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在大鼠肝脏中,ecto-5'-核苷酸酶/CD73 与特定的 NTPDases 的共表达差异调节腺苷的形成。

Coexpression of ecto-5'-nucleotidase/CD73 with specific NTPDases differentially regulates adenosine formation in the rat liver.

机构信息

Centre de Recherche en Rhumatologie et Immunologie, Québec, QC, Canada.

出版信息

Am J Physiol Gastrointest Liver Physiol. 2012 Feb 15;302(4):G447-59. doi: 10.1152/ajpgi.00165.2011. Epub 2011 Dec 1.

Abstract

Ectonucleotidases modulate purinergic signaling by hydrolyzing ATP to adenosine. Here we characterized the impact of the cellular distribution of hepatic ectonucleotidases, namely nucleoside triphosphate diphosphohydrolase (NTPDase)1/CD39, NTPDase2/CD39L1, NTPDase8, and ecto-5'-nucleotidase/CD73, and of their specific biochemical properties, on the levels of P1 and P2 receptor agonists, with an emphasis on adenosine-producing CD73. Immunostaining and enzyme histochemistry showed that the distribution of CD73 (protein and AMPase activity) overlaps partially with those of NTPDase1, -2, and -8 (protein levels and ATPase and ADPase activities) in normal rat liver. CD73 is expressed in fibroblastic cells located underneath vascular endothelial cells and smooth muscle cells, which both express NTPDase1, in portal spaces in a distinct fibroblast population next to NTPDase2-positive portal fibroblasts, and in bile canaliculi, together with NTPDase8. In fibrotic rat livers, CD73 protein expression and activity are redistributed but still overlap with the NTPDases mentioned. The ability of the observed combinations of ectonucleotidases to generate adenosine over time was evaluated by reverse-phase HPLC with the recombinant rat enzymes at high "inflammatory" (500 μM) and low "physiological" (1 μM) ATP concentrations. Overall, ATP was rapidly converted to adenosine by the NTPDase1+CD73 combination, but not by the NTPDase2+CD73 combination. In the presence of NTPDase8 and CD73, ATP was sequentially dephosphorylated to the CD73 inhibitor ADP, and then to AMP, thus resulting in a delayed formation of adenosine. In conclusion, the specific cellular cocompartmentalization of CD73 with hepatic NTPDases is not redundant and may lead to the differential activation of P1 and P2 receptors, under normal and fibrotic conditions.

摘要

核苷酸酶通过水解 ATP 为腺苷来调节嘌呤能信号。在这里,我们描述了肝外核苷酸酶的细胞分布,即核苷三磷酸二磷酸水解酶 (NTPDase)1/CD39、NTPDase2/CD39L1、NTPDase8 和外核苷酸酶/CD73,以及它们特定的生化特性,对 P1 和 P2 受体激动剂水平的影响,重点是产生腺苷的 CD73。免疫染色和酶组织化学显示,CD73(蛋白和 AMPase 活性)的分布与正常大鼠肝中 NTPDase1、-2 和 -8(蛋白水平以及 ATPase 和 ADPase 活性)的分布部分重叠。CD73 在血管内皮细胞和平滑肌细胞下方的成纤维细胞中表达,NTPDase1 也在这些细胞中表达,在门脉空间中,NTPDase2 阳性的门脉成纤维细胞旁有一个独特的成纤维细胞群体,在胆小管中,与 NTPDase8 一起表达。在纤维化大鼠肝脏中,CD73 蛋白表达和活性重新分布,但仍与上述 NTPDases 重叠。通过在高“炎症”(500 μM)和低“生理”(1 μM)ATP 浓度下用重组大鼠酶进行反相高效液相色谱法评估了观察到的外核苷酸酶组合随时间产生腺苷的能力。总体而言,NTPDase1+CD73 组合可快速将 ATP 转化为腺苷,但 NTPDase2+CD73 组合则不能。在存在 NTPDase8 和 CD73 的情况下,ATP 依次被磷酸化为 CD73 抑制剂 ADP,然后转化为 AMP,从而导致腺苷的形成延迟。总之,在正常和纤维化条件下,CD73 与肝 NTPDases 的特定细胞共位不是多余的,可能导致 P1 和 P2 受体的差异激活。

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