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利用啮齿动物泌尿生殖窦间充质和人类干细胞的组织重组形成人前列腺上皮。

Formation of human prostate epithelium using tissue recombination of rodent urogenital sinus mesenchyme and human stem cells.

作者信息

Cai Yi, Kregel Steven, Vander Griend Donald J

机构信息

Department of Surgery, Section of Urology, University of Chicago, USA.

出版信息

J Vis Exp. 2013 Jun 22(76):50327. doi: 10.3791/50327.

Abstract

Progress in prostate cancer research is severely limited by the availability of human-derived and hormone-naïve model systems, which limit our ability to understand genetic and molecular events underlying prostate disease initiation. Toward developing better model systems for studying human prostate carcinogenesis, we and others have taken advantage of the unique pro-prostatic inductive potential of embryonic rodent prostate stroma, termed urogenital sinus mesenchyme (UGSM). When recombined with certain pluripotent cell populations such as embryonic stem cells, UGSM induces the formation of normal human prostate epithelia in a testosterone-dependent manner. Such a human model system can be used to investigate and experimentally test the ability of candidate prostate cancer susceptibility genes at an accelerated pace compared to typical rodent transgenic studies. Since Human embryonic stem cells (hESCs) can be genetically modified in culture using inducible gene expression or siRNA knock-down vectors prior to tissue recombination, such a model facilitates testing the functional consequences of genes, or combinations of genes, which are thought to promote or prevent carcinogenesis. The technique of isolating pure populations of UGSM cells, however, is challenging and learning often requires someone with previous expertise to personally teach. Moreover, inoculation of cell mixtures under the renal capsule of an immunocompromised host can be technically challenging. Here we outline and illustrate proper isolation of UGSM from rodent embryos and renal capsule implantation of tissue mixtures to form human prostate epithelium. Such an approach, at its current stage, requires in vivo xenografting of embryonic stem cells; future applications could potentially include in vitro gland formation or the use of induced pluripotent stem cell populations (iPSCs).

摘要

前列腺癌研究的进展受到人类来源且未接触激素的模型系统可用性的严重限制,这些模型系统限制了我们理解前列腺疾病发生背后的遗传和分子事件的能力。为了开发更好的研究人类前列腺癌发生的模型系统,我们和其他人利用了胚胎啮齿动物前列腺基质独特的前列腺诱导潜能,即泌尿生殖窦间充质(UGSM)。当与某些多能细胞群体如胚胎干细胞重组时,UGSM以睾酮依赖的方式诱导正常人类前列腺上皮的形成。与典型的啮齿动物转基因研究相比,这种人类模型系统可用于以更快的速度研究和实验测试候选前列腺癌易感基因的能力。由于人类胚胎干细胞(hESCs)在组织重组前可在培养中使用诱导型基因表达或siRNA敲低载体进行基因改造,这种模型便于测试被认为促进或预防癌症发生的基因或基因组合的功能后果。然而,分离UGSM细胞的纯群体技术具有挑战性,学习通常需要有经验的人亲自指导。此外,在免疫受损宿主的肾包膜下接种细胞混合物在技术上也具有挑战性。在这里,我们概述并说明从啮齿动物胚胎中正确分离UGSM以及将组织混合物植入肾包膜以形成人类前列腺上皮的方法。在现阶段,这种方法需要对胚胎干细胞进行体内异种移植;未来的应用可能包括体外腺体形成或使用诱导多能干细胞群体(iPSCs)。

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