膜磷脂酰肌醇-4,5-二磷酸与受体介导的天然神经元M通道抑制之间的关系
Relationship between membrane phosphatidylinositol-4,5-bisphosphate and receptor-mediated inhibition of native neuronal M channels.
作者信息
Winks Joanna S, Hughes Simon, Filippov Alexander K, Tatulian Lucine, Abogadie Fe C, Brown David A, Marsh Stephen J
机构信息
1Ion Channel Pharmacology Group, IPC 388, Pfizer Global Research and Development, Sandwich Laboratories, Sandwich, Kent CT13 9NJ, United Kingdom.
出版信息
J Neurosci. 2005 Mar 30;25(13):3400-13. doi: 10.1523/JNEUROSCI.3231-04.2005.
The relationship between receptor-induced membrane phosphatidylinositol-4'5'-bisphosphate (PIP2) hydrolysis and M-current inhibition was assessed in single-dissociated rat sympathetic neurons by simultaneous or parallel recording of membrane current and membrane-to-cytosol translocation of the fluorescent PIP2/inositol 1,4,5-trisphosphate (IP3)-binding peptide green fluorescent protein-tagged pleckstrin homology domain of phospholipase C (GFP-PLCdelta-PH). The muscarinic receptor agonist oxotremorine-M produced parallel time- and concentration-dependent M-current inhibition and GFP-PLCdelta-PH translocation; bradykinin also produced parallel time-dependent inhibition and translocation. Phosphatidylinositol-4-phosphate-5-kinase (PI5-K) overexpression reduced both M-current inhibition and GFP-PLCdelta-PH translocation by both oxotremorine-M and bradykinin. These effects were partly reversed by wortmannin, which inhibits phosphatidylinositol-4-kinase (PI4-K). PI5-K overexpression also reduced the inhibitory action of oxotremorine-M on PIP2-gated G-protein-gated inward rectifier (Kir3.1/3.2) channels; bradykinin did not inhibit these channels. Overexpression of neuronal calcium sensor-1 protein (NCS-1), which increases PI4-K activity, did not affect responses to oxotremorine-M but reduced both fluorescence translocation and M-current inhibition by bradykinin. Using an intracellular IP3 membrane fluorescence-displacement assay, initial mean concentrations of membrane [PIP2] were estimated at 261 microm (95% confidence limit; 192-381 microm), rising to 693 microm (417-1153 microm) in neurons overexpressing PI5-K. Changes in membrane [PIP2] during application of oxotremorine-M were calculated from fluorescence data. The results, taken in conjunction with previous data for KCNQ2/3 (Kv7.2/Kv7.3) channel gating by PIP2 (Zhang et al., 2003), accorded with the hypothesis that the inhibitory action of oxotremorine-M on M current resulted from depletion of PIP2. The effects of bradykinin require additional components of action, which might involve IP3-induced Ca2+ release and consequent M-channel inhibition (as proposed previously) and stimulation of PIP2 synthesis by Ca2+-dependent activation of NCS-1.
通过同时或平行记录膜电流以及与荧光磷脂酰肌醇-4',5'-二磷酸(PIP2)/肌醇1,4,5-三磷酸(IP3)结合的肽——绿色荧光蛋白标记的磷脂酶C的pleckstrin同源结构域(GFP-PLCδ-PH)从膜到胞质溶胶的转位,在单离的大鼠交感神经元中评估受体诱导的膜PIP2水解与M电流抑制之间的关系。毒蕈碱受体激动剂氧化震颤素-M产生了平行的时间和浓度依赖性的M电流抑制以及GFP-PLCδ-PH转位;缓激肽也产生了平行的时间依赖性抑制和转位。磷脂酰肌醇-4-磷酸-5-激酶(PI5-K)的过表达减少了氧化震颤素-M和缓激肽对M电流的抑制以及GFP-PLCδ-PH转位。渥曼青霉素(一种抑制磷脂酰肌醇-4-激酶(PI4-K)的物质)部分逆转了这些效应。PI5-K过表达还降低了氧化震颤素-M对PIP2门控的G蛋白门控内向整流(Kir3.1/3.2)通道的抑制作用;缓激肽不抑制这些通道。神经元钙传感器-1蛋白(NCS-1)的过表达增加了PI4-K的活性,它不影响对氧化震颤素-M的反应,但减少了缓激肽引起的荧光转位和M电流抑制。使用细胞内IP3膜荧光位移测定法,估计膜[PIP2]的初始平均浓度为261微摩尔(95%置信限;192 - 381微摩尔),在过表达PI5-K的神经元中升至693微摩尔(417 - 1153微摩尔)。根据荧光数据计算了氧化震颤素-M作用期间膜[PIP2]的变化。这些结果与先前关于PIP2对KCNQ2/3(Kv7.2/Kv7.3)通道门控的数据(Zhang等人,2003年)相结合,符合氧化震颤素-M对M电流的抑制作用是由PIP2耗竭引起的这一假设。缓激肽的作用需要其他作用成分,这可能涉及IP3诱导的Ca2+释放以及随之而来的M通道抑制(如先前提出的),以及Ca2+依赖性激活NCS-1对PIP2合成的刺激。
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