Sirica A E, Gainey T W
Department of Pathology, Virginia Commonwealth University-Medical College of Virginia, Richmond 23298-0297, USA.
Hepatology. 1997 Sep;26(3):537-49. doi: 10.1002/hep.510260302.
The rat treated with bile duct ligation (BDL) and furan is a unique animal model of massive bile ductular hyperplasia in which normal liver parenchyma is largely replaced with well-differentiated proliferated bile ductules. We have now developed a simple cell isolation procedure to obtain and culture viable bile ductular epithelial cells in high numbers and with a high degree of purity from the livers of BDL/furan-treated rats. Primary monolayer cell cultures were readily established when the isolated bile ductular epithelial cells were cultured in plastic tissue culture wells coated with rat tail tendon type I collagen plus bovine plasma fibronectin. Under these conditions, epidermal growth factor (EGF) was mitogenic for the cultured cells, and they retained phenotypic features typical of hyperplastic bile ductular epithelium but did not show evidence of ductal morphogenesis in vitro. In contrast, when the isolated bile ductular cells were cultured for 7 to 16 days in the presence of 25 ng EGF/mL and 10% fetal bovine serum on type I collagen gels, they formed into branching ductal structures whose ultrastructural features very closely resembled those of polarized hyperplastic bile ductules/ducts in vivo. Histological preparations of these gel cultures further showed that numerous ductal structures with defined lumens were present. Phenotypically, these ductal structures were completely surrounded by a thickened basement membrane that was strongly immunoreactive for laminin. Like their in vivo biliary cell counterparts, the epithelial cells comprising these ductal structures in culture also exhibited strong immunocytochemical staining reactions for cytokeratins 8 and 19, for glutathione S-transferase pi 7, and for luminal gamma-glutamyl transpeptidase, but they did not express immunoreactive albumin or alpha-fetoprotein. Occasional epithelial cells of the ductal structures, when examined in 10-day-old primary gel culture, showed strong nuclear staining for incorporated 5-bromo-2'deoxyuridine, indicating active cell proliferation. Our results support the development of a novel biliary epithelial cell culture model that has the potential of serving as a powerful tool for investigation of factors that regulate hyperplastic bile ductular morphogenesis, cell proliferation, and polarized cell functions in a structural form in vitro that mimics that of hyperplastic bile ductules induced in vivo.
经胆管结扎(BDL)和呋喃处理的大鼠是一种独特的大量胆管增生动物模型,其中正常肝实质大部分被分化良好的增生性胆小管所取代。我们现已开发出一种简单的细胞分离程序,可从经BDL/呋喃处理的大鼠肝脏中大量且高度纯化地获取并培养有活力的胆小管上皮细胞。当将分离出的胆小管上皮细胞培养在涂有大鼠尾腱I型胶原蛋白加牛血浆纤连蛋白的塑料组织培养孔中时,很容易建立原代单层细胞培养。在这些条件下,表皮生长因子(EGF)对培养的细胞有促有丝分裂作用,它们保留了增生性胆小管上皮的典型表型特征,但在体外未显示导管形态发生的证据。相反,当将分离出的胆小管细胞在含有25 ng EGF/mL和10%胎牛血清的I型胶原凝胶上培养7至16天时,它们形成分支导管结构,其超微结构特征与体内极化增生性胆小管/导管的特征非常相似。这些凝胶培养物的组织学制剂进一步显示存在许多具有明确管腔的导管结构。从表型上看,这些导管结构完全被增厚的基底膜包围,该基底膜对层粘连蛋白有强烈的免疫反应性。与它们在体内的胆管细胞对应物一样,构成培养中这些导管结构的上皮细胞对细胞角蛋白8和19、谷胱甘肽S-转移酶pi 7以及管腔γ-谷氨酰转肽酶也表现出强烈的免疫细胞化学染色反应,但它们不表达免疫反应性白蛋白或甲胎蛋白。在10日龄的原代凝胶培养物中检查时,导管结构的偶尔上皮细胞对掺入的5-溴-2'-脱氧尿苷显示出强烈的核染色,表明细胞活跃增殖。我们的结果支持开发一种新型胆管上皮细胞培养模型,该模型有可能成为一种强大的工具,用于研究调节增生性胆小管形态发生、细胞增殖以及体外模拟体内诱导的增生性胆小管结构形式的极化细胞功能的因素。
