Project Summary During pregnancy, alcohol abuse produces persistent changes in the fetal brain, causing behavioral impairments throughout life. These conditions are defined as fetal alcohol spectrum disorder (FASD). Most concerningly, regular binge drinking during pregnancy causes cognitive and socio-behavioral deficits in offspring. However, the molecular mechanisms underlying persistent alcohol-induced neurobehavioral impairments are not fully understood. Our previous studies demonstrated that alcohol exposure results in CB1 signaling defects in neonatal mice (P7) that cause neurodegeneration and behavioral deficits in adults. Other data also implicate CB1 in the teratogenic effects of alcohol. However, whether synaptic and behavioral deficits are due to alcohol-induced changes in CB1 and its signaling events within the adult hippocampus (HP) and prefrontal cortical (PFC) regions remains largely unknown. CB1s are mainly expressed in glutamatergic and GABAergic neurons. They can elicit cell-type-specific signaling depending on where they are activated and contribute to neuronal and behavior outcomes. CB1 activity also regulates gene expression via epigenetics; however, the mechanisms are unknown. Our recent pilot findings suggested that human third-trimester-equivalent alcohol exposure in neonatal mice caused persistent cognitive and social behavior deficits. These behavioral changes were accompanied by increased CB1 expression, histone methylation, and reduced expression of genes essential for synaptic structure and function in specific neuronal types. These findings suggest that alcohol alters the transcriptional control of gene expression and synaptic function in a given cell type in the PFC and HP. This proposal will test the hypothesis that a mechanism underlying synaptic dysfunction in the PFC and HP contributing to behavioral deficits is enhanced CB1 activity and histone methylation by postnatal alcohol leading to aberrant synaptic gene expression. This proposal will test these hypotheses in PFC and HP using cell-type-specific (Cre or CreERT2) RiboTag (TRAP) technology to study CB1 and histone methylation events altered by postnatal alcohol exposure (PAE). We will pay special attention to evidence of aberrant regulation of histone methylation responsive genes related to spine and synaptic vesicle function. Additionally, we will investigate the role of histone methylation on synaptic structure and function by conditional deletion (cKO) of the CB1 gene or a gene encoding a histone-methylation-related enzyme (FloxP lines) in the specific neuronal type (CreERT2) in the adult PFC and HP. Finally, we will mechanistically test the effects of modulating histone methylation levels using cKO of CB1 or histone methylation enzyme function in specific neuronal types to rescue adult cognitive and social behaviors. These studies will use sex-dependent models to perform a combined epigenetic, synaptic, and behavioral analysis of the response to PAE. Our...