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ADP-sensitive purinoceptors induce steroidogenesis via adenylyl cyclase activation in bovine adrenocortical fasciculata cells

机译:ADP敏感的嘌呤受体通过牛肾上腺皮质筋膜细胞中的腺苷酸环化酶激活诱导类固醇生成

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摘要

The role of P2Y receptors in the production of cAMP and the activation of protein kinase A (PKA) was studied with respect to the regulation of the steroidogenesis in primary cultures of bovine adrenocortical fasciculata cells (BAFCs).ADP and ATP stimulated cAMP production with EC50 values of 23.7±6.8 μM and 40.1±5.5 μM, respectively. In contrast, the EC50 of BzATP for cAMP production was 153.0±37.4 μM. Adenosine and AMP (0.1–1000 μM) were much less effective than ADP and ATP. 2MeSADP and UTP did not exert detectable effects. ADP (10 and 100 μM) significantly stimulated steroidogenesis; the process was blocked by an adenylyl cyclase inhibitor SQ22536 (100 μM) but not by the P2Y1 receptor antagonist MRS2179 (100 μM).Real-time imaging of the PKA activity with the dye ARII, which became less fluorescent upon phosphorylation, revealed that ADP (100 μM) immediately activated PKA. These effects could be mimicked by forskolin (100 μM) and were blocked by the PKA inhibitor H89 (50 μM). UTP (100 μM) did not activate PKA.The cytoplasm harvested from morphologically and electrophysiologically identified single BAFCs contained mRNA for P2Y2 but not for P2Y1, P2Y4, P2Y11 or P2Y12 receptors, as confirmed by single-cell RT–PCR amplification (50 cycles).These results suggest an expression of an ADP-sensitive Gs-coupled purinoceptor in BAFCs. We propose that this not yet described type of P2Y receptor might mediate the extracellular purine-activated steroidogenesis via cAMP/PKA-mediated pathways, independently from the pathways involving InsP3 production and consequent intracellular Ca2+ increase.
机译:研究了P2Y受体在cAMP产生和蛋白激酶A(PKA)激活中对牛肾上皮束状细胞(BAFC)原代培养中类固醇生成的调节作用.ADP和ATP通过EC50刺激cAMP产生分别为23.7±6.8μM和40.1±5.5μM。相反,BzATP对cAMP产生的EC50为153.0±37.4μM。腺苷和AMP(0.1–1000μM)的效力远低于ADP和ATP。 2MeSADP和UTP没有发挥可检测的作用。 ADP(10和100μM)显着刺激了类固醇生成;该过程被腺苷酸环化酶抑制剂SQ22536(100μM)阻断,但未被P2Y1受体拮抗剂MRS2179(100μM)阻断。染料ARII实时成像显示PKA活性,该染料在磷酸化后荧光减弱,表明ADP (100μM)立即激活PKA。这些作用可以被毛喉素(100μM)模仿,并被PKA抑制剂H89(50μM)阻断。 UTP(100μM)不会激活PKA。通过单细胞RT-PCR扩增(50个循环)证实,从形态和电生理学上鉴定的单个BAFC收集的细胞质中含有P2Y2的mRNA,但不含P2Y1,P2Y4,P2Y11或P2Y12受体的mRNA。这些结果表明ADP敏感的Gs偶联嘌呤受体在BAFC中的表达。我们建议这种尚未描述的P2Y受体类型可能通过cAMP / PKA介导的途径介导细胞外嘌呤激活的类固醇生成,独立于涉及InsP3产生和随后细胞内Ca2 +增加的途径。

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