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利用人外分泌胰腺部分,对无血清悬浮培养和单层培养过程中导管细胞富集过程进行研究与表征。

Investigation and characterization of the duct cell-enriching process during serum-free suspension and monolayer culture using the human exocrine pancreas fraction.

作者信息

Klein Tino, Heremans Yves, Heimberg Harry, Pipeleers Daniel, Madsen Ole D, Serup Palle, Heller R Scott

机构信息

Department of Developmental Biology, Hagedorn Research Institute, Gentofte, Denmark.

出版信息

Pancreas. 2009 Jan;38(1):36-48. doi: 10.1097/MPA.0b013e3181816547.

DOI:10.1097/MPA.0b013e3181816547
PMID:18665014
Abstract

OBJECTIVES

We aimed to characterize a serum-free culture system resulting in highly enriched duct cells from human exocrine pancreas. In addition, we tested the effect of vascular endothelial growth factor (VEGF) on endothelial cell proliferation and endocrine differentiation of the duct cells.

METHODS

The exocrine pellet fraction was cultivated in suspension followed by monolayer culture. Time course analysis of multiple acinar and duct cell markers was performed using reverse transcription-polymerase chain reaction and immunocytochemistry. The effects of VEGF and placental growth factor on the quantities of endothelial, duct, and endocrine cells and fibroblasts were investigated using computerized imaging analysis.

RESULTS

Suspension culture of the exocrine material efficiently enriched the cultures for duct cells. Frequent acinar cell death as well as cell selective adherence of acinar cells to the culture dish was the underlying cause of the enrichment. Confocal microscopy demonstrated the virtual absence of cells coexpressing duct cell- and acinar cell-specific markers. The endothelial immunoreactivity of the suspension culture system could be increased 2-fold by VEGF treatment, yet no effect was observed on endocrine cell numbers.

CONCLUSIONS

We have characterized a serum-free in vitro culture system to enrich human duct cells and further show that the contribution of acinoductal transdifferentiation to the enrichment of duct cells is negligible.

摘要

目的

我们旨在表征一种无血清培养系统,该系统能从人外分泌胰腺中产生高度富集的导管细胞。此外,我们测试了血管内皮生长因子(VEGF)对导管细胞内皮细胞增殖和内分泌分化的影响。

方法

将外分泌沉淀部分进行悬浮培养,随后进行单层培养。使用逆转录-聚合酶链反应和免疫细胞化学对多种腺泡和导管细胞标志物进行时间进程分析。使用计算机成像分析研究VEGF和胎盘生长因子对内皮细胞、导管细胞、内分泌细胞和成纤维细胞数量的影响。

结果

外分泌物质的悬浮培养有效地富集了导管细胞培养物。腺泡细胞频繁死亡以及腺泡细胞对培养皿的选择性黏附是富集的根本原因。共聚焦显微镜显示几乎不存在同时表达导管细胞和腺泡细胞特异性标志物的细胞。VEGF处理可使悬浮培养系统的内皮免疫反应性增加2倍,但对内分泌细胞数量未观察到影响。

结论

我们已经表征了一种无血清体外培养系统来富集人导管细胞,并进一步表明腺泡导管转分化对导管细胞富集的贡献可忽略不计。

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