sed expression of Beclin-1 and class III PI3K or the increased Bcl-2 expression by propofol in the OGDinjured PC12 eventually inhibits autophagy. Increased Expression of Autophagy-related Proteins in PC12 Cells Following OGD Propofol Prevents Autophagic Cell Death The Injury of Hippocampal Pyramidal Neurons Following I/R Studies have reported an early decline in the number of (-)-Blebbistatin site hippocampus CA1 pyramidal neurons following severe ischemic insults. To specifically investigate the temporal effects of I/ R on hippocampal pyramidal neuron function, we measured the number of pyramidal neurons in the CA1 region of the hippocampus following severe ischemic insults at ” various time points using histochemical techniques. The results revealed that, as compared with the control group, there was no robust change in the number of hippocampal pyramidal neurons at 1 h after ischemia. This result was consistent with the observation the lack of LC3 expression in the CA1 hippocampus at that time point. However, the 
number of hippocampal pyramidal neurons was reduced in the ischemic CA1 hippocampus at 3 h and was further decreased at 624 h after ischemia. Moreover, the damaged pyramidal neurons in the ischemic CA1 hippocampus exhibited various stages of fragmentation, which is characteristic of dying cells, indicating that the hippocampal pyramidal neurons were damaged and died in a time-dependent manner following I/R. We also measured the expression of LC3 II by immunohistochemistry at various time points following the ischemic insult. LC3 II is a marker for autophagic vacuoles. When the hippocampal pyramidal neurons were examined by fluorescence microscopy after I/R treatment, the immunohistochemistrylabeled AVs appeared as distinct puncta distributed throughout the cytoplasm, the perinuclear regions ” and the processes. As compared with the control group, there was a significant increase in the number of LC3 II-labeled vesicles at 1 h, which peaked at 36 h after I/R treatment, suggesting an induction of AV formation in hippocampal pyramidal neurons after I/R. Activation of Autophagy”2533479
” in Rat Hippocampal Pyramidal Neurons after I/R The ultrastructural changes in rat hippocampal pyramidal neurons were observed by transmission electron microscopy at 1 Propofol Prevents Autophagic Cell Death 4 Propofol Prevents Autophagic Cell Death 24 h after I/R. The smooth cytoplasmic, normal appearance of the mitochondria, nuclei and chromatin were observed in the control hippocampal pyramidal neurons. After the I/R insult, the pyramidal neurons exhibited typical signs of autophagic/lysosomal activation and apoptosis, as shown in . The most abundant autophagosomes were observed at 3 h after I/R. Occasionally, autophagosomes with engulfed organelles were observed. The fusion of autophagosomes with lysosomes was occasionally observed. The mitochondria displayed swelling, dilation and cristae disruption, and the 5 Propofol Prevents Autophagic Cell Death 6 Propofol Prevents Autophagic Cell Death PI3K, Beclin-1, Bcl-2, LC3-I and LC3-II expression. Each protein shown in Fig. 5A, B, E, F was quantified after a densitometric scan and normalized to GAPDH. The optical densities of the respective protein bands were analyzed using Sigma Scan Pro 5 and normalized to the loading control. The results are expressed as the mean 6 SD from three independent experiments. Statistical comparisons were conducted using an ANOVA followed by the Tukey test. p, 0.01 vs. control group; p, 0.05, p, 0.01 vs
