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一氧化氮从视网膜无长突细胞的酸性细胞器中释放氯离子。

Nitric oxide releases Cl(-) from acidic organelles in retinal amacrine cells.

作者信息

Krishnan Vijai, Gleason Evanna

机构信息

Department of Biological Sciences, Louisiana State University Baton Rouge, LA, USA.

出版信息

Front Cell Neurosci. 2015 Jun 8;9:213. doi: 10.3389/fncel.2015.00213. eCollection 2015.

Abstract

Determining the factors regulating cytosolic Cl(-) in neurons is fundamental to our understanding of the function of GABA- and glycinergic synapses. This is because the Cl(-) distribution across the postsynaptic plasma membrane determines the sign and strength of postsynaptic voltage responses. We have previously demonstrated that nitric oxide (NO) releases Cl(-) into the cytosol from an internal compartment in both retinal amacrine cells and hippocampal neurons. Furthermore, we have shown that the increase in cytosolic Cl(-) is dependent upon a decrease in cytosolic pH. Here, our goals were to confirm the compartmental nature of the internal Cl(-) store and to test the hypothesis that Cl(-) is being released from acidic organelles (AO) such as the Golgi, endosomes or lysosomes. To achieve this, we made whole cell voltage clamp recordings from cultured chick retinal amacrine cells and used GABA-gated currents to track changes in cytosolic Cl(-). Our results demonstrate that intact internal proton gradients are required for the NO-dependent release of internal Cl(-). Furthermore, we demonstrate that increasing the pH of AO leads to release of Cl(-) into the cytosol. Intriguingly, the elevation of organellar pH results in a reversal in the effects of NO. These results demonstrate that cytosolic Cl(-) is closely linked to the regulation and maintenance of organellar pH and provide evidence that acidic compartments are the target of NO.

摘要

确定调节神经元胞质氯离子(Cl⁻)的因素对于我们理解γ-氨基丁酸(GABA)能和甘氨酸能突触的功能至关重要。这是因为突触后质膜上的Cl⁻分布决定了突触后电压反应的正负和强度。我们之前已经证明,一氧化氮(NO)能使视网膜无长突细胞和海马神经元胞质中的Cl⁻从内部隔室释放到胞质溶胶中。此外,我们还表明胞质Cl⁻的增加依赖于胞质pH值的降低。在这里,我们的目标是确认内部Cl⁻储存的区室性质,并检验Cl⁻从酸性细胞器(AO)如高尔基体、内体或溶酶体释放的假设。为了实现这一目标,我们对培养的鸡视网膜无长突细胞进行了全细胞电压钳记录,并使用GABA门控电流来追踪胞质Cl⁻的变化。我们的结果表明,完整的内部质子梯度是NO依赖性释放内部Cl⁻所必需的。此外,我们证明增加AO的pH值会导致Cl⁻释放到胞质溶胶中。有趣的是,细胞器pH值的升高导致NO的作用发生逆转。这些结果表明胞质Cl⁻与细胞器pH值的调节和维持密切相关,并提供了证据表明酸性区室是NO的作用靶点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/917a/4459082/9dbd3f1cea5e/fncel-09-00213-g0001.jpg

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