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丙酸睾酮与胰岛素在骨再生和生长中的作用

[Role of testosterone propionate and insulin in the regeneration and growth of bone].

作者信息

Nishimura S

机构信息

Department of Dental Pharmacology, Meikai University School of Dentistry, Saitama, Japan.

出版信息

Meikai Daigaku Shigaku Zasshi. 1990;19(3):291-309.

PMID:2152002
Abstract

In order to clarify the effects of androgens and insulin (Ins) on the growth and regeneration of bone in growing rats, and to examine the interaction of the two hormones on the bone growth and regeneration, I carried out both in vivo and in vitro experiments using male rats and clonal osteoblastic cells, respectively. In vivo: 1) Three week-old male rats were castrated, and one week after the castration two holes were drilled into their calvariae, followed by subcutaneous administration of 2 mg/kg of testosterone propionate (TP) and/or 20 mg/kg of cyproterone acetate (CPA). After the daily administration of the drugs for two weeks, the calvariae containing wound holes were isolated, and a soft X-ray photograph was taken. The area of the hole in the X-ray film was measured. The calcium (Ca) and the hydroxyproline (HP) contents and alkaline phosphatase (ALPase) activity in the wound and non-wound portions of the calvariae were also determined. 2) Streptozotocin (STZ, 80 mg/kg) was administered intravenously to immature male rats (25-day-old); and three days after the administration, wound holes were made in their calvariae. Ins (10 units/kg) and/or TP (2 mg/kg) were/was administered daily for two weeks starting two weeks after the operation. The length and weight of the femur, and the area of the hole of the calvariae seen in a soft X-ray photograph were measured. The Ca and HP contents in the wound portion, and serum Ca and phosphate (P) levels and ALPase activity were also determined. In vitro: Mouse clonal osteoblastic cells (MC3T3-E1) were incubated in alpha-MEM mudium containing 10% FBS or 0.1% BSA with or without 10(-9)-10(-6) M TP and/or 10(-9)-10(-6) M Ins, the number of cells was counted, and [3H] thymidine incorporation into the cells was assayed for assessment of DNA synthesis. ALPase activity of the cells was also assayed. The results obtained were as follows: 1. The reduction in the wound-hole area was significantly delayed after the castration and was accelerated by TP. This effect of TP was inhibited about 60% by the simultaneous administration of CPA, though this inhibition was not statistically significant. 2. The reduction in HP content of the wound portion by castration was inhibited by TP, and this effect was antagonized by CPA.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

为了阐明雄激素和胰岛素(Ins)对生长中大鼠骨骼生长和再生的影响,并研究这两种激素在骨骼生长和再生方面的相互作用,我分别使用雄性大鼠和克隆成骨细胞进行了体内和体外实验。体内实验:1)对3周龄雄性大鼠进行阉割,阉割1周后在其颅骨上钻两个孔,随后皮下注射2mg/kg丙酸睾酮(TP)和/或20mg/kg醋酸环丙孕酮(CPA)。每天给药两周后,分离含有伤口孔的颅骨,并拍摄软X线照片。测量X线片上孔的面积。还测定了颅骨伤口和非伤口部分的钙(Ca)、羟脯氨酸(HP)含量以及碱性磷酸酶(ALPase)活性。2)对未成熟雄性大鼠(25日龄)静脉注射链脲佐菌素(STZ,80mg/kg);给药3天后,在其颅骨上制造伤口孔。从手术后两周开始,每天注射Ins(10单位/kg)和/或TP(2mg/kg),持续两周。测量股骨的长度和重量,以及软X线照片中颅骨孔的面积。还测定了伤口部分的Ca和HP含量、血清Ca和磷酸盐(P)水平以及ALPase活性。体外实验:将小鼠克隆成骨细胞(MC3T3-E1)在含有10%胎牛血清或0.1%牛血清白蛋白的α-MEM培养基中培养,添加或不添加10⁻⁹ - 10⁻⁶ M的TP和/或10⁻⁹ - 10⁻⁶ M的Ins,计数细胞数量,并检测[³H]胸腺嘧啶核苷掺入细胞的情况以评估DNA合成。还检测了细胞的ALPase活性。得到的结果如下:1. 阉割后伤口孔面积的减小明显延迟,TP可加速这种减小。同时给予CPA可使TP的这种作用受到约60%的抑制,尽管这种抑制无统计学意义。2. 阉割导致的伤口部分HP含量降低可被TP抑制,且这种作用可被CPA拮抗。(摘要截断于400字)

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