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本文引用的文献

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Vasomotor sympathetic neurons are more excitable than secretomotor sympathetic neurons in bullfrog paravertebral ganglia.在牛蛙脊柱旁神经节中,血管运动交感神经元比分泌型交感神经元更易兴奋。
Auton Neurosci. 2010 Jun 24;155(1-2):19-24. doi: 10.1016/j.autneu.2009.12.009. Epub 2010 Jan 27.
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Reporting ethical matters in the Journal of Physiology: standards and advice.《生理学杂志》中的伦理问题报告:标准与建议
J Physiol. 2009 Feb 15;587(Pt 4):713-9. doi: 10.1113/jphysiol.2008.167387.
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The self-tuning neuron: synaptic scaling of excitatory synapses.自调节神经元:兴奋性突触的突触缩放
Cell. 2008 Oct 31;135(3):422-35. doi: 10.1016/j.cell.2008.10.008.
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A carboxy-terminal inter-helix linker as the site of phosphatidylinositol 4,5-bisphosphate action on Kv7 (M-type) K+ channels.一种羧基末端螺旋间连接子作为磷脂酰肌醇4,5-二磷酸作用于Kv7(M型)钾通道的位点。
J Gen Physiol. 2008 Sep;132(3):361-81. doi: 10.1085/jgp.200810007.
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Functional significance of axonal Kv7 channels in hippocampal pyramidal neurons.海马锥体神经元中轴突Kv7通道的功能意义
Proc Natl Acad Sci U S A. 2008 Jun 3;105(22):7869-74. doi: 10.1073/pnas.0802805105. Epub 2008 May 30.
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J Physiol. 2008 Apr 1;586(7):1811-21. doi: 10.1113/jphysiol.2007.148304. Epub 2008 Jan 31.
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Inositol triphosphate-mediated Ca2+ signals direct purinergic P2Y receptor regulation of neuronal ion channels.肌醇三磷酸介导的钙离子信号传导直接调控神经元离子通道的嘌呤能P2Y受体。
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Somatodendritic Kv7/KCNQ/M channels control interspike interval in hippocampal interneurons.体细胞树突状 Kv7/KCNQ/M 通道控制海马中间神经元的峰间间隔。
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9
Excitatory muscarinic modulation strengthens virtual nicotinic synapses on sympathetic neurons and thereby enhances synaptic gain.兴奋性毒蕈碱调节增强了交感神经元上的虚拟烟碱突触,从而提高了突触增益。
J Neurophysiol. 2006 Dec;96(6):3104-13. doi: 10.1152/jn.00589.2006. Epub 2006 Sep 27.
10
Rapid chemically induced changes of PtdIns(4,5)P2 gate KCNQ ion channels.化学诱导下磷脂酰肌醇 -4,5- 二磷酸(PtdIns(4,5)P2)对钾离子通道(KCNQ)的快速变化
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内稳态调节的 M 电流调节分泌运动神经元,而不是血管运动神经元中的突触整合在牛蛙。

Homeostatic regulation of M-current modulates synaptic integration in secretomotor, but not vasomotor, sympathetic neurons in the bullfrog.

机构信息

Department of Neurobiology, E 1440 Starzl Biomedical Science Tower, University of Pittsburgh School of Medicine, Pittsburgh, PA 15261, USA.

出版信息

J Physiol. 2010 Mar 15;588(Pt 6):923-38. doi: 10.1113/jphysiol.2009.182873. Epub 2010 Jan 25.

DOI:10.1113/jphysiol.2009.182873
PMID:20100739
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2849959/
Abstract

We compared how vasomotor C neurons and secretomotor B neurons integrated identical patterns of virtual synaptic activity using dynamic clamp, perforated-patch recordings from dissociated bullfrog sympathetic ganglion cells. The synaptic template modelled one strong nicotinic synapse and nine weak synapses, each firing randomly at 5 Hz, with strength normalized to each cell. B neurons initially fired at 12 Hz, but this declined within seconds, decreasing 27% after 40 s and recovering slowly as evidenced by the threshold synaptic conductance for firing (tau(recovery) = 136 + or - 23 s). C neurons gave an identical initial response that remained steady, declining only 6% after 40 s. The difference resulted from an activity-dependent 379 + or - 65% increase in M-current (I(M)) in B cells (tau(recovery) = 153 + or - 22 s), which was absent in C cells. In addition, action potential afterhyperpolarizations were 2-fold longer in B cells, but this did not produce the differential response to synaptic stimulation. Activity-dependent increases in I(M) were sensitive to 100 microm Cd(2+) and 2.5 microm oxotremorine M (oxo-M), a muscarinic agonist, and fully blocked by zero Ca(2+), 10 microm oxo-M and 2.5 microm oxo-M plus 50 microm wortmannin, a PIP(2) synthesis inhibitor. A leftward shift in voltage-dependent activation could not fully account for the I(M) increase. Firing at 0.5 Hz was sufficient to modulate I(M). Opposing influences of activity and muscarinic excitation thus produce homeostatic I(M) regulation, to stabilize excitability and postsynaptic output in secretomotor sympathetic neurons. Absence of this regulation in vasomotor neurons suggests a different integrative function, where synaptic gain increases in proportion to presynaptic activity.

摘要

我们比较了血管运动神经元 C 和分泌神经元 B 如何整合相同模式的虚拟突触活动,使用从分离的牛蛙交感神经节细胞进行的动态钳位、穿孔膜片钳记录。该突触模板模拟了一个强烟碱型突触和九个弱突触,每个突触以 5 Hz 的随机频率发射,强度归一化为每个细胞。B 神经元最初以 12 Hz 的频率发射,但在几秒钟内下降,在 40 秒后下降 27%,并随着发射阈值突触电导(tau(recovery)=136+/-23s)的缓慢恢复而恢复。C 神经元给出了相同的初始反应,该反应保持稳定,在 40 秒后仅下降 6%。这种差异是由于 B 细胞中活动依赖性的 M 电流(I(M))增加 379+/-65%(tau(recovery)=153+/-22s),而 C 细胞中则没有。此外,B 细胞中的动作电位后超极化延长了 2 倍,但这并没有产生对突触刺激的差异反应。I(M)的活动依赖性增加对 100µM Cd(2+)和 2.5µM 氧托溴铵(oxo-M)敏感,后者是一种毒蕈碱激动剂,并且完全被零 Ca(2+)、10µM oxo-M 和 2.5µM oxo-M 加 50µM wortmannin 阻断,后者是一种 PIP(2)合成抑制剂。电压依赖性激活的左移不能完全解释 I(M)的增加。以 0.5Hz 的频率发射足以调节 I(M)。因此,活动和毒蕈碱兴奋的相反影响产生了 I(M)的稳态调节,以稳定分泌运动神经元的兴奋性和突触后输出。血管运动神经元中不存在这种调节表明了不同的整合功能,其中突触增益与突触前活动成比例增加。