Yasuda Yoshiyuki, Saito Masaru, Yamamura Takehira, Yaguchi Takahiro, Nishizaki Tomoyuki
Department of Physiology, Hyogo College of Medicine, 1-1 Mukogawa, Nishinomiya, 663-8501, Japan.
J Gastroenterol. 2009;44(1):56-65. doi: 10.1007/s00535-008-2273-7. Epub 2009 Jan 22.
Extracellular adenosine has been shown to induce apoptosis in a variety of cells via an intrinsic pathway linked to adenosine uptake into cells and the ensuing signaling cascades and an extrinsic pathway linked to adenosine receptors. The present study was designed to understand the mechanism underlying adenosine-induced apoptosis of Caco-2 human colonic cancer cells.
To observe cell viability, an MTT assay was carried out in Caco-2 cells untransfected or transfected with the A(2a) adenosine receptor pcDNA3.1. Apoptotic cell death was assessed with flow cytometry using propidium iodide and annexin V and internucleosomal DNA fragmentation analysis. Activities of caspase-3, -8, and -9 were measured using a caspase fluorometric assay kit. Mitochondrial membrane potentials were monitored using a DePsipher kit. Expression of adenosine receptors was examined with the reverse transcription-polymerase chain reaction (RT-PCR) method.
Extracellular adenosine induced Caco-2 cell apoptosis in a concentration-dependent (1-20 mM) and treatment time-dependent (24-72 h) manner. The adenosine effect was inhibited by DMPX, an inhibitor of A(2a) adenosine receptors and SQ22536, an inhibitor of adenylate cyclase. CGS21680, an agonist of A(2a) adenosine receptors, and forskolin, an adenylate cyclase activator, mimicked the adenosine action. Caco-2 cell death was still induced by overexpressing A(2a) adenosine receptors, and adenosine further promoted the cell death. Adenosine disrupted mitochondrial membrane potentials and activated caspase-9 and -3, but not caspase-8.
Extracellular adenosine induces apoptosis in Caco-2 cells by activating caspase-9 and the downstream effector caspase caspase-3 in association with mitochondrial damage via A(2a) adenosine receptors.
细胞外腺苷已被证明可通过与腺苷摄入细胞及随后的信号级联相关的内在途径以及与腺苷受体相关的外在途径,诱导多种细胞发生凋亡。本研究旨在了解腺苷诱导Caco-2人结肠癌细胞凋亡的潜在机制。
为观察细胞活力,对未转染或转染了A(2a)腺苷受体pcDNA3.1的Caco-2细胞进行MTT试验。使用碘化丙啶和膜联蛋白V通过流式细胞术以及核小体间DNA片段分析评估凋亡细胞死亡情况。使用半胱天冬酶荧光检测试剂盒测量半胱天冬酶-3、-8和-9的活性。使用DePsipher试剂盒监测线粒体膜电位。采用逆转录-聚合酶链反应(RT-PCR)方法检测腺苷受体的表达。
细胞外腺苷以浓度依赖性(1-20 mM)和处理时间依赖性(24-72小时)的方式诱导Caco-2细胞凋亡。A(2a)腺苷受体抑制剂DMPX和腺苷酸环化酶抑制剂SQ22536可抑制腺苷的作用。A(2a)腺苷受体激动剂CGS21680和腺苷酸环化酶激活剂福斯可林模拟了腺苷的作用。过表达A(2a)腺苷受体仍可诱导Caco-2细胞死亡,且腺苷进一步促进细胞死亡。腺苷破坏线粒体膜电位并激活半胱天冬酶-9和-3,但不激活半胱天冬酶-8。
细胞外腺苷通过A(2a)腺苷受体激活半胱天冬酶-9和下游效应半胱天冬酶半胱天冬酶-3,并伴有线粒体损伤,从而诱导Caco-2细胞凋亡。
