Effects of Limited Exposure of Rabbit Chondrocyte Cultures to Parathyroid Hormone and Dibutyryl Adenosine 3′,5′-Monophosphate on Cartilage-Characteristic Proteoglycan Synthesis*

Abstract

Treatment of rabbit chondrocyte cultures with PTH or (Bu)₂cAMP for 30 h increased by 2- to 3-fold the incorporation of [³⁵S]sulfate and ³H radioactivity with glucosamine as the precursor into large chondroitin sulfate proteoglycans characteristically found in cartilage matrix. However, PTH and (Bu)₂cAMP did not increase either [³⁵S]sulfate incorporation into small proteoglycans or the incorporation of 3H radioactivity into hyaluronic acid and other glycosaminoglycans. PTH and (Bu)₂cAMP also increased the incorporation of [3H] serine into both proteoglycans and total protein. In all cultures described above, the stimulation of [3H]serine incorporation into proteoglycans exceeded that of [3H]serine incorporation into total protein. These data indicate that PTH and (Bu)₂cAMP selectively stimulate cartilage proteoglycan synthesis while they increase total protein synthesis. Since cAMP seems to play a mediatory role in the action of PTH, we elected to examine the effects of a limited exposure of chondrocytes_to PTH or (Bu)₂cAMP on the synthesis of proteoglycans. Treatment with PTH or (Bu)₂cAMP for only the initial 2-7 h “dldTTOf increase the rates of incorporation of [³⁵S] sulfate, the 3H radioactivity with glucosamine, and [3H]serine into proteoglycans, as measured at 30 h, despite the fact that this treatment brought about a rapid and transient rise in the cAMP level. Furthermore, the application of prostaglandin I2 at concentrations that increased cAMP levels in a similar fashion as did PTH did not affect [38S] sulfate incorporation into proteoglycans. These observations suggest that in addition to the transient rise of cAMP, other biochemical changes are required for elaboration of the effect of PTH on proteoglycan synthesis. Although cAMP analogs mimic some of the effects of PTH in chondrocytes, the nucleotides and PTH appear to stimulate proteoglycan synthesis by different mechanisms. (Endocrinology122: 1991–1997, 1988)