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机构地区:[1]中国科学院上海药物研究所 [2]核医学国家重点实验室
出 处:《生理学报》1999年第1期65-72,共8页Acta Physiologica Sinica
基 金:国家自然科学基金
摘 要:为了进一步阐明SPD对大鼠纹状体突触后D1受体的激动作用特性,本文应用反磷酸化在体内测定及放射配体结合方法,分别观察SPD对6OHDA损毁大鼠纹状体DARPP32体内磷酸化作用及突触后D1受体密度的影响。结果表明:皮下给予SPD(20,40mg/kg,21d),损毁侧纹状体DARPP32体外[32P]的掺入量较健侧下降50%(P<001)。换言之,损毁侧纹状体内DARPP32的磷酸化程度增加了。然而,SPD使损毁导致D1受体上调的作用减弱(Bmax从3850±261fmol/mg降至3197±201fmol/mg水平)。因此,SPD激动D1受体,使6OHDA损毁大鼠纹状体内DARPP32磷酸化作用加强,而受体密度减少。这是SPD调节脑内D1受体信号转导功能的重要机制。In order to explore the characteristics of l stepholidine (SPD) activating the postsynaptic D 1 receptors, the effects of SPD on DARPP 32 phosphorylation in vivo with back phosphorylation assay and on the postsynaptic D 1 receptor densities with radioligand assay were observed in the striatum of 6 OHDA lesioned rat. The results showed that following subcutaneously administration of 20 or 40 mg/kg SPD for 21 d, [ 32 P]phosphate incorporation into the DARPP 32 protein in the denervated striatum showed a 50% reduction ( P <0 01) vs the intact striatum, indicating an increase of DARPP 32 phosphorylation in vivo in the denervated striatum. However, the D 1 receptor B max was decreased from 385 0±26 1 to 319 7±20 1 fmol/mg protein. It is suggested that D 1 agonist action of SPD decreases the D 1 receptor density but increases the phosphorylation of DARPP 32 in the striatum of 6 OHDA lesioned rat, which may be responsible for the regulation of D 1 receptor signal transduction in brain neurons.
关 键 词:左旋千金藤啶碱 DARPP-32 磷酸化 6-OHDA
分 类 号:R338.13[医药卫生—人体生理学]
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