Abstract
Hypothermia and hypothermic preconditioning are known to be profoundly cardioprotective, but the molecular mechanisms of this protection have not been fully explained. In this study, temperature preconditioning (16 °C) was found to be cardioprotective in isolated adult rat ventricular myocytes, enhancing contractile recovery and preventing calcium dysregulation after oxidative stress. Hypothermic preconditioning preserved mitochondrial function by delaying the pathological opening of the mitochondrial permeability transition pore (mPTP), whereas transient mPTP flickering remained unaltered. For the first time, reactive oxygen species (ROS) from the mitochondria are shown to be released exclusively during the hypothermic episodes of the temperature-preconditioning protocol. Using a mitochondrially targeted ROS biosensor, ROS release was shown during the brief bursts to 16 °C of temperature preconditioning. The ROS scavenger N-(2-mercaptopropionyl) glycine attenuated ROS accumulation during temperature preconditioning, abolishing the protective delay in mPTP opening. Temperature preconditioning induces ROS-dependant phosphorylation of the prosurvival kinase extracellular signal-regulated kinase (ERK)1/2. ERK1/2 activation was shown to be downstream of ROS release, as the presence of a ROS scavenger during temperature preconditioning completely blocked ERK1/2 activation. The cardioprotective effects of temperature preconditioning on mPTP opening were completely lost by inhibiting ERK1/2 activation. Thus, mitochondrial ROS release and ERK1/2 activation are both necessary to signal the cardioprotective effects of temperature preconditioning in cardiac myocytes.
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Main
Mitochondria are the gatekeepers of cardiac myocyte death or survival, particularly in ischaemic heart disease. The opening of the mitochondrial permeability transition pore (mPTP) is considered to be the ‘point of no return’, after which the myocyte is irreversibly committed to necrotic or apoptotic death pathways.1 This is responsible for the production of necrotic regions that are routinely observed after long periods of ischaemia followed by reperfusion.2 When the mPTP opens, low molecular weight molecules (<1.5 kDa) equilibrate across the inner membrane, resulting in mitochondrial swelling and outer membrane rupture. Oxidative phosphorylation is uncoupled when the mitochondrial membrane potential depolarises so that ATP can no longer be synthesised leading to ATP depletion and necrotic cell death.1 The situation is exacerbated as mitochondria begin to consume ATP through reversal of the F1/F0 ATPase in an effort to maintain the mitochondrial membrane potential.3 Strong evidence suggests that inhibiting the mPTP is a powerful means to protect the heart against ischaemia/reperfusion injury.4, 5 One example of an mPTP inhibitor is cyclosporine A (CsA), which binds to cyclophilin-D, a core component of the mPTP. CsA has been shown to significantly decrease infarct size in both an animal model and in humans, 6, 7 and to delay the time to mPTP opening in single cell analysis.8 In addition to irreversible mPTP opening, the mPTP has been reported to flicker,9 which may serve as a way for mitochondria to remove excess mitochondrial reactive oxygen species (ROS) and calcium during respiration.10
Cardioprotection is a phenomenon whereby the myocardium can be protected from damage by ischaemia/reperfusion injury. Cardioprotection can be conferred by many protocols, including pre-treatment with mitochondrial uncouplers, such as DNP, and hormones, such as insulin, and profound protection is observed with ischaemic preconditioning, in which short bursts of mild ischaemia are applied before prolonged ischaemia.11, 12, 13 More recently, profound cardioprotective effects of temperature preconditioning have been described, which involve brief bursts of hypothermia before ischaemia.14
Hypothermia is now considered to be one of the most potent cardioprotective strategies available and is used clinically to protect the heart against ischaemia in a number of surgical procedures, such as coronary bypass, valve repair and transplantation.15, 16 Many animal models have shown that hypothermia is protective, including a study in dogs in which whole-body hypothermia protected the ischaemic myocardium.17 Also, hypothermia localised to the myocardial risk zone early after the onset of coronary occlusion salvaged 18% of the risk region and significantly decreased the area of infarct in rabbit studies.15 Since then, myocardial hypothermia by endovascular cooling has been shown to decrease infarct size in pigs if administered during ischaemia, but not to be beneficial if administered at reperfusion.18 It is proposed that a 1-°C drop in body temperature slows metabolic rate by approximately 8%, 19 which may preserve ATP levels and explain some of the protection to the ischaemic myocardium by hypothermia. However, modest hypothermia (34 °C) only has a very mild effect on ATP levels, yet is still very protective, which suggests that the protection is more complex than just a case of energy preservation alone.20 The molecular mechanisms of hypothermic preconditioning are not fully understood.
The signalling pathways that are activated in response to a cardioprotective stimuli are not fully elucidated, but what is known is that preventing pathological mPTP opening underlies the infarct-limiting effects and may represent the end point of cardioprotective signalling pathways.8, 21 One set of signalling molecules characterised as having a role in myocyte survival signalling is the reperfusion injury salvage kinases (RISK).22 Involvement of the pro-survival kinase, extracellular signal-regulated kinase (ERK)1/2, a member of the RISK family, in preconditioning has been shown in a number of cardioprotective strategies, including ischaemic preconditioning.21, 23 Indeed, ERK1/2 phosphorylation is maintained during a 30 min ischemic period in isolated rabbit hearts perfused with hypothermic solutions, whereas ERK1/2 phosphorylation falls markedly after 10 min during normothermic ischaemia.24 ROS, possibly released from the mitochondria by mPTP flickering during ischemic preconditioning, has been postulated as a signal that may initiate subsequent survival pathways.21
In this study, the focus was on the effect of temperature preconditioning using rapid bursts of profound (16 °C) hypothermia in an isolated rat ventricular myocyte model of ischaemia/reperfusion injury. The effects of temperature preconditioning on contractile recovery and calcium homeostasis following exposure to simulated ischaemia/reperfusion injury were investigated. Using two independent fluorescence assays, the effect of temperature preconditioning on pathological mPTP opening was tested. How temperature preconditioning affected mPTP flickering rates was assessed with a calcein–cobalt quench assay. Using a novel mitochondrially targeted ROS biosensor,25 the timing of ROS release from the mitochondria during the temperature preconditioning protocol was investigated, and how this affects the downstream ERK1/2 activation is shown.
Results
Temperature preconditioning improves recovery of contractile function and calcium homeostasis following simulated ischaemia/reperfusion injury
Temperature preconditioning, like ischaemic preconditioning, has been reported in whole-heart studies to significantly increase cardioprotection.14 To investigate the molecular mechanisms of temperature preconditioning in cardioprotection, adult rat hearts were dissociated into single ventricular myocytes and subjected to simulated ischaemia/reperfusion injury. The myocytes were perfused with Tyrode buffer and contracted in response to electrical field stimulation (1 Hz; Figure 1ai). Ischaemia was simulated by rapidly preventing myocyte ATP production using a ‘metabolic inhibition (MI) solution’. After several minutes, the myocytes lost their ability to contract and shortened into a state of rigor contracture (Figure 1aii). After 7 min of using the MI solution, reperfusion was simulated by re-energising the myocytes by perfusion with Tyrode buffer to wash out the inhibitors and reintroduce metabolic substrates for ATP generation. The number of myocytes that had regained their contractile function was quantified after 10 min of reperfusion (Figure 1aiii).
Isolated ventricular myocytes, temperature preconditioned by two 2-min incubations at 16 °C, showed a significant increase in recovery of contractile function when compared with control cells (51.6±5.7 versus 28.1±3.4%, Figure 1b). This improvement in contractile recovery was comparable to those produced by other known cardioprotective agents: the mitochondrial uncoupler, dinitrophenol (DNP) and the mPTP inhibitor, CsA (56.5±8.5 and 58.8±6.8%, respectively; Figure 1b).
The effects of preconditioning protocols on calcium homeostasis after simulated ischaemia/reperfusion of contracting myocytes were investigated using Fura2-loaded myocytes to report intracellular calcium changes. Temperature preconditioning had no effect on calcium homeostasis before MI (Figures 2ai and bi). However, following cessation of field stimulation at the end of the MI/reperfusion protocol, intracellular calcium was significantly lower for temperature preconditioned cells (132±17 nM) compared with control (301±52 nM; Figures 2aii and b). Temperature preconditioning resulted in a significant increase in the percentage of myocytes with a cellular calcium estimate <150 nM (Figure 2bii). Temperature preconditioning resulted in a significant improvement in the percentage of myocytes that regained synchronous calcium transients after MI/reperfusion compared with control. (Figure 2biii). Also, both pretreatment with the mitochondrial uncoupler DNP and the presence of CsA protected against the loss of calcium homeostasis after MI/reperfusion (Figures 2c and d).
Temperature preconditioning delays pathological mPTP opening in a model of reperfusion injury
The mPTP is considered to be the central determinant of myocyte fate following ischaemia/reperfusion injury, and cardioprotective signalling cascades are thought to converge on the mPTP to prevent opening and thus inhibit myocyte death.7, 26, 27, 28 The effect of temperature preconditioning on time to mPTP opening was investigated with two independent assays to quantify mitochondrial membrane potential in intact cardiac myocytes. In the first assay, the myocytes were loaded with a relatively high tetramethylrhodamine, methyl ester (TMRM) concentration (5 μM), which accumulates in the mitochondria and autoquenches to become non-fluorescent. Depolarisation of the mitochondrial membrane potential, due to mPTP opening, causes TMRM to be redistributed into the cytosol and dequenched, giving an increase in fluorescence. The mPTP opening was induced by oxidative stress caused by continuous illumination of TMRM at 546 nm.8 Under these conditions, both temperature preconditioning and DNP resulted in a significant delay in the time to fluorescence increase (mPTP opening) relative to control (2.5- and 1.7-fold increase, respectively) (Figures 3a–c). The presence of the known mPTP inhibitor, CsA, also resulted in a significant delay in the time required for mPTP opening to occur (Figure 3c). To exclude the possibility of a non-specific effect of CsA on calcineurin accounting for the delay in mPTP opening, experiments were conducted in the presence of FK-506, a calcineurin inhibitor, and no delay in mPTP opening was observed (Figure 3c). Conversely, carboxyatractyloside, an mPTP opener, resulted in a significant acceleration in the time to mPTP opening (Figure 3c).
As TMRM was used to both record and stimulate mPTP opening in this assay, a second assay was developed to confirm the results. Continuous illumination was avoided, and the myocytes were loaded with a relatively low concentration of TMRM (50 nM), which accumulates in the mitochondria, but not at a concentration high enough to quench so the fluorescence remains high. Myocyte mPTP opening was induced by ROS generated by addition of xanthine and xanthine oxidase. Upon mPTP opening, the fluorescence signal decreased as the TMRM redistributed into the cytosol and then into the bathing solution. No photodamage-induced mPTP opening was observed using this protocol, as fluorescence was measured at a sampling rate of 0.2 Hz (Figures 4ai and ii). The ROS donor, xanthine and xanthine oxidase caused a significant decrease in myocyte fluorescence (Figures 4a and b). Temperature preconditioning resulted in a significant delay in mitochondrial mPTP opening relative to control (15.1±1.3 min compared with 10.3±0.9 min, respectively) (Figures 4b and c). The presence of the mPTP inhibitor, CsA, also resulted in a significant delay in the time to mPTP opening compared with control (15.5±1.1 min compared with 10.3±0.9 min, respectively, Figure 4c).
Transient mPTP flickering is not altered by temperature preconditioning
It has been demonstrated that non-pathological, transient mPTP flickering occurs under basal conditions, and may serve as a way to regulate mitochondrial ROS and Ca2+ concentration within myocytes.29 The effect of temperature preconditioning on non-pathological mPTP flickering was investigated using a calcein–cobalt quench assay. Isolated ventricular myocytes were co-loaded with calcein-AM (1 μM) and cobalt chloride (1 mM). Calcein-AM readily crosses cell and mitochondrial membranes, whereas cobalt chloride is spatially restricted to the cytosol. Cobalt chloride quenches cytosolic calcein fluorescence to reveal a punctate pattern of mitochondrial calcein fluorescence. During basal mPTP flickering, calcein is released from mitochondria into the cytosol where its fluorescence is quenched by cobalt chloride. This is observed as a change in the fluorescence pattern from a mitochondrial punctuate pattern (Figure 5ai) to a decreased and diffuse fluorescence (Figure 5aii). Temperature-preconditioned myocytes showed a decrease in cellular fluorescence over the 30-min period to 78.8±4.1% of initial fluorescence, which was similar to that observed in control myocytes (80.2±7.2% of initial fluorescence; Figures 5b and c). However, when experiments were conducted in the presence of the known mPTP inhibitor, CsA, there was no decrease in cellular fluorescence (101.2±2.9% of initial fluorescence; Figures 5b and c).
Mitochondrial ROS production is essential for the protective effects of temperature preconditioning
Although excessive amounts of ROS are detrimental to myocyte viability, small amounts have been shown to have beneficial effects and are crucial to certain cardioprotective interventions, including ischaemic preconditioning.21, 30 To investigate the involvement of ROS in the signalling cascade of temperature preconditioning, isolated ventricular myocytes were infected with adenovirus, containing DNA encoding a mitochondrially targeted superoxide biosensor.25 After a 48-h infection, the myocytes expressing the biosensor were characterised by low-level fluorescence that increased after the addition of exogenous ROS. To confirm the sensitivity of the biosensor to ROS, myocytes were challenged with exogenous ROS by addition of xanthine and xanthine oxidase, and an increase in fluorescence was detected (Figures 6a and b). Infected myocytes were loaded with mitoTracker deep red, and co-localisation confirmed the mitochondrial localisation (Figure 6c). The table (Figure 6d) shows the infection efficiency for four representative experiments. The mitochondrial ROS increased, indicated by an increase in biosensor fluorescence, during the 2-min decrease in temperature to 16 °C (Figure 6e). Fluorescence rose rapidly upon the switch to the lower temperature and quickly reversed when the temperature was restored to 37 °C. To confirm the increase in ROS during the hypothermic steps of the temperature-preconditioning protocol, the experiments were repeated in the presence of a ROS scavenger, N-(2-mercaptopropionyl) glycine (MPG). Scavenging ROS significantly decreased the 16°C-induced increase in fluorescence observed during the temperature-preconditioning protocol (Figure 6e and f). Significantly, MPG also prevented the protective delay in time to mitochondrial depolarisation in response to photodamage, which was observed with temperature preconditioning (Figure 6g).
ERK activation is downstream of mitochondrial ROS production and is necessary for the protection induced by temperature preconditioning
The RISK pathway is a protective pathway shown to be activated by a number of cardioprotective interventions, including ischaemic preconditioning.31 A number of kinases have been demonstrated to be involved in the RISK pathway, one of which is the ERK.
The activation of ERK by temperature preconditioning was investigated by western blotting for active phosphorylated ERK (pERK). Control myocytes and myocytes that were analysed 10 min after the completion of the temperature preconditioning protocol were examined for pERK levels, with total ERK included as a loading control (Figure 7a and b). Temperature-preconditioned myocytes were found to have significantly greater levels of pERK compared with untreated control myocytes. The temperature-preconditioning-induced increase in pERK was abolished if temperature preconditioning was conducted in the presence of ERK activation inhibitors, either PD98059 or U0126 (Figure 7a and b). Furthermore, the temperature-preconditioning-induced activation of ERK was also abolished by the presence of the ROS scavenger, MPG, during the temperature-preconditioning protocol (Figure 7a and b).
The functional importance of the temperature-preconditioning-induced ERK activation was investigated by the temperature-preconditioning of myocytes in the presence of an ERK inhibitor, and testing the delay to photodamage-induced mPTP opening. Inhibition of ERK with either PD98095 or U0126 abolished the protective delay in time to mitochondrial membrane depolarisation conferred by temperature preconditioning (Figure 7c).
Discussion
The results of this study demonstrate that temperature preconditioning by two brief episodes of profound hypothermia (16 °C) results in strong cardioprotection of isolated ventricular myocytes against oxidative stress. Temperature preconditioning delays pathological mPTP opening, which is considered to be the end effector for preconditioning pathways. However, non-pathological transient mPTP opening or ‘flickering’ remains unaltered after the bursts of hypothermia. Mitochondrial ROS were produced during the brief bursts of hypothermia, which was shown to be necessary to signal cardioprotection. ERK activation is known to have an essential role in cardioprotective signalling, and mitochondrial ROS production was shown in this study to be required for ERK1/2 phosphorylation in temperature preconditioning.
The cardioprotective effects of hypothermia have been known for some time, but the mechanism of protection has not been clear. Although certainly preservation of ATP content during cooling is an attractive hypothesis, the profound protection observed, especially in mild hypothermia (32 °C), cannot be explained fully by ATP preservation alone.20 Hypothermic conditioning has been used advantageously in many clinical intracardiac settings, especially in transplantation.18 Indeed, the use of therapeutic hypothermia has the potential to reduce myocardial infarct size.32 The signalling events, which initiate the hypothermic cardioprotection, are described here.
Two cycles of hypothermia to 16 °C for 2 min, interspersed with normothermia at 37 °C for 3 min resulted in a significant improvement in recovery of contractile function after simulated ischaemia/reperfusion injury. This shows that the signalling pathways involved in temperature preconditioning exist at the level of individual myocytes and are independent of any signalling influence from other cell types present within the heart, such as endothelial cells or fibroblasts. These results are consistent with the observation that temperature preconditioning in the isolated whole heart improves haemodynamic recovery, decreases arrhythmia and reduces necrotic damage when assessed during reperfusion.14 Previous reports investigating the response of ex vivo whole hearts found that preconditioning at 26 °C gives optimal cardioprotection.33 In this study, although 26 °C preconditioning did result in cardioprotection, 16 °C gave a larger and more consistent cardioprotective effect. The reasons for this discrepancy are unclear and may relate to the fact that the myocytes in this study are isolated.
Elevated calcium in myocytes following ischaemia/reperfusion injury has pathophysiological implications associated with cellular injury. High intracellular calcium underlies hypercontracture, development of areas of cell death by necrosis,34, 35 and the activation of pro-apoptotic proteins and calcium-dependent proteases.36 Temperature preconditioning led to a significant increase in the number of myocytes with healthy calcium levels (calcium<150 nM) at the end of re-energisation compared with control myocytes. Temperature preconditioning also increased the percentage of myocytes that regained synchronous calcium transients and the proportion of myocytes that regained their contractile function in response to field stimulation. In addition, high mitochondrial matrix calcium concentration is a critical factor for the opening of the mPTP, which is believed to be central to myocyte death in the setting of ischaemia/reperfusion injury.37 Therefore, maintenance of calcium homeostasis of the hypothermically preconditioned myocytes may underlie many of the therapeutic benefits of temperature preconditioning already reported, including decreased infarct size.15
The opening of the mPTP was first proposed to be a mediator of cell death in the setting of acute ischaemia/reperfusion injury by Crompton et al. in 1986.38 Since then, the opening of mPTP has become well established as the key determinant of cell fate, although how mPTP opening is modulated is not fully understood.39 Inhibiting mPTP opening with agents, such as CsA, result in cardioprotection.6, 8 Temperature preconditioning of isolated cardiac myocytes delays the time to mitochondrial membrane potential depolarisation, which occurs on mPTP opening. This is consistent with reports that de-energised, isolated mitochondria harvested from temperature-preconditioned myocytes can inhibit calcium-induced mitochondrial swelling, which is also a reflection of the mPTP opening.14
Basal transient mPTP ‘flickering’ is proposed to allow release of excess mitochondrial ROS and calcium from the mitochondrial matrix.10 Moreover, hypoxic preconditioning has been shown to augment mPTP flickering, which was necessary for the development of cardioprotection.30 However, in this study, no changes in mPTP flickering were observed between the control and the temperature-preconditioned myocytes, but in all myocytes, the mPTP flickering was sensitive to CsA. This suggests that the modulation of mPTP that delays opening may be separate from that which affects basal flickering rates.
This study shows that mitochondrial ROS are produced during the hypothermic steps of temperature preconditioning, and that this is responsible for downstream activation of ERK1/2. A mitochondrially targeted superoxide biosensor 25 was used to report mitochondrial ROS production in cardiac myocytes. Bursts of mitochondrial ROS production were detected exclusively during the two hypothermic (16 °C) periods of the temperature-preconditioning protocol. Hypothermia-induced mitochondrial ROS production is an obligatory signalling event required for temperature preconditioning, because the presence of a ROS scavenger during temperature preconditioning ablates the protective delay in mitochondrial depolarisation. ROS production during hypothermia may be due to a respiratory ‘slow down’. ROS production was observed during metabolic depression of isolated mouse brain mitochondria that were maintained in hypothermic conditions.40 This may result from decreased activity of the F1/F0 ATPase and reduced oxygen consumption by the electron transport chain, which results in increased mitochondrial oxygen levels that can promote ROS production. Also consistent with these findings, hypothermia (17 °C) by cold perfusion of the isolated whole heart resulted in dihydroethidium fluorescence changes across the intact myocardial wall, suggesting an increase in ROS production.41
The activation of the pro-survival kinase, ERK1/2, is well established in cardioprotective pathways.21, 23 The cardioprotective effects of ischaemic preconditioning are, in part, due to activation of ERK1/2 within the first few minutes of reperfusion.22 However, it has recently been shown that when isolated whole hearts were maintained in mild hypothermia (35 °C) during ischaemia, ERK1/2 phosphorylation was preserved for the duration of the ischaemic period instead of steadily declining that occurs in normothermia.24 The preservation of ERK1/2 during the hypothermic ischaemic period conferred a significant cardioprotection.24 Temperature preconditioning results in a robust phosphorylation of ERK1/2 when measured 10 min after the temperature-preconditioning stimulus, but before the ischaemic insult. The cardioprotection by temperature preconditioning was blocked by inhibition of ERK1/2 activation, showing that this is a key step in the cardioprotective pathway. A critical role of ROS in the activation of ERK1/2 is shown, as scavenging ROS during the temperature preconditioning protocol was sufficient to abolish ERK1/2 activation and any subsequent cardioprotection. This shows that mitochondrial ROS production is upstream of and necessary for ERK1/2 activation in the temperature-preconditioning signalling cascade in cardiac myocytes. Temperature preconditioning may therefore share common cardioprotective signalling pathways with many preconditioning stimuli, such as ischaemic preconditioning, and mitochondrial uncouplers, such as DNP. The common pathway may stem from a decrease in mitochondrial respiration, leading to increased release of ROS and subsequent ERK1/2 activation.
Materials and Methods
Isolation of adult rat ventricular myocytes
Adult male Wistar rats (200–350 g) were killed by cervical dislocation in accordance with the UK Animals (Scientific Procedures) Act, 1986. The heart was rapidly excised and placed in nominally Ca2+-free Tyrode solution titrated to pH 7.4 with NaOH, containing 135 mM NaCl, 6 mM KCl, 0.33 mM NaH2PO4, 5 mMNa pyruvate, 10 mM glucose, 1 mM MgCl2 and 10 mM HEPES. Within 1 min, the heart was cannulated at the aorta and retrogradely perfused using a Langendorff apparatus for 6 min at a constant flow rate of 10 ml/min with Ca2+-free Tyrode at 37 °C, vigorously bubbled with 95% O2/5% CO2. The heart was then perfused with Ca2+-free Tyrode solution containing Type I collagenase (approximately 0.4 units/ml), protease type XIV (approximately 2.7 units/ml) and 0.05% bovine serum albumin for 7–10 min, to digest the heart. This was followed by perfusion for 3 min with Tyrode solution (containing 2 mM CaCl2) to remove the enzymes. Isolated ventricular myocytes were obtained by cutting the ventricular mass in two and gently agitating in Tyrode solution at 37 °C, in a shaking water bath. The isolation procedure typically yielded 70–90% viable rod-shaped myocytes. Following isolation, myocytes were stored in Tyrode solution at room temperature (approximately 21 °C) at a density of approximately 0.4 million cells/ml and were used for experimentation within 10 h. All compounds used throughout this study were acquired from Sigma-Aldrich (Gillingham, UK), unless otherwise stated.
MI and re-energisation
In this study, the MI solution was the substrate-free Tyrode solution containing 140 mM NaCl, 6 mM KCl, 0.33 mM NaH2PO4, 10 mM sucrose, 1 mM MgCl2, 2 mM CaCl2 and 10 mM HEPES, and was titrated to pH 7.4 using NaOH with cyanide (2 mM) and iodoacetic acid (1 mM). The MI solution contained iodoaectic acid (1 mM) to inhibit glyceraldehyde 3-phosphate dehydrogenase and cyanide (2 mM) to block electron transfer from complex IV of the electron transport chain. The MI solution also lacked the metabolic substrates, glucose and pyruvate, which are necessary for ATP generation.11 Isolated myocytes were superfused with MI solution for 7 min, followed by 10 min of re-energisation by superfusion with Tyrode solution to simulate reperfusion injury. For assays in which MI was used, all cardiac myocytes were subjected to the MI/reperfusion protocol, and the control group were populations of cardiac myocytes that had not had prior hypothermia or drug treatment.
Temperature preconditioning of isolated ventricular myocytes
For the purposes of temperature preconditioning, isolated ventricular myocytes in Tyrode solution (approximately 0.4 million cells/ml) was placed in a water bath to reach a final temperature of 16 °C for a 2-min period. The myocytes were then immersed in a water bath at 37 °C for 3 min. Temperature preconditioning using confocal microscopy of the mt-cpYFP superoxide biosensor was conducted within the microscope chamber and was achieved by superfusing myocytes with Tyrode solution cooled to 16 °C for 2 min and 37 °C for 3 min for two cycles.
Measurement of myocyte contractile recovery
Isolated ventricular myocytes were placed in a diamond-shaped chamber with a parallel alignment of two platinum electrodes for electric-field stimulation at 1 Hz (physiological stimulator, Farnell, Leeds, UK) on the stage of a Nikon (Kingston upon Thames, UK) inverted light microscope. Myocytes were perfused at 33–35 °C at a rate of 4.5 ml/min. Viable rod-shaped cells that were synchronously contracting in response to electric-field stimulation were identified, and the contractile response of these myocytes was then tracked throughout 7 min of superfusion with MI and 10 min of re-energisation with Tyrode solution. Those myocytes that were contractile at 10 min of re-energisation were considered to have recovered their contractile function. Myocytes that did not respond to the electrical field stimulation or contracted asynchronously were deemed not to have recovered contractile function. For the purposes of temperature preconditioning, myocytes were temperature preconditioned before being placed in the chamber. For DNP preconditioning, myocytes were superfused within the chamber for 5 min in substrate-free Tyrode containing DNP (50 μM), followed by 5 min in substrate-free Tyrode solution immediately before MI. Where CsA was used, 4 μM was present throughout the entire experiment.
Fluorescence imaging
Isolated ventricular myocytes were placed in the chamber of a Nikon (Eclipse TE200) inverted epifluorescence microscope. Myocytes were superfused with Tyrode solution at a rate of 4.5 ml/min at 34 °C (Dagan, Minneapolis, MN, USA). For calcium imaging experiments, myocytes were stimulated in an electrical field at 1 Hz (Research Stimulator, Harvard Apparatus, Kent, UK). For fluorescence imaging, myocytes were illuminated at the appropriate wavelength using a monochromator (PTI deltaRAM), emission was measured using a CCD camera (Photometrics Cascade: 512B; Roper Scientific, Inc., Tucson, AZ, USA) and EasyRatioPro software was used for all analysis (PTI, Birmingham, NJ, USA).
For calcium imaging, isolated ventricular myocytes were loaded for 20 min at room temperature (approximately 21 °C) in Tyrode solution with the ratiometric calcium-sensitive dye, fura-2AM (Invitrogen, Paisley, UK; 2.5 μM in Tyrode solution). Myocytes were imaged with a × 20 fluorescence objective and were alternately excited at 340 and 380 nm. Emission was recorded at >520 nm. All rod-shaped myocytes that responded to the electrical field stimulation (1 Hz) at the start of the experiment were included in the study. A calcium calibration was achieved by exposing fura-2-loaded and ionomycin (10 μM)-treated myocytes to a high calcium solution (10 mM), followed by exposure to a calcium-free solution (EGTA, 15 mM). Fluorescence was measured after 10 min of re-energisation, when the stimulator had been turned off to measure basal cellular calcium levels. A calcium calibration kit was used to estimate free calcium (Invitrogen). This method of calcium calibration is crude and was only intended to give a rough estimate of cellular calcium concentrations for the purposes of comparison.
For measurements of mPTP opening, a well-established assay was used, which takes advantage of both the facts that TMRM, continuously illuminated at 546 nm, will produce ROS that induce mPTP opening, and that TMRM fluorescence reports changes in mitochondrial membrane potential.8 Isolated ventricular myocytes were loaded with the fluorescent dye TMRM (5 μM) at 37 °C for 15 min, washed and imaged using a × 60 oil immersion objective. TMRM-loaded myocytes were continuously excited at 546 nm and the emission measured using a long-pass filter at >560 nm. Depolarisation of the mitochondrial membrane potential was reported by an increase in TMRM fluorescence, as it dequenched on leaving the mitochondria.
For experiments with relatively low TMRM (50 nM), a low sampling rate (0.2 Hz) was used to decrease TMRM excitation. Xanthine (2 mM) and xanthine oxidase (20 mU) were superfused onto the myocytes to provide ROS for induction of mPTP opening. Depolarisation of the mitochondrial membrane potential was reported by a decrease in TMRM fluorescence, as the dye diffused from the mitochondria and the cell.
For the detection of mPTP flickering, isolated ventricular myocytes were loaded with calcein-AM (1 μM; Invitrogen) and cobalt chloride (1 mM; Invitrogen) for 15 min at room temperature (approximately 21 °C), imaged using a × 60 oil immersion objective and were excited at 488 nm, and the calcein fluorescence emission collected using a long-pass filter >505 nm. Three images of calcein fluorescence were measured at times 0, 10 and 30 min from rod-shaped myocytes. When mPTP flickering occurs, calcein is redistributed to the cytoplasm and quenched by cobalt, which is measured as a decrease in fluorescence.
For measuring mitochondrial ROS formation, ventricular myocytes were infected with adenovirus encoding mt-cpYFP for 48 h. Ventricular myocytes were cultured in media 199 supplemented with ITS+3 (2 mg/ml), carnitine (2 mM), creatine (5 mM), taurine (5 mM), T3 (1.5 pM), and penicillin and streptomycin (100 units) at 37 °C and 5% CO2. After 48 h, approximately 70% of myocytes were infected. The mt-cpYFP fluorescence was measured using confocal microscopy on an Olympus IX70 confocal microscope (Olympus, Southend-on-Sea, UK) with a × 60 oil immersion objective, and myocytes were excited using the argon laser (Melles Griot, Albuquerque, NW, USA) at 488 nm, and the mt-cpYFP emission was collected at 0.2 Hz using a long-pass filter >515 nm.
For co-localisation analysis, 48 h infected myocytes were loaded with MitoTracker deep red (500 nM; Invitrogen) for 20 min at room temperature (approximately 21 °C) and washed. For measurement of the MitoTracker deep red fluorescence, myocytes were illuminated using red helium-neon laser (Melles Griot) at 633 nm, and fluorescence was measured using a 660 nm long-pass filter.
Western blotting
A sample of cardiac myocytes were temperature preconditioned in the presence or absence of ERK1/2 inhibitors, either PD98095 (10 μM) or U0126 (0.5 μM), or the ROS scavenger MGP (300 μM). The myocytes were then lysed, and the collected protein was subjected to SDS-PAGE. Equal amounts of protein, measured by the Bradford assay, from each treatment group were loaded in each well. The phosphorylation state of ERK1/2 (p42/p44) protein level was determined for each treatment group. Both ERK1/2 antibodies were obtained from Cell Signaling Technology (Hitchin, UK) and were used in accordance with the manufacturer’s instructions. The pERK levels were normalised to the respective total-ERK levels in each well. Relative densitometry was determined using Felix, a computerised software analysis package.
Statistics
Values are expressed as mean±S.E.M. Data were analysed by an unpaired Student’s t-test or a one-way analysis of variance, as appropriate, P<0.05 was considered significant. Where data is expressed as ‘normalised to control’, this indicates that all data values were divided by the mean control value for the data set.
Abbreviations
- mPTP:
-
mitochondrial permeability transition pore
- ROS:
-
reactive oxygen species
- MPG:
-
N-(2-mercaptopropionyl) glycine
- ERK:
-
extracellular signal-regulated kinases
- RISK:
-
reperfusion injury salvage kinases
- MI:
-
metabolic inhibition solution
- TMRM:
-
tetramethylrhodamine, methyl ester
- CsA:
-
cyclosporine A
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Acknowledgements
We are grateful to the British Heart Foundation for research funding for this project (FS/08/045/25508), Dr. Heping Cheng for the gift of mt-cpYFP, and Mrs. Sonja Khemiri for assistance with adenovirus preparation.
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Bhagatte, Y., Lodwick, D. & Storey, N. Mitochondrial ROS production and subsequent ERK phosphorylation are necessary for temperature preconditioning of isolated ventricular myocytes. Cell Death Dis 3, e345 (2012). https://doi.org/10.1038/cddis.2012.84
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DOI: https://doi.org/10.1038/cddis.2012.84
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