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Evaluating forearm vascular adaptations to training interventions : an in vivo and in vitro approachThompson, Emilia January 2014 (has links)
Exercise training promotes a beneficial endothelial cell (EC) phenotype and results in conduit vessel adaptation. The specific underlying mechanisms have been proposed (shear stress, circumferential stress, hypoxia, metabolic) but are yet to be fully elucidated. This thesis investigated the predominant stimuli responsible for conduit vessel adaptation with training. Further, it developed a method of in situ EC extraction to allow for determination of the cellular and molecular mechanisms underpinning these adaptations. The methodology utilised two-dimensional (2D) Doppler ultrasound, strain gauge plethysmography, immunocytochemistry and RT-qPCR to provide insight in to vascular characteristics, predominantly of the brachial artery and peripheral EC. Long-term repeated isometric forearm muscle contractions as performed by well-trained rock climbers promoted greater resting, peak (in response to 5 min ischaemia) and maximal (in response to ischaemic exercise) brachial artery diameters compared with controls. This structural response is dependent upon confounders associated with exercise additional to shear stress as evidenced by the lack of brachial artery remodelling in response to 8 weeks of ischaemic preconditioning (IPC). A transient increase in flow-mediated dilation (FMD)% was observed following 6 weeks exposure to IPC, which became significant when controlled for baseline artery diameter, despite an absence of augmentation following long-term (≥ 8 weeks) exposure to a shear stimulus. This is in line with the suggested timeline of conduit vessel adaptation to exercise training of a transient increase in function at 2-4 weeks. Underpinning molecular mechanisms responsible were not determined but may be further investigated given that the endovascular biopsy technique was developed and improved in this thesis. The endovascular biopsy successfully yields approximately 2100 ± 1700 EC per sample, providing sufficient material for determination of expression of both mRNA (RT-qPCR) and protein (immunocytochemistry). Specifically, type 2 diabetics (T2DM) with symptomatic cardiac abnormalities exhibited augmented eNOS mRNA and protein in brachial artery EC as compared with non-diabetic controls with symptomatic cardiac abnormalities. In conclusion, this thesis demonstrates that although shear stress promotes a transient trend for enhancement in function of the peripheral conduit arteries, additional factors are required for long-term structural adaptations. Further, the endovascular biopsy technique offers a novel method of extracting and analysing EC for genes and proteins of interest to vascular health. The use of this technique to decipher the underlying cellular and molecular mechanisms involved in vascular adaptations with exercise requires further investigation.
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Ischaemic preconditioning in exercise and disease : one size fits all?Seeger, Joost January 2016 (has links)
Ischaemia reperfusion injury (IR-injury) occurs when blood supply to a certain area of the body is blocked, and is subsequently followed by reperfusion. During the period of ischaemia, tissue is damaged as a result of lack of oxygen. Rapid reperfusion is mandatory, but unfortunately causes damage in addition to the damage induced by ischaemia alone. While a prolonged period of ischaemia is harmful to the bodily tissue, short periods of ischaemia interspersed with short bouts of reperfusion have protective effects. This mechanism is called ischaemic preconditioning (IPC). In this thesis, the impact of co-morbidity and age on IR-injury and IPC are explored. Moreover, the possible role of IPC to enhance exercise performance is investigated. Finally an attempt is made to understand the interchangeable effects of IPC and exercise performance in the prevention of IR-injury. Using the brachial artery endothelial function as a surrogate marker, first the consequences of IR-injury in both young and older individuals on endothelial function were studied. It was also assessed whether IPC could prevent endothelial IR-injury. It was found that endothelial function in both groups declined, when IR-injury was not preceded with IPC. However, when IPC was applied prior to IR-injury, a protective effect was detected in young subjects, but not in older participants. In chapter 5, this study was repeated in patients with heart failure, as they are at an increased risk for IR-injury. While in both groups a significant decline in endothelial function was observed, a much larger decline was established in the heart failure group. Moreover, IPC failed to protect against endothelial dysfunction in heart failure patients after IR-injury. The third study presented in this thesis, focused on the question whether exercise performance enhancement during a 5-km time trial was comparable when IPC on the upper legs was applied immediately before the time trial versus 24 hours (24-IPC) prior to exercise. Interestingly, a significant and strong correlation was found in finish time between acute IPC and 24-IPC, suggesting comparable effects of IPC and 24-IPC on exercise performance. In a follow-up study, it was determined whether local IPC applied on the upper arm, or remote IPC applied on the legs, would lead to an improved maximum incremental arm crank exercise test in individuals with a complete spinal cord lesion. The main finding was that upper arm IPC led to an increased performance enhancement, whilst remote IPC (stimulus below the lesion) did not lead to any significant differences. These studies help to inform the best or most practical application of IPC in daily life situations. Some previous work has suggested that exercise may resemble some of the effects of IPC. More specifically, acute exercise might possess the same protective effects against ischaemia-reperfusion injury as IPC. Therefore, in young healthy individuals it was studied, whether an acute bout of endurance or interval exercise is able to protect against brachial endothelial IR-injury. It was established that interval exercise prevented endothelial dysfunction after an IR stimulus, while no protective effect of endurance exercise was found. It was concluded that interval exercise, but not endurance exercise, prevented endothelial dysfunction after an ischaemic period. In conclusion, this thesis provides further evidence for the protective effects of (remote) IPC, both on the prevention of endothelial IR-injury as well as improvement in exercise performance. However, effects may depend on the protocol and population studied.
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In Vitro Ischaemic Preconditioning of Isolated Rabbit Cardiomyocytes: Effects of Selective Adenosine Receptor Blockade and Calphostin CArmstrong, S., Ganote, C. E. 01 January 1995 (has links)
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.
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In Vitro Ischaemic Preconditioning of Isolated Rabbit Cardiomyocytes: Effects of Selective Adenosine Receptor Blockade and Calphostin CArmstrong, Stephen, Ganote, Charles E. 01 September 1994 (has links)
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.
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Adenosine Receptor Specificity in Preconditioning of Isolated Rabbit Cardiomyocytes: Evidence of a<sub>3</sub> Receptor InvolvementArmstrong, Stephen, Ganote, Charles E. 01 January 1994 (has links)
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.
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Preconditioning of Isolated Rabbit Cardiomyocytes: Effects of Glycolytic Blockade, Phorbol Esters, and IschaemiaArmstrong, Stephen, Ganote, Charles E. 01 January 1994 (has links)
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.
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Adenosine and a<sub>1</sub> Selective Agonists Offer Minimal Protection Against Ischaemic Injury to Isolated Rat CardiomyocytesGanote, Charles E., Armstrong, Stephen, Downey, James M. 01 January 1993 (has links)
Objective: The aim was to determine if isolated rat cardiomycytes could be protected from ischaemic cell death by preincubation with adenosine or adenosine agonists. Methods: Cardiomyocytes isolated from rat hearts were preincubated in the presence of adenosine, CCPA (2-chloro-N6-cyclopentyladenosine), or carbachol prior to concentration into an ischaemic slurry. Effects of glycolysis and of isoprenaline were determined by addition of iodoacetic acid or isoprenaline to the ischaemic incubates and by exclusion of glucose from all media. Rates of ischaemic contracture were determined and survival of the myocytes versus paired control preparations was determined after various times of ischaemia, following resuspension of the cells in isotonic or hypotonic media. Results: Adenosine and CCPA produced only a small reduction of the rates of contracture and death of isolated myocytes. Carbachol gave no significant protection. Neither the degree of injury of control cells nor the amount of protection by CCPA was altered in the presence of added isoprenaline. Protection was abolished by the A1 receptor blocker sulphophenyl theophylline, iodoacetic acid, and exclusion of glucose. Conclusions: Adenosine and adenosine agonists afford a minimal degree of protection to ischaemic isolated myocytes by a glucose dependent mechanism. This protection does not appear to account for the larger degree of protection seen in intact hearts, following similar preconditioning protocols. The failure of adenosine to protect may be related to the quiescent state of isolated cardiomyocytes, or be species specific in that adenosine may not be the trigger for preconditioning in rats.Cardiovascular Research 1993;27:1670-1676.
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Potassium Channels and Preconditioning of Isolated Rabbit Cardiomyocytes: Effects of Glyburide and PinacidilArmstrong, Stephen C., Liu, Guang S., Downey, James M., Ganote, Charles E. 01 January 1995 (has links)
Calcium tolerant rabbit cardiomyocytes, isolated by collagenase perfusion, were preincubated for varying periods of time followed by resuspension in fresh media and centrifugation into an ischaemic pellet with restricted extracellular fluid. Pellets were incubated for 240 min under oil at 37°C to mimic severe ischaemia. Time to onset of ischaemic contracture (rod to square transformation) and trypan blue permeability following resuspension in 85 mOsm media were monitored at sequential times. The protocol of Series 1 was a 5-10 min pre-incubation, immediately followed by ischaemic pelleting. Preincubation with pinacidil (50 μm) protected cells from ischaemic insult, but pinacidil added only into the ischaemic pellet did not protect. Protection was abolished by the protein kinase (PKC) inhibitors chelerythrine (10 μm) added with pinacidil and calphostin C (200nm) added only into the ischaemic pellet. Neither PKC inhibitor had an effect on injury of untreated ischaemic myocytes (data not shown). Series 2-5 were preconditioning protocols with a 10 min intervention period, followed by a 30 min oxygenated drug-free period, prior to ischaemic pelleting. In series 2 pinacidil protected cells from ischaemic insult and this protection was abolished when glyburide (10 μm) was present during preincubation, or during post-incubation and ischaemia. Glyburide only partially inhibited the protection when glyburide was added only into the ischaemic pellet. In Series 3, 8-sulfophenyltheophyline (SPT)(100 μm) or adenosine deaminase during preincubation, or SPT only added into the ischaemic pellet abolished pinacidil’s protection. In Series 4, cardiomyocytes were ischaemically preconditioned by pelleting for 10 min followed by 30 min reoxygenation. Glyburide during initial ischaemic blocked protection, but when added during post incubation and into the final pellet protection was not reduced. In Series 5 8-cyclopentyl-1,3, dipropylxanthine (DPCPX) (10 μm) added into the final pellet abolished protection by pinacidil, but not protection following ischaemic preconditioning. In contrast to pinacidil, ischaemically preconditioned cells maintain protection in the presence of glyburide, indicating that: (1) pinacidil does not exactly mimic preconditioning and (2) ischaemically preconditioned cells do not require opened K+ATP channels for protection, although they appear to be important during initiation of the preconditioned state. It is hypothesized that pinacidil opening of K+ channels may facilitate induction of preconditioning.
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The phenomenon of 'second window of protection' : effect of beta-adrenergic stimulation and melatoninDavids, Ashraf 03 1900 (has links)
Thesis (MSc)--Stellenbosch University, 2004. / ENGLISH ABSTRACT:
Please see fulltext for abstract. / AFRIKAANSE OPSOMMING:
Sien asb volteks vir opsomming.
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Ischaemic preconditioning : an investigation of the patterns of kinase activation and protein expression profiles during reperfusion in the rat heartHattingh, Susanna Maria (Suzel) 12 1900 (has links)
Thesis (PhD)--Stellenbosch University, 2013. / ENGLISH ABSTRACT: Introduction: Coronary heart disease (CHD) is the leading cause of death
worldwide with 3.8 million men and 3.4 million women dying globally each year.
Although existing myocardial reperfusion strategies such as thrombolysis and
percutaneous coronary intervention (PCI), if applied in a timely manner, limit
myocardial infarct size, the mortality and morbidity remains significantly high.
Ischaemic preconditioning (IPC) may offer the potential to attenuate myocardial
ischaemia/reperfusion injury through cardioprotective signaling pathways which is
recruited at the time of myocardial reperfusion, thereby improving clinical
outcomes in patients with coronary artery disease.
Ischaemic preconditioning is a phenomenon whereby short intermittent episodes
of coronary occlusion followed by reperfusion protect the myocardium against a
subsequent period of sustained ischaemia. This protection is reflected in the
limitation of infarct size and improved functional recovery of the ischaemic heart
during reperfusion. Despite intensive research efforts, the promise of an effective
cardioprotective strategy using the endogenous protective mechanisms of the
heart which underlies IPC, has not yet been materialized. Although progress has
been made in terms of signaling mechanisms in the preconditioned heart, the
identification of the myocardial reperfusion phase as the critical “window” for
cardioprotection, requires the elucidation of the signal transduction pathways
during the reperfusion phase after IPC.
In view of the above, the aims of the present study were to investigate:
i. the involvement of the RISK pathway and p38 MAP kinase pathway in IPC
during early and late reperfusion
ii. the involvement of heat shock protein-27 (HSP-27), heat shock protein-70
(HSP-70), GSK-3β, CAMKII, AMPK and the transcription factor CREB in
the context of IPC during early reperfusion
iii. the involvement of autophagy and apoptosis during early and late
reperfusion after IPC iv. the correlation of the protein kinases with the hemodynamic parameters of
the heart
v. the mechanism of IPC by means of two-dimensional (2D) proteomics
Methods: The isolated perfused working rat heart model was used with
functional recovery as end-point. Hearts were preconditioned (IPC) for 3x5 min
global ischaemia, alternated with 5 min reperfusion. Hearts were subjected to 25
min sustained global ischaemia, followed by 5, 10, 15 or 30 min reperfusion when
hearts were snap-frozen for western blotting analysis. Alternatively, hearts were
reperfused for 30 min to record hemodynamic parameters and measure
functional recovery. Non-preconditioned (Non-IPC) hearts were stabilized for 30
min and subjected to 25 min sustained global ischaemia followed by 5, 10, 15 or
30 min reperfusion when hearts were snap-frozen. Alternatively Non-IPC hearts
were reperfused for 30 min to serve as control for the 30 min reperfused IPC
group. Activation of the protein kinases was determined by western blotting
analysis.
For the proteomic study mitochondrial and cytosolic proteins were isolated from
heart tissue and separated in the first dimension by isoelectric focusing, followed
by separation in the second dimension by two dimensional gel electrophoresis.
The PD Quest software programme was used to identify significantly expressed
protein spots. Protein spots of interest were excised and subjected to in-gel
digestion and the resulting peptides were analysed by mass spectrometry.
Proteins were identified by Mascot and the Swiss Prot database.
Results: Western blotting analysis demonstrated that the RISK pathway and p38
MAPK are activated very early in reperfusion, but the activation is not sustained
during the reperfusion period. Autophagy is also upregulated during this early
reperfusion phase; it is attenuated in the middle reperfusion phase and increase
for a second peak of upregulation in the late reperfusion phase. In addition, we
identified CAMKII as a novel marker of functional recovery in IPC after
reperfusion. The proteomic analysis identified twenty differentially expressed mitochondrial
and thirty six differentially expressed cytosolic proteins between Non-IPC and IPC hearts. Functions ascribed to the majority of these individual proteins were
directly related to cardiac metabolism.
Conclusion: Activation of the majority of the protein kinases investigated in the
present study is associated with the hemodynamic parameters of the heart
instead of functional recovery. Results indicated that the variable signaling
patterns could be attributed to differences in heart rate and the effect thereof
(ejection fraction, minimum and maximum rate of contraction), as a result of
sympathetic stimulation due to psychological stress in the animals before
slaughtering. Proteomics results demonstrated that IPC hearts which failed after
ischaemia /reperfusion are metabolically compromised and “worse off” compared
to non-IPC hearts. / AFRIKAANSE OPSOMMING: Inleiding: Koronêre hartsiekte is die vernaamste oorsaak van sterftes wêreldwyd
met 3.8 miljoen mans en 3.4 miljoen vrouens wat jaarliks sterf. Alhoewel
bestaande miokardiale herperfusie strategieë soos trombolise en perkutane
koronêre intervensie (PKI), wanneer betyds toegepas, miokardiale infarktgrootte
beperk, bly mortaliteit en morbiditeit steeds hoog. Isgemiese prekondisionering
(IPK) beskik oor die potensiaal om miokariale isgemie/herperfusie skade te
verminder deur beskermende seinoordragpaaie tydens miokardiale herperfusie te
aktiveer en sodoende die pasiënte wat aan koronêre arterie siekte ly, se
prognose te verbeter.
Isgemiese prekondisionering verwys na die verskynsel waartydens kort episodes
van isgemie opgevolg deur herperfusie, die miokardium teen ‘n daaropvolgende
langdurige isgemiese insident beskerm. Hierdie beskerming word gereflekteer in
die beperking van infarktgrootte en verbeterde funksionele herstel van die
isgemiese hart tydens herperfusie. Ten spyte van intensiewe navorsingspogings
is die presiese meganisme van endogene beskerming tydens IPK nog nie ten
volle ontrafel nie. Die identifisering van die miokardiale herperfusie fase se
kritiese “vensterperiode” van beskerming, noodsaak ‘n volledige analise van die
seinoordragpaaie wat geaktiveer word tydens die herperfusie fase na IPK.
In die lig van bogenoemde, was die doel van die huidige studie om die volgende
te ondersoek:
i. die betrokkenheid van die RISK seinoordragpad en p38 MAP kinase
tydens vroeë en laat herperfusie na IPK
ii. die betrokkenheid van “heat shock protein-27” (HSP-27), “heat shock
protein- 70” (HSP-70), GSK -3β, CAMKII, AMPK en die transkripsie faktor,
CREB, in die konteks van IPK tydens vroeë herperfusie
iii. die betrokkenheid van outofagie en apoptose tydens vroeë en laat
herperfusie na IPK
iv. die korrelasie van die proteïenkinases met die hemodinamiese parameters
van die hart v. die meganisme van IPK deur middel van twee dimensionele proteomika
Metodes: Die geïsoleerde werkende rothart model, met funksionele herstel as
eindpunt, is gebruik. Harte is geprekondisioneer (IPK) met 3x5 min globale
isgemie, afgewissel met 5 min herperfusie. Daarna is harte blootgestel aan 25
min volgehoue globale isgemie, gevolg deur 5, 10, 15 of 30 min herperfusie,
waartydens harte gevriesklamp is. Alternatiewelik, is harte blootgestel aan 30 min
herperfusie ten einde funksionele herstel te meet en hemodinamiese parameters
te registreer. Nie-geprekondisioneerde (Non-IPK) harte is gestabiliseer vir 30
min, waarna dit onderwerp is aan 25 min volgehoue globale isgemie, gevolg deur
5, 10, 15 of 30 min herperfusie, waartydens harte gevriesklamp is vir westelike
klad analise. Alternatiewelik, is Non-IPK harte onderwerp aan 30 min herperfusie
om te dien as kontrole vir die 30 min IPK groep. Aktivering van die
proteïenkinases is bepaal deur westelike klad analise.
Vir die proteomiese studie, is onderskeidelik mitokondriale en sitosoliese
proteïene geïsoleer en geskei in die eerste dimensie met behulp van isoelektriese
fokusering, gevolg deur skeiding in die tweede dimensie met behulp
van twee dimensionele gel elektroforese. Die PDQuest sagteware program is
gebruik om proteïenkolle te identifiseer wat statisties beduidende verskille toon.
Proteïenkolle van belang is uitgesny en onderwerp aan in-gel tripsinering en die
peptiede wat sodoende verkry is, is deur middel van massa spektrometrie
geanaliseer. Proteïene is geïdentifiseer deur Mascot en die Swiss Prot databasis. Resultate: Westelike klad analise het aangetoon dat die RISK pad en p38 MAPK
geaktiveer is tydens vroeë herperfusie, maar die aktivering word nie volgehou
tydens die hele herperfusie periode nie. Outofagie word gestimuleer tydens die
vroeë herperfusie fase; dit word onderdruk in die middel herperfusie fase en
bereik ‘n tweede piek van stimulering in die laat herperfusie fase. Die
proteomiese analise het onderskeidelik twintig differensieel gereguleerde
mitokondriale proteïene en ses en dertig differensieel gereguleerde sitosoliese
proteïene geïdentifiseer tussen Non-IPK en IPK. Die grootste persentasie van
hierdie proteïene is direk betrokke by miokardiale energie metabolisme. CAMKII
is geidentifiseer as ‘n unieke merker van funksionele herstel in IPK tydens
reperfusie. Gevolgtrekking: Aktivering van die meeste van die proteïenkinases wat
ondersoek is in die huidige studie, is geassosieer met die hemodinamiese
parameters van die hart, in plaas van funksionele herstel. Die resultate het
aangetoon dat die varierende patrone van kinase aktivering toegeskryf kan word
word aan verskille in harttempo en die effek daarvan (ejeksie fraksie, minimum
en maksimum tempo van kontraksie), as gevolg van simpatiese stimulasie
toegeskryf aan sielkundige stres in die diere voor slagting. Proteomiese analise
het getoon dat IPK harte wat faal na isgemie/reperfusie metabolies
gekompromiseer is en “slegter daaraan toe” is, in vergelyking met Non-IPK harte.
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