Calcio
Calcio
Calcio
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Most of the Ca2+ in a resting cell is sequestered in organelles, particularly the endoplasmic or sarcoplasmic reticulum (ER or SR) and the mitochondria, and the free [Ca2+]i is kept to a low level, about 10-7M. The Ca2+ concentration in tissue fluid [Ca2+]o, is about 2.4 mM, so there is a large concentration gradient favouring Ca2+ entry. [Ca2+]i is kept low (a) by the operation of active transport mechanisms that eject cytosolic Ca2+ through the plasma membrane and pump it into the ER, and (b) by the normally low Ca2+ permeability of the plasma and ER membranes. Regulation of [Ca2+]i involves three main mechanisms: control of Ca2+ entry control of Ca2+ extrusion exchange of Ca2+ between the cytosol and the intracellular stores. These mechanisms are described in more detail below and are summarised in Figure 4.1 (see reviews by Berridge et al., 2000, 2003).
Figure 4-1 Regulation of intracellular calcium. The main routes of transfer of Ca2+ into, and out of, the cytosol and endoplasmic reticulum are shown for a typical cell (see text for details). Black arrows: routes into the cytosol. Blue arrows: routes out of the cytosol. Red arrows: regulatory mechanisms. Most of the channels and transporters have been characterised at the molecular level, but the mechanism by which store-operated calcium channels (SOCs) are linked to the state of the intracellular Ca2+ store is uncertain. Normally, [Ca2+]i is regulated to about 10-7mol/l in a 'resting' cell. Mitochondria (not shown) also function as Ca2+ storage organelles but release Ca2+ only under pathological conditions, such as ischaemia (see text). There is also evidence for an intracellular store (not shown) activated by the second messenger nicotinic acid dinucleotide phosphate. GPCR, G-protein-coupled receptor; IP3, inositol trisphosphate; IP3R, inositol
trisphosphate receptor; LGC, ligand-gated cation channel; NCX, Na+-Ca2+ exchange transporter; PMCA, plasma membrane Ca2+-ATPase;
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RyR, ryanodine receptor; SERCA, sarcoplasmic/endoplasmic reticulum ATPase; VGCC, voltage-gated calcium channel.
The pioneering work of Hodgkin and Huxley on the ionic basis of the nerve action potential (see below) identified voltage-dependent Na+ and K+ conductances as the main participants. It was later found that some invertebrate nerve and muscle cells could produce action potentials that depended on Ca2+ rather than Na+, and improved voltage clamp methods revealed that vertebrate cells also possess voltage-activated calcium channels capable of allowing substantial amounts of Ca2+ to enter the cell when the membrane is depolarised. These voltage-gated channels are highly selective for Ca2+ (although they also conduct Ba2+ ions, which are often used as a substitute in electrophysiological experiments), and do not conduct Na+ or K+; they are ubiquitous in excitable cells and allow Ca2+ to enter the cell whenever the membrane is depolarised, for example by a conducted action potential.
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A combination of electrophysiological and pharmacological criteria suggests that there are five distinct subtypes of voltage-gated calcium channels: L, T, N, P and R.1 The subtypes vary with respect to their activation and inactivation kinetics, their voltage threshold for activation, their conductance, and their sensitivity to blocking agents, as summarised in Table 4.1. The molecular basis for this heterogeneity has been worked out in some detail. The main pore-forming subunits (termed 1, see Fig. 3.4) occur in at least 10 molecular subtypes, and they are associated with other subunits (, , ) that also exist in different forms. Different combinations of these subunits give rise to the different physiological subtypes. In general, L channels are particularly important in regulating contraction of cardiac and smooth muscle (see below), and N channels (and also P/Q) are involved in neurotransmitter and hormone release, while T channels mediate Ca2+ entry into neurons and thereby control various Ca2+-dependent functions such as regulation of other channels, enzymes, etc. Clinically used drugs that act directly on these channels include the group of 'Ca2+ antagonists' consisting of dihydropyridines (e.g. nifedipine), verapamil and diltiazem (used for their cardiovascular effects; see Chs 18 and 19), and also gabapentin and pregabalin (used to treat epilepsy and pain; see Chs 40, 41). Many drugs affect calcium channels indirectly by acting on G-protein-coupled receptors (see Ch. 3; Triggle, 1999). A number of toxins act selectively on one or other type of calcium channel (Table 4.1), and these are used as experimental tools. LIGAND-GATED CHANNELS Table 4-1. Types and functions of calcium channels Gated by: Voltage Main types Characteristics Location and function L High activation threshold. Plasma membrane of Slow inactivation. many cells. Main Ca2+ source for contraction in smooth and cardiac muscle. N Low activation threshold. Slow inactivation. Main Ca2+ source for transmitter release by nerve terminals. Drug effects Blocked by dihydropyridines, verapamil, diltiazem. Activated by BayK 8644. Blocked by -conotoxin (component of Conus snail venom).
Widely distributed. Blocked by mibefradil. Important in cardiac pacemaker and atria (role in dysrhythmias). Nerve terminals. Transmitter release. Blocked by agatoxin (component of funnel web spider venom). Not directly targeted by drugs. Some experimental blocking agents known (e.g. heparin, injected
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P/Q
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activation.
intracellularly). Responds to GPCR agonists and antagonists in many cells. Activated by caffeine (high concentrations). Blocked by ryanodine. Mutations may lead to drug-induced malignant hyperthermia. Activated indirectly by agents that deplete intracellular stores (e.g. GPCR agonists, thapsigargin). Not directly targeted by drugs. -
Ca2+, Ryanodine Directly activated in striated muscle via sensitised by receptor dihydropyridine receptor cyclic ADP of T tubules. ribose
Located in endoplasmic/sarcoplasmic reticulum. Mediates Ca2+-evoked Ca2+ release in muscle. Also activated by the second messenger cyclic ADP ribose.
Store depletion
Storeoperated channels
NAADP
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Most ligand-gated cation channels (see Ch. 3) that are activated by excitatory neurotransmitters are relatively nonselective, and conduct Ca2+ ions as well as other cations. Most important in this respect is the glutamate receptor of the NMDA type (Ch. 33), which has a particularly high permeability to Ca2+ and is a major contributor to Ca2+ uptake by postsynaptic neurons (and also glial cells) in the central nervous system. Activation of this receptor can readily cause so much Ca2+ entry that the cell dies, mainly through activation of Ca2+-dependent proteases but also by triggering apoptosis (see Ch. 5). This mechanism, termed excitotoxicity, probably plays a part in various neurodegenerative disorders (see Ch. 35). For many years, there has been dispute about the existence of 'receptor-operated channels' in smooth muscle, responding directly to mediators such as adrenaline (epinephrine), acetylcholine and histamine. Now it seems (see Kuriyama et al., 1998) that the P2X receptor (see Ch. 3), activated by ATP, is the only example of a true ligand-gated channel in smooth muscle, and this constitutes an important route of entry for Ca2+. Other mediators, acting on Gprotein-coupled receptors, affect Ca2+ entry indirectly, mainly by regulating voltage-gated calcium channels or potassium channels. STORE-OPERATED CALCIUM CHANNELS These are channels that occur in the plasma membrane and open to allow Ca2+ entry when the ER stores are depleted. They are distinct from other membrane calcium channels, and belong to the large, recently discovered group of TRP (standing for 'transient receptor potential') channels, which have many different functions (see Clapham, 2003). SOCs remain somewhat mysterious, because it is unclear what kind of linkage couples them to the ER (see Berridge, 1997; Barritt, 1999). Like the ER and SR channels, they can serve to amplify the rise in [Ca2+]i resulting from Ca2+ release from the stores. So far, only experimental compounds are known to block these channels, but efforts are being made to develop specific blocking agents for therapeutic use as relaxants of smooth muscle.
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blocks the ER pump, causing loss of Ca2+ from the ER. It is a useful experimental tool but has no therapeutic significance. Calcium is also extruded from cells in exchange for Na+, by Na+-Ca2+ exchange. The transporter that does this has been fully characterised and cloned, and (as you would expect) comes in several molecular subtypes whose functions remain to be worked out. The exchanger transfers three Na+ ions for one Ca2+, and therefore produces a net depolarising current when it is extruding Ca2+. The energy for Ca2+ extrusion comes from the electrochemical gradient for Na+, not directly from ATP hydrolysis. This means that a reduction in the Na+ concentration gradient resulting from Na+ entry will reduce Ca2+ extrusion by the exchanger, causing a secondary rise in [Ca2+]i, a mechanism that is particularly important in cardiac muscle (see Ch. 18). The exchanger can actually function in reverse if [Na+]i rises excessively, resulting in increased Ca2+ entry into the cell (see above). The effect of digoxin on cardiac muscle (Ch. 18) is produced in this way.
induced calcium release (CICR), which serves to amplify the Ca2+ signal produced by other mechanisms such as opening of calcium channels in the plasma membrane. CICR means that release tends to be regenerative, because an initial puff of Ca2+ releases more, resulting in localised 'sparks' or 'waves' of Ca2+ release (see Berridge, 1997).
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Figure 4-2 Increase in intracellular calcium concentration in response to receptor activation. The records were obtained from a single rat sensory neuron grown in tissue culture. The cells were loaded with the fluorescent Ca2+ indicator Fura-2, and the signal from a single cell monitored with a fluorescence microscope. A brief exposure to the peptide bradykinin, which causes excitation of sensory neurons (see Ch. 41), causes a transient increase in [Ca2+]i from the resting value of about 150 nmol/l. When Ca2+ is removed from the extracellular Ca2+ represents the release of stored intracellular Ca2+ resulting from the intracellular production of inositol trisphosphate. The difference between this and the larger response when Ca2+ is present extracellularly is believed to represent Ca2+ entry through storeoperated ion channels in the cell membrane. (Figure kindly provided by G M Burgess and A Forbes, Novartis Institute for Medical Research.) extracellular solution, the bradykinin-induced increase in [Ca2+]i is still present but is smaller and briefer. The response in the absence of
The functions of IP3Rs and RyRs are modulated by a variety of other intracellular signals (see Berridge et al., 2003),
which affect the magnitude and spatiotemporal patterning of Ca2+ signals. Fluorescence imaging techniques have revealed a remarkable level of complexity of Ca2+ signals, and much remains to be discovered about the importance of this patterning in relation to physiological and pharmacological mechanisms. The Ca2+ sensitivity of RyRs is increased by caffeine, causing Ca2+ release from the SR even at resting levels of [Ca2+]i. This is used experimentally but rarely happens in humans, because the other pharmacological effects of caffeine (see Ch. 42) occur at much
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lower doses. The blocking effect of dantrolene, a compound related to ryanodine, is used therapeutically to relieve muscle spasm in the rare condition of malignant hyperthermia (see Ch. 36), which is associated with inherited abnormalities in the RyR protein. There are as yet few other examples of drugs that directly affect these Ca2+ release mechanisms. A typical [Ca2+]i signal resulting from activation of a G-protein-coupled receptor is shown in Figure 4.2. The response produced in the absence of extracellular Ca2+ represents release of intracellular Ca2+. The larger and more prolonged response when extracellular Ca2+ is present shows the contribution of SOC-mediated Ca2+ entry. OTHER SECOND MESSENGERS Two intracellular metabolites, cyclic ADP-ribose (cADPR; see Guse, 2000) and nicotinic acid dinucleotide phosphate (NAADP; see Chini & De Toledo, 2002), formed from the ubiquitous coenzymes nicotinamide adenine dinucleotide (NAD) and NAD phosphate, also affect Ca2+ signalling. cADPR acts by increasing the sensitivity of RyRs to Ca2+, thus increasing the 'gain' of the CICR effect. NAADP releases Ca2+ from lysosomes by activating channels not yet identified but evidently distinct from the IP3R and RyR. The levels of these messengers in mammalian cells may be regulated mainly in response to changes in the metabolic status of the cell, although the details are not yet clear. Abnormal Ca2+ signalling is involved in many pathophysiological conditions, such as ischaemic cell death, endocrine disorders and cardiac dysrhythmias, where the roles of cADPR and NAADP, and their interaction with other mechanisms that regulate [Ca2+]I, are the subject of much current work (see Berridge et al., 2003). THE ROLE OF MITOCHONDRIA Under normal conditions, mitochondria accumulate Ca2+ passively as a result of the intramitochondrial potential, which is strongly negative with respect to the cytosol. This negativity is maintained by active extrusion of protons, and is lost-thus releasing Ca2+ into the cytosol-if the cell runs short of ATP, for example under conditions of hypoxia. This only happens in extremis, and the resulting Ca2+ release contributes to the cytotoxicity associated with severe metabolic disturbance. Cell death resulting from brain ischaemia or coronary ischaemia (see Chs 18 and 35) involves this mechanism, along with others that contribute to an excessive rise in [Ca2+]i.
CALMODULIN
Calcium regulation Intracellular Ca2+ concentration, [Ca2+]i, is critically important as a regulator of cell function. Intracellular Ca2+ is determined by (a) Ca2+ entry; (b) Ca2+ extrusion; and (c) Ca2+ exchange between the cytosol, endoplasmic reticulum (ER) and mitochondria. Calcium entry occurs by various routes, including voltage- and ligand-gated calcium channels and Na+-Ca2+ exchange. Calcium extrusion depends mainly on an ATP-driven Ca2+ pump. Calcium ions are stored by the ER or sarcoplasmic reticulum (SR), from which they are released in response to various stimuli. Calcium ions are released from ER/SR stores by (a) the second messenger inositol trisphosphate acting on inositol trisphosphate receptors; or (b) increased [Ca2+]i itself acting on ryanodine receptors, a mechanism known as Ca2+-induced Ca2+ release. Other second messengers, cyclic ADP-ribose and nicotinic acid dinucleotide phosphate, also promote the release of Ca2+ from Ca2+ stores. Depletion of ER/SR Ca2+ stores promotes Ca2+ entry through the plasma membrane, via store-operated channels. Calcium ions affect many aspects of cell function by binding to proteins such as calmodulin, which in turn bind other proteins and regulate their function.
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Calcium exerts its control over cell functions by virtue of its ability to regulate the activity of many different proteins, including enzymes (particularly kinases and phosphatases), channels, transporters, transcription factors, synaptic vesicle proteins, and many others. In most cases, a Ca2+-binding protein serves as an intermediate between Ca2+ and the regulated functional protein, the best known such binding protein being the ubiquitous calmodulin. This regulates at least 40 different functional proteins-indeed a powerful fixer. Calmodulin is a dimer, with four Ca2+binding sites. When all are occupied, it undergoes a conformational change, exposing a 'sticky' hydrophobic domain that lures many proteins into association, thereby affecting their functional properties.
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