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首页> 外文期刊>The Journal of Experimental Biology >The role of muscarinic receptors and intracellular Ca2+ in the spectral reflectivity changes of squid iridophores
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The role of muscarinic receptors and intracellular Ca2+ in the spectral reflectivity changes of squid iridophores

机译:毒蕈碱受体和细胞内Ca2 +在鱿鱼虹吸体光谱反射率变化中的作用

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In this paper we describe changes in spectral reflectivity of the light reflectors (iridophores) of the squid Alloteuthis subulata. The spectral changes that can be seen in living squid, can also be brought about by superfusing whole skin preparations with acetylcholine (ACh) (20 micro mol l(-1)) and muscarine (30 micro mol l(-1)) but not nicotine (up to 50 mmol l(-1)), suggesting that cholinergic muscarinic receptors are involved. Changing the osmolarity of the external solution had no effect on spectral reflectivity. To study the iridophores at the cellular level, iridophores were isolated enzymatically. Lucifer Yellow filled the iridophores uniformly, showing cellular individuality. Isolated iridophore cells were loaded with Fura-2 AM and cytoplasmic Ca(2+) was recorded ratiometrically. Intracellular Ca(2+) (resting concentration at 66.16 nmol l(-1)) increased transiently after addition of ACh (50 micro mol l(-1)), muscarine (25 micro mol l(-1)), but not nicotine (up to 5 mmol l(-1)). Ca(2+) also increased when superfused with potassium chloride (10 mmol l(-1)) and caffeine (2.5 mmol l(-1)). Hypo- and hyperosmotic solutions had no effects on the cytoplasmic Ca(2+). By presenting direct evidence that iridophores are polarised cellular structures containing Ca(2+) stores and that they are activated via cholinergic muscarinic receptors, we demonstrate that Ca(2+) is involved in the reflectivity changes of the iridophores of A. subulata. Specimens were prepared for transmission electron microscopy. It was found that the orientations of the plates with respect to the skin surface are in good agreement with the expected orientations based on the prediction that the iridophores act as multilayer reflectors.
机译:在本文中,我们描述了鱿鱼Alloteuthis subulata的光反射器(虹膜)的光谱反射率变化。在活鱿鱼中可以看到的光谱变化也可以通过将整个皮肤制剂与乙酰胆碱(ACh)(20 micro mol l(-1))和毒蕈碱(30 micro mol l(-1))融合来实现,但不能尼古丁(最高50 mmol l(-1)),提示胆碱能毒蕈碱受体参与其中。改变外部溶液的渗透压对光谱反射率没有影响。为了在细胞水平上研究iridophores,通过酶法分离iridophores。路西法·黄(Lucifer Yellow)均匀地填充了虹膜,显示出细胞的个性。分离的虹膜细胞加载Fura-2 AM,并按比例记录细胞质Ca(2+)。加入ACh(50 micro mol l(-1)),毒蕈碱(25 micro mol l(-1))而非尼古丁后,细胞内Ca(2+)(在66.16 nmol l(-1)处的静止浓度)瞬时增加(至多5 mmol l(-1))。当与氯化钾(10 mmol l(-1))和咖啡因(2.5 mmol l(-1))融合时,Ca(2+)也增加。低渗和高渗溶液对细胞质的Ca(2+)没有影响。通过提供直接的证据,iridophores是极化的细胞结构,包含Ca(2+)存储,并通过胆碱能毒蕈碱受体被激活,我们证明Ca(2+)参与了A. subulata iridophores的反射率变化。准备用于透射电子显微镜的样品。根据对虹彩体充当多层反射体的预测,发现板相对于皮肤表面的取向与预期取向非常一致。

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