Reznikoff C A, Loretz L J, Pesciotta D M, Oberley T D, Ignjatovic M M
J Cell Physiol. 1987 Jun;131(3):285-301. doi: 10.1002/jcp.1041310302.
Conditions have been described for the selective growth, serial cultivation, and postconfluent morphological differentiation in vitro of normal adult human uroepithelial cells (HUC) on collagen gel substrates in a serum-free medium without the deliberate addition of undefined components and without a requirement for a polypeptide growth factor. The culture medium used (F12) was the standard Ham's F12 medium (0.3 mM calcium) supplemented with 1 microgram/ml hydrocortisone, 5 micrograms/ml transferrin, 10 micrograms/ml insulin, 0.1 mM nonessential amino acids, 2.0 mM L-glutamine, 2.7 mg/ml D-glucose, 10(-4) M ethanolamine or 10(-4) M phosphoethanolamine, and 5 X 10(-8) M selenium. HUC grown in F12 on Type I collagen gel substrates had a generation time of 33 hours and could be serially passed 3-5 times during log phase of growth (20-25 population doublings) before spontaneously senescing. Transmission electron microscopy showed that cultures of HUC grown entirely in serum-free F12 on collagen gel substrates morphologically differentiate postconfluence to resemble in some respects the stratified uroepithelium in vivo, although neither a basal lamina nor an asymmetric unit membrane develop. The addition of epidermal growth factor (EGF) to the F12 did not improve either the growth rate or the lifespan in vitro of HUC. In contrast, the addition of fetal bovine serum (FBS) to F12 was mitogenic to HUC in a dose-dependent manner in the concentration range 0.01-1.00% (4-400 micrograms/ml protein), but higher concentrations of FBS did not improve growth further. The generation time of HUC in 1% FBS-F12 decreased to 21 hours, and the potential population doublings in vitro increased to 31-36. Small amounts (140 micrograms/ml) of bovine pituitary extract (BPE) were similarly mitogenic to HUC in F12. Altering the calcium concentration in the standard Ham's F12 medium (0.3 mM), however, did not improve the growth of HUC in serum-containing or serum-free medium. Higher calcium concentrations (0.30-0.90 mM) were neither mitogenic nor inhibitory to HUC growth, but resulted in decreasing viability of HUC in growing cultures, suggesting an accelerating rate of cellular differentiation. In contrast HUC in low calcium, serum-free F12 (0.1 mM) failed to stratify and morphologically differentiate even in postconfluent cultures. This failure of HUC to differentiate in low calcium F12 medium did not confer a long-term growth advantage.(ABSTRACT TRUNCATED AT 400 WORDS)
已描述了在无血清培养基中,于胶原凝胶底物上正常成人人类尿路上皮细胞(HUC)进行选择性生长、连续培养及汇合后形态分化的条件,该培养基不刻意添加成分不明的物质,也无需多肽生长因子。所用培养基(F12)为标准的哈姆氏F12培养基(0.3 mM钙),添加了1微克/毫升氢化可的松、5微克/毫升转铁蛋白、10微克/毫升胰岛素、0.1 mM非必需氨基酸、2.0 mM L-谷氨酰胺、2.7毫克/毫升D-葡萄糖、10⁻⁴ M乙醇胺或10⁻⁴ M磷酸乙醇胺以及5×10⁻⁸ M硒。在I型胶原凝胶底物上于F12中生长的HUC代时为33小时,在对数生长期(20 - 25次群体倍增)可连续传代3 - 5次,之后自发衰老。透射电子显微镜显示,完全在无血清F12中于胶原凝胶底物上生长的HUC培养物在汇合后形态上发生分化,在某些方面类似于体内的复层尿路上皮,尽管既未形成基底层也未形成不对称单位膜。向F12中添加表皮生长因子(EGF)既未提高HUC的体外生长速率,也未延长其寿命。相反,向F12中添加胎牛血清(FBS)在0.01 - 1.00%(4 - 400微克/毫升蛋白质)浓度范围内对HUC有促有丝分裂作用,呈剂量依赖性,但更高浓度的FBS并未进一步促进生长。在1% FBS - F12中HUC的代时降至21小时,体外潜在群体倍增数增加至31 - 36。少量(140微克/毫升)牛垂体提取物(BPE)在F12中对HUC同样有促有丝分裂作用。然而,改变标准哈姆氏F12培养基中的钙浓度(0.3 mM),并未改善含血清或无血清培养基中HUC的生长。更高的钙浓度(0.30 - 0.90 mM)对HUC生长既无促有丝分裂作用也无抑制作用,但导致生长培养物中HUC的活力下降,提示细胞分化速率加快。相反,在低钙、无血清F12(0.1 mM)中的HUC即使在汇合后培养物中也未能分层和进行形态分化。HUC在低钙F12培养基中无法分化并未赋予其长期生长优势。(摘要截短于400字)
