一种在器官培养系统中使用荧光肿瘤细胞的浅表性膀胱癌模型。

A model of superficial bladder cancer using fluorescent tumour cells in an organ-culture system.

作者信息

Crook T J, Hall I S, Solomon L Z, Birch B R, Cooper A J

机构信息

MDR Research Group, Department of Urology, Southampton General Hospital, Southampton, UK.

出版信息

BJU Int. 2000 Nov;86(7):886-93. doi: 10.1046/j.1464-410x.2000.00923.x.

DOI:10.1046/j.1464-410x.2000.00923.x

PMID:11069418

Abstract

OBJECTIVE

To develop a reproducible in vitro simulation of superficial bladder cancer for testing cytotoxic agents at clinically relevant concentrations.

MATERIALS AND METHODS

Square explants (5 mm) of rat bladder were cultured in Petri dishes in minimal volumes of Waymouth's MB 752/1 medium supplemented with 10% fetal calf serum, antibiotics and glutamine. Parental and resistant MGH-U1 urothelial cancer cells were transfected with a green fluorescent protein (GFP) vector. Transfectants were purified by flow cytometry. Cells were seeded onto the prepared organ cultures and images obtained using confocal microscopy. The tumour colonies were confirmed using scanning electron microscopy. Conventional intravesical cytotoxic agents including epirubicin, mitomycin-C and estramustine were tested in the system.

RESULTS

Colonies of GFP-MGH-U1 cells became established on the explants and were identified by confocal microscopy; the development of the colonies was then followed over several days. Staining the explant for viability allowed imaging of normal urothelium on the explant surface or surrounding skirt of urothelial cells. The conventional cytotoxic agents epirubicin, mitomycin C and estramustine showed the expected differential responses to parental and resistant cell types. The colonies were able to survive high concentrations of the drug, equivalent to those in clinical use. The colonies were imaged serially over a period of several days.

CONCLUSION

This system provides a more realistic model for testing cytotoxic agents for use in intravesical therapy, by allowing clinically relevant concentrations of drugs to be tested. The differential properties of the parental and resistant cells are maintained. The model also enables the same tumour colony to be imaged over several days in culture. The model may also be adapted for use in testing the effects of drugs on normal urothelium and the study of the effects of growth factors.

摘要

目的

建立一种可重复的浅表性膀胱癌体外模拟模型，用于测试临床相关浓度的细胞毒性药物。

材料与方法

将大鼠膀胱的方形外植体（5毫米）培养在培养皿中，培养基为添加了10%胎牛血清、抗生素和谷氨酰胺的少量Waymouth's MB 752/1培养基。将亲代和耐药的MGH-U1膀胱癌细胞系用绿色荧光蛋白（GFP）载体转染。通过流式细胞术纯化转染细胞。将细胞接种到制备好的器官培养物上，并用共聚焦显微镜获取图像。使用扫描电子显微镜确认肿瘤集落。在该系统中测试了包括表柔比星、丝裂霉素-C和雌莫司汀在内的传统膀胱内细胞毒性药物。

结果

GFP-MGH-U1细胞的集落在外植体上形成，并通过共聚焦显微镜进行鉴定；随后对集落的发育情况进行了数天的跟踪观察。对外植体进行活力染色，可对正常膀胱上皮细胞在外植体表面或周围的尿路上皮细胞裙进行成像。传统细胞毒性药物表柔比星、丝裂霉素C和雌莫司汀对亲代和耐药细胞类型表现出预期的不同反应。这些集落能够在相当于临床使用浓度的高浓度药物环境中存活。在数天时间内对集落进行了连续成像。