Abstract

Memory is the result of molecular, cellular, and brain system interactions. To better treat and diagnose mental health disorders that affect memory and cognition, we must understand the complex interactions that occur at these different levels in the brain. The long-term objective of this research program is to increase understanding on the role of experience-dependent neuronal gene expression in the formation of long-term memory (LTM). Within this broad framework, the experiments of this proposal will help determine: (1) how sensory information affects immediate-early gene (IEG) transcription in the hippocampal formation (HF) and (2) how task demands influence IEG transcription in defined neuronal populations in the HF. While the central focus of this research is at the level of systems neurobiology and behavior, the findings from the proposed studies will provide important primary information for future focused studies on the molecular mechanisms that control IEG expression under different physiologic conditions. We will use a modified fluorescent in situ hybridization (FISH) protocol that we developed recently to visualize multiple different IEG RNAs in brain tissue. This FISH assay is extremely sensitive and is capable of detecting the putative sites of active IEG transcription (transcription foci, or TF) in brain neurons. We have performed a series of experiments in rats to show that TF for a number of IEGs can be visualized within 2 minutes of either an electrical stimulus or by exploration of a new environment. Moreover, this induced transcription is transient with IEG TF at baseline levels by 30 minutes after behavioral and electrical stimulus, and the nascent mRNA found distributed in the cytoplasm at this time point. Because the time course of nuclear versus cytoplasmic RNA accumulation is distinct, the subcellular distribution of RNA, determined by confocal microscopy, can be used to infer the activity history of individual neurons at two different times. We have termed this approach to functional brain imaging cellular compartment analysis of temporal activity by FISH, or catFISH. We have begun to use IEG catFISH to examine the role that discrete sensory information has on patterns of IEG transcriptional activation in the HF. In many of these studies, we exploit the temporal resolution properties of catFISH to see how discrete behavioral experiences, separated in time by 20 minutes, influence transcriptional patterns in different neuronal populations. Our early data show that two populations of CA1 neurons induce transcription of the IEG Arc following exploration of two environments, whereas exploration of the same environment twice only activates transcription of Arc RNA in one population of neurons. This provides compelling evidence that IEG transcription in CA1 neurons is linked to information processing, and is not driven by generalized or nonspecific influences. Data from the proposed studies will provide new insights into the role of experience-dependent IEG expression during memory formation, and in the neuronal population interactions that occur within the HF as an animal processes different types of information.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Mental Health (NIMH)
Type
Research Project (R01)
Project #
1R01MH060123-01A1
Application #
6128360
Study Section
Special Emphasis Panel (ZRG1-IFCN-7 (01))
Program Officer
Edwards, Emmeline
Project Start
2000-04-15
Project End
2003-03-31
Budget Start
2000-04-15
Budget End
2001-03-31
Support Year
1
Fiscal Year
2000
Total Cost
$319,091
Indirect Cost

  Institution

Name
University of Arizona
Department
Type
Organized Research Units
DUNS #
City
Tucson
State
AZ
Country
United States
Zip Code
85721

  Publications

Chawla, M K; Sutherland, V L; Olson, K et al. (2018) Behavior-driven arc expression is reduced in all ventral hippocampal subfields compared to CA1, CA3, and dentate gyrus in rat dorsal hippocampus. Hippocampus 28:178-185
Kubik, Stepan; Miyashita, Teiko; Kubik-Zahorodna, Agnieszka et al. (2012) Loss of activity-dependent Arc gene expression in the retrosplenial cortex after hippocampal inactivation: interaction in a higher-order memory circuit. Neurobiol Learn Mem 97:124-31
Miyashita, Teiko; Kubik, Stepan; Haghighi, Nahideh et al. (2009) Rapid activation of plasticity-associated gene transcription in hippocampal neurons provides a mechanism for encoding of one-trial experience. J Neurosci 29:898-906
Bramham, Clive R; Worley, Paul F; Moore, Melissa J et al. (2008) The immediate early gene arc/arg3.1: regulation, mechanisms, and function. J Neurosci 28:11760-7
Miyashita, Teiko; Kubik, Stepan; Lewandowski, Gail et al. (2008) Networks of neurons, networks of genes: an integrated view of memory consolidation. Neurobiol Learn Mem 89:269-84
Kubik, Stepan; Miyashita, Teiko; Guzowski, John F (2007) Using immediate-early genes to map hippocampal subregional functions. Learn Mem 14:758-70
Steward, Oswald; Huang, Fen; Guzowski, John F (2007) A form of perforant path LTP can occur without ERK1/2 phosphorylation or immediate early gene induction. Learn Mem 14:433-45
Fletcher, Bonnie R; Baxter, Mark G; Guzowski, John F et al. (2007) Selective cholinergic depletion of the hippocampus spares both behaviorally induced Arc transcription and spatial learning and memory. Hippocampus 17:227-34
Tafoya, Lawrence C R; Mameli, Manuel; Miyashita, Teiko et al. (2006) Expression and function of SNAP-25 as a universal SNARE component in GABAergic neurons. J Neurosci 26:7826-38
Vazdarjanova, Almira; Ramirez-Amaya, Victor; Insel, Nathan et al. (2006) Spatial exploration induces ARC, a plasticity-related immediate-early gene, only in calcium/calmodulin-dependent protein kinase II-positive principal excitatory and inhibitory neurons of the rat forebrain. J Comp Neurol 498:317-29

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