Long-term memories are believed to be due to persistent changes in synaptic strength. Although the molecular mechanisms initiating these changes have been extensively studied, the mechanisms maintaining these changes, which may contribute to storing long-term memory, have been unknown. Recently, however, a candidate molecular mechanism has emerged for maintaining a persistent form of synaptic enhancement triggered by strong afferent stimulation of synapses, known as long-term potentiation (LTP). The key molecule in this maintenance mechanism is a brain-specific, protein kinase C isoform, PKM6. Unlike other PKC isoforms that require second messengers for activation, PKM6 consists of an independent PKC catalytic domain that is constitutively active. PKM6 is produced from a PKM6 mRNA, and the amount of the kinase increases with LTP induction. The persistent activity of the kinase is then both necessary and sufficient for maintaining the synaptic enhancement. Postsynaptic perfusion of PKM6 enhances synaptic transmission, and inhibition of PKM6 activity reverses previously established LTP. Recently, PKM6 inhibition has been found to disrupt the storage of previously established long-term memories. These data indicate that PKM6 is a candidate molecule uniquely important for information storage at synapses and during behavior. Thus the overall goal of this application is to elucidate in mechanistic detail the function of PKM6 in persistent synaptic enhancement and memory storage. Our 3 Specific Aims are: 1) To characterize the mechanisms by which PKM6 enhances synaptic strength. We found that PKM6 potentiates synaptic strength by increasing the number of postsynaptic AMPA receptors (AMPARs) through interactions between the AMPAR GluR2 subunit and the trafficking protein NSF. We will examine whether this potentiation is through increased exocytosis and/or decreased endocytosis of postsynaptic AMPARs and the function of this altered trafficking in memory maintained by PKM6. 2) To determine whether preexisting and newly translated PKM6 mediate distinct phases of potentiation during LTP. Preliminary evidence indicates that antisense oligodeoxynucleotides blocking new PKM6 synthesis prevents the persistence of a phase of LTP. We will determine whether this new synthesis occurs at dendritic sites. 3) To determine the role of preexisting, newly translated, and new gene transcription of PKM6 in distinct phase of memory. PKM6 maintains memory up to several months after training. We will employ both antisense to block translation of PKM6 mRNA and conditional genetic deletion of PKM6 to examine the function of distinct mechanisms of expression of PKM6 in different phases of memory. These 3 aims will provide fundamental new information on a potential molecular mechanism for maintaining synaptic and behavioral information storage, which may be relevant to both normal memory and its disorders.
How long-term memories are stored in the brain is a fundamental neurobiological question, with many implications for neurology and psychiatry, but the molecular mechanisms of memory maintenance have been unknown. Recently, however, the persistent action of a protein kinase, termed PKMzeta, has been found to be one potential mechanism for maintaining memory. This application is to characterize the functional mechanisms by which PKMzeta maintains long-term information at synapses and during behavioral memory storage.
|Jalil, Sajiya J; Sacktor, Todd Charlton; Shouval, Harel Z (2015) Atypical PKCs in memory maintenance: the roles of feedback and redundancy. Learn Mem 22:344-53|
|Dong, Zhifang; Han, Huili; Li, Hongjie et al. (2015) Long-term potentiation decay and memory loss are mediated by AMPAR endocytosis. J Clin Invest 125:234-47|
|Hernandez, A Ivan; Oxberry, William C; Crary, John F et al. (2014) Cellular and subcellular localization of PKMÃ½Ã½. Philos Trans R Soc Lond B Biol Sci 369:20130140|
|Eom, Taesun; Muslimov, Ilham A; Tsokas, Panayiotis et al. (2014) Neuronal BC RNAs cooperate with eIF4B to mediate activity-dependent translational control. J Cell Biol 207:237-52|
|Yao, Yudong; Shao, Charles; Jothianandan, Desingarao et al. (2013) Matching biochemical and functional efficacies confirm ZIP as a potent competitive inhibitor of PKMÎ¶ in neurons. Neuropharmacology 64:37-44|
|VÃ©lez-HernÃ¡ndez, MarÃa E; VÃ¡zquez-Torres, Rafael; Velasquez-Martinez, Maria C et al. (2013) Inhibition of Protein kinase Mzeta (PKMÎ¶) in the mesolimbic system alters cocaine sensitization in rats. J Drug Alcohol Res 2:235669|
|Sacktor, Todd Charlton (2012) Memory maintenance by PKMÃ½Ã½--an evolutionary perspective. Mol Brain 5:31|
|Shao, Charles Y; Sondhi, Rachna; van de Nes, Paula S et al. (2012) PKMÎ¶ is necessary and sufficient for synaptic clustering of PSD-95. Hippocampus 22:1501-7|
|Wang, Jun; Meng, Fanli; Cottrell, James E et al. (2012) Metabotropic actions of the volatile anaesthetic sevoflurane increase protein kinase M synthesis and induce immediate preconditioning protection of rat hippocampal slices. J Physiol 590:4093-107|
|Barry, Jeremy M; Rivard, Bruno; Fox, Steven E et al. (2012) Inhibition of protein kinase MÃ½Ã½ disrupts the stable spatial discharge of hippocampal place cells in a familiar environment. J Neurosci 32:13753-62|
Showing the most recent 10 out of 21 publications