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培养的肝细胞具有祖细胞特征,并表现出重新填充肝脏的双能能力。

Cultured hepatocytes adopt progenitor characteristics and display bipotent capacity to repopulate the liver.

作者信息

Krause Petra, Unthan-Fechner Kirsten, Probst Irmelin, Koenig Sarah

机构信息

Department of General and Visceral Surgery, University Medical Centre Goettingen, Goettingen, Germany.

出版信息

Cell Transplant. 2014;23(7):805-17. doi: 10.3727/096368913X664856. Epub 2013 Mar 5.

Abstract

Clinical studies have proved the therapeutic potential of hepatocyte transplantation as a promising alternative to whole organ liver transplantation in the treatment of hereditary or end-stage liver disease. However, donor shortage seriously restricts cell availability, and the lack of appropriate cell culture protocols for the storage and maintenance of donor cells constitutes a significant obstacle. The aim of this study was to stimulate mature hepatocytes in culture to multiply in vitro and track their fate on transplantation. Rat hepatocytes isolated nonenzymatically were cultured serum free for up to 10 days. They were stimulated into proliferation in the presence of growth factors and conditioned media from nonparenchymal and hepatocyte culture supernatants, as well as 10 mM lithium chloride (LiCl). Cell proliferation was assessed by determining DNA content. Additionally, the extent of cell differentiation was estimated using immunofluorescence staining of hepatic, biliary, progenitor, and mesenchymal markers and gene expression analyses. Transplantation studies were performed on the Fischer CD26-mutant rat following pretreatment with retrorsine and partial hepatectomy. Proliferating hepatocytes increasingly adopted precursor characteristics, expressing progenitor (OV6, CD133), hepatic lineage (CK18), biliary (CD49f, CK7, CK19), and mesenchymal (vimentin) markers. The supplement of LiCl further enhanced the proliferative capacity by 30%. Transplantation studies revealed extensive repopulation by large donor hepatocyte clusters. Furthermore, bile duct-like structures deriving from donor cells proved to be immunoreactive to ductular markers and formed in close proximity to endogenous bile ducts. Mature hepatocytes reveal their potential to "switch" between phenotypes, adopting progenitor characteristics during proliferation in vitro. Following transplantation, these "retrodifferentiated" cells further expanded in vivo, thereby generating bipotentially differentiated progenies (hepatocytes and bile duct-like structures). This apparent plasticity of mature hepatocytes may open new approaches for cell-based strategies to treat liver disease.

摘要

临床研究已证明,肝细胞移植作为全器官肝移植的一种有前景的替代方法,在治疗遗传性或终末期肝病方面具有治疗潜力。然而,供体短缺严重限制了细胞的可获得性,并且缺乏用于储存和维持供体细胞的合适细胞培养方案构成了重大障碍。本研究的目的是在培养中刺激成熟肝细胞在体外增殖,并追踪其移植后的命运。非酶法分离的大鼠肝细胞在无血清条件下培养长达10天。在生长因子、非实质细胞和肝细胞培养上清液的条件培养基以及10 mM氯化锂(LiCl)存在的情况下,刺激它们增殖。通过测定DNA含量评估细胞增殖。此外,使用肝、胆管、祖细胞和间充质标志物的免疫荧光染色以及基因表达分析来估计细胞分化程度。在经雷琐辛预处理和部分肝切除的Fischer CD26突变大鼠上进行移植研究。增殖的肝细胞越来越多地呈现前体特征,表达祖细胞(OV6、CD133)、肝谱系(CK18)、胆管(CD49f、CK7、CK19)和间充质(波形蛋白)标志物。LiCl的添加进一步将增殖能力提高了30%。移植研究显示大量供体肝细胞簇广泛再填充。此外,源自供体细胞的胆管样结构被证明对胆管标志物具有免疫反应性,并在内源性胆管附近形成。成熟肝细胞显示出在表型之间“转换”的潜力,在体外增殖过程中呈现祖细胞特征。移植后,这些“逆分化”细胞在体内进一步扩增,从而产生双潜能分化后代(肝细胞和胆管样结构)。成熟肝细胞这种明显的可塑性可能为基于细胞的肝病治疗策略开辟新途径。

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