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Journal of Reproduction and Fertility (1998) 112 69-77
DOI: 10.1530/jrf.0.1120069
Copyright © 1998 Society for Reproduction and Fertility
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Effects of dose of LH on androgen production and luteinization of ovine theca cells cultured in a serum-free system

B. K. Campbell, D. T. Baird and R. Webb

The study reports the development of a serum-free culture system for sheep thecal cells that overcomes the problem of spontaneous luteinization and the use of this system to study the control of proliferation and differentiation. Theca cells were isolated by enzymatic dispersion from small follicles (< 3.5 mm) and the effect of plating densities (25–100 x 103 cells per well), LH (0.001–100 µg l–1), insulin (1–5000 µg l–1), insulin-like growth factor I (IGF-I) analogue (1–100 µg LR3-IGF-Il–1) and epidermal growth factor (EGF) (0.005–50 µg l–1) on the number of cells and androstenedione and progesterone production were determined. Plating density had a marked effect on the pattern of hormone secretion with densities between 50 and 75 x 103 cells per well resulting in a high androstenedione: progesterone ratio at optimum doses of LH (0.1 µg l–1: P < 0.001). In the first 48 h, the production of both androstenedione and progesterone was stimulated in a dose-dependent manner by LH (P < 0.001). However, the production of androstenedione was ten times higher than that of progesterone and was more sensitive to LH (ED50 value 0.08 µg l–1 for androstenedione and 1 µg l–1 for progesterone). From 48–144 h of culture higher doses of LH (> 1 ng ml–1) inhibited androstenedione (P < 0.001) and stimulated progesterone (P < 0.001) and resulted in a marked change in cell morphology, thus reflecting both functional and morphological luteinization. At optimum doses of LH, both insulin and IGF stimulated cell proliferation (P < 0.001) and androstenedione production (P < 0.001) in a dose responsive manner and there was a significant (P < 0.001) interaction between them. In contrast, both insulin and IGF-I inhibited (P < 0.001) progesterone production in a dose responsive manner. EGF stimulated cell proliferation (P < 0.001) and progesterone production (P < 0.001), but inhibited androstenedione production (P < 0.001), in a dose responsive manner. In conclusion, this culture system exhibits physiologically relevant responses to known in vivo modulators of follicle development. The biphasic nature of the theca cell response to LH emphasises the exquisite sensitivity of theca cells to LH stimulation and highlights the importance of dose–response relationships in the gonadotrophic control of ovarian function.




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