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解离的大鼠颈上神经节神经元中的5-羟色胺3型受体通道

5-HT3 receptor channels in dissociated rat superior cervical ganglion neurons.

作者信息

Yang J, Mathie A, Hille B

机构信息

Department of Physiology and Biophysics, University of Washington, Seattle 98195.

出版信息

J Physiol. 1992 Mar;448:237-56. doi: 10.1113/jphysiol.1992.sp019039.

Abstract
  1. Whole-cell and single-channel voltage-clamp techniques were used to record the 5-HT3 receptor-mediated currents in neurons freshly dissociated from rat superior cervical ganglia. 2. Whole-cell currents elicited by brief pressure ejection of 5-HT (10 microM) reversed at -4.5 mV when extracellular and intracellular solutions mainly contained NaCl and CsCl. The peak current-voltage relation showed modest inward rectification that was fully developed within less than 2 ms of the applied voltage step. 3. With prolonged application of 5-HT (10 microM) using a fast perfusion system, the response desensitized in two phases with fast and slow time constants of 0.57 and 6.0 s at -74 mV. The time constants showed little voltage dependence; however, the relative amplitude of the two components was significantly dependent on voltage. The time course of desensitization was not affected by agents that increase the levels of intracellular cyclic AMP. 4. The relative permeability of the channel was determined from reversal potential changes. The channel passed small cations non-selectively, with permeability ratios (PX/PNa) of 0.93 and 1.24 for Cs+ and K+. The organic cations Tris and glucosamine were measurably permeant with permeability ratios of 0.19 and 0.06. Ca2+ was fairly permeant with a relative permeability of 0.55 in 20 mM solution and of 0.16 when the concentration of CaCl2 was increased to 115 mM. No permeability was detected for Cl-. 5. Fluctuation analysis of the whole-cell current revealed an apparent single-channel current of approximately 0.18 pA at -74 mV. 6. 5-HT-activated single-channel currents were recorded in excised outside-out patches. When 5-HT (10 microM) was delivered by pressure ejection, channel openings appeared rapidly with a delay of 28 ms. The unitary current was about approximately 0.80 pA at -74 mV. The channel activity induced by bath perfusion of 5-HT (0.8 microM) was significantly reduced by 100 nM of the 5-HT3 receptor-specific antagonists 3-tropanyl-3,5-dichlorobenzoate (MDL 72222) or 3-tropanyl-indole-3-carboxylate (ICS 205-930). 7. The single-channel current-voltage relation was non-linear, with moderate inward rectification similar to that of the whole-cell current. The chord conductance of the channel decreased with membrane depolarization from 14.6 pS at -104 mV to only 9.9 pS at -54 mV. Open-time distributions consisted of two components with mean time constants of 0.45 and 2.8 ms at -104 mV. Burst-length distributions were also made up of two components with time constants of 0.45 and 4.6 ms.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 采用全细胞和单通道电压钳技术,记录从大鼠颈上神经节新鲜分离的神经元中5-羟色胺(5-HT)3受体介导的电流。2. 当细胞外和细胞内溶液主要含有氯化钠和氯化铯时,由短暂压力喷射5-HT(10微摩尔)引发的全细胞电流在-4.5毫伏时发生反转。峰值电流-电压关系显示出适度的内向整流,在施加电压阶跃后不到2毫秒内充分发展。3. 使用快速灌注系统长时间施加5-HT(10微摩尔)时,在-74毫伏下,反应以0.57秒和6.0秒的快速和慢速时间常数分两个阶段脱敏。时间常数几乎没有电压依赖性;然而,两个成分的相对幅度明显依赖于电压。脱敏的时间进程不受增加细胞内环磷酸腺苷水平的药物影响。4. 通道的相对通透性由反转电位变化确定。该通道非选择性地通过小阳离子,铯离子和钾离子的通透率(PX/PNa)分别为0.93和1.24。有机阳离子三羟甲基氨基甲烷和葡糖胺可测量地通透,通透率分别为0.19和0.06。钙离子相当通透,在20毫摩尔溶液中的相对通透性为0.55,当氯化钙浓度增加到115毫摩尔时为0.16。未检测到氯离子的通透性。5. 全细胞电流的波动分析显示,在-74毫伏时,明显的单通道电流约为0.18皮安。6. 在切除的外侧向外膜片中记录了5-HT激活的单通道电流。当通过压力喷射递送5-HT(10微摩尔)时,通道开口迅速出现,延迟28毫秒。在-74毫伏时,单位电流约为0.80皮安。用100纳摩尔的5-HT3受体特异性拮抗剂3-托烷-3,5-二氯苯甲酸酯(MDL 72222)或3-托烷-吲哚-3-羧酸酯(ICS 205-930)可显著降低由浴灌注5-HT(0.8微摩尔)诱导的通道活性。7. 单通道电流-电压关系是非线性的,具有与全细胞电流类似的适度内向整流。通道的弦电导随着膜去极化从-104毫伏时的14.6皮西门子降至-54毫伏时的仅9.9皮西门子。开放时间分布由两个成分组成,在-104毫伏时平均时间常数分别为0.45毫秒和2.8毫秒。爆发长度分布也由两个成分组成,时间常数分别为0.45毫秒和4.6毫秒。(摘要截断于4

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