钙释放激活钙通道研究进展

库操纵的钙(Store Operated Calcium,SOC)进入参与许多重要Ca2+信号生理过程,如细胞分化和凋亡虽然SOC的许多生物物理特性被表述,但研究最清楚的是钙释放激活的钙(Ca2+ release-activated Ca2+,CRAC)通道.最近通过RNA干扰技术在果蝇和哺乳动物细胞上鉴定出CRAC通道的两个组成蛋白STIM1和Orail细胞静息时,STIM1均匀分布在内质网膜(ER)上.一当钙库耗竭,ER上STIM1会聚集迁移到细胞膜下,相比而言,Orail是一个形成CRAC通道孔的四次跨膜蛋白.有报道说STIM1作为ER上一个Ca2+感受器向细胞膜传导钙库耗竭信号.虽然钙库耗竭激活CRAC通道的过程在最近的研究中被定量描述为四个步骤,但还有很多细节仍然不清楚.如STIM1是如何感受钙库耗竭而导致其发生聚集的不清楚,又如STIM1是如何定位到细胞膜下又如何传导信息的不清楚,STIM1和Orai1直接到底是如何相互作用的等都有待进一步的研究.本文对CRAC通道的研究历史和最新进展进行了讨论.     

Exchangeability of Colloidal Calcium in Milk with Soluble Calcium

Approximately 40% of the calcium existing in colloidal phase of skimmilk was estimated to be hardly exchanged with the calcium psesent in soluble phase by applying a radioisotopic technique. This type of calcium was designated hard-to-exchange calcium. Hard-to-exchange calcium was absent or nearly zero in calcium caseinate dispersion or colloidal phosphate-free milk, but was present in composite calcium caseinate phosphate dispersion. It is suggested that hard-to-exchange calcium is present in a part of colloidal phosphate portion of casein micelles.     

Calcium Oscillations

Calcium signaling results from a complex interplay between activation and inactivation of intracellular and extracellular calcium permeable channels. This complexity is obvious from the pattern of calcium signals observed with modest, physiological concentrations of calcium-mobilizing agonists, which typically present as sequential regenerative discharges of stored calcium, a process referred to as calcium oscillations. In this review, we discuss recent advances in understanding the underlying mechanism of calcium oscillations through the power of mathematical modeling. We also summarize recent findings on the role of calcium entry through store-operated channels in sustaining calcium oscillations and in the mechanism by which calcium oscillations couple to downstream effectors.Calcium ions participate in a multiplicity of physiological and pathological functions. Among the most intensely studied, and the major focus of this article, is the role of Ca²⁺ as a cellular signal. Elevations in cytoplasmic Ca²⁺ mediate a plethora of cellular responses, ranging from extremely rapid events (muscle contraction, neurosecretion), to slower more subtle responses (cell division, differentiation, apoptosis). In contrast to most cellular signals, it is a relatively simple matter to observe changes in cytoplasmic Ca²⁺ in real time in living cells. As a result, the truly complex nature of Ca²⁺ signaling pathways has been revealed. The challenge is to understand what regulates these signals and what the biological significance of their complexity is.In the majority of laboratory experiments examining effects of various stimulants on Ca²⁺ signaling, supramaximal concentrations of activating agonists are employed resulting in rapid, robust, and often sustained increases in cytoplasmic Ca²⁺. It has long been appreciated that these signals result from a coordinated release of intracellular stores and increased Ca²⁺ influx across the plasma membrane (Bohr, 1973; Putney et al. 1981). The intracellular release of Ca²⁺ most commonly results from the Ca²⁺ releasing action of the phospholipase C-derived second messenger, inositol 1,4,5-trisphosphate (InsP₃) (Streb et al. 1983), whereas the entry of Ca²⁺ is because of the activation of store-operated channels in the plasma membrane (Putney 1986). However, it is becoming increasingly clear that these large sustained elevations seldom occur with physiological levels of stimulants. Rather the more common pattern of Ca²⁺ signaling, in both excitable and nonexcitable cells is a pattern of periodic discharges and/or entry of Ca²⁺. In excitable cells, such as the heart for example, these may be comprised of, or initiated by regenerative all-or-none plasma membrane channel activation, the Ca²⁺ action potential (Tsien et al. 1986) with amplification by intracellular Ca²⁺ release (Fabiato 1983). In nonexcitable cells, these spikes of cytoplasmic Ca²⁺ arise from regenerative discharge of stored Ca²⁺, a process generally termed Ca²⁺ oscillations (Prince and Berridge 1973; Woods et al. 1986). Like Ca²⁺ action potentials, these all-or-none discharges of Ca²⁺ represent a form of excitable behavior of the intracellular Ca²⁺ release signaling mechanism. However, because it is not possible to easily monitor and control the transmembrane chemical and biophysical parameters, as is the case for excitable plasma membrane behavior, it has been more difficult to fully understand the basic mechanisms by which these Ca²⁺ oscillations arise. Thus, although the question has been exhaustively studied for well over twenty years, there is still uncertainty and controversy over the underlying processes that give rise to Ca²⁺ oscillations. A number of reviews have discussed these issues at some length (Berridge and Galione 1988; Rink and Jacob 1989; Berridge 1990; Petersen and Wakui 1990; Berridge 1991; Cuthbertson and Cobbold 1991; Meyer and Stryer 1991; Hellman et al. 1992; Tepikin and Petersen 1992; Thomas et al. 1992; Dupont and Goldbeter 1993; Keizer 1993; Sneyd et al. 1994; Li et al. 1995; Thomas et al. 1996; Shuttleworth 1999; Lewis 2003; Dupont et al. 2007). In the current treatment, we have chosen to focus on two important aspects of Ca²⁺ oscillations. First, we review the available evidence for various computational models of Ca²⁺ oscillations that employ a quantitative approach to validate or repudiate specific mechanisms. Second, we consider the interrelationship between Ca²⁺ oscillations and plasma membrane Ca²⁺ influx mechanisms, with the view that we may learn more of the physiological function that these intracellular discharges of Ca²⁺ provide.     

Calcium waves

Waves through living systems are best characterized by their speeds at 20 degrees C. These speeds vary from those of calcium action potentials to those of ultraslow ones which move at 1-10 and/or 10-20 nm s(-1). All such waves are known or inferred to be calcium waves. The two classes of calcium waves which include ones with important morphogenetic effects are slow waves that move at 0.2-2 microm s(-1) and ultraslow ones. Both may be propagated by cycles in which the entry of calcium through the plasma membrane induces subsurface contraction. This contraction opens nearby stretch-sensitive calcium channels. Calcium entry through these channels propagates the calcium wave. Many slow waves are seen as waves of indentation. Some are considered to act via cellular peristalsis; for example, those which seem to drive the germ plasm to the vegetal pole of the Xenopus egg. Other good examples of morphogenetic slow waves are ones through fertilizing maize eggs, through developing barnacle eggs and through axolotl embryos during neural induction. Good examples of ultraslow morphogenetic waves are ones during inversion in developing Volvox embryos and across developing Drosophila eye discs. Morphogenetic waves may be best pursued by imaging their calcium with aequorins.     

Competitive Calcium Binding: Implications for Dendritic Calcium Signaling

Action potentials evoke calcium transients in dendrites of neocortical pyramidal neurons with time constants of <100 ms at physiological temperature. This time period may not be sufficient for inflowing calcium ions to equilibrate with all present Ca²⁺-binding molecules. We therefore explored nonequilibrium dynamics of Ca²⁺ binding to numerous Ca²⁺ reaction partners within a dendritelike compartment using numerical simulations. After a brief Ca²⁺ influx, the reaction partner with the fastest Ca²⁺ binding kinetics initially binds more Ca²⁺ than predicted from chemical equilibrium, while companion reaction partners bind less. This difference is consolidated and may result in bypassing of slow reaction partners if a Ca²⁺ clearance mechanism is active. On the other hand, slower reaction partners effectively bind Ca²⁺ during repetitive calcium current pulses or during slower Ca²⁺ influx. Nonequilibrium Ca²⁺ distribution can further be enhanced through strategic placement of the reaction partners within the compartment. Using the Ca²⁺ buffer EGTA as a competitor of fluo-3, we demonstrate competitive Ca²⁺ binding within dendrites experimentally. Nonequilibrium calcium dynamics is proposed as a potential mechanism for differential and conditional activation of intradendritic targets.     

Lectin-Induced Enhancement of Voltage-Dependent Calcium Flux and Calcium Channel Antagonist Binding

Concanavalin A (Con A), a tetravalent lectin with preferential affinity for mannosyl and glucosyl residues of membrane glycoconjugates, increased K+ depolarization-evoked uptake of 45Ca2+ in the PC12 neural cell line. Enhancement of uptake by Con A was concentration dependent, with maximal (24%) stimulation at 100 micrograms/ml of Con A, and was preferentially inhibited by mannoside and glucoside. Succinyl-Con A, a divalent analog with reduced biological potency, increased uptake by only 7%. The effect of Con A on 45Ca2+ uptake was dependent on membrane depolarization, was abolished by ionic Ca2+ channel blockers and organic Ca2+ channel antagonists, and was accompanied by an equivalent increase in Ca2+ channel 3H-labeled antagonist binding, observations suggesting that the voltage-dependent Ca2+ channel was the site of Ca2+ entry. The mechanism for enhancement of 45Ca2+ uptake by Con A appeared to be separate from that used by the Ca2+ channel agonist BAY K 8644 and independent of that involved in Ca2+ channel regulation by phorbol esters. These findings suggest that voltage-dependent Ca2+ channels may link cell surface carbohydrate interactions with intracellular effector processes.