体外扩增小鼠去势抵抗性中间前列腺干细胞。
Expansion of mouse castration-resistant intermediate prostate stem cells in vitro.
机构信息
Institute for Translational Medicine, The Affiliated Hospital of Qingdao University, Medical College, Qingdao University, Qingdao, 266021, China.
School of Basic Medicine, Qingdao University, Qingdao, 266021, China.
出版信息
Stem Cell Res Ther. 2022 Jul 15;13(1):299. doi: 10.1186/s13287-022-02978-x.
BACKGROUND
Most castration-resistant prostate cancers (CRPCs) have a luminal phenotype with high androgen receptor (AR) and prostate-specific antigen (PSA) expression. Currently, it is difficult to culture castration-resistant luminal cells with AR and PSA expression.
METHODS
We formulated a custom-made medium and isolated primary cells from the prostate of adult wild-type (WT) and TRAMP mice. The cells were characterized by immunofluorescence staining, transcriptomic analysis, and qRT-PCR verification. Their self-renewal and differentiation potential in vitro and in vivo were examined. We treated the cells with androgen deprivation and enzalutamide and performed immunofluorescence staining and western blotting to analyze their expression of AR and PSA.
RESULTS
We isolated a novel type of castration-resistant intermediate prostate stem cells (CRIPSCs) from adult WT and TRAMP mice. The mouse CRIPSCs proliferated rapidly in two-dimensional (2D) culture dishes and can be cultured for more than six months. The mouse CRIPSCs expressed luminal markers (AR, PSA, and Dsg4), basal markers (CK5 and p63), Psca, and the intermediate cell marker (Ivl). Transcriptomic analysis showed that the mouse CRIPSCs had upregulated signaling pathways related to cancer development and drug resistance. In the long-term culture, TRAMP CRIPSCs had higher expression of the genes related to stem cells and cancers than WT mice. Both WT and TRAMP CRIPSCs formed organoids in Matrigel. WT CRIPSCs did not form prostate tissues when transplanted in vivo without urogenital sinus mesenchyme (UGM) cells. In contrast, TRAMP CRIPSCs formed prostate ducts in NOG mice without UGM cells and differentiated into luminal, basal, and neuroendocrine cells. Androgens regulated AR translocation between the nucleus and cytoplasm in the mouse CRIPSCs. Treatment of androgen deprivation (ADT) and enzalutamide reduced AR expression in WT and TRAMP CRIPSCs; however, this treatment promoted PSA expression in TRAMP, while not WT CRIPSCs, similar to the clinical observations of CRPC.
CONCLUSIONS
Our study established a method for isolating and expanding mouse CRIPSCs in 2D culture dishes. Mouse CRIPSCs had markers of basal and luminal cells, including AR and PSA, and can differentiate into prostate organoids and tissues. TRAMP CRIPSCs had elevated PSA expression upon ADT and enzalutamide treatment. Our method can be translated into clinical settings for CRPC precision medicine.
背景
大多数去势抵抗性前列腺癌(CRPC)具有腔型表型,雄激素受体(AR)和前列腺特异性抗原(PSA)表达水平较高。目前,培养具有 AR 和 PSA 表达的去势抵抗性腔细胞比较困难。
方法
我们设计了一种定制的培养基,并从成年野生型(WT)和 TRAMP 小鼠的前列腺中分离原代细胞。通过免疫荧光染色、转录组分析和 qRT-PCR 验证对细胞进行鉴定。检测细胞在体外和体内的自我更新和分化潜能。我们用雄激素剥夺和恩扎鲁胺处理细胞,进行免疫荧光染色和 Western blot 分析,检测 AR 和 PSA 的表达。
结果
我们从成年 WT 和 TRAMP 小鼠中分离出一种新型的去势抵抗性中间前列腺干细胞(CRIPSCs)。小鼠 CRIPSCs 在二维(2D)培养皿中快速增殖,可培养超过 6 个月。小鼠 CRIPSCs 表达腔细胞标志物(AR、PSA 和 Dsg4)、基底细胞标志物(CK5 和 p63)、Psca 和中间细胞标志物(Ivl)。转录组分析表明,小鼠 CRIPSCs 中与癌症发展和耐药性相关的信号通路被上调。在长期培养中,TRAMP CRIPSCs 中与干细胞和癌症相关的基因表达水平高于 WT 小鼠。WT 和 TRAMP CRIPSCs 在 Matrigel 中均可形成类器官。在没有尿生殖窦间质(UGM)细胞的情况下,WT CRIPSCs 体内移植不能形成前列腺组织。相比之下,TRAMP CRIPSCs 在没有 UGM 细胞的情况下可在 NOG 小鼠中形成前列腺导管,并分化为腔细胞、基底细胞和神经内分泌细胞。雄激素调节小鼠 CRIPSCs 中 AR 在核质间的易位。去势(ADT)和恩扎鲁胺处理降低了 WT 和 TRAMP CRIPSCs 中 AR 的表达;然而,这种治疗促进了 TRAMP CRIPSCs 中 PSA 的表达,而不是 WT CRIPSCs,这与 CRPC 的临床观察结果相似。
结论
本研究建立了在 2D 培养皿中分离和扩增小鼠 CRIPSCs 的方法。小鼠 CRIPSCs 具有基底细胞和腔细胞标志物,包括 AR 和 PSA,可分化为前列腺类器官和组织。TRAMP CRIPSCs 在 ADT 和恩扎鲁胺治疗后 PSA 表达水平升高。我们的方法可转化为 CRPC 精准医学的临床应用。
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