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长期无血清人胎肝细胞培养的特征和移植。

Characterization and engraftment of long-term serum-free human fetal liver cell cultures.

机构信息

Department of Transplantation Surgery, Sahlgrenska University Hospital, University of Gothenburg, Gothenburg, Sweden.

出版信息

Cytotherapy. 2010 Apr;12(2):201-11. doi: 10.3109/14653240903398053.

DOI:10.3109/14653240903398053
PMID:19929451
Abstract

BACKGROUND AIMS

Cultured human hepatocytes have extensive diagnostic and clinical applications. However, the setting-up of new in vitro culture techniques allowing the long-term survival and functional maintenance of adult human hepatocytes represents a formidable challenge. Fetal liver cells (FLC) are attractive candidate donor cells because of their high proliferative capacity.

METHODS

Using cell culture and molecular techniques, we studied the in vitro and in vivo characteristics of FLC grown long-term in serum-free conditions.

RESULTS

Serum-free FLC obtained from 6-10-week-old human fetal livers grew as multiple clusters in suspension and could be subcultured for at least six passages. These cells maintained stable hepatocyte phenotypes and gene expression patterns in culture for up to 6 months. When a cluster of these cells in various passages was placed on collagen-coated plates, they formed a monolayer and morphologically resembled hepatocytes. The cells expressed alpha -fetoprotein, cytokeratin (CK) 8, CK18 and CK19 and albumin (ALB). Hepatocyte nuclear factor 4alpha and 1beta and cytochrome P450 (CYP) 3A4 and CYP3A7 mRNA expression was demonstrated by reverse transcriptase-polymerase chain reaction (RT-PCR). Cells at different passages, when transplanted into nude mice with liver injury, engrafted successfully, as detected by in situ hybridization using a human-specific DNA probe. Colonies of human-specific CK8, CK18, c-Met nuclear antigen (Ag), mitochondrial Ag, hepatocyte-specific Ag and ALB-expressing cells were present in the livers of recipient animals.

CONCLUSIONS

Primary human FLC can be kept in culture consistently over a long time period and are potential candidates for cell therapy and in vitro diagnostics.

摘要

背景与目的

培养的人肝细胞具有广泛的诊断和临床应用价值。然而,建立新的体外培养技术,使成人肝细胞长期存活和功能维持,这是一个巨大的挑战。由于其高增殖能力,胎肝细胞(FLC)是有吸引力的候选供体细胞。

方法

我们使用细胞培养和分子技术,研究了在无血清条件下长期培养的 FLC 的体外和体内特征。

结果

从 6-10 周龄人胎肝中获得的无血清 FLC 在悬浮状态下以多个细胞簇生长,可以至少传代培养 6 次。这些细胞在培养中保持稳定的肝细胞表型和基因表达模式,长达 6 个月。当这些细胞的一个细胞簇在不同的传代中放置在胶原涂层的平板上时,它们形成单层,形态上类似于肝细胞。这些细胞表达α-胎蛋白、细胞角蛋白(CK)8、CK18 和 CK19 以及白蛋白(ALB)。通过逆转录聚合酶链反应(RT-PCR)证实了肝细胞核因子 4alpha 和 1beta 以及细胞色素 P450(CYP)3A4 和 CYP3A7 mRNA 的表达。在用人类特异性 DNA 探针进行原位杂交时,当移植到有肝损伤的裸鼠中时,在不同传代的细胞中成功植入,检测到。在受体动物的肝脏中存在人特异性 CK8、CK18、c-Met 核抗原(Ag)、线粒体 Ag、肝细胞特异性 Ag 和表达 ALB 的细胞的克隆。

结论

原代人 FLC 可以在很长一段时间内保持在培养中,是细胞治疗和体外诊断的潜在候选者。

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