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血清诱导的哺乳动物视网膜神经胶质细胞生理变化:溶血磷脂酸的作用

Serum-induced changes in the physiology of mammalian retinal glial cells: role of lysophosphatidic acid.

作者信息

Kusaka S, Kapousta-Bruneau N, Green D G, Puro D G

机构信息

Department of Ophthalmology, University of Michigan, Ann Arbor 48105, USA.

出版信息

J Physiol. 1998 Jan 15;506 ( Pt 2)(Pt 2):445-58. doi: 10.1111/j.1469-7793.1998.445bw.x.

Abstract
  1. With a breakdown of the vascular-CNS barrier, serum enters the nervous system. Although this is a frequent pathophysiological event, knowledge of the effects of serum on the function of the nervous system is limited. In this study, we examined the effects of serum on the activity of ion channels in Müller cells: the principal glia of the retina. 2. Freshly dissociated Müller cells from the bovine and human retina were studied with the perforated-patch configuration of the patch clamp technique. In other experiments, electroretinograms (ERGs) were recorded from isolated rat retinas. 3. Perforated-patch recordings revealed that serum induced a calcium-permeable, non-specific cation (NSC) current. Approximately 40 s after induction of this current, an outwardly rectifying K+ current was also detected. Sensitivity to charybdotoxin and margatoxin indicated that this K+ current was due to the activation of Kv1.3 channels. This increase in the Kv1.3 current was dependent on extracellular calcium. 4. The NSC and Kv1.3 currents were activated by serum in 100% and 95% of the sampled Müller cells, respectively. Also, in a minority (21%) of the cells, the inwardly rectifying K+ current was inhibited slightly. These changes in ion channel activity were associated with depolarization of the Müller cells. 5. We hypothesized that activation of NSC channels would reduce the siphoning of K+ via the Müller cells. Consistent with this idea, ERGs from isolated retinas showed serum-induced reductions in the slow PIII component, which is generated by Müller cells responding to light-evoked changes in the extracellular K+ concentration. 6. Lysophosphatidic acid (LPA), a component of serum, had effects on Müller cells that were qualitatively similar to those induced by serum. 7. Our observations demonstrate that exposure to serum alters the activity of multiple types of ion channels in Müller glial cells of the mammalian retina. When there is a breakdown of the blood-retina barrier, LPA may be one of the serum-derived molecules which regulates the physiology of Müller cells.
摘要
  1. 随着血管 - 中枢神经系统屏障的破坏,血清进入神经系统。尽管这是一种常见的病理生理事件,但关于血清对神经系统功能影响的了解却很有限。在本研究中,我们检测了血清对 Müller 细胞(视网膜主要神经胶质细胞)中离子通道活性的影响。2. 采用膜片钳技术的穿孔膜片配置研究了从牛和人视网膜新鲜分离的 Müller 细胞。在其他实验中,从分离的大鼠视网膜记录视网膜电图(ERG)。3. 穿孔膜片记录显示血清诱导了一种钙通透性非特异性阳离子(NSC)电流。在诱导该电流后约40秒,还检测到外向整流钾电流。对蝎毒素和玛格毒素的敏感性表明该钾电流是由于Kv1.3通道的激活。Kv1.3电流的这种增加依赖于细胞外钙。4. NSC电流和Kv1.3电流分别在100%和95%的采样Müller细胞中被血清激活。此外,在少数(21%)细胞中,内向整流钾电流略有抑制。离子通道活性的这些变化与Müller细胞的去极化有关。5. 我们假设NSC通道的激活会减少通过Müller细胞对钾离子的虹吸作用。与此观点一致,分离视网膜的ERG显示血清诱导慢PIII成分减少,慢PIII成分是由Müller细胞对细胞外钾离子浓度的光诱发变化作出反应而产生的。6. 溶血磷脂酸(LPA)是血清的一种成分,对Müller细胞的作用在性质上与血清诱导的作用相似。7. 我们的观察结果表明,暴露于血清会改变哺乳动物视网膜Müller神经胶质细胞中多种类型离子通道的活性。当血视网膜屏障破坏时,LPA可能是调节Müller细胞生理学的血清衍生分子之一。

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