yoshiyasu, Ajiki Tetsuo, Kamigaki Takashi, Okazaki Taro, Hori Hiroshige, Horiuchi Hideki, Hirata Kenro, Fujita Tsunenori, Fujimori Takahiro, Kuroda Yoshikazu
Department of Gastroenterological Surgery, Kobe University Graduate School of Medical Sciences, Kobe, Japan.
Ann Surg Oncol. 2007 Apr;14(4):1374-80. doi: 10.1245/s10434-006-9191-9. Epub 2007 Jan 18.
The prognosis of gallbladder carcinoma is poor; therefore, investigating the efficacy of new chemotherapy agents is essential for the treatments for this tumor. Recently, several studies have reported clinical trials using gemcitabine as treatment for advanced gallbladder cancers. However, the antitumor effects of gemcitabine on gallbladder carcinoma have not been examined in in vitro and in vivo model systems.
We examined the cytotoxicity of gemcitabine in four biliary tract cancer cell lines using the WST-1 assay. In addition, we examined the effect of gemcitabine on gallbladder cancers resulting from orthotopic inoculation of NOZ gallbladder tumor cells into nude mice. One week after transplantation, the mice were randomized into two groups: In Group A, the mice were treated by an intra-peritoneal injection of 0.9% sodium chloride for three weeks after inoculation (control). In Group B, the mice were treated by an intra-peritoneal injection of gemcitabine (125 mg / kg) for three weeks. All mice were sacrificed one week after the end of treatment, and macroscopic and histological findings were evaluated. The expression levels of proliferating-cell nuclear antigen (PCNA) were examined to investigate cellular proliferation activity, and Tunnel assays were performed to determine apoptotic status. Survival duration of the mice after gemcitabine treatment was compared to that of untreated mice.
The gemcitabine sensitivity of the four biliary tract cancer cell lines was similar in a dose dependent manner. In the in vivo models, the Group A mice showed huge tumors of the gallbladder, with liver invasion and lymph node metastases. However, there were no abdominal tumors in the Group B mice, and microscopic gallbladder cancer could only be detected from histological findings. The mean percent of PCNA-positive tumor cells was significantly higher in tumors from mice in Group A (71.9%) compared to those of Group B (34.7%). The mean percent of Tunnel-positive tumor cells was significantly lower in mice from Group A (2.0%) than those from Group B (5.7%). Survival duration was prolonged significantly in the gemcitabine-treated mice relative to untreated mice.
Gemcitabine treatment may inhibit tumor progression and prolong survival in gallbladder cancer by inhibiting cell proliferation and inducing apoptosis.
胆囊癌预后较差,因此,研究新型化疗药物的疗效对该肿瘤的治疗至关重要。最近,多项研究报道了使用吉西他滨治疗晚期胆囊癌的临床试验。然而,吉西他滨对胆囊癌的抗肿瘤作用尚未在体外和体内模型系统中进行研究。
我们使用WST-1法检测了吉西他滨在四种胆管癌细胞系中的细胞毒性。此外,我们研究了吉西他滨对将NOZ胆囊肿瘤细胞原位接种到裸鼠体内所产生的胆囊癌的影响。移植一周后,将小鼠随机分为两组:A组小鼠在接种后腹腔注射0.9%氯化钠,持续三周(对照组)。B组小鼠腹腔注射吉西他滨(125mg/kg),持续三周。治疗结束一周后,处死所有小鼠,评估大体和组织学结果。检测增殖细胞核抗原(PCNA)的表达水平以研究细胞增殖活性,并进行Tunnel试验以确定细胞凋亡状态。将吉西他滨治疗后小鼠的生存时间与未治疗小鼠的生存时间进行比较。
四种胆管癌细胞系对吉西他滨的敏感性呈剂量依赖性且相似。在体内模型中,A组小鼠胆囊出现巨大肿瘤,伴有肝侵犯和淋巴结转移。然而,B组小鼠未出现腹部肿瘤,仅从组织学结果中可检测到微小胆囊癌。A组小鼠肿瘤中PCNA阳性肿瘤细胞的平均百分比(71.9%)显著高于B组(34.7%)。A组小鼠Tunnel阳性肿瘤细胞的平均百分比(2.0%)显著低于B组(5.7%)。与未治疗小鼠相比,吉西他滨治疗的小鼠生存时间显著延长。
吉西他滨治疗可能通过抑制细胞增殖和诱导凋亡来抑制胆囊癌的肿瘤进展并延长生存期。
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