Top Notch Items Intended for IOX1
Data were visualized on a Power Macintosh G3 personal computer (Apple Macintosh, Cork, Ireland). All data are expressed as means ��s.e.m. Single repeated measures ANOVA or two-factor ANOVA was used with Bonferroni post hoc test for multiple group comparisons where appropriate. P IOX1 left ventricular pressure (LVP) and Ca2+ transients were monitored during autonomic nerve stimulation in two sets of conditions, as follows: (1) when the heart rate of the intrinsic sinus rhythm of the heart was varying as a result of nerve stimulation; and (2) when hearts were paced at a constant rate via the right ventricle. Autonomic nerve stimulation was allowed to continue until heart rate, LVP and calcium fluorescence diglyceride reached steady state. A minimum period of 3 min between stimulation frequencies was maintained throughout the experiment. We allowed hearts to remain in either sinus rhythm whilst monitoring changes in heart rate, or in constant pacing at 240 beats min�C1 when we investigated nerve stimulation whilst maintaining heart rate. During right ventricular pacing, SS and VS were tested separately and in combination. Right atrial electrograms were recorded during ventricular pacing to ascertain the presence of underlying effects of nerve stimulation. Baseline and peak heart rate achieved during autonomic nerve stimulation before and after perfusion with 5 ��m decamethonium bromide are shown in Table 1. Whilst there was a trend for a decrease in heart rate values during decamethonium bromide perfusion, the chronotropic effect of sympathetic and vagus nerve stimulation was unaffected, suggesting that decamethonium bromide does not interfere with the cardiac effects of the autonomic nerves. Data representing the change in fluorescence during the loading protocol are shown in Fig. 1. Before loading, there was no beat-to-beat variation in F340, F380 or the calcium Selleckchem I-BET-762 transient, whilst reducing the temperature of the perfusing solution prior to loading did not alter fluorescence. Within 2 min of loading, measurable increases in F340 and F380 were seen, with a greater increase in F380 compared with F340 (Fig. 1) being detected throughout the loading period. During this time, the fluorescence ratio decreased. Phasic changes correlating to the cardiac cycle appeared in all fluorescence signals within 5 min of loading but were not recognizable as calcium-dependent changes until after 10 min loading as the signal to noise ratio improved. On return to normal Tyrode solution, fluorescence values at each wavelength were higher than those obtained at baseline.