Error bars represent the SEM. Statistical analyses usually consisted of one- or two-way anova and Bonferroni’s post hoc tests. Statistical significance was set at 0.05. In two-way anova, the two this website variables typically were ‘drugs’ (drug combinations or concentrations) and ‘stimulus’ (by comparing the side of the slice ipsilateral or contralateral to the stimulus). The Bonferroni’s post hoc test was applied to the variable ‘drugs’ to compare effects on the ipsilateral side. NK1R internalization in the contralateral side was consistently low and unaffected by the drugs used in this study. Concentration–response data were fitted using nonlinear

regression by a sigmoidal dose–response function: where the IC50 is the concentration of drug that produces half of the inhibition. Baseline measures (zero concentration of drug) were included in the nonlinear regression by assigning them a concentration value three log units lower than the estimated IC50. Parameter constraints were: 0% < top < 100%, 0% < bottom. Statistical errors of the EC50 or IC50 were expressed as 95% confidence intervals (CI). Prism was set to detect and exclude outliers by using the ‘robust regression and outlier removal’ (ROUT) algorithm with

Q = 1% (Motulsky buy Inhibitor Library & Brown, 2006). An F-test (Motulsky & Christopoulos, 2003) was used to compare alternative nonlinear regression fittings with different number of parameters, i.e., when one parameter was constrained to a fixed value. First, we studied the effect of CB1 receptors on substance P release in rat spinal cord slices. Using an approach developed in our laboratory (Marvizon et al., 1997; Adelson et al., 2009), we prepared spinal cord slices with one contiguous Rucaparib dorsal root that was electrically stimulated

to induce substance P release, which was measured as NK1R internalization. As we previously reported, neurons showing NK1R internalization were virtually absent in the contralateral dorsal horn (Fig. 1A) but numerous in the ipsilateral dorsal horn, particularly in its central part (Fig. 1B). Two electrical stimulation protocols were used, low (1 Hz) and high (100 Hz) frequency, because we previously found that the stimulation frequency influences substance P release and its modulation by GABA and other neurotransmitters (Marvizon et al., 1999; Lao & Marvizon, 2005; Adelson et al., 2009). The electrical pulses used were of sufficient amplitude (20 V) and duration (0.4 ms) to recruit C-fibers (Adelson et al., 2009). Dorsal root stimulation at 1 Hz induced NK1R internalization in nearly half of the NK1R neurons in lamina I (Fig. 2A). The number of NK1R neurons with internalization was increased by the selective CB1 receptor agonist ACEA (100 nm) and decreased by the selective CB1 antagonist AM251 (100 nm; Fig. 2A). Combining ACEA with AM251 cancelled their effects and brought NK1R internalization back to control levels.