Global ETD Search

131	Adenosine and a<sub>1</sub> Selective Agonists Offer Minimal Protection Against Ischaemic Injury to Isolated Rat Cardiomyocytes Ganote, 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. adenosine agonists adenosine antagonists adenosine receptors glycolysis heart ischaemic injury ischaemic preconditioning reperfusion
132	Protein Phosphatase Inhibitors Calyculin a and Fostriecin Protect Rabbit Cardiomyocytes in Late Ischemia Armstrong, Stephen C., Gao, W., Lane, J. R., Ganote, C. E. 01 January 1998 (has links) Calcium-tolerant rabbit cardiomyocytes were isolated using retrograde aortic perfusion with a nominally calcium-free, collagenase buffer. In vitro ischemic preconditioning was induced by a 10-min episode of ischemic pelleting, followed by a 15-min post-incubation and a prolonged period of ischemic pelleting. Injury was assessed by determination of cell contracture and trypan blue permeability following hypotonic swelling and correlated with metabolic assays of lactate and adenine nucleotides. The protein phosphatase PP1/2A inhibitor calyculin A and PP2A-selective fostriecin protected isolated rabbit cardiomyocytes from lethal injury after a 10-min pre-incubation and when added late into ischemic pellets after a delay of 75 min. At the time of late drug addition, cells were severely ATP-depleted and in rigor contracture. Protection with Calyculin A from 1 nM to 1 μM was dose-related. Cells pre-incubated with 10 nM to 10 μM fostriecin 10 min prior to ischemic pelleting were protected with an EC50 approximating 71 nM, implying protection at a PP2A-selective dose. The selective protein kinase C inhibitor, calphostin C, blocked ischemic preconditioning protection but not protection from 1 μM calyculin A. Protection of severely ischemic cardiomyocytes following protein phosphatase inhibition appears not to require PKC activity or ATP conservation. Pre-incubation of cells with calyculin A induced high levels of phosphorylation in p38 mitogen activated protein kinase (MAPK), as compared to the ischemia-induced phosphorylation observed in the untreated group only at 30 min of ischemia, providing evidence of protein phosphatase activity in cardiomyocytes. Pharmacological protection in late ischemia has been demonstrated, but the mechanism of protection is undetermined. fostriecin ischemic injury isolated cardiomyocyte myocardial infarction preconditioning protein phosphatase 2A
133	Preconditioning of Isolated Rabbit Cardiomyocytes: No Evident Separation of Induction, Memory and Protection Armstrong, Stephen C., Hoover, D. B., Shivell, L. C., Ganote, C. E. 01 January 1997 (has links) Cardiomyocytes isolated from rabbit hearts were preconditioned in vitro by 10 min of ischemia or treatment with 100 μM adenosine. Protection was assessed as average integrated mortality following osmotic swelling and determination of viability by trypan blue exclusion over 60-180 min ischemia. Repetitive submaximal stimulations with 1 μM adenosine amplified the protective response. Treatment with adenosine only at the onset of prolonged ischemia afforded a dose-dependent protection. The PKC inhibitor calphostin C (500 nM) blocked preconditioning and, when added during ischemic incubation of non-preconditioned cells, significantly increased injury. The memory of adenosine-induced preconditioning decayed over a 60 min post-incubation period. Light activation of calphostin C initially added to preconditioned ischemic cells in the dark indicated that a 10 min period of PKC activity at the onset of ischemia affords full protection. The reversible PKC inhibitors chelerythrine (5 μM) or staurosporine (100 nM) added only to bracket induction of ischemia, reduced but did not abolish protection. Protection was abolished when either drug was present during induction and a subsequent 30 min post-incubation period. Staurosporine included during initiation and post-incubation but washed out in the final 5 min of post-incubation allowed significant protection to occur. It is concluded that a single adenosine receptor-stimulation induces protection as it preconditions, and PKC activity appears to be required for both induction and protection. Memory may reside in post-receptor amplification of an initial protective response. adenosine protection ischemic injury isolated cardiomyocyte preconditioning protein kinase c Biomedical Sciences
134	Translocation of PKC, Protein Phosphatase Inhibition and Preconditioning of Rabbit Cardiomyocytes Armstrong, Stephen C., Hoover, Donald B., Delacey, Martha H., Ganote, Charles E. 01 January 1996 (has links) This study was designed to test the hypothesis that induction of the preconditioned state results in a sustained translocation of protein kinase C (PKC) which accounts for the memory associated with preconditioning. Isolated rabbit cardiomyocytes were subjected to established preconditioning protocols using either adenosine or transient ischemia. At timed intervals during induction of preconditioning (PC), post-incubation or final sustained ischemia, cells were harvested, subjected to digitonin lysis and separated into cytosolic and particulate fractions. Samples were evaluated by Western blot analysis with monoclonal antibodies to alpha, epsilon, zeta and gamma PKC isozymes, and bands were quantified by densitometry. Internal controls for each experiment included oxygenated cardiomyocytes and cells with PKC translocation evoked by treatment with phorbol 12-myristate 13-acetate (PMA). For control oxygenated cells, the particulate fraction contained about 30% of PKC epsilon, 5-10% of PKC alpha and 60-70% of PKC zeta. Preconditioning with adenosine (100 μM) or 10 min ischemia had no significant effect on these percentages. Furthermore, the relative amounts of the PKC isozymes associated with the particulate fraction of control and preconditioned cells did not differ after a post-incubation in oxygenated buffer or during a final ischemic incubation. PMA and ingenol completely translocated the epsilon and alpha isoforms, while thymeleatoxin totally translocated PKC alpha but only partially (50%) translocated PKC epsilon. The distribution of PKC zeta between fractions was not affected by any drug, The protein phosphatase inhibitor calyculin A protected cells mimicking preconditioning. This protection was blocked by preincubation with the selective PKC inhibitor calphostin C but was largely retained if calphostin C was added only during the final ischemic period. It is concluded that PKC activity is required for preconditioning, but a sustained translocation of PKC above basal levels is not necessary for protection of rabbit cardiomyocytes in vitro. ischemic preconditioning isolated cardiomyocytes protein kinase C protein phosphatases Biomedical Sciences
135	Potassium Channels and Preconditioning of Isolated Rabbit Cardiomyocytes: Effects of Glyburide and Pinacidil Armstrong, 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. adenosine adenosine receptors glibenclamide ischaemic injury ischaemic preconditioning isolated cardiomyocyte pinacidil potassium channels protein kinase C
136	Pre-Wounding and Free Gingival Grafts: A Pilot Investigation Delima, Suzanne Lynn 29 August 2013 (has links) No description available. Dentistry Prewounding ischemic preconditioning periodontal plastic soft tissue grafts free gingival grafts
137	A Global Preconditioning Method for the Euler Equations Yildirim, B. Gazi 02 August 2003 (has links) This study seeks to validate a recently introduced global preconditioning technique for the Euler equations. Energy and enthalpy equations are nondimensionalized by means of a reference enthalpy, resulting in increased numerical accuracy for low-speed flows. A cellbased, finite volume formulation is used, with Roe flux difference splitting and both explicit and implicit time integration schemes. A Newton-linearized iterative implicit algorithm is implemented, with Symmetric Gauss-Seidel (LU/SGS) nested sub-iterations. This choice allows one to retain time accuracy, and eliminates approximate factorization errors, which become dominant at low speed flows. The linearized flux Jacobians are evaluated by numerical differentiation. Higher-order discretization is constructed by means of the MUSCL approach. Locally one-dimensional characteristic variable boundary conditions are implemented at the farfield boundary. The preconditioned scheme is successfully applied to the following traditional test cases used as benchmarks for local preconditioning techniques: point disturbance, flow angle disturbance, and stagnation point arising from the impingement of two identical jets. The flow over a symmetric airfoil and a convergentdivergent nozzle are then simulated for arbitrary Mach numbers. The preconditioned scheme greatly enhances accuracy and convergence rate for low-speed flows (all the way down to M ≈ 10E − 4). Some preliminary tests of fully unsteady flows are also conducted. Newton formulation flux difference splitting euler equations preconditioning
138	Isoform Specific Effect of Ischemia/Reperfusion on Cardiac Na,K-ATPase: Protection by Ouabain Preconditioning Stebal, Cory J. 14 July 2009 (has links) No description available. Molecular Biology Pharmacology Physiological Psychology Na+,K+-ATPase preconditioning Ouabain ischemia reperfusion Langendorff-perfusion
139	Parallel ILU Preconditioning for Structured Grid Matrices Eisenlohr, John Merrick 20 May 2015 (has links) No description available. Computer Science high-performance computing numerical linear algebra preconditioning parallel programming SIMD vectorization
140	The Effect of an Acute Bout of Exercise on Endothelial Function following Ischemic-Reperfusion Injury Lawrence, Jennifer L. January 2011 (has links) No description available. Health Sciences Exercise Endothelial Function Ischemic-Reperfusion Injury Exercise Preconditioning Flow-Mediated Dilation

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