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生长激素对大鼠脂肪组织和分离的大鼠脂肪细胞中胰岛素样生长因子-I mRNA的调节作用。

Growth hormone regulation of insulin-like growth factor-I mRNA in rat adipose tissue and isolated rat adipocytes.

作者信息

Vikman K, Isgaard J, Edén S

机构信息

Department of Physiology, University of Göteborg, Sweden.

出版信息

J Endocrinol. 1991 Oct;131(1):139-45. doi: 10.1677/joe.0.1310139.

Abstract

The effects of hypophysectomy and hormonal replacement therapy on insulin-like growth factor-I (IGF-I) mRNA in rat adipose tissue and adipocytes were studied. The effects of GH and IGF-I in vitro on IGF-I mRNA and IGF-I production were also studied in cultured rat adipocytes. Male rats were hypophysectomized at about 50 days of age and given replacement therapy with cortisol (400 micrograms/kg per day) and thyroxine (10 micrograms/kg per day). GH was given as a single i.v. or s.c. injection and also as a continuous s.c. infusion for 6 days. Epididymal fat pads were excised and used either for isolation of adipocytes or for determination of IGF-I mRNA in adipose tissue. A solution hybridization assay was used. The IGF-I mRNA content of adipocytes was analysed either immediately after isolation or after short-term (2-3 days) culture with or without GH or IGF-I. Hypophysectomy resulted in a marked decrease in IGF-I mRNA in both tissue and cells. Replacement therapy (in vivo) with cortisol and thyroxine alone had no effect, whereas additional treatment with GH caused a dose-dependent increase in IGF-I mRNA. IGF-I mRNA was also increased after a continuous s.c. infusion of GH. A single i.v. injection of GH (100 micrograms) resulted in an increase in IGF-I mRNA after approximately 2 h, with maximal levels around 6 h after the injection. In cultured adipocytes, addition of GH to the culture medium increased IGF-I mRNA in a dose-dependent manner and a marked increase was observed with a concentration of GH of 1 ng/ml. Addition of IGF-I (100 ng/ml) had no effect. The increase in IGF-I mRNA after addition of GH (100 ng/ml) was detectable after 3 h. The concentration of IGF-I in the culture medium was increased 24 h after the addition of GH. These results demonstrate that GH induces IGF-I mRNA in both adipose tissue and isolated fully differentiated adipocytes and that this increase in IGF-I mRNA results in increased IGF-I production.

摘要

研究了垂体切除及激素替代疗法对大鼠脂肪组织和脂肪细胞中胰岛素样生长因子-I(IGF-I)mRNA的影响。还在培养的大鼠脂肪细胞中研究了体外生长激素(GH)和IGF-I对IGF-I mRNA及IGF-I产生的影响。雄性大鼠在约50日龄时接受垂体切除,并给予皮质醇(400微克/千克/天)和甲状腺素(10微克/千克/天)进行替代疗法。GH通过单次静脉内或皮下注射给药,也通过皮下持续输注给药6天。切除附睾脂肪垫,用于分离脂肪细胞或测定脂肪组织中的IGF-I mRNA。采用溶液杂交测定法。脂肪细胞的IGF-I mRNA含量在分离后立即分析,或在添加或不添加GH或IGF-I的情况下短期(2 - 3天)培养后分析。垂体切除导致组织和细胞中的IGF-I mRNA显著降低。单独使用皮质醇和甲状腺素进行替代疗法(体内)没有效果,而额外给予GH导致IGF-I mRNA呈剂量依赖性增加。皮下持续输注GH后IGF-I mRNA也增加。单次静脉注射GH(100微克)在约2小时后导致IGF-I mRNA增加,注射后约6小时达到最高水平。在培养的脂肪细胞中,向培养基中添加GH以剂量依赖性方式增加IGF-I mRNA,当GH浓度为1纳克/毫升时观察到显著增加。添加IGF-I(100纳克/毫升)没有效果。添加GH(100纳克/毫升)后3小时可检测到IGF-I mRNA增加。添加GH后24小时培养基中IGF-I的浓度增加。这些结果表明,GH在脂肪组织和分离的完全分化脂肪细胞中均诱导IGF-I mRNA,且这种IGF-I mRNA的增加导致IGF-I产生增加。

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