Homosynaptic plasticity

Last updated

Homosynaptic plasticity is one type of synaptic plasticity. [1] Homosynaptic plasticity is input-specific, meaning changes in synapse strength occur only at post-synaptic targets specifically stimulated by a pre-synaptic target. [2] Therefore, the spread of the signal from the pre-synaptic cell is localized.

Contents

In homosynaptic plasticity, only neurons that are specifically innervated undergo changes in synaptic plasticity Homosynaptic Plasticity-1.jpg
In homosynaptic plasticity, only neurons that are specifically innervated undergo changes in synaptic plasticity

Another type of synaptic plasticity, heterosynaptic plasticity, is not input-specific and differs from homosynaptic plasticity in many mechanisms.

In addition to being input-specific, the strengthening of a synapse via homosynaptic plasticity is associative, because it is dependent on the firing of a presynaptic and postsynaptic neuron closely in time. This associativity increases the chances that the postsynaptic neuron will also fire. [3] These mechanisms are theorized to underlie learning and short-term memory. [3]

Overview

Hebb's postulate

Donald Hebb theorized that strengthening of synaptic connections occurred because of coordinated activity between the pre-synaptic terminal and post-synaptic dendrite. According to Hebb, these two cells are strengthened because their signaling occurs together in space and/or time, also known as coincident activity. This postulate is often summarized as Cells that fire together, wire together, which means that the synapses that have neurons with coincident firing are strengthened, while the other synapses on these neurons remain unchanged. [3] Hebb's postulate has provided a conceptual framework for how synaptic plasticity underlies long-term information storage. [1]

Mechanisms for input-specificity

Changes in plasticity often occurs via the insertion or internalization of AMPA receptors (AMPARs) into the postsynaptic membrane of the synapse undergoing a change in connective strength. [1] Ca2+ is one signaling ion that causes this AMPA receptor density change by inducing a cascade of biological changes within the cell. To induce long-term potentiation (LTP), Ca2+ activates CAMKII and PKC, causing phosphorylation and insertion of AMPARs, while long-term depression (LTD) occurs by Ca2+ activating protein phosphatases, which dephosphorylate and cause internalization of AMPARs. [1]

In order to create input-specific changes in synaptic strength, the Ca2+ signal must be restricted to specific dendritic spines. Dendritic restriction of Ca2+ is mediated by several mechanisms. Extracellular Ca2+ can enter the spine through NMDA receptors (NMDARs) and voltage gated Ca2+ channels (VGCCs). Both NMDARs and VGCCs are concentrated on dendritic spines, mediating spine specific Ca2+ influx. Intracellular stores of Ca2+ in the endoplasmic reticulum and mitochondria may also contribute to spine restricted signaling, although some studies have failed to find evidence for this. [4] Clearance of Ca2+ is controlled by buffer proteins, which bind to Ca2+ and keep it from trickling out to other spines. Restricted diffusion of Ca2+ across the neck of the dendritic spine also helps isolate it to specific dendrites. [4]

Another mechanism for input-specific long-term potentiation is temporal. NMDARs require both depolarization, to remove their magnesium block, and glutamate activation, to open their channels, to allow Ca2+ influx. LTP is thus localized at sites where NMDA channels are opened by active synaptic inputs that are releasing glutamate and causing depolarization of the postsynaptic cell, and will not affect nearby inactive synapses. [1]

Maintaining Long-Term Changes

In order to stabilize LTP and make it last longer periods of time, new proteins supporting this change are synthesized in response to stimulation at a potentiating synapse. The challenge that arises is how to get specific, newly synthesized proteins to the correct input-specific synapses they are need at. Two solutions to this problem include synaptic tagging and local protein synthesis.

Synaptic Tagging

In a neuron, synaptic tagging occurs in a series of steps in order to provide information on synaptic plasticity. Synaptic Tagging.jpg
In a neuron, synaptic tagging occurs in a series of steps in order to provide information on synaptic plasticity.

Synaptic tags mark where synaptic plasticity has occurred and can thus provide information on synaptic strength and potential for long-term plastic changes. [5] The tag is temporary and involves a large number of proteins, activated by the influx of Ca2+ into the postsynaptic cell. [5] In addition, depending on the type and magnitude of synaptic change, different proteins are used for tagging. For example, when plastic changes lead to long-term depression, calcineurin is used. Conversely, when plasticity leads to long-term potentiation, CaMKII is used. [5] In order for synaptic plasticity to be input-specific, these synaptic tags are essential on post-synaptic targets, to ensure synaptic potentiation is localized. [5] These tags will later initiate protein synthesis that will in turn cause synaptic plasticity changes at these activated neurons. [1]

Local Protein Synthesis

Protein synthesis at dendrites is necessary for homosynaptic plasticity. The depolarization and resulting activation of AMPA and NMDA receptors in the postsynaptic cell causes endocytosis of these receptors. Local protein synthesis is required to maintain the number of surface receptors at the synapse. These new proteins help stabilize the structural changes induced by homosynaptic plasticity. [6] There is evidence of ribosomes in dendrites, which can manufacture these proteins. Furthermore, there is also evidence of granules of RNA in dendrites, which indicates the presence of newly made proteins. LTP can be induced from dendrites severed from the soma of the post-synaptic target neuron. Contrarily, LTP can be blocked in these dendrites by protein synthesis blockers, such as Endomyacin, which further indicates a site for local protein synthesis. This evidence shows local protein synthesis is necessary for L-LTP to be stabilized and maintained. [1]

Related Research Articles

<span class="mw-page-title-main">Chemical synapse</span> Biological junctions through which neurons signals can be sent

Chemical synapses are biological junctions through which neurons' signals can be sent to each other and to non-neuronal cells such as those in muscles or glands. Chemical synapses allow neurons to form circuits within the central nervous system. They are crucial to the biological computations that underlie perception and thought. They allow the nervous system to connect to and control other systems of the body.

<span class="mw-page-title-main">Dendritic spine</span> Small protrusion on a dendrite that receives input from a single axon

A dendritic spine is a small membranous protrusion from a neuron's dendrite that typically receives input from a single axon at the synapse. Dendritic spines serve as a storage site for synaptic strength and help transmit electrical signals to the neuron's cell body. Most spines have a bulbous head, and a thin neck that connects the head of the spine to the shaft of the dendrite. The dendrites of a single neuron can contain hundreds to thousands of spines. In addition to spines providing an anatomical substrate for memory storage and synaptic transmission, they may also serve to increase the number of possible contacts between neurons. It has also been suggested that changes in the activity of neurons have a positive effect on spine morphology.

<span class="mw-page-title-main">Long-term potentiation</span> Persistent strengthening of synapses based on recent patterns of activity

In neuroscience, long-term potentiation (LTP) is a persistent strengthening of synapses based on recent patterns of activity. These are patterns of synaptic activity that produce a long-lasting increase in signal transmission between two neurons. The opposite of LTP is long-term depression, which produces a long-lasting decrease in synaptic strength.

<span class="mw-page-title-main">AMPA receptor</span> Transmembrane protein family

The α-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid receptor is an ionotropic transmembrane receptor for glutamate (iGluR) that mediates fast synaptic transmission in the central nervous system (CNS). It has been traditionally classified as a non-NMDA-type receptor, along with the kainate receptor. Its name is derived from its ability to be activated by the artificial glutamate analog AMPA. The receptor was first named the "quisqualate receptor" by Watkins and colleagues after a naturally occurring agonist quisqualate and was only later given the label "AMPA receptor" after the selective agonist developed by Tage Honore and colleagues at the Royal Danish School of Pharmacy in Copenhagen. The GRIA2-encoded AMPA receptor ligand binding core was the first glutamate receptor ion channel domain to be crystallized.

In neuroscience, synaptic plasticity is the ability of synapses to strengthen or weaken over time, in response to increases or decreases in their activity. Since memories are postulated to be represented by vastly interconnected neural circuits in the brain, synaptic plasticity is one of the important neurochemical foundations of learning and memory.

In neurophysiology, long-term depression (LTD) is an activity-dependent reduction in the efficacy of neuronal synapses lasting hours or longer following a long patterned stimulus. LTD occurs in many areas of the CNS with varying mechanisms depending upon brain region and developmental progress.

In neuroscience, a silent synapse is an excitatory glutamatergic synapse whose postsynaptic membrane contains NMDA-type glutamate receptors but no AMPA-type glutamate receptors. These synapses are named "silent" because normal AMPA receptor-mediated signaling is not present, rendering the synapse inactive under typical conditions. Silent synapses are typically considered to be immature glutamatergic synapses. As the brain matures, the relative number of silent synapses decreases. However, recent research on hippocampal silent synapses shows that while they may indeed be a developmental landmark in the formation of a synapse, that synapses can be "silenced" by activity, even once they have acquired AMPA receptors. Thus, silence may be a state that synapses can visit many times during their lifetimes.

Schaffer collaterals are axon collaterals given off by CA3 pyramidal cells in the hippocampus. These collaterals project to area CA1 of the hippocampus and are an integral part of memory formation and the emotional network of the Papez circuit, and of the hippocampal trisynaptic loop. It is one of the most studied synapses in the world and named after the Hungarian anatomist-neurologist Károly Schaffer.

An apical dendrite is a dendrite that emerges from the apex of a pyramidal cell. Apical dendrites are one of two primary categories of dendrites, and they distinguish the pyramidal cells from spiny stellate cells in the cortices. Pyramidal cells are found in the prefrontal cortex, the hippocampus, the entorhinal cortex, the olfactory cortex, and other areas. Dendrite arbors formed by apical dendrites are the means by which synaptic inputs into a cell are integrated. The apical dendrites in these regions contribute significantly to memory, learning, and sensory associations by modulating the excitatory and inhibitory signals received by the pyramidal cells.

Metaplasticity is a term originally coined by W.C. Abraham and M.F. Bear to refer to the plasticity of synaptic plasticity. Until that time synaptic plasticity had referred to the plastic nature of individual synapses. However this new form referred to the plasticity of the plasticity itself, thus the term meta-plasticity. The idea is that the synapse's previous history of activity determines its current plasticity. This may play a role in some of the underlying mechanisms thought to be important in memory and learning such as long-term potentiation (LTP), long-term depression (LTD) and so forth. These mechanisms depend on current synaptic "state", as set by ongoing extrinsic influences such as the level of synaptic inhibition, the activity of modulatory afferents such as catecholamines, and the pool of hormones affecting the synapses under study. Recently, it has become clear that the prior history of synaptic activity is an additional variable that influences the synaptic state, and thereby the degree, of LTP or LTD produced by a given experimental protocol. In a sense, then, synaptic plasticity is governed by an activity-dependent plasticity of the synaptic state; such plasticity of synaptic plasticity has been termed metaplasticity. There is little known about metaplasticity, and there is much research currently underway on the subject, despite its difficulty of study, because of its theoretical importance in brain and cognitive science. Most research of this type is done via cultured hippocampus cells or hippocampal slices.

Coincidence detection in the context of neurobiology is a process by which a neuron or a neural circuit can encode information by detecting the occurrence of temporally close but spatially distributed input signals. Coincidence detectors influence neuronal information processing by reducing temporal jitter, reducing spontaneous activity, and forming associations between separate neural events. This concept has led to a greater understanding of neural processes and the formation of computational maps in the brain.

The spine apparatus (SA) is a specialized form of endoplasmic reticulum (ER) that is found in a subpopulation of dendritic spines in central neurons. It was discovered by Edward George Gray in 1959 when he applied electron microscopy to fixed cortical tissue. The SA consists of a series of stacked discs that are connected to each other and to the dendritic system of ER-tubules. The actin binding protein synaptopodin is an essential component of the SA. Mice that lack the gene for synaptopodin do not form a spine apparatus. The SA is believed to play a role in synaptic plasticity, learning and memory, but the exact function of the spine apparatus is still enigmatic.

<span class="mw-page-title-main">Nonsynaptic plasticity</span> Form of neuroplasticity

Nonsynaptic plasticity is a form of neuroplasticity that involves modification of ion channel function in the axon, dendrites, and cell body that results in specific changes in the integration of excitatory postsynaptic potentials and inhibitory postsynaptic potentials. Nonsynaptic plasticity is a modification of the intrinsic excitability of the neuron. It interacts with synaptic plasticity, but it is considered a separate entity from synaptic plasticity. Intrinsic modification of the electrical properties of neurons plays a role in many aspects of plasticity from homeostatic plasticity to learning and memory itself. Nonsynaptic plasticity affects synaptic integration, subthreshold propagation, spike generation, and other fundamental mechanisms of neurons at the cellular level. These individual neuronal alterations can result in changes in higher brain function, especially learning and memory. However, as an emerging field in neuroscience, much of the knowledge about nonsynaptic plasticity is uncertain and still requires further investigation to better define its role in brain function and behavior.

Plasticity Product is a term coined by Jerry Rudy to refer to mRNA genetic artifacts and protein products triggered by transcription factors leading to long-lasting long term potentiation.

Synaptic tagging, or the synaptic tagging hypothesis, was first proposed in 1997 by Uwe Frey and Richard G. Morris; it seeks to explain how neural signaling at a particular synapse creates a target for subsequent plasticity-related product (PRP) trafficking essential for sustained LTP and LTD. Although the molecular identity of the tags remains unknown, it has been established that they form as a result of high or low frequency stimulation, interact with incoming PRPs, and have a limited lifespan.

Actin remodeling is a biochemical process in cells. In the actin remodeling of neurons, the protein actin is part of the process to change the shape and structure of dendritic spines. G-actin is the monomer form of actin, and is uniformly distributed throughout the axon and the dendrite. F-actin is the polymer form of actin, and its presence in dendritic spines is associated with their change in shape and structure. Actin plays a role in the formation of new spines as well as stabilizing spine volume increase. The changes that actin brings about lead to the formation of new synapses as well as increased cell communication.

Long-term potentiation (LTP), thought to be the cellular basis for learning and memory, involves a specific signal transmission process that underlies synaptic plasticity. Among the many mechanisms responsible for the maintenance of synaptic plasticity is the cadherin–catenin complex. By forming complexes with intracellular catenin proteins, neural cadherins (N-cadherins) serve as a link between synaptic activity and synaptic plasticity, and play important roles in the processes of learning and memory.

Memory allocation is a process that determines which specific synapses and neurons in a neural network will store a given memory. Although multiple neurons can receive a stimulus, only a subset of the neurons will induce the necessary plasticity for memory encoding. The selection of this subset of neurons is termed neuronal allocation. Similarly, multiple synapses can be activated by a given set of inputs, but specific mechanisms determine which synapses actually go on to encode the memory, and this process is referred to as synaptic allocation. Memory allocation was first discovered in the lateral amygdala by Sheena Josselyn and colleagues in Alcino J. Silva's laboratory.

<span class="mw-page-title-main">Heterosynaptic plasticity</span>

Synaptic plasticity refers to a chemical synapse's ability to undergo changes in strength. Synaptic plasticity is typically input-specific, meaning that the activity in a particular neuron alters the efficacy of a synaptic connection between that neuron and its target. However, in the case of heterosynaptic plasticity, the activity of a particular neuron leads to input unspecific changes in the strength of synaptic connections from other unactivated neurons. A number of distinct forms of heterosynaptic plasticity have been found in a variety of brain regions and organisms. These different forms of heterosynaptic plasticity contribute to a variety of neural processes including associative learning, the development of neural circuits, and homeostasis of synaptic input.

<span class="mw-page-title-main">Synaptic stabilization</span> Modifying synaptic strength via cell adhesion molecules

Synaptic stabilization is crucial in the developing and adult nervous systems and is considered a result of the late phase of long-term potentiation (LTP). The mechanism involves strengthening and maintaining active synapses through increased expression of cytoskeletal and extracellular matrix elements and postsynaptic scaffold proteins, while pruning less active ones. For example, cell adhesion molecules (CAMs) play a large role in synaptic maintenance and stabilization. Gerald Edelman discovered CAMs and studied their function during development, which showed CAMs are required for cell migration and the formation of the entire nervous system. In the adult nervous system, CAMs play an integral role in synaptic plasticity relating to learning and memory.

References

  1. 1 2 3 4 5 6 7 Purves, D., Augustine, G. J., Fitzpatrick, D., Hall, W. C., LaMantia, A. S., White, L. E. (2012). Synaptic Plasticity. In Neuroscience (5th ed.) (pp. 163-182). Sunderland, Massachusetts: Sinauer Associates.
  2. Byrne, J. (1997). Synaptic Plasticity. In Neuroscience Online (Section 1, Chapter 7).
  3. 1 2 3 Bailey, C., Giustetto, M., Huang, Y., Hawkins, R., Kandel, E. (Oct. 2000). Reviews: Is Heterosynaptic Modulation Essential for Stabilizing Hebbian Plasticity and Memory?. In Macmillan Magazines Ltd (Vol. 1). Retrieved from www.nature.com/reviews/neuroscience
  4. 1 2 Higley, M.J., Sabatini, B. L. (Feb. 2012.) Calcium Signaling in Dendritic Spines. Cold Spring Harbor Perspectives in Biology. Retrieved from http://cshperspectives.cshlp.org/. doi:10.1101/cshperspect.a005686.
  5. 1 2 3 4 Redondo, Roger L., and Richard G. M. Morris. (2011) "Making Memories Last: The Synaptic Tagging and Capture Hypothesis." Nature Reviews Neuroscience, 12, 17-30.
  6. Pfeiffer B. E., Huber K. M. (2006). Current advances in Local Protein Synthesis and Synaptic Plasticity. The Journal of Neuroscience, 26(27), 7147-7150.