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Analysis of growth factor “relaxation” in chinese hamster lung fibroblasts required for tumoral expression
Author(s) -
van ObberghenSchilling E.,
PérezRodríguez R.,
Franchi A.,
Chambard J. C.,
Pouysségur J.
Publication year - 1983
Publication title -
journal of cellular physiology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.529
H-Index - 174
eISSN - 1097-4652
pISSN - 0021-9541
DOI - 10.1002/jcp.1041150204
Subject(s) - chinese hamster , growth factor , hamster , thrombin , insulin like growth factor , endocrinology , cell culture , stimulation , in vivo , transforming growth factor , medicine , biology , chemistry , microbiology and biotechnology , receptor , genetics , platelet
Abstract The Chinese hamster lung fibroblast line, CCI39, displays the properties characteristic of normal secondary cultures of Chinese hamster fibroblasts including: reversible GO growth arrest (<2% labeled nuclei), anchorage dependence, and high serum‐growth factor dependence. Injection of CCI39 cells, or anchorage‐independent variants, in nude mice leads to tumor formation; however, as we have previously shown (Pérez‐Rodriguez et al., 1981b), the resulting tumor clones no longer possess the high serum dependence of injected CCI39 cells. Hormonal growth restraints imposed by the host create an in vivo selection for diminished, or “relaxed,” growth factor requirement. To characterize this growth factor “relaxation” further, we have analyzed the mitogenic response of parental CCI39 cells, anchorage‐independent clones, and selected tumoral derivatives, to purified growth factors. Two highly purified growth factors, thrombin and insulin, together fulfill the growth factor requirements of CCI39 cells; thrombin (1 U/ml) stimulates the reinitiation of DNA synthesis in GO‐arresed CCI39 cells, and insulin (10 μ/ml) maximally potentiates this stimulation to the level obtained with 10% fetal calf serum. First, we found no correlation between loss of anchorage dependence and growth factor relaxation. Second, we found that A71 (anchorage independent), a tumoral variant of CCI39 capable of growth arrest, and tumor‐derived cells all display an increased sensitivity to thrombin and a diminished requirement for the potentiating action of insulin. Examination of thrombin binding to CCI39, A51 (nontumoral, anchorage independent), and A71 cells revealed that the increased sensitivity to thrombin of A71 cells is not attributable to an alteration in thrombin cell surface receptor number or affinity for thrombin. Rather, under standard conditions of serum or growth factor removal (30 hr), A71 cells maintain a metabolically elevated growth‐arrested state, different from that of their nontumoral counterparts. Consequently, much lower concentrations of growth factors are needed to induce a proliferative response in these tumoral cells.