Gordon P B, Conn G, Hatcher V B
J Cell Physiol. 1985 Dec;125(3):596-607. doi: 10.1002/jcp.1041250332.
An endothelial cell (EC) growth factor isolated from bovine brain stimulates in vitro growth of human umbilical vein endothelial cells, and permits long term serial propagation. In the presence of increasing concentrations of EC growth factor, confluent cultures of early (CPDL less than or equal to 20) and late (CPDL greater than 20) passage human endothelial cells exhibit an increased incorporation of 3H-glucosamine and Na235SO4 into the glycosaminoglycans (GAG), hyaluronic acid, chondroitin, chondroitin-4-sulfate, dermatan-4-sulfate, and chondroitin-6-sulfate. An increase in both labelled sulfated and nonsulfated GAG was observed in the cytosol, membrane, secreted and extracellular matrix fractions. In contrast, endothelial cells grown in the presence of EC growth factor contained decreased amounts of labelled heparan sulfate than cells grown without EC growth factor. Confluent cultures of early passage cells had significantly more labelled GAG but significantly less heparan sulfate than cultures of late passage cells on a per cell basis. Extracellular matrix from early passage cells contained about two- to seven-fold more labelled GAG than extracellular matrix from late passage cells, but only about half as much labelled heparan sulfate. Cell adhesion was enhanced when cells were grown in the presence of EC growth factor as compared to adhesion of cells grown without EC growth factor. Conversely, trypsin-mediated detachment of cells grown in the presence of growth factor was inhibited as compared to detachment of cells grown in medium without EC growth factor. The composition of the extracellular matrix influenced incorporation of labelled GAG into extracellular matrix. Early passage cells grown to confluence on a matrix from late passage cells incorporated significantly less labelled GAG into extracellular matrix than when grown to confluence on matrix from early passage cells. Incorporation of labelled GAG into extracellular matrix was significantly higher when late passage cells were grown on a matrix from early passage endothelial cells than when grown on matrix from late passage cells. We conclude that EC growth factor selectively stimulates incorporation of isotopic precursors into GAG in cultures of early and late passage endothelial cells but inhibits incorporation of radiolabel into heparan sulfate; early passage cells contain more GAG but less heparan sulfate than late passage cells, extracellular matrix controls the amount of GAG and heparan sulfate incorporated into matrix.(ABSTRACT TRUNCATED AT 400 WORDS)
从牛脑中分离出的一种内皮细胞(EC)生长因子可刺激人脐静脉内皮细胞的体外生长,并能使其长期连续传代培养。在EC生长因子浓度不断增加的情况下,早期传代(群体倍增水平(CPDL)小于或等于20)和晚期传代(CPDL大于20)的人内皮细胞汇合培养物中,3H-葡萄糖胺和Na235SO4掺入糖胺聚糖(GAG)、透明质酸、软骨素、硫酸软骨素-4、硫酸皮肤素-4和硫酸软骨素-6的量增加。在胞质溶胶、细胞膜、分泌成分和细胞外基质部分均观察到标记的硫酸化和非硫酸化GAG增加。相比之下,在EC生长因子存在下生长的内皮细胞中,标记的硫酸乙酰肝素含量比在无EC生长因子条件下生长的细胞少。以单个细胞计,早期传代细胞的汇合培养物中标记的GAG显著更多,但硫酸乙酰肝素显著更少。早期传代细胞的细胞外基质中标记的GAG比晚期传代细胞的细胞外基质多约2至7倍,但标记的硫酸乙酰肝素仅为其一半左右。与在无EC生长因子条件下生长的细胞的黏附相比,在EC生长因子存在下生长的细胞的黏附增强。相反,与在无EC生长因子的培养基中生长的细胞的脱离相比,胰蛋白酶介导的在生长因子存在下生长的细胞的脱离受到抑制。细胞外基质的组成影响标记的GAG掺入细胞外基质。早期传代细胞在晚期传代细胞的基质上生长至汇合时,掺入细胞外基质的标记GAG比在早期传代细胞的基质上生长至汇合时显著更少。当晚期传代细胞在早期传代内皮细胞的基质上生长时,标记的GAG掺入细胞外基质的量比在晚期传代细胞的基质上生长时显著更高。我们得出结论,EC生长因子选择性地刺激早期和晚期传代内皮细胞培养物中同位素前体掺入GAG,但抑制放射性标记掺入硫酸乙酰肝素;早期传代细胞比晚期传代细胞含有更多的GAG但更少的硫酸乙酰肝素,细胞外基质控制掺入基质的GAG和硫酸乙酰肝素的量。(摘要截短至400字)
