Rana B, Mischoulon D, Xie Y, Bucher N L, Farmer S R
Department of Biochemistry, Boston University School of Medicine, Massachusetts 02118.
Mol Cell Biol. 1994 Sep;14(9):5858-69. doi: 10.1128/mcb.14.9.5858-5869.1994.
Previous investigations have shown that culture of freshly isolated hepatocytes under conventional conditions, i.e., on dried rat tail collagen in the presence of growth factors, facilitates cell growth but also causes an extensive down-regulation of most liver-specific functions. This dedifferentiation process can be prevented if the cells are cultured on a reconstituted basement membrane gel matrix derived from the Englebreth-Holm-Swarm mouse sarcoma tumor (EHS gel). To gain insight into the mechanisms regulating this response to extracellular matrix, we are analyzing the activities of two families of transcription factors, C/EBP and AP-1, which control the transcription of hepatic and growth-responsive genes, respectively. We demonstrate that isolation of hepatocytes from the normal quiescent rat liver by collagenase perfusion activates the immediate-early growth response program, as indicated by increased expression of c-jun, junB, c-fos, and c-myc mRNAs. Adhesion of these activated cells to dried rat tail collagen augments the elevated levels of these mRNAs for the initial 1 to 2 h postplating; junB and c-myc mRNA levels then drop steeply, with junB returning to normal quiescence and the c-myc level remaining slightly elevated during the 3-day culture period. Levels of c-jun mRNA and AP-1 DNA binding activity, however, remain elevated from the outset, while C/EBP alpha mRNA expression is down-regulated, resulting in a decrease in the steady-state levels of the 42- and 30-kDa C/EBP alpha polypeptides and C/EBP alpha DNA binding activity. In contrast, C/EBP beta mRNA production remains at near-normal hepatic levels for 5 to 8 days of culture, although its DNA binding activity decreases severalfold during this time. Adhesion of hepatocytes to the EHS gel for the same period of time dramatically alters this program: it arrests growth and inhibits AP-1 DNA binding activity and the expression of c-jun, junB, and c-myc mRNAs, but, in addition, it restores C/EBP alpha mRNA and protein as well as C/EBP alpha and C/EBP beta DNA binding activities to the abundant levels present in freshly isolated hepatocytes. These changes are not due merely to growth inhibition, because suppression of hepatocyte proliferation on collagen by epidermal growth factor starvation or addition of transforming growth factor beta does not inhibit AP-1 activity or restore C/EBP alpha DNA binding activity to normal hepatic levels. These data suggest that expression of the normal hepatic phenotype requires that hepatocytes exist in a G0 state of growth arrest, facilitated here by adhesion of cells to the EHS gel, in order to express high levels of hepatic transcription factors such as C/EBP alpha.
先前的研究表明,在传统条件下,即在生长因子存在的情况下于干燥的大鼠尾胶原上培养新鲜分离的肝细胞,虽有助于细胞生长,但也会导致大多数肝脏特异性功能的广泛下调。如果将细胞培养在源自恩格尔布雷特 - 霍尔姆 - 斯旺小鼠肉瘤肿瘤的重组基底膜凝胶基质(EHS凝胶)上,则可防止这种去分化过程。为深入了解调节这种对细胞外基质反应的机制,我们正在分析两类转录因子的活性,即C/EBP和AP-1,它们分别控制肝脏和生长反应性基因的转录。我们证明,通过胶原酶灌注从正常静止的大鼠肝脏中分离肝细胞会激活即刻早期生长反应程序,这表现为c-jun、junB、c-fos和c-myc mRNA表达增加。这些活化细胞在接种后最初1至2小时内黏附于干燥的大鼠尾胶原会增强这些mRNA的升高水平;然后junB和c-myc mRNA水平急剧下降,junB恢复到正常静止状态,而c-myc水平在3天培养期内仍略有升高。然而,c-jun mRNA水平和AP-1 DNA结合活性从一开始就保持升高,而C/EBPα mRNA表达下调,导致42 kDa和30 kDa的C/EBPα多肽的稳态水平以及C/EBPα DNA结合活性降低。相比之下,在培养5至8天期间,C/EBPβ mRNA产生保持在接近正常肝脏水平,尽管在此期间其DNA结合活性降低了数倍。肝细胞在相同时间段内黏附于EHS凝胶会显著改变这一程序:它会抑制生长并抑制AP-1 DNA结合活性以及c-jun、junB和c-myc mRNA的表达,但此外,它会将C/EBPα mRNA和蛋白质以及C/EBPα和C/EBPβ DNA结合活性恢复到新鲜分离的肝细胞中存在的丰富水平。这些变化不仅仅是由于生长抑制,因为通过表皮生长因子饥饿或添加转化生长因子β来抑制胶原上肝细胞的增殖并不会抑制AP-1活性或使C/EBPα DNA结合活性恢复到正常肝脏水平。这些数据表明,正常肝脏表型的表达要求肝细胞处于生长停滞的G0状态,在这里细胞黏附于EHS凝胶有助于这种状态的形成,以便表达高水平的肝脏转录因子,如C/EBPα。
