Concentration-Response Relationships for Adenosine Agonists During Preconditioning of Rabbit Cardiomyocytes

Rice, Peter J., Armstrong, Stephen C., Ganote, Charles E.

01 January 1996

Although adenosine receptors have been implicated in the induction of preconditioning in a variety of experimental models, there is controversy concerning the specific adenosine receptor subtypes mediating this effect. Concentration-protection relationships for adenosine and adenosine agonists in rabbit cardiomyocytes were used to characterize the role of adenosine receptor subtypes in preconditioning. Isolated cells were ischemically preconditioned or pre-incubated for 10 min with increasing concentrations of adenosine, CCPA (2-chloro-N6-cyclopentyladenosine) APNEA (N6-2-(4-aminophenyl)ethyladenosine), or BNECA (N6-benzyl-5'-N-ethyl-carboxamidoadenosine) in the presence or absence of 1 or 10 μM of the selective A1-adenosine antagonist DPCPX (8-Cyclopentyl-1,3-dipropylxanthine). Following a 30-min post-incubation period, cells were pelleted, layered with oil and ischemically incubated for 180 min. Injury was assessed by osmotic swelling and trypan blue exclusion of sequential samples, and determination of the areas beneath the mortality curves. Adenosine produced a broad concentration-protection curve which was displaced to the right by DPCPX. The curve for A1-selective agonist CCPA was biphasic, with an initial response below 1 nM and a second above 1 μM. DPCPX abolished the early response leaving a steep monophasic curve between 0.1 and 10 μM CCPA. The APNEA curve appeared monophasic, the major slope occurring between 1-100 nM; DPCPX (1 μM) shifted the concentration-response curve ≃ 30-fold and decreased the slope. Adenosine receptor agonist BNECA produced preconditioning characterized by a shallow monophasic concentration-protection curve with a maximal effect of 49% and an EC50 of ≃ 5 nM; DPCPX shifted the BNECA concentration-protection relationship ≃ 40-fold with only a modest increase in slope. Analysis of the data suggests that induction of preconditioning results from interaction of agonists with the A1 receptor and a second adenosine receptor having properties consistent with the A3 receptor. Adenosine, CCPA, APNEA, BNECA and DPCPX each appear to be selective for the A1 adenosine receptor subtype in isolated rabbit cardiomyocytes.

adenosine receptors

ischemic injury

ischemic preconditioning

isolated myocyte

Biomedical Sciences

Effects of Calcium Depletion and Loading on Injury During Metabolic Inhibition of Isolated Adult Rat Myocytes

Rim, Dianne S., Altschuld, Ruth A., Ganote, Charles E.

01 January 1990

The hypothesis that calcium influxes from the extracellular space play an important role in the pathogenesis of irreversible anoxic injury was tested using isolated adult rat myocytes. Myocytes treated with 6 mm amytal and 3 mm iodoacetate and subsequently incubated in either calcium-containing (1.12 mm) or calcium-free media (with or without 1 mm EGTA) developed rigor contracture (cell squaring) and cell death (trypan blue permeability) at the same rate. The rates of cell death in both calcium-containing and calcium-free media were increased by incubation in hypotonic media even though the rates of contracture development remained unaltered. Cells developed osmotic fragility prior to membrane permeability increases. The calcium ionophore, A23187 (10 μm), induced rapid rounding of rod-shaped cells subjected only to mitochondrial inhibition in calcium containing media, confirming its ability to cause an increase in cellular permeability to calcium. However, A23187 did not alter the rates of cell death of totally metabolically inhibited myocytes in either calcium-containing or calcium-free media with EGTA. The results indicate that influxes of calcium are not necessary for the development of irreversible injury in metabolically inhibited, isolated myocytes.

anoxic injury

calcium

isolated myocyte

membrane injury

osmotic fragility

In Vitro Ischaemic Preconditioning of Isolated Rabbit Cardiomyocytes: Effects of Selective Adenosine Receptor Blockade and Calphostin C

Armstrong, S., Ganote, C. E.

01 January 1995

Objective: The aim was to determine if in vitro ischaemic preincubation can precondition cardiomyocytes and if the responses to adenosine receptor antagonists are similar to those previously determined during 'metabolic' preconditioning with glucose deprivation or adenosine agonists. Methods: Isolated rabbit cardiomyocytes were preconditioned with 10 min of ischaemic preincubation, followed by a 30 min postincubation before the final sustained ischaemic period. The protein kinase C inhibitor calphostin C or the adenosine receptor antagonists 8-sulphophenyltheophylline (SPT), BW 1433U, and 1,3-dipropyl-8-cyclopentylxanthine (DPCPX) were added either during the preincubation or into the final ischaemic pellet. Adenosine deaminase (10 U·ml-1) was added during ischaemic preincubation. Rates of contracture and extent of injury were determined by sequential sampling and assessment of trypan blue permeability following 85 mOsM swelling. Results: Myocytes were preconditioned by a 10 min in vitro ischaemic preincubation. Preincubation with 100 μM SPT or with adenosine deaminase, or addition of 200 nM calphostin C into the final ischaemic pellet did not alter rates of rigor contracture but nearly abolished protection. A significant degree of protection was maintained following ischaemic preincubation with the highly selective adenosine A1 receptor blocker DPCPX (10 μM), while the A1/A3 antagonist BW 1433U (1 μM) severely limited protection. SPT and BW 1433U added only into the final ischaemic pellet of preconditioned cells significantly blocked protection, while protection was maintained in the presence of DPCPX. Conclusions: Ischaemic preconditioning of cardiomyocytes is blocked by adenosine receptor antagonists known to bind to A3 receptors but not by DPCPX which has high affinity for A1 receptors, but little affinity for A3 receptors. Maintenance of protection during the final ischaemic phase has a similar receptor specificity. Blockade of protein kinase C activity abolishes protection. Ischaemic and metabolic preconditioning in vitro appear to occur through similar pathways.

adenosine A receptor 3

adenosine receptors

ischaemic injury

ischaemic preconditioning

isolated myocyte

protein kinase C

In Vitro Ischaemic Preconditioning of Isolated Rabbit Cardiomyocytes: Effects of Selective Adenosine Receptor Blockade and Calphostin C

Armstrong, Stephen, Ganote, Charles E.

01 September 1994

Objective: The aim was to determine if in vitro ischaemic preincubation can precondition cardiomyocytes and if the responses to adenosine receptor antagonists are similar to those previously determined during "metabolic" preconditioning with glucose deprivation or adenosine agonists. Methods: Isolated rabbit cardiomyocytes were preconditioned with 10 min of ischaemic preincubation, followed by a 30 min postincubation before the final sustained ischaemic period. The protein kinase C inhibitor calphostin C or the adenosine receptor antagonists 8-sulphophenyltheophylline (SPT), BW 1433U, and 1,3-dipropyl-8-cyclopentylxanthine (DPCPX) were added either during the preincubation or into the final ischaemic pellet. Adenosine deaminase (10 U · ml-1) was added during ischaemic preincubation. Rates of contracture and extent of injury were determined by sequential sampling and assessment of trypan blue permeability following 85 mOsM swelling. Results: Myocytes were preconditioned by a 10 min in vitro ischaemic preincubation. Preincubation with 100 μM SPT or with adenosine deaminase, or addition of 200 nM calphostin C into the final ischaemic pellet did not alter rates of rigor contracture but nearly abolished protection. A significant degree of protection was maintained following ischaemic preincubation with the highly selective adenosine A1 receptor blocker DPCPX (10 μM), while the antagonist BW 1433U (1 μM) severely limited protection. SPT and BW 1433U added only into the final ischaemic pellet of preconditioned cells significantly blocked protection, while protection was maintained in the presence of DPCPX. Conclusions: Ischaemic preconditioning of cardiomyocytes is blocked by adenosine receptor antagonists known to bind to A3 receptors but not by DPCPX which has high affinity for A1 receptors, but little affinity for A3 receptors. Maintenance of protection during the final ischaemic phase has a similar receptor specificity. Blockade of protein kinase C activity abolishes protection. Ischaemic and metabolic preconditioning in vitro appear to occur through similar pathways.

adenosine A3 receptor

adenosine receptors

ischaemic injury

Ischaemic preconditioning

isolated myocyte

protein kinase C

Adenosine Receptor Specificity in Preconditioning of Isolated Rabbit Cardiomyocytes: Evidence of a₃ Receptor Involvement

Armstrong, Stephen, Ganote, Charles E.

01 January 1994

Objective: The aim was to further characterise an experimental model of preconditioning of isolated rabbit cardiomyocytes and to determine the role of adenosine receptor subtypes in initiation of the protective response. Methods: Isolated myocytes were subjected to 5 min preincubation in the presence or absence of glucose and various agonists and antagonists of adenosine receptors. Ischaemic pelleting was preceded by a 30 min postincubation period. Rate and extent of injury during ischaemia was determined by sequential sampling of the pelleted cells and assessment of trypan blue permeability following 85 mOsm swelling. Results: Myocytes were preconditioned with a 30-50% reduction of injury by a 5 min glucose-free preincubation. Substitution of 5 mM pyruvate for glucose during preincubation did not prevent the protective response. Protection was maintained over a 60-180 min postincubation period. Protection was blocked by 100 μM of the non-specific adenosine A1A2, antagonist SPT, both when added only during preincubation or only into the ischaemic pellet. Calphostin C, a specific protein kinase C inhibitor at 200 nM, added to the ischaemic pellet blocked protection. Preincubation with R-PIA, the adenosine A1 agonist, did not precondition at an A1 selective dose of 1 μM, but did at 100 μM. The selective A2 agonist CGS 12680 (1 μM) did not precondition. The selective A1/A3 adenosine agonist, APNEA, preconditioned at 1 μM and 200 nM dose levels. Preconditioning induced either by 200 nM APNEA or by glucose-free preincubation was not blocked by 200 nM or 10 μM of the A1 antagonist DPCPX, which has extremely low affinity for A3 receptors, but was blocked by 1 μM of the A1/A3 adenosine antagonist BW 1433U83. Conclusions: Preconditioning can be induced in isolated myocytes by a 5 min preincubation/30 min postincubation protocol, and a similar protection induced by adenosine agonists with A3, but not A1 selectivity. Preconditioning is blocked by non-selective or selective A1/A3 adenosine antagonists and a specific protein kinase C inhibitor, but not by A1 antagonists with little affinity for A3 receptors. The results suggest that preconditioning in isolated rabbit myocytes requires participation of adenosine receptors with agonist/antagonist binding characteristics of the A3 subtype, and is likely to be mediated by activation of protein kinase C.Cardiovascular Research 1994;28:1049-1056.

adenosine agonists

adenosine receptors

heart

ischaemic injury

ischaemic preconditioning

isolated myocyte

Preconditioning of Isolated Rabbit Cardiomyocytes: Effects of Glycolytic Blockade, Phorbol Esters, and Ischaemia

Armstrong, Stephen, Ganote, Charles E.

01 January 1994

Objective: The aim was to discriminate among several hypotheses of preconditioning of isolated rabbit cardiomyocytes and to determine if ischaemic preincubation would evoke a protective response. Methods: Isolated myocytes were subjected to 5 min of preincubation, in the presence or absence of glucose, and incubated in the presence of 1 mM iodoacetic acid during the final sustained ischaemic period. In a second series, the protein kinase C (PKC) activators phorbol 12-myristate 13-acetate (PMA), ingenol 3, 20-dibenzoate, and thymeleatoxin were added during preincubation. In a third series, preincubation periods were substituted by brief ischaemic pelleting of cells. Final prolonged ischaemic pelleting was preceded by a 30 min postincubation period. Rate and extent of injury was determined by sequential sampling and assessment of trypan blue permeability following 85 mOsM swelling. Results: Myocytes were preconditioned by a 5 min glucose-free preincubation. Addition of iodoacetic acid into the final ischaemic pellet increased the rates of rigor contracture and injury, but did not abolish the protective response. Direct protein kinase C activation with PMA, a non-selective phorbol ester, and ingenol, an ε, δ-PKC isozyme selective activator, protected cells, but thymeleatoxin, an α,β,γ-PKC isozyme selective activator, did not. A 10 min ischaemic preincubation preconditioned, but the protection was not enhanced when ischaemia was extended to 30 min, or when PMA was included during the initial ischaemic preincubation. Adenosine partially inhibited the response. Conclusions: (1) Preconditioning of isolated myocytes is not dependent on glycolysis or glucose transport. (2) Preconditioning appears dependent on activation of the ε-PKC isoformn. (3) Ischaemia is capable of preconditioning isolated myocytes in vitro, and initiation of this effect is modified by simultaneous additional of adenosine but not by direct protein kinase C activation with PMA. Induction of protection by PMA and ingenol shows that protection requires protein kinase C activation, but direct potassium channel activation by regulatory G proteins is not critical.Cardiovascular Research 1994;28:1700-1706.

adenosine receptors

glycolysis

ischaemic injury

ischaemic preconditioning

isolated myocyte

phorbol esters

protein kinase C

Effects of 2,3-Butanedione Monoxime (BDM) on Contracture and Injury of Isolated Rat Myocytes Following Metabolic Inhibition and Ischemia

Armstrong, Stephen C., Ganote, Charles E.

01 January 1991

The relationship between myocardial cell contracture and injury during total metabolic inhibition (amylobarbital and iodacetic acid) and ischemia was examined, using 5-50 mm butanedione monoxime (BDM) as an inhibitor of contracture. BDM had no apparent effect on control myocytes during 180 min incubations, but inhibited contracture following anoxia or ischemia in a dose-dependent fashion, as directly quantitated by length/width ratios. Cellular ATP levels decreased at a similar rate in the absence or presence of BDM, following metabolic inhibition. BDM-mediated inhibition of contracture was associated with accelerated cell injury, as defined by: the uptake of an extracellular marker (trypan blue) by the cardiomyocytes, by direct analysis of myoglobin released into the supernatant and by ultrastructural demonstration of defects in sarcolemmal membrane integrity. Calcium was not required for BDM's enhancement of injury, in that cells incubated in calcium free-EGTA buffer showed a similar BDM-mediated acceleration of injury. In the presence or absence of calcium, enhancement of injury was more marked in cells osmotically stressed with a brief incubation in hypotonic buffer, than in cells resuspended in isotonic media. It is concluded that BDM enhances development of osmotic fragility of inhibited or ischemic cardiomyocytes and that contracture is not a necessary contributing factor to myocardial cell death.

ATP

BDM

butanedione monoxime

calcium

contracture

ischemic injury

isolated myocyte

osmotic fragility

Atividade contratil e mobilização de calcio em miocitos ventriculares na presença de solução hiperosmotica de NaCI / Contractile activity and calcium cycling in ventricular myocytes exposed to NaCI hyperosmotic solution

Ricardo, Rafael de Almeida

08 March 2005

Orientadores: Jose Wilson Magalhães Bassani, Rosana Almada Bassani / Dissertação (mestrado) - Universidade Estadual de Campinas, Faculdade de Engenharia Eletrica e de Computação / Made available in DSpace on 2018-08-05T08:06:24Z (GMT). No. of bitstreams: 1 Ricardo_RafaeldeAlmeida_M.pdf: 2095157 bytes, checksum: 9fa58fb47d65f96bb946104c547ac025 (MD5) Previous issue date: 2005 / Resumo: A infusão intravenosa de solução hiperosmótica de NaCI tem se mostrado eficaz como tratamento único para a condição de choque hemorrágico, mas o conhecimento de seus efeitos sobre o coração ainda é limitado. Neste trabalho, desenvolvemos instrumentação para registro de encurtamento celular e investigamos o efeito direto de soluções hiperosmóticas de NaCI sobre a atividade contrátil e transientes de Ca2+ em miócitos ventriculares isolados de rato. A amplitude do encurtamento celular (?EC) e dos transientes de Ca2+ (?[Ca2+]i, medida com indo-1) foi registrada em miócitos estimulados a 0,5 Hz antes e depois do incremento da osmolaridade extracelular em 85 mOsm/l pela adição de sacarose (HiperSac) ou NaCI (HiperNac) à solução de perfusão. Variações do conteúdo de Ca2+ e da liberação fracional de Ca2+ do retículo sarcoplasmático (RS) também foram avaliadas. Simulação computacional (LabHeart v. 4.9.5) de transientes de Ca2+ e curva corrente-tensão da troca Na+-Ca2+ (NCX) foram usados para auxiliar o entendimento dos resultados. A perfusão dos miócitos com solução HiperNac provocou redução transitória, seguida de recuperação de ?[Ca2+]i e ?EC. Por outro lado, a perfusão com HiperSac reduziu de maneira persistente a ?EC, sem alterar ?[Ca2+];. O aumento da liberação fracional de Ca2+ do RS (p< 0,05) provocado pela solução HiperNac pode ter contribuído para a recuperação de ?[Ca2+];. A hiperosmolalidade per se prolongou o relaxamento, sem afetar a cinética de {Ca2+]j, possivelmente por aumento da viscosidade intracelular. A queda mais lenta de [Ca2+]; durante o transiente induzido por cafeína é compatível com redução da extrusão de Ca2+ via NCX devida ao acúmulo intracelular lento de Na+ na condição de hiperosmolaridade. Os resultados da simulação computacional estão de acordo com esta hipótese / Abstract: Intravenous injection of hyperosmolar NaCI solution has been used as the sole treatment for hemorrhagic shock, but its effects on heart muscle are not completely elucidated. In this work, we developed instrumentation for cell shortening measurement and investigated the direct effects of hyperosmolar NaCI solution on contractile activity and cytosolic Ca2+ concentration ([Ca2+]i) in isolated rat ventricular myocyte. Cell shortening (LlEC) and Ca2+ transient amplitude (?[Ca2+]j, measured with indo-1) were recorded in myocytes stimulated at 0.5 Hz before and after increasing extracellular osmolarity in 85 mOsm/l by sucrose (HiperSac) or NaCI (HiperNac) addition to the perfusate. Sarcoplasmatic reticulum (RS) Ca2+ load and fractional release were estimated. Computational simulation (LabHeart, v. 4.9.5) of Ca2+ transient and Na+-Ca2+ exchange voltage-current relationship was performed. HiperNac perfusion caused transient decrease of ?[Ca2+]i and LlEC, followed bya gradual recovery. HiperSac perfusion caused a monophasic decrease of LlEC, but did not change ?[Ca2+]i. Increased fractional RS Ca2+ release (pc:; 0.05) in the presence of HiperNac may have contributed to the delayed recovery of ?[Ca2+]i. Hyperosmolarity per se prolonged cell relaxation, but did not affect [Ca2+]i decline kinetics, possibly by increased intracellular viscosity. Slower [Ca2+]i decay during caffeine-induced transients indicates decreased NCX-mediated Ca2+ efflux transport following progressive intracellular [Na+] accumulation due to extracellular hyperosmolarity. Computational simulation results agree with this hypothesis / Mestrado / Engenharia Biomedica / Mestre em Engenharia Elétrica

Coração - Ventriculo esquerdo

Células musculares

Cálcio

Fluorescência

Choque hemorragico

Uso terapeutico de solução hipertonica

Heart

Isolated myocyte

Calcium

Fluorescence

Hemorrhagic shock

Hypersosmolarity

Sodium chloride