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首页> 外文期刊>Brain research >Involvement of nitric oxide synthase and ROS-mediated activation of L-type voltage-gated Ca2+ channels in NMDA-induced DPYSL3 degradation.
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Involvement of nitric oxide synthase and ROS-mediated activation of L-type voltage-gated Ca2+ channels in NMDA-induced DPYSL3 degradation.

机译:一氧化氮合酶的参与和ROS介导的NMDA诱导的DPYSL3降解中L型电压门控Ca2 +通道的激活。

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Dihydropyrimidinase-like 3 (DPYSL3), a member of TUC (TOAD-64/Ulip/CRMP), is believed to play a role in neuronal differentiation, axonal outgrowth and possibly in neuronal regeneration. Recently, we have shown that in primary cortical neurons (PCN) NMDA and oxidative stress (H(2)O(2)) caused a calpain-dependent cleavage of DPYSL3 (62 kDa) resulting in the appearance of a lower molecular weight form (60 kDa) of DPYSL3. Our preliminary results had shown that antioxidants significantly reduced NMDA-induced DPYSL3 degradation, indicating involvement of ROS in calpain activation. The aim of this study was to investigate the possible involvement of NOS in NMDA-induced DPYSL3 degradation. We found that NOS inhibitor (L-NAME) significantly prevented NMDA-induced ROS formation, as well as intracellular Ca(2+) increase [Ca(2+)](i), DPYSL3 degradation and cell death. Further, exposure of PCN to NO donor (SNP) resulted in significant [Ca(2+)](i) increase, ROS generation and probable calpain-mediated DPYSL3 truncation. The NMDA- and oxidative stress (ROS)-induced DPYSL3 truncation was totally dependent on extracellular [Ca(2+)](i). While NMDA-induced DPYSL3 truncation was blocked by both NMDA receptor antagonist (MK801) [Kowara, R., Chen, Q., Milliken, M., Chakravarthy, B., 2005. Calpain-mediated degradation of dihydropyrimidinase-like 3 protein (DPYSL3) in response to NMDA and H(2)O(2) toxicity. J. Neurochem. 95 (2), 466-474] and L-VGCC (nimodipine) inhibitors, H(2)O(2)-induced increase in [Ca(2+)](i), ROS generation and DPYSL3 truncation was blocked only by nimodipine. These results indicate that changes in Ca(2+) homeostasis resulting from ROS-dependent activation of L-VGCC are sufficient to induce probable calpain-mediated DPYSL3 truncation and demonstrate for the first time the role of ROS in the mechanism leading to glutamate-induced calpain activation and DPYSL3 protein degradation. The probable calpain-mediated DPYSL3 truncation may have significant impact on its interaction with actin and its assembly, and in turn on growth cone integrity.
机译:TUC(TOAD-64 / Ulip / CRMP)成员二氢嘧啶酶样3(DPYSL3)被认为在神经元分化,轴突生长以及可能在神经元再生中起作用。最近,我们已经表明,在初级皮层神经元(PCN)中,NMDA和氧化应激(H(2)O(2))引起了DPYSL3(62 kDa)的钙蛋白酶依赖性裂解,从而导致了较低分子量形式的出现( 60 kDa)的DPYSL3。我们的初步结果表明,抗氧化剂可显着降低NMDA诱导的DPYSL3降解,表明ROS参与了钙蛋白酶的活化。这项研究的目的是调查NOS可能参与NMDA诱导的DPYSL3降解。我们发现,NOS抑制剂(L-NAME)可以显着阻止NMDA诱导的ROS形成,以及细胞内Ca(2+)增加[Ca(2 +)](i),DPYSL3降解和细胞死亡。此外,PCN暴露于NO供体(SNP)导致[Ca(2 +)](i)显着增加,ROS生成和可能的钙蛋白酶介导的DPYSL3截短。 NMDA和氧化应激(ROS)诱导的DPYSL3截短完全取决于细胞外[Ca(2 +)](i)。虽然NMDA诱导的DPYSL3截短被两个NMDA受体拮抗剂(MK801)阻断[Kowara,R.,Chen,Q.,Milliken,M.,Chakravarthy,B.,2005。钙蛋白酶介导的二氢嘧啶酶样3蛋白降解( DPYSL3)响应NMDA和H(2)O(2)毒性。 J.神经化学。 95(2),466-474]和L-VGCC(尼莫地平)抑制剂,H(2)O(2)诱导的[Ca(2 +)](i)增加,ROS生成和DPYSL3截短仅由尼莫地平。这些结果表明,由ROS依赖性激活L-VGCC引起的Ca(2+)稳态变化足以诱导可能的钙蛋白酶介导的DPYSL3截短,并首次证明了ROS在导致谷氨酸诱导的机制中的作用。钙蛋白酶激活和DPYSL3蛋白降解。钙蛋白酶介导的DPYSL3截短可能对其与肌动蛋白的相互作用及其组装产生重大影响,进而对生长锥的完整性产生重大影响。

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