THE ESTABLISHMENT OF A NEW BIOLOGICAL ASSAY SYSTEM FOR SIMULTANEOUS MEASUREMENT OF BONE RESORPTION AND BONE MINERALIZATION IN ORGAN CULTURES OF CHICK EMBRYONIC FEMUR
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概要
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A biological assay system has been developed for the simultaneous measurement of bone resorption and bone mineralization. In this system we (1) used chick embryonic femur as the biological material because of the easy handling and easy specification of developmental stages compared with rat and mouse, (2) labeled bone with ^<45>Ca in vitro, (3) calculated the biological half life (T_<1/2>) of ^<45>Ca incorporated into bone salts for quantitative estimation of the bone resorbing activity, and (4) investigated bone-mineralizing activity by determining the calcium content before and after cultivation. Eleven-day-old chick embryonic femur was labeled with ^<45>Ca in a chemically defined medium in vitro and thereafter labeled bones were transferred to chase medium. T_<1/2> was calculated from the sequential release of the label into the medium from the cultured bone. No one heretofore had determined the T_<1/2> of Ca in bone salts. We first determined in this study that the T_<1/2> of Ca in the chick embryonic femur is about 50 h. The decrease in T_<1/2> by parathyroid hormone, prostaglandin E_1 and E_2 and lipopolysaccharide, well-known stimulators of bone resorption, showed that this system works well in terms of bone resorption. By using this system, we demonstrated that immunomodulators such as Bacillus Calmette Guerin and Corynebacterium paruvum stimulate bone resorption and therefore affect bone metabolism. On the contrary, sodium fluoride (NaF) and hydrocortisone increased T_<1/2>, indicating that they inhibit bone resorption. These agents were also tested to determine if they would alter total calcium in the bone during cultivation. Those which resulted in the shortening of T_<1/2> decreased total calcium during the cultivation period, probably because they stimulated bone resorption. On the contrary, NaF increased calcium content during cultivation. Fluorine ion, therefore, keeps bone hard not only by its direct incorporation into bone salts but also by aiding the accumulation of calcium into bone salts by inhibiting bone resorption. 1α, 25-dihydroxyvitamin D_3 and calcitonin, known as a stimulator and an inhibitor of bone resorption, respectively, had no effect on the T_<1/2> in this system, indicating that some of the agents which affect bone resorption are not evaluated in this system. Our system, however, offers a simple and quantitative method for simultaneous measurement of bone resorption and bone mineralization. Therefore, we can use this system as the initial assay system for the identification of new drugs for the treatment of bone disease, even though there are some limitations in this system.
- 公益社団法人日本薬学会の論文
著者
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Endo Hiroyoshi
Research Development Corporation Of Japan:(present Address)research Laboratories Sumitomo Pharmaceut
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SAITO Makoto
Research and Development Division, Kikkoman Corporation
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Saito Makoto
Research And Development Division Kikkoman Corporation
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Kawashima Kohtaro
Research Development Corporation Of Japan:(present Address)research Laboratories Sumitomo Pharmaceut
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Saito Makoto
Research Development Corporation Of Japan:(present Address)research Laboratories Sumitomo Pharmaceut
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Saito Makoto
Research & Development Division Kikkoman Corporation
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