大鼠逼尿肌不稳定模型的建立及逼尿肌T型钙通道亚型表达的初步研究

目的:建立膀胱逼尿肌不稳定的大鼠模型并初步研究逼尿肌T型钙通道亚型的表达。方法:以增加膀胱出口梗阻的方法诱导膀胱逼尿肌不稳定的出现;以RT-PCR的方法检测正常膀胱和不稳定膀胱逼尿肌上T通道亚型的表达。结果:梗阻后5、6周逼尿肌不稳定发生率高且稳定;不稳定逼尿肌细胞与正常逼尿肌细胞均有α1I亚型表达且无数量差异,逼尿肌细胞有α1G亚型的表达,而正常逼尿肌上无此亚型表达。结论:梗阻第5、6周的动物是用来研究DI产生机制的良好模型;α1G亚型可能与逼尿肌不稳定的发生具有一定关系。     

钾通道在大鼠支气管平滑肌张力调控中作用的研究

目的：探讨延迟整流钾通道（Kv),高电导钙激活钾通道（BKCa)和ATP敏感钾通道（KATP)在大鼠支气管平滑肌张力调控中的作用。方法：以特异性钾通道阻断剂为工具,采用体外等长张力测定观察钾通道对静息和收缩状态下支气管张力的影响。结果：（1）KV阻断剂4－aminopyridine(4-AP)诱发大鼠支气管平滑肌产生浓度依赖性收缩反应,而BKCa阻断剂tetraethylammonium(TEA)和KATP阻断剂glibenclamide(Glib)对其无影响。（2）去除上皮对4－AP诱发大鼠支气管平滑肌收缩反应无影响,而钙通道阻断剂nifedipine对其有显著抑制效应。（3）在0.1mmol/L组胺或50mmol/L KCl诱发支气管平滑肌收缩之前或之后,加入TEA（1,5mmol/L)或0.1mmol/L 4-AP均显著增强二者诱发的收缩反应;而Glib(10μmol/L）对其无明显影响。结论：Kv参与大鼠支气管平滑肌静息张力的调控,而BKCa和KATP对其无影响。Kv和BKCa的关闭增强组胺及高浓度钾离子诱发大鼠离体支气管产生的收缩张力。     

模拟失重增强大鼠脑动脉血管平滑肌细胞大电导钙激活钾通道功能

本工作旨在探讨短期模拟失重大鼠脑动脉血管平滑肌细胞（vascular smooth muscle cells,VSMCs）大电导钙激活钾通道（large conductance calcium-activated potassium channels,BKCa channels）功能的改变。以尾部悬吊大鼠模型模拟失重对脑血管的影响。应用激光扫描共聚焦显微镜测定VSMCs胞内游离钙浓度（[Ca^2＋]i）;采用细胞贴附模式,记录BKCa通道的单通道活动。结果表明,模拟失重1周后,大鼠脑动脉VSMCs的[Ca^2＋]i比对照组显著升高（P〈0．05）：BKCa通道的开放概率（Po）与平均开放时间（To）显著增加（P〈0．05）,而单通道电导与平均关闭时间（Tc）则无显著变化。总之,1周模拟失重可引起脑动脉VSMCs的BKCa通道功能显著增强,且与细胞[Ca^2＋]i的升高同步出现。结果提示,脑动脉VSMCs的离子通道机制可能参与介导模拟失重引起的脑血管适应性变化。     

慢性吸烟大鼠气道平滑肌大电导的钙激活钾通道和Kv1.5表达的变化

复制大鼠的慢性吸烟模型,采用气道反应性的测定、HE染色、免疫组织化学染色、原位杂交和免疫印迹实验等方法,观察吸烟对大鼠支气管平滑肌大电导的钙激活的钾通道(BKca)和电压依赖性延迟整流钾通道Kv1．5蛋白和mRNA表达的影响,以阐明吸烟引起的气道高反应性发病机制中钾通道表达变化的作用。结果显示：(1)慢性吸烟可降低大鼠大气道和小气道BKca和Kv1．5蛋白和mRNA表达;(2)大气道BKca的降低程度大于Kv1．5,小气道BKca和Kv1．5的降低程度无明显差异：(3)吸烟对全肺组织BKca和Kv1．5的蛋白表达无明显影响。上述结果提示,慢性吸烟可下调大鼠气道平滑肌钾通道BKca和Kv1．5的表达水平,是导致气道高反应的机制之一。     

Ca2+对骨骼肌钙释放通道的调节

钙释放通道（calcium release channel）又称Ryanodine受体（RyR）,是细胞内质网膜上介导细胞内钙信号转导的离子通道。RyR1在骨骼肌细胞的兴奋-收缩偶联过程中起重要作用,是肌质网快速释放Ca^2＋的通道。许多调节因素,如一些内源性蛋白（FK结合蛋白、钙调素、钙结合蛋白）和一些离子（Ca^2＋、Mg^2＋）,通过不同的作用位点与RyR1结合,调控RyR1的结构与功能。研究表明,Ca^2＋是众多调节RyR1因素中的核心成分和前提条件,其对RyR1的结构与功能有重要的调控作用。     

T型Ca2+通道在心脏中的表达

电生理学研究表明心脏组织细胞主要存在L型和T型两种不同的Ca2 通道,其中T型Ca2 通道主要存在于正常成熟心脏的浦肯野纤维和起搏点细胞以及胚胎心室肌细胞,而正常成熟心肌细胞中存在很少,但在心脏肥大和心衰等心脏疾病的心肌细胞中表达明显增加,提示T型Ca2 通道与心脏正常节律的形成和心脏发育以及一些心脏疾病的发生与发展密切相关.     

ATP敏感性钾通道在心血管系统中的作用

ＡＴＰ敏感性钾通道对Ｋ＾＋有较高的选择性,且有相当高的电导。磺酰脲类药物对ＡＴＰ敏感性钾通道有特异的抑制作用,而一些开放剂对其有激活作用。缺血或其它代谢抑制时,ＡＴＰ浓度下降,腺苷产生产增加,两者激活ＡＴＰ敏感性钾通道,对心肌缺血再灌注损伤起保持作用;ＡＴＰ敏感性钾通道开放剂对高血压有一定的治疗效用。     

钙离子调控蛋白在肿瘤血管形成及肿瘤发展中的研究进展

[目的]探讨钙离子调控蛋白在肿瘤血管生成及肿瘤发展中的作用。[内容]Ca2+作为第二信使参与生命活动中多种途径的调控,钙离子调控蛋白作为Ca2+的生物信息传递载体在此过程中起着重要作用。肿瘤组织中血管内皮细胞及平滑肌细胞的激活是肿瘤新生的第一步,新生血管的形成能促进实体瘤生长、侵袭和转移。该文综述了参与钙离子浓度调控的钙调控蛋白S100蛋白、膜联蛋白(Annexin)、钙网蛋白(CRT)、钙调蛋白Ca M及其他非直接钙离子结合的钙调控蛋白,这些蛋白在肿瘤细胞中的表达水平,及如何通过调控血管内皮细胞及平滑肌细胞的功能进而影响肿瘤血管生成与肿瘤转移,该综述聚焦重点是肺癌的研究,也对其他常见癌症有涉及。[结论]钙离子调控蛋白是一种重要的调节血管形成和肿瘤发展的一类蛋白,是肿瘤发展的标志物及肿瘤治疗的潜在靶点。     

下丘脑神经元电压依赖性钾电流活动在大鼠出生后发育过程中的变化

采用膜片钳细胞贴附式技术,比较研究SD大鼠下丘脑神经元电压依赖性钾通道(voltage-dependent potassium channel,Kv)单通道电流活动的动力学特性,在出生后发育过程中的变化。出生不同天数的大鼠,其下丘脑神经元上Kv通道的电流强度和电导无显著差别(P>0.05),通道电导接近120 pS;单位时间内封接膜片上N个通道的开放概率的总和升高,由第1天的0.19±0.08(n=10)上升到第9天的0.30±0.09(n=10,P<0.05),单通道活动密度增加,由0.14 channel/μm2升高至0.26 channel/μm2。上述结果提示大鼠下丘脑神经元在出生发育过程中,Kv单通道活动的动力学发生显著变化。     

Alterations in KATP and KCa channel function in cerebral arteries of insulin-resistant rats

We examined whether insulin resistance alters the function of ATP-dependent and Ca(2+)-activated K(+) channels (K(ATP) and K(Ca) channels, respectively) in pressurized isolated middle cerebral arteries (MCAs) from fructose-fed insulin-resistant (IR) and control rats. Blockade of K(Ca) channels with tetraethylammonium chloride (TEA, 2.5 mM) or iberiotoxin (IBTX, 0.1 microM) increased the spontaneously developed tone in control MCAs by 10.5 +/- 1.3% (n = 10) and 13.3 +/- 2.3% (n = 6), respectively. In the IR arteries, TEA induced similar constrictions (8.0 +/- 1.1%, n = 10), but IBTX constricted the IR arteries by only 3.1 +/- 0.9% (n = 8; P < 0.01). Bradykinin (BK)-induced endothelium-mediated relaxation was reduced in IR MCAs. Maximum relaxation to BK (10(-6) M) was 42 +/- 4% in control (n = 9) and 19 +/- 2% in IR (n = 10; P < 0.01) arteries. Pretreatment with TEA, IBTX, or the K(ATP) channel blocker glibenclamide (10 microM) inhibited relaxation to BK in control MCAs but did not alter dilation in IR arteries. Relaxation to the K(ATP) channel opener cromakalim was also diminished in IR MCAs. Maximum relaxation to cromakalim (10(-5) M) was 48 +/- 3% in control (n = 6) and 19 +/- 2% in IR arteries (n = 6; P < 0.01). These findings demonstrate that insulin resistance alters the function of K(ATP) and K(Ca) channels in isolated MCAs and affects the control of resting vascular tone and the mediation of dilator stimuli.     

Evaluation of flurbiprofen in detrusor instability.

Thirty women with detrusor instability (27 cases idiopathic, and three secondary to multiple sclerosis) completed a double-blind, cross-over trial of the prostaglandin synthetase inhibitor flurbiprofen and a placebo, results being evaluated by questionnaire and cystometry. Frequency, urgency, and urge incontinence were all significantly reduced with flurbiprofen (P less than 0.001, P less than 0.025, and P less than 0.025 respectively), as was the detrusor-pressure rise during bladder filling (P less than 0.01). Side effects, however, occurred in 13 patients while taking flurbiprofen compared with five while taking placebo (P less than 0.025). After the trial 19 patients wished to continue with flurbiprofen. Flurbiprofen is a useful treatment for idiopathic detrusor instability and is well tolerated by most patients.     

Inhibition of KCa2.2 and KCa2.3 channel currents by protonation of outer pore histidine residues

Ion channels are often modulated by changes in extracellular pH, with most examples resulting from shifts in the ionization state of histidine residue(s) in the channel pore. The application of acidic extracellular solution inhibited expressed K_Ca2.2 (SK2) and K_Ca2.3 (SK3) channel currents, with K_Ca2.3 (pIC₅₀ of ∼6.8) being approximately fourfold more sensitive than K_Ca2.2 (pIC₅₀ of ∼6.2). Inhibition was found to be voltage dependent, resulting from a shift in the affinity for the rectifying intracellular divalent cation(s) at the inner mouth of the selectivity filter. The inhibition by extracellular protons resulted from a reduction in the single-channel conductance, without significant changes in open-state kinetics or open probability. K_Ca2.2 and K_Ca2.3 subunits both possess a histidine residue in their outer pore region between the transmembrane S5 segment and the pore helix, with K_Ca2.3 also exhibiting an additional histidine residue between the selectivity filter and S6. Mutagenesis revealed that the outer pore histidine common to both channels was critical for inhibition. The greater sensitivity of K_Ca2.3 currents to protons arose from the additional histidine residue in the pore, which was more proximal to the conduction pathway and in the electrostatic vicinity of the ion conduction pathway. The decrease of channel conductance by extracellular protons was mimicked by mutation of the outer pore histidine in K_Ca2.2 to an asparagine residue. These data suggest that local interactions involving the outer turret histidine residues are crucial to enable high conductance openings, with protonation inhibiting current by changing pore shape.     

Blockade of a KCa channel with synthetic peptides from noxiustoxin: A K+ channel blocker

Using the outside-out configuration of the patch-clamp method, we studied the effect of several synthetic peptides corresponding to various segments from the N-terminal region of noxiustoxin (NTX) on single Ca²⁺-activated K⁺ (K_Ca) channels of small conductance obtained from cultured bovine aortic endothelial cells. These peptides induced diverse degrees of fast blockade in the endothelial K_Ca channel. The most effective blockers were the peptides NTX_1–39 (IC₅₀=0.5 m) and NTX_1–20 comprising the first 20 amino acids from the native toxin (IC₅₀ 5 m), while less effective was the hexapeptide NTX_1–6, from the first six amino acid residues of NTX (IC₅₀ = 500 m). This was the minimum sequence required to block the channel.By testing overlapping sequences from the entire molecule, specially those corresponding to the N-terminal region of NTX, we have been able to determine their different apparent affinities for the K_Ca channel. Synthetic peptides from the C-terminal region produced no effect on the K_Ca channel at the concentrations tested (up to 1 mm). These results confirm that in the N-terminal region of the NTX is located part of the sequence that may recognize K⁺ channels, as we have suggested previously from in vivo experiments. The blockade induced by native NTX was poorly affected by changes in membrane potential; however, the blockage induced by synthetic peptides lacking the C-terminal region was partially released by depolarization.This study was supported by grant HL-45880 from the National Institutes of Health, and by grant 900946 from the American Heart Association to D.L.K. and Howard Hughes Medical Institute No. 75191-527104, CONACyT-Mexico No. 0018-N9105, and DGAPA-UNAM No. IN 202689 to L.D.P. This work was partially supported by a Grant-in-aid No. 92014250 from the American Heart Association to L.V.     

Role of S3 and S4 transmembrane domain charged amino acids in channel biogenesis and gating of KCa2.3 and KCa3.1

The role of positively charged arginines in the fourth transmembrane domain (S4) and a single negatively charged amino acid in the third transmembrane domain (S3) on channel biogenesis and gating of voltage-gated K(+) channels (Kv) has been well established. Both intermediate (KCa3.1) and small (KCa2.x) conductance, Ca(2+)-activated K(+) channels have two conserved arginines in S4 and a single conserved glutamic acid in S3, although these channels are voltage-independent. We demonstrate that mutation of any of these charged amino acids in KCa3.1 or KCa2.3 to alanine, glutamine, or charge reversal mutations results in a rapid degradation (<30 min) of total protein, confirming the critical role of these amino acids in channel biogenesis. Mutation of the S4 arginine closest to the cytosolic side of KCa3.1 to histidine resulted in expression at the cell surface. Excised patch clamp experiments revealed that this Arg/His mutation had a dramatically reduced open probability (P(o)), relative to wild type channels. Additionally, we demonstrate, using a combination of short hairpin RNA, dominant negative, and co-immunoprecipitation studies, that both KCa3.1 and KCa2.3 are translocated out of the endoplasmic reticulum associated with Derlin-1. These misfolded channels are poly-ubiquitylated, recognized by p97, and targeted for proteasomal degradation. Our results suggest that S3 and S4 charged amino acids play an evolutionarily conserved role in the biogenesis and gating of KCa channels. Furthermore, these improperly folded K(+) channels are translocated out of the endoplasmic reticulum in a Derlin-1- and p97-dependent fashion, poly-ubiquitylated, and targeted for proteasomal degradation.     

Heat shock protein modulation of KATP and KCa channel cerebrovasodilation after brain injury

Fluid percussion brain injury (FPI) impairs pial artery dilation to activators of the ATP-sensitive (K(ATP)) and calcium-activated (K(Ca)) K(+) channels. This study investigated the role of heat shock protein (HSP) in the modulation of K(+) channel-induced pial artery dilation after FPI in newborn pigs equipped with a closed cranial window. Under nonbrain injury conditions, topical coadministration of exogenous HSP-27 (1 mug/ml) blunted dilation to cromakalim, CGRP, and NS-1619 (10(-8) and 10(-6) M; cromakalim and CGRP are K(ATP) agonists and NS-1619 is a K(Ca) agonist). In contrast, coadministration of exogenous HSP-70 (1 mug/ml) potentiated dilation to cromakalim, CGRP, and NS-1619. FPI increased the cerebrospinal fluid (CSF) concentration of HSP-27 from 0.051 +/- 0.012 to 0.113 +/- 0.035 ng/ml but decreased the CSF concentration of HSP-70 from 50.42 +/- 8.96 to 30.9 +/- 9.9 ng/ml at 1 h postinsult. Pretreatment with topical exogenous HSP-70 (1 mug/ml) before FPI fully blocked injury-induced impairment of cromakalim and CGRP dilation and partially blocked injury-induced impairment of dilation to NS-1619. These data indicate that HSP-27 and HSP-70 contribute to modulation of K(+) channel-induced pial artery dilation. These data suggest that HSP-70 is an endogenous protectant of which its actions may be unmasked and/or potentiated with exogenous administration before brain injury.     

Direct molecular interaction of caveolin-3 with KCa1.1 channel in living HEK293 cell expression system

Caveolin family is supposed to be essential molecules for the formation of not only caveola structure on cell membrane but also functional molecular complexes in them with direct and/or indirect interaction with other membrane and/or submembrane associated proteins. The direct coupling of caveolin-1 (cav1) with large conductance Ca²⁺-activated K⁺ channel, KCa1.1 has been established in several types of cells and in expression system as well. The possible interaction of caveolin-3 (cav3), which shows expression in some differential tissues from cav1, with KCa1.1 remains to be determined. In the present study, the density of KCa1.1 current expressed in HEK293 cells was significantly reduced by the co-expression of cav3, as well as cav1. The co-localization and direct interaction of GFP- or CFP-labeled cav3 (GFP/CFP-cav3) with YFP- or mCherry-labeled KCa1.1 (KCa1.1-YFP/mCherry) were clearly demonstrated by single molecular image analyses using total internal reflection fluorescence (TIRF) microscopy and fluorescence resonance energy transfer (FRET) analyses with acceptor photobleaching method. The deletion of suggested cav1-binding motif in C terminus region of KCa1.1 (KCa1.1ΔCB-YFP) resulted in the marked decrease in cell surface expression, co-localization and FRET efficiency with CFP-cav3 and CFP-cav1. The FLAG-KCa1.1 co-immunoprecipitation with GFP-cav3 or GFP-cav1 also supported their direct molecular interaction. These results strongly suggest that cav3 possesses direct interaction with KCa1.1, presumably at the same domain for cav1 binding. This interaction regulates KCa1.1 expression to cell surface and the formation of functional molecular complex in caveolae in living cells.