The ATP-sensitive potassium channel from the inner mitochondrial membrane (mitoK ATP ) is a highly selective conductor of K ؉ ions. When isolated in the presence of nonionic detergent and reconstituted in liposomes, mitoK ATP is inhibited with high affinity by ATP (K 1/2 ؍ 20 -30 M). We have suggested that holo-mitoK ATP is a heteromultimer consisting of an inwardly rectifying K The importance of the mitochondrial K ϩ cycle for volume regulation, reviewed by Garlid and Paucek (1) was recognized by Mitchell (2) long before any of the components of this cycle were discovered. K ϩ is driven into the matrix by the high membrane potential (⌬⌿) 1 generated by the proton-pumping electron transport system, and excess K ϩ is removed by the regulated K ϩ /H ϩ antiporter. Electrophoretic K ϩ influx occurs by diffusion and by means of ATP-sensitive potassium channel from the inner mitochondrial membrane (mitoK ATP ). At the high values of ⌬⌿ maintained by mitochondria, both of these processes increase exponentially with ⌬⌿ (3, 4) and are consequently very sensitive to fluctuations in ⌬⌿. These fluctuations, in turn, are high in tissues such as heart, which undergo large variations in energy demand and ATP synthesis rates (5). Thus, regulation of K ϩ influx and efflux pathways can be seen as a means of regulating volume in the face of the changing energy requirements of the cell. MitoK ATP plays more than a housekeeping role in cell physiology. There is now general agreement that mitoK ATP plays a key role in cardioprotection against ischemia-reperfusion injury (6, 7). The proposed mechanisms of this protective effect of mitoK ATP opening (5, 8, 9) are plausible; however, it is evident that more needs to be known about the functional properties of mitoK ATP before its role in vivo can be ascertained.By using a novel ethanol extraction technique, Mironova et al. (10) were the first to report reconstitution in lipid bilayer membranes of a 55-kDa K ϩ channel from mitochondria. Paucek et al. (3) used a detergent extraction technique and were the first to report reconstitution of mitoK ATP in liposomes. The latter channel was associated with two proteins of molecular mass 55 and 63 kDa, and we hypothesized that mitoK ATP is a heteromultimeric complex consisting of a 55-kDa inwardly rectifying K ϩ channel (mitoKIR) and a 63-kDa sulfonylurea receptor (mitoSUR), analogous to the plasma membrane ATPdependent K ϩ channel (cellK ATP ) (11,12). In this report, we focus on three interactions that address the key question of whether the 55-kDa K ϩ channel protein observed in the ethanol purification is the same as the 55-kDa protein purified with detergents. First, we show that UDP reverses ATP-inhibition of K ϩ flux mediated by both mitoKIR and mitoK ATP reconstituted in liposomes. Moreover, UDP exerts the same action in isolated mitochondria, and the affinities for the opening effect of UDP are about the same in each preparation. Second, we show that the mitoKIR opener p-diethylaminoethylbenzoate (DEB) also activates K ϩ flux via ...
The ATP-dependent K+ channel (KATP) was purified from the inner mitochondrial membrane and reconstituted into lipid bilayer membranes. KATP activity was inhibited by high concentrations of ATP and ADP, but activated by low concentrations (up to 200 microM) of ADP. p-Diethylaminoethylbenzoate (DEB) acted as a KATP opener: at micromolar concentrations, it reversed inhibition by ATP and ADP and it also prevented KATP rundown. Pelargonidine, extracted from flowers of Pelargonium, reduced spontaneous activity of KATP channels and diminished their potentiation by DEB. Their opposite action on KATP corresponded with their opposite redox properties in reactions with free radicals: DEB behaved as an electron donor, whereas pelargonidine acted as an electron acceptor. We hypothesize that thiol groups on mitoKATP are targets for redox-active ligans.
The Ca(2+) release channel (CRC) from sarcoplasmic reticulum (SR) is rich in thiol groups, and their oxidation/- reduction by thiol reagents activates/inhibits the CRC. Most channel regulators are not thiol reagents, and the mechanism of their action is illusive. Here the authors show that many channel activators act as electron acceptors, while many channel inhibitors act as electron donors in free radical reactions. The channel activator, caffeine, and the CRC inhibitor, tetracaine, are shown to interact competitively, which suggests that there exists a common site(s) on the CRC, that integrates the donor/acceptor effects of ligands. Moreover, channel activators shift the redox potential of reactive thiols on the ryanodine receptor (RyR) to more negative values and decrease the number of reactive thiols, while channel inhibitors shift the redox potential to more positive values and increase the number of reactive thiols. These observations suggest that the non-thiol channel modulators shift the thiol-disulfide balance within CRC by transiently exchanging electrons with the Ca(2+) release protein.
The calcium release channel (CRC) of the skeletal sarcoplasmic reticulum is rich in thiol groups and is strongly regulated by covalent modification of these thiols. Oxidizing reagents activate the release channel, whereas reducing reagents inhibit the channel. However, most CRC regulators are not thiol reagents. Here, we propose that reversible redox interactions are involved in regulation of the CRC by nonthiol reagents. This hypothesis was tested with several CRC regulators. The local anesthetics tetracaine, procaine and QX-314, which block the CRC, behaved as electron donors in reactions with dye free radicals. In contrast, ryanodine, caffeine, doxorubicin and daunorubicin, compounds known to activate the release channel, all accepted electrons from dye anion radicals. Moreover, release of Ca2+ from SR initiated by doxorubicin (acceptor) was antagonized by local anesthetics (donors). Based on the redox characterization of CRC modulators, we propose a functional model in which channel inhibitors and activators act as weak electron donors and acceptors, respectively, and shift the thiol-disulfide balance within the release protein. The consequence of this model is that, in spite of the chemical diversity of CRC modulators, a common mechanism of channel regulation involves the transient exchange of electrons between the activator/inhibitor and the CRC.
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