生物物理学报 第十八卷 2002年总目录

第一期综述与专论劳埃晶体学时代的到来……………………………………任重Dominique BourgeoisJohn R. Helliwell等( 1 )研究热点与进展HIV-1进攻靶细胞的机制及相应环节抑制剂的研究进展…………………………………………………………邱阳( 11)研究论文外源氯化胆碱可提高小麦线粒体膜的流动性……………………………………刘世名季玉龙陈靠山等( 19)CPM抑制了由1,4NQ诱导的对骨肌肌质网SR钙通道RyR1的激活效应………………………………………………………………………………………………………………………夏若虹ABRAMSON J.J…     

调控剂的电子传递性质对骨骼肌型钙释放通道的调控效应研究

肌质网(sarcoplasmic reticulum,SR)中的钙释放通道利阿诺定受体(ryanodine receptor,RyR)是调控胞浆钙离子浓度的重要蛋白,其活性受多种调控剂影响．调控剂的不同电子传递性质可能作用于RyR的功能性巯基,进而影响其门控状态．了解具有不同电子传递性质的调控剂影响钙通道的作用机制具有重要意义．本研究采用光子相关光谱法(PCS)、CPM(7-二乙 基-3-(4′-马来酰亚胺苯基)4-甲基香豆素)荧光标记法及[³H]-ryanodine结合等实验,分别检测多种调控剂对RyR1的蛋白及复合体粒度分布、自由巯基量及对通道状态的影响,利用光漂白法检测各调控剂的电子传递性质．结果显示,激活剂和巯基氧化剂具有类似电子受体的性质并产生相似作用,即自由蛋白粒度增加,自由巯基量减少,具有激活通道作用;抑制剂和巯基还原剂则具有类似电子供体的性质,作用效果相反．     

DNMT3a通过提升基因内部甲基化介导紫杉醇诱导的LINE-1异常表达

药物诱导的长散在重复序列LINE-1异常激活可促进细胞基因组不稳定,而基因组不稳定是促进肿瘤发生发展和耐药表型形成的重要因素。因此,探索LINE-1异常激活的分子机制具有重要的理论和临床意义。DNA甲基化是调控基因表达的重要方式,已知DNA甲基转移酶家族成员DNMT3a不仅能通过促进基因启动子甲基化抑制基因表达,还可通过增强基因内部甲基化上调基因表达。本实验室前期研究发现,将乳腺癌细胞暴露于化疗药物可诱导LINE-1异常高表达,但LINE-1启动子甲基化水平并无显著改变。本研究进一步探讨了在化疗药物压力下DNMT3a是否可通过增强LINE-1基因内部甲基化水平促进LINE-1在乳腺癌细胞中的异常高表达。ChIP实验和甲基分析结果显示,用化疗药物紫杉醇(PTX)处理乳腺癌细胞,不仅可以诱导DNMT3a表达,而且可以促进DNMT3a与LINE-1基因内部区域的结合,提升其基因内部甲基化水平,进而上调LINE-1的表达水平。利用表达载体增加细胞内DNMT3a的表达水平,可显著上调LINE-1基因内部的甲基化及基因的表达水平,而下调DNMT3a的表达可有效抑制LINE-1表达。上述研究结果表明,DNMT3a介导的基因非启动子区甲基化在药物诱导的LINE-1异常激活中发挥重要作用,为认识LINE-1在乳腺癌化疗耐药性形成过程中异常激活的机制提供了新思路。     

曲古抑菌素A对体外培养牛成纤维细胞组蛋白乙酰化和甲基化的影响

Trichostatin A(TSA)是一种特异的组蛋白去乙酰化酶抑制剂。研究显示,TSA可以特异地抑制组蛋白去乙酰化酶活性,提高细胞的组蛋白乙酰化水平,激活基因的表达。但是,目前还不是很清楚TSA处理是否对组蛋白甲基化产生影响。本研究以成纤维细胞为研究对象,利用免疫细胞化学技术及激光共聚焦显微镜,探讨了TSA处理体细胞对其组蛋白乙酰化及甲基化修饰的影响。结果显示,随TSA浓度增加,体细胞形态发生明显的改变,细胞变得扁平且核区较大,处理后组蛋白H4K8位点的乙酰化水平随着TSA浓度的增加明显提高。检测组蛋白H3上两个甲基化位点发现,随组蛋白乙酰化水平的增加,H3K4位点的三甲基化（H3K4me3）水平也显著提高。但是,对于H3K9的二甲基化水平（H3K9me2）则没有明显变化。以上结果显示,TSA的处理不仅可以提高体细胞的组蛋白乙酰化水平,同时也增加了与基因表达激活相关组蛋白修饰位点的甲基化水平,但是对于与沉默基因相关的组蛋白修饰位点则没有明显的影响。     

酸性鞘磷脂水解酶和MAPK信号通路在UVA诱导细胞凋亡中的作用

为了探讨酸性鞘磷脂水解酶 (ASM)和MAPK信号通路在UVA诱导的细胞凋亡中的作用 ,用DNA梯形条带 (DNAladder)和荧光显微镜鉴定细胞凋亡 ,Western印迹分析MAPK信号通路的激活情况 .结果显示 :①经UVA照射 ,正常的淋巴母细胞JY出现严重的细胞凋亡 ,而ASM遗传性缺陷的淋巴母细胞MS1 4 1 8出现轻微凋亡 ;给予ASM特异性抑制剂NB6 ,UVA诱导的JY细胞凋亡明显减轻 ,表明UVA诱导的细胞凋亡依赖于ASM .②UVA照射后 ,磷酸化ERK含量在MS1 4 1 8细胞中明显升高 ,在JY细胞中受到抑制 ;UVA照射前给予NB6 ,JY细胞中磷酸化ERK含量上升 ,表明ASM能抑制ERK的激活 .③UVA照射后 ,磷酸化JNK含量在MS1 4 1 8细胞中几乎没有变化 ,而在JY细胞中含量升高 ;UVA照射前给予NB6 ,JY细胞中磷酸化JNK含量没有明显升高 ,表明ASM激活JNK通路 .④NB6对UVA激活的p38MAPK信号通路没有影响 ,表明p38的激活与ASM关系不大 .研究表明 ,UVA诱导的细胞凋亡是通过激活ASM、激活JNK信号通路并抑制ERK信号通路来完成的     

cAMP和cGMP对棉铃虫神经细胞高电压激活钙通道的调节作用

用全细胞膜片钳法研究了cAMP和cGMP对棉铃虫Helicoverpa armigera 3龄幼虫胸腹神经节细胞高电压激活钙通道的调节作用。细胞外液中加入腺苷酸环化酶（AC）激活剂福斯克林（forskolin） 0.1 mmol/L,对于Ba²⁺介导的钙通道电流激活电压、峰电压、峰电流变化以及通道激活和电流达到峰值的时间无影响。电极内液中加入1 mmol/L的cGMP则明显抑制峰电流,且抑制作用呈时间依赖性和浓度依赖性,而对激活电压、峰电压无影响。结果提示,棉铃虫神经细胞高电压激活钙通道的活动可能不受细胞内cAMP水平提高的影响,但被cGMP抑制。     

低剂量顺铂通过p38MAPK介导的DNMT1下调降低p21与p16启动子甲基化上调p21与p16表达

低剂量顺铂可通过诱导p21与p16表达而诱导肿瘤细胞早衰,但其机制不明。本研究探讨了低剂量顺铂诱导的HeLa细胞衰老过程中p21与p16的上调机制。低剂量顺铂（4 μmol/L）处理HeLa细胞后,DNA甲基转移酶DNMT1蛋白水平降低;p21与p16启动子甲基化水平降低,二者mRNA及蛋白质水平升高;顺铂对DNMT1蛋白水平的降低作用与其激活p38MAPK有关,用SB203580抑制p38MAPK可部分逆转顺铂对DNMT1蛋白水平以及p21与p16启动子甲基化的降低作用,从而部分逆转顺铂对p21与p16表达的诱导;抑制p38MAPK 也可部分逆转低剂量顺铂诱导的HeLa细胞早衰。上述结果表明,低剂量顺铂可通过p38MAPK信号通路下调p21与p16启动子甲基化水平,进而上调二者的表达。这些结果为解析低剂量顺铂诱导肿瘤细胞早衰的信号转导机制提供了实验依据。     

ERK1/2信号通路活化对Tamoxifen所致胶质瘤细胞凋亡的影响

为了探讨ERK1/2信号通路在他莫昔芬(tamoxifen, TAM)所致胶质瘤细胞凋亡中的作用,以C6和U87MG胶质瘤细胞为研究对象,经TAM处理后,采用MTT法检测细胞的存活率;倒置显微镜和DAPI染色观察细胞的形态;流式细胞术检测细胞凋亡; Western-blot法检测细胞内ERK1/2磷酸化水平。最后应用ERK1/2抑制剂(PD98059)与TAM共同作用,观察其对胶质瘤细胞内ERK1/2磷酸化水平和细胞凋亡的影响。实验结果显示:TAM可呈浓度和时间依赖性地抑制胶质瘤细胞生长; TAM处理组的细胞凋亡明显增加且呈浓度依赖性;TAM能增加细胞内ERK1/2磷酸化水平;以PD98059阻断ERK1/2的激活,能增强TAM诱导细胞凋亡的作用。实验结果表明TAM能够抑制胶质瘤细胞生长和促进其细胞凋亡, ERK1/2信号通路的激活参与调控TAM所致胶质瘤细胞凋亡。     

蛇床子素对L-和N-型钙通道的影响

目的:比较蛇床子素对不同钙通道亚型的作用差异方法:首先在tsA201细胞上瞬时转染Cav1.2,Cav1.3,Cav2.2e[37a],和Cav2.2e[37b]通道,然后采用全细胞膜片钳技术,记录tsA201细胞上的钙电流,并观察蛇床子素对各种钙通道亚型的影响结果:蛇床子素可以浓度依赖性抑制Cav1.2和Cav1.3电流,抑制的半有效浓度分别为162.1μmol·L^-1和56.2μmol·L^-1。此外,蛇床子素对Cav2.2通道也有一定的抑制作用,在300μmol·L^-1的浓度下,抑制38%的Cav2.2e[37a]电流和61%的Cav2.2e[37b]电流蛇床子素对钙电流的抑制是快速可逆的蛇床子素在各个测试电位水平均能抑制上述四种钙通道电流,但不改变电流的激活阈值和最大峰值电流的激活电压。结论:蛇床子素以浓度依赖的方式抑制多种钙通道亚型并表现出不同的亲和力     

木黄酮对小鼠胰岛β细胞电压依赖性钙通道表达和电流的影响

目的:研究长期抑制酪氨酸激酶活性对胰岛β细胞中电压依赖性钙通道的影响,探讨酪氨酸激酶在胰岛β细胞中的作用.方法:原代培养小鼠胰岛和胰岛β细胞,经0.1 mmol/L酪氨酸激酶抑制剂木黄酮处理12 h后,运用全细胞电流记录的方法观察电压依赖性钙电流以及动作电位的改变,RT-PCR方法观察电压依赖性钙通道α1亚单位的表达改变.结果:木黄酮处理12 h后,小鼠胰岛β细胞的电压依赖性钙电流明显减小(13.83±1.515pA/pFvs 7.012±1.502 pA/pF,P＜0.01,n=6),动作电位幅度明显减弱(38.50±7.46 mV vs 15.95±4.39 mV,P＜0.01,n=6).木黄酮处理12 h后,小鼠胰岛中电压依赖性钙通道的α1亚单位的表达明显减少,降低为对照组的0.792±0.078(P＜0.01,n=5).结论:木黄酮处理可以抑制小鼠胰岛β细胞中电压依赖性钙通道的表达和电流,提示长期抑制酪氨酸激酶活性在胰岛β细胞功能损害中具有重要作用.     

Classes of thiols that influence the activity of the skeletal muscle calcium release channel

The skeletal muscle Ca(2+) release channel/ryanodine receptor (RyR1) is a prototypic redox-responsive ion channel. Nearly half of the 101 cysteines per RyR1 subunit are kept in a reduced (free thiol) state under conditions comparable with resting muscle. Here we assessed the effects of physiological determinants of cellular redox state (oxygen tension, reduced (GSH) or oxidized (GSSG) glutathione, and NO/O(2) (released by 3-morpholinosydnonimine)) on RyR1 redox state and activity. Oxidation of approximately 10 RyR1 thiols (from approximately 48 to approximately 38 thiols/RyR1 subunit) had little effect on channel activity. Channel activity increased reversibly as the number of thiols was further reduced to approximately 23/subunit, whereas more extensive oxidation (to approximately 13 thiols/subunit) inactivated the channel irreversibly. Neither S-nitrosylation nor tyrosine nitration contributed to these effects. The results identify at least three functional classes of RyR1 thiols and suggest that 1) the channel may be protected from oxidation by a large reservoir of functionally inert thiols, 2) the channel may be designed to respond to moderate oxidative stress by a change in activation setpoint, and 3) the channel is susceptible to oxidative injury under more extensive conditions.     

Effects of pO2 on the activation of skeletal muscle ryanodine receptors by NO: a cautionary note

Eu et al., reported that O2 dynamically controls the redox state of 6-8 out of 50 thiols per skeletal ryanodine receptor (RyR1) subunit and thereby tunes the response of Ca2+-release channels to authentic nitric oxide (NO) [J.P. Eu, J. Sun, L. Xu, J.S. Stamler, G. Meissner, The skeletal muscle calcium release channel: coupled O2 sensor and NO signaling functions, Cell 102 (2000) 499-509]. A role for O2 was based on the observation that RyR1 can be activated by submicromolar NO at physiological ( approximately 10 mmHg) but not ambient (approximately 150 mmHg) pO2. At ambient pO2, these critical thiols were oxidized but incubation at low pO2 reset the redox state of these thiols, closed RyR1 channels and made these thiols available for nitrosation by low NO concentrations. Eu et al., postulated the existence of a redox/O2sensor that couples channel activity to NO and pO2 and explained that "the nature of the 'redox/O2 sensor' that couples channel activity to intracellular redox chemistry is a mystery". Here, we re-examined the effect of pO2 on RyR1 and find that incubation of RyR1 at low pO2 did not alter channel activity and NO (0.5-50 microM) failed to activate RyR1 despite a wide range of pO2 pre-incubation conditions. We show that low levels of NO do not activate RyR1, do not reverse the inhibition of RyR1 by calmodulin (CaM) even at physiological pO2. Similarly, the pre-incubation of SR vesicles in low pO2 (for 10-80 min) did not inhibit channel activity or sensitization of RyR1 to NO. We discuss the significance of these findings and propose that caution should be taken when considering a role for pO2 and nitrosation by NO as mechanisms that tune RyRs in striated muscles.     

The toxicity of menadione (2-methyl-1,4-naphthoquinone) and two thioether conjugates studied with isolated renal epithelial cells

Menadione (2-methyl-1,4-naphthoquinone) was used as a model compound to test the hypothesis that thioether conjugates of quinones can be toxic to tissues associated with their elimination through a mechanism involving oxidative stress. Unlike menadione, the glutathione (2-methyl-3-(glutathion-S-yl)-1,4-naphthoquinone; MGNQ) and N-acetyl-L-cysteine (2-methyl-3-(N-acetylcysteine-S-yl)-1,4-naphthoquinone; M(NAC)NQ) thioether conjugates were not able to arylate protein thiols but were still able to redox cycle with cytochrome c reductase/NADH and rat kidney microsomes and mitochondria. Interestingly, menadione and M(NAC)NQ were equally toxic to isolated rat renal epithelial cells (IREC) while MGNQ was nontoxic. The toxicity of both menadione and M(NAC)NQ was preceded by a rapid depletion of soluble thiols and was associated with a depletion of soluble thiols and was associated with a depletion of protein thiols. Treatment of IREC with the glutathione reductase inhibitor, 1,3-bis(2-chloroethyl)-1-nitrosourea, potentiated the thiol depletion and toxicity observed with menadione and M(NAC)NQ indicating the involvement of oxidative stress in this model of renal cell toxicity. The lack of MGNQ toxicity can be attributed to an intramolecular cyclization reaction which destroys the quinone nucleus and therefore eliminates its ability to redox cycle. These findings have important implications with regard to our understanding of the toxic potential of quinone thioether conjugates and of quinone toxicity in general.     

Nitric oxide,NOC-12, and S-nitrosoglutathione modulate the skeletal muscle calcium release channel/ryanodine receptor by different mechanisms. An allosteric function for O2 in S-nitrosylation of the channel

The skeletal muscle Ca(2+) release channel/ryanodine receptor (RyR1) contains approximately 50 thiols per subunit. These thiols have been grouped according to their reactivity/responsiveness toward NO, O(2), and glutathione, but the molecular mechanism enabling redox active molecules to modulate channel activity is poorly understood. In the case of NO, very low concentrations (submicromolar) activate RyR1 by S-nitrosylation of a single cysteine residue (Cys-3635), which resides within a calmodulin binding domain. S-Nitrosylation of Cys-3635 only takes place at physiological tissue O(2) tension (pO(2); i.e. approximately 10 mm Hg) but not at pO(2) approximately 150 mm Hg. Two explanations have been offered for the loss of RyR1 responsiveness to NO at ambient pO(2), i.e. Cys-3635 is oxidized by O(2) versus O(2) subserves an allosteric function (Eu, J. P., Sun, J. H., Xu, L., Stamler, J. S., and Meissner, G. (2000) Cell 102, 499-509). Here we report that the NO donors NOC-12 and S-nitrosoglutathione both activate RyR1 by release of NO but do so independently of pO(2). Moreover, NOC-12 activates the channel by S-nitrosylation of Cys-3635 and thereby reverses channel inhibition by calmodulin. In contrast, S-nitrosoglutathione activates RyR1 by oxidation and S-nitrosylation of thiols other than Cys-3635 (and calmodulin is not involved). Our results suggest that the effect of pO(2) on RyR1 S-nitrosylation is exerted through an allosteric mechanism.     

The skeletal muscle calcium release channel: coupled O2 sensor and NO signaling functions

Ion channels have been studied extensively in ambient O2 tension (pO2), whereas tissue PO2 is much lower. The skeletal muscle calcium release channel/ryanodine receptor (RyR1) is one prominent example. Here we report that PO2 dynamically controls the redox state of 6-8 out of 50 thiols in each RyR1 subunit and thereby tunes the response to NO. At physiological pO2, nanomolar NO activates the channel by S-nitrosylating a single cysteine residue. Among sarcoplasmic reticulum proteins, S-nitrosylation is specific to RyR1 and its effect on the channel is calmodulin dependent. Neither activation nor S-nitrosylation of the channel occurs at ambient PO2. The demonstration that channel cysteine residues subserve coupled O2 sensor and NO regulatory functions and that these operate through the prototypic allosteric effector calmodulin may have general implications for the regulation of redox-related systems.     

1,4萘醌和谷胱甘肽对Ryanodine受体初始结合率的影响及其意义

采用ｒｙａｎｏｄｉｎｅ 动态结合方法,考察了１,４ 萘醌（１,４ＮＱ） 和谷胱甘肽（ＧＳＳＧ） 作用于兔骨骼肌肌质网（ＳＲ）ｒｙａｎｏｄｉｎｅ 敏感钙通道（ＲｙＲ） 所产生的对ｒｙａｎｏｄｉｎｅ 初结合率（Ｒ０） 的影响。类似于１,４ＮＱ 对ｒｙａｎｏｄｉｎｅ 平衡结合的实验结果［７ ］ ,１ ,４ＮＱ 对Ｒ０ 也诱导出浓度依赖性的多相性变化规律,还原态１ , ４ＮＱ 的Ｒ０ 曲线则没有这种多相性。而ＧＳＳＧ 在３７°Ｃ 时所有浓度或时间区间都没有对ｒｙａｎｏｄｉｎｅ 结合对或Ｒ０ 诱导出明显的多相性行为;还原态的谷胱甘肽（ＧＳＨ） 亦只能产生出单相的抑制作用。这些氧化还原试剂也对ｒｙａｎｏｄｉｎｅ 结合率系数ｋ ＋ １ ,但不是ｋ － １ ,产生了相应的影响。     

Conformation-dependent stability of junctophilin 1 (JP1) and ryanodine receptor type 1 (RyR1) channel complex is mediated by their hyper-reactive thiols

Junctophilin 1 (JP1), a 72-kDa protein localized at the skeletal muscle triad, is essential for stabilizing the close apposition of T-tubule and sarcoplasmic reticulum membranes to form junctions. In this study we report that rapid and selective labeling of hyper-reactive thiols found in both JP1 and ryanodine receptor type 1 (RyR1) with 7-diethylamino-3-(4'-maleimidylphenyl)-4-methylcoumarin, a fluorescent thiol-reactive probe, proceeded 12-fold faster under conditions that minimize RyR1 gating (e.g. 10 mM Mg2+) compared with conditions that promote high channel activity (e.g. 100 microM Ca2+, 10 mM caffeine, 5 mM ATP). The reactivity of these thiol groups was very sensitive to oxidation by naphthoquinone, H2O2, NO, or O2, all known modulators of the RyR1 channel complex. Using preparative SDS-PAGE, in-gel tryptic digestion, high pressure liquid chromatography, and mass spectrometry-based peptide sequencing, we identified 7-diethylamino-3-(4'-maleimidylphenyl)-4-methylcoumarin-thioether adducts on three cysteine residues of JP1 (101, 402, and 627); the remaining five cysteines of JP1 were unlabeled. Co-immunoprecipitation experiments demonstrated a physical interaction between JP1 and RyR1 that, like thiol reactivity, was sensitive to RyR1 conformation and chemical status of the hyper-reactive cysteines of JP1 and RyR1. These findings support a model in which JP1 interacts with the RyR1 channel complex in a conformationally sensitive manner and may contribute integral redox-sensing properties through reactive sulfhydryl chemistry.     

Aldolase potentiates DIDS activation of the ryanodine receptor in rabbit skeletal sarcoplasmic reticulum

DIDS (4,4'-di-isothiocyanostilbene-2,2'-disulfonate), an anion channel blocker, triggers Ca2+ release from skeletal muscle SR (sarcoplasmic reticulum). The present study characterized the effects of DIDS on rabbit skeletal single Ca2+-release channel/RyR1 (ryanodine receptor type 1) incorporated into a planar lipid bilayer. When junctional SR vesicles were used for channel incorporation (native RyR1), DIDS increased the mean P(o) (open probability) of RyR1 without affecting unitary conductance when Cs+ was used as the charge carrier. Lifetime analysis of single RyR1 activities showed that 10 microM DIDS induced reversible long-lived open events (P(o)=0.451+/-0.038) in the presence of 10 microM Ca2+, due mainly to a new third component for both open and closed time constants. However, when purified RyR1 was examined in the same condition, 10 microM DIDS became considerably less potent (P(o)=0.206+/-0.025), although the caffeine response was similar between native and purified RyR1. Hence we postulated that a DIDS-binding protein, essential for the DIDS sensitivity of RyR1, was lost during RyR1 purification. DIDS-affinity column chromatography of solubilized junctional SR, and MALDI-TOF (matrix-assisted laser-desorption ionization-time-of-flight) MS analysis of the affinity-column-associated proteins, identified four major DIDS-binding proteins in the SR fraction. Among them, aldolase was the only protein that greatly potentiated DIDS sensitivity. The association between RyR1 and aldolase was further confirmed by co-immunoprecipitation and aldolase-affinity batch-column chromatography. Taken together, we conclude that aldolase is physically associated with RyR1 and could confer a considerable potentiation of the DIDS effect on RyR1.     

Activation of cardiac ryanodine receptors by cardiac glycosides

This study investigated the effects of cardiac glycosides on single-channel activity of the cardiac sarcoplasmic reticulum (SR) Ca2+ release channels or ryanodine receptor (RyR2) channels and how this action might contribute to their inotropic and/or toxic actions. Heavy SR vesicles isolated from canine left ventricle were fused with artificial planar lipid bilayers to measure single RyR2 channel activity. Digoxin and actodigin increased single-channel activity at low concentrations normally associated with therapeutic plasma levels, yielding a 50% of maximal effect of approximately 0.2 nM for each agent. Channel activation by glycosides did not require MgATP and occurred only when digoxin was applied to the cytoplasmic side of the channel. Similar results were obtained in human RyR2 channels; however, neither the crude skeletal nor the purified cardiac channel was activated by glycosides. Channel activation was dependent on [Ca2+] on the luminal side of the bilayer with maximal stimulation occurring between 0.3 and 10 mM. Rat RyR2 channels were activated by digoxin only at 1 microM, consistent with the lower sensitivity to glycosides in rat heart. These results suggest a model in which RyR2 channel activation by digoxin occurs only when luminal [Ca2+] was increased above 300 microM (in the physiological range). Consequently, increasing SR load (by Na+ pump inhibition) serves to amplify SR release by promoting direct RyR2 channel activation via a luminal Ca2+-sensitive mechanism. This high-affinity effect of glycosides could contribute to increased SR Ca2+ release and might play a role in the inotropic and/or toxic actions of glycosides in vivo.