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在极限[Ca2+]条件下肌浆网Ca2+-ATP酶对Ca2+转运的调节

Regulation of Ca2+ transport by sarcoplasmic reticulum Ca2+-ATPase at limiting [Ca2+].

作者信息

Berman M C

机构信息

Department of Chemical Pathology, University of Cape Town Medical School, Observatory 7925, Cape Town, South Africa.

出版信息

Biochim Biophys Acta. 1999 Apr 14;1418(1):48-60. doi: 10.1016/s0005-2736(99)00017-6.

Abstract

The factors regulating Ca2+ transport by isolated sarcoplasmic reticulum (SR) vesicles have been studied using the fluorescent indicator Fluo-3 to monitor extravesicular free [Ca2+]. ATP, in the presence of 5 mM oxalate, which clamps intravesicular [Ca2+] at approximately 10 microM, induced a rapid decline in Fluo-3 fluorescence to reach a limiting steady state level. This corresponds to a residual medium [Ca2+] of 100 to 200 nM, and has been defined as [Ca2+]lim, whilst thermodynamic considerations predict a level of less than 1 nM. This value is similar to that measured in intact muscle with Ca2+ fluophores, where it is presumed that sarcoplasmic free [Ca2+] is a balance between pump and leaks. Fluorescence of Fluo-3 at [Ca2+]lim was decreased 70% to 80% by histidine, imidazole and cysteine. The K0.5 value for histidine was 3 mM, suggesting that residual [Ca2+]lim fluorescence is due to Zn2+. The level of Zn2+ in preparations of SR vesicles, measured by atomic absorption, was 0.47+/-0.04 nmol/mg, corresponding to 0.1 mol per mol Ca-ATPase. This is in agreement with findings of Papp et al. (Arch. Biochem. Biophys., 243 (1985) 254-263). Histidine, 20 mM, included in the buffer, gave a corrected value for [Ca2+]lim of 49+/-1.8 nM, which is still higher than predicted on thermodynamic grounds. A possible 'pump/leak' mechanism was tested by the effects of varying active Ca2+ transport 1 to 2 orders with temperature and pH. [Ca2+]lim remained relatively constant under these conditions. Alternate substrates acetyl phosphate and p-NPP gave similar [Ca2+]lim levels even though the latter substrate supported transport 500-fold slower than with ATP. In fact, [Ca2+]lim was lower with 10 mM p-NPP than with 5 mM ATP. The magnitude of passive efflux from Ca-oxalate loaded SR during the steady state of [Ca2+]lim was estimated by the unidirectional flux of 45Ca2+, and directly, following depletion of ATP, by measuring release of 40Ca2+, and was 0.02% of Vmax. Constant infusion of CaCl2 at [Ca2+]lim resulted in a new steady state, in which active transport into SR vesicles balances the infusion rate. Varying infusion rates allows determination of [Ca2+]-dependence of transport in the absence of chelating agents. Parameters of non-linear regression were Vmax=853 nmol/min per mg, K0.5(Ca)=279 nM, and nH(Ca)=1.89. Since conditions employed in this study are similar to those in the sarcoplasm of relaxed muscle, it is suggested that histidine, added to media in studies of intracellular Ca2+ transients, and in the relaxed state, will minimise contribution of Zn2+ to fluophore fluorescence, since it occurs at levels predicted in this study to cause significant overestimation of cytoplasmic free [Ca2+] in the relaxed state. Similar precautions may apply to non-muscle cells as well. This study also suggests that [Ca2+]lim in the resting state is a characteristic feature of Ca2+ pump function, rather than a balance between active transport and passive leakage pathways.

摘要

利用荧光指示剂Fluo-3监测囊泡外游离[Ca2+],对分离的肌浆网(SR)囊泡中Ca2+转运的调节因素进行了研究。在5 mM草酸盐存在的情况下,ATP可使囊泡内[Ca2+]维持在约10 μM,导致Fluo-3荧光迅速下降,达到一个稳定的极限水平。这对应于100至200 nM的残余介质[Ca2+],已被定义为[Ca2+]lim,而热力学考虑预测该水平应低于1 nM。该值与在完整肌肉中用Ca2+荧光团测量的值相似,据推测,肌浆游离[Ca2+]是泵与泄漏之间的平衡。组氨酸、咪唑和半胱氨酸可使Fluo-3在[Ca2+]lim时的荧光降低70%至80%。组氨酸的K0.5值为3 mM,表明残余的[Ca2+]lim荧光是由Zn2+引起的。通过原子吸收法测量,SR囊泡制剂中的Zn2+水平为0.47±0.04 nmol/mg,相当于每摩尔Ca-ATPase有0.1摩尔。这与帕普等人(《生物化学与生物物理学报》,243 (1985) 254 - 263)的研究结果一致。缓冲液中加入20 mM组氨酸后,[Ca2+]lim的校正值为49±1.8 nM,仍高于热力学预测值。通过改变温度和pH使活性Ca2+转运变化1至2个数量级的影响,测试了一种可能的“泵/漏”机制。在这些条件下,[Ca2+]lim保持相对恒定。替代底物乙酰磷酸和对硝基苯磷酸酯(p-NPP)产生的[Ca2+]lim水平相似,尽管后一种底物支持的转运速度比ATP慢500倍。实际上,10 mM p-NPP时的[Ca2+]lim低于5 mM ATP时的[Ca2+]lim。在[Ca2+]lim的稳定状态下,通过45Ca2+的单向通量以及在ATP耗尽后直接测量40Ca2+的释放,估算了从负载草酸钙的SR中被动流出的量,为Vmax的0.02%。在[Ca2+]lim持续输注CaCl2会导致新的稳定状态,其中向SR囊泡的主动转运与输注速率平衡。改变输注速率可在不存在螯合剂的情况下确定转运的[Ca2+]依赖性。非线性回归参数为Vmax = 853 nmol/min per mg,K0.5(Ca) = 279 nM,nH(Ca) = 1.89。由于本研究采用的条件与松弛肌肉肌浆中的条件相似,因此建议在细胞内Ca2+瞬变研究中以及在松弛状态下添加到培养基中的组氨酸,将使Zn2+对荧光团荧光的贡献最小化,因为在本研究预测的水平下,它会导致在松弛状态下对细胞质游离[Ca2+]的显著高估。类似的预防措施也可能适用于非肌肉细胞。本研究还表明,静息状态下的[Ca2+]lim是Ca2+泵功能的一个特征,而不是主动转运与被动泄漏途径之间的平衡。

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