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.
As the opposing process to long-term potentiation (LTP), LTD is one of several processes that serves to selectively weaken specific synapses in order to make constructive use of synaptic strengthening caused by LTP. This is necessary because, if allowed to continue increasing in strength, synapses would ultimately reach a ceiling level of efficiency, which would inhibit the encoding of new information.
As the opposing process to long-term potentiation (LTP), LTD is one of several processes that serves to selectively weaken specific synapses in order to make constructive use of synaptic strengthening caused by LTP. This is necessary because, if allowed to continue increasing in strength, synapses would ultimately reach a ceiling level of efficiency, which would inhibit the encoding of new information.
Characterisation
LTD
in the hippocampus and cerebellum have been the best characterized, but
there are other brain areas in which mechanisms of LTD are understood.[1]
LTD has also been found to occur in different types of neurons that
release various neurotransmitters, however, the most common
neurotransmitter involved in LTD is L-glutamate. L-glutamate acts on the
N-methyl-D- aspartate receptors (NMDARs), α-amino-3-hydroxy-5-methylisoxazole-4-propionic acid receptors (AMPARs), kainate receptors (KARs) and metabotropic glutamate receptors (mGluRs) during LTD. It can result from strong synaptic stimulation (as occurs in the cerebellar Purkinje cells) or from persistent weak synaptic stimulation (as in the hippocampus). Long-term potentiation
(LTP) is the opposing process to LTD; it is the long-lasting increase
of synaptic strength. In conjunction, LTD and LTP are factors affecting
neuronal synaptic plasticity. LTD is thought to result mainly from a
decrease in postsynaptic receptor
density, although a decrease in presynaptic neurotransmitter release
may also play a role. Cerebellar LTD has been hypothesized to be
important for motor learning.
However, it is likely that other plasticity mechanisms play a role as
well. Hippocampal LTD may be important for the clearing of old memory
traces.
Hippocampal/cortical LTD can be dependent on NMDA receptors, metabotropic glutamate receptors (mGluR), or endocannabinoids.
The result of the underlying-LTD molecular mechanism is the
phosphorylation of AMPA glutamate receptors and their elimination from
the surface of the parallel fiber-Purkinje cell (PF-PC) synapse.
Neural homeostasis
It is highly important for neurons to maintain a variable range of neuronal output. If synapses were only reinforced by positive feedback,
they would eventually come to the point of complete inactivity or too
much activity. To prevent neurons from becoming static, there are two
regulatory forms of plasticity that provide negative feedback: metaplasticity and scaling. Metaplasticity is expressed as a change in the capacity to provoke subsequent synaptic plasticity, including LTD and LTP. The Bienenstock, Cooper and Munro model
(BCM model) proposes that a certain threshold exists such that a level
of postsynaptic response below the threshold leads to LTD and above it
leads to LTP. BCM theory further proposes that the level of this
threshold depends upon the average amount of postsynaptic activity. Scaling has been found to occur when the strength of all of a neuron’s excitatory inputs are scaled up or down. LTD and LTP coincide with metaplasticity and synaptic scaling to maintain proper neuronal network function.
General forms of LTD
Long-term depression can be described as either homosynaptic plasticity or heterosynaptic plasticity. Homosynaptic LTD is restricted to the individual synapse that is activated by a low frequency stimulus.
In other words, this form of LTD is activity-dependent, because the
events causing the synaptic weakening occur at the same synapse that is
being activated. Homosynaptic LTD is also associative in that it
correlates the activation of the postsynaptic neuron with the firing of
the presynaptic neuron.
Heterosynaptic LTD, in contrast, occurs at synapses that are not
potentiated or are inactive. The weakening of a synapse is independent
of the activity of the presynaptic or postsynaptic neurons as a result
of the firing of a distinct modulatory interneuron. Thus, this form of
LTD impacts synapses nearby those receiving action potentials.
Mechanisms that weaken synapses
Hippocampus
LTD affects hippocampal synapses between the Schaffer collaterals and the CA1 pyramidal cells. LTD at the Schaffer collateral-CA1 synapses depends on the timing and frequency of calcium influx.
LTD occurs at these synapses when Schaffer collaterals are stimulated
repetitively for extended time periods (10–15 minutes) at a low
frequency (approximately 1 Hz). Depressed excitatory postsynaptic potentials (EPSPs)
result from this particular stimulation pattern. The magnitude of
calcium signal in the postsynaptic cell largely determines whether LTD
or LTP occurs; LTD is brought about by small, slow rises in postsynaptic calcium levels. When Ca2+ entry is below threshold, it leads to LTD.
The threshold level in area CA1 is on a sliding scale that depends on
the history of the synapse. If the synapse has already been subject to
LTP, the threshold is raised, increasing the probability that a calcium
influx will yield LTD. In this way, a "negative feedback" system
maintains synaptic plasticity. Activation of NMDA-type glutamate receptors, which belong to a class of ionotropic glutamate receptors (iGluRs), is required for calcium entry into the CA1 postsynaptic cell.[13] Change in voltage provides a graded control of postsynaptic Ca2+ by regulating NMDAR-dependent Ca2+ influx, which is responsible for initiating LTD.
While LTP is in part due to the activation of protein kinases,
which subsequently phosphorylate target proteins, LTD arises from
activation of calcium-dependent phosphatases that dephosphorylate the
target proteins. Selective activation of these phosphatases by varying
calcium levels might be responsible for the different effects of calcium
observed during LTD.
The activation of postsynaptic phosphatases causes internalization of
synaptic AMPA receptors (also a type of iGluRs) into the postsynaptic
cell by clathrin-coated endocytosis mechanisms, thereby reducing sensitivity to glutamate released by Schaffer collateral terminals.
A model for the mechanisms of depotentiation and de novo LTD.
Cerebellum
LTD occurs at synapses in cerebellar Purkinje neurons, which receive two forms of excitatory input, one from a single climbing fiber and one from hundreds of thousands of parallel fibers.
LTD decreases the efficacy of parallel fiber synapse transmission,
though, according to recent findings, it also impairs climbing fiber
synapse transmission.
Both parallel fibers and climbing fibers must be simultaneously
activated for LTD to occur. With respect to calcium release however, it
is best if the parallel fibers are activated a few hundred milliseconds
before the climbing fibres. In one pathway, parallel fiber terminals
release glutamate to activate AMPA and metabotropic
glutamate receptors in the postsynaptic Purkinje cell. When glutamate
binds to the AMPA receptor, the membrane depolarizes. Glutamate binding
to the metabotropic receptor activates phospholipase C (PLC) and produces diacylglycerol (DAG) and inositol triphosphate (IP3) second messengers. In the pathway initiated by activation of climbing fibers, calcium enters the postsynaptic cell through voltage-gated ion channels,
raising intracellular calcium levels. Together, DAG and IP3 augment the
calcium concentration rise by targeting IP3-sensitive receptors
triggering release of calcium from intracellular stores as well as
protein kinase C (PKC)
activation (which is accomplished jointly by calcium and DAG). PKC
phosphorylates AMPA receptors, which promotes their dissociation from
scaffold proteins in the post-synaptic membrane and subsequent
internalization. With the loss of AMPA receptors, the postsynaptic
Purkinje cell response to glutamate release from parallel fibers is
depressed.
Calcium triggering in the cerebellum is a critical mechanism involved
in long-term depression. Parallel fibre terminals and climbing fibres
work together in a positive feedback loop for invoking high calcium
release.
Ca2+ involvement
Further
research has determined calcium's role in long-term depression
induction. While other mechanisms of long-term depression are being
investigated, calcium's role in LTD is a defined and well understood
mechanism by scientists. High calcium concentrations in the
post-synaptic Purkinje cells is a necessity for the induction of
long-term depression. There are several sources of calcium signaling
that elicit LTD: climbing fibres and parallel fibres which converge onto
Purkinje cells. Calcium signaling in the post-synaptic cell involved
both spatial and temporal overlap of climbing fibre induced calcium
release into dendrites as well as parallel fibre induced mGluRs and IP3
mediated calcium release. In the climbing fibres, AMPAR-mediated
depolarization induces a regenerative action potential that spreads to
the dendrites, which is generated by voltage-gated calcium channels.
Paired with PF-mediated mGluR1 activation results in LTD induction.
In the parallel fibres, GluRs are activated by constant activation of
the parallel fibres which indirectly induces the IP3 to bind to its
receptor (IP3) and activate calcium release from intracellular storage.
In calcium induction, there is a positive feedback loop to regenerate
calcium for long-term depression. Climbing and parallel fibres must be
activated together to depolarize the Purkinje cells while activating
mGlur1s.
Timing is a critical component to CF and PF as well, a better calcium
release involves PF activation a few hundred milliseconds before CF
activity.
AMPAR phosphorylation
There
is a series of signaling cascades, MAPK, in the cerebellum that plays a
critical role in cerebellum LTD. The MAPK cascade is important in
information processing within neurons and other various types of cells.
The cascade includes MAPKKK, MAPKK, and MAPK. Each is dual
phosphorylated by the other, MAPKKK dual phosphorylates MAPKK and in
turn dual phosphorylates MAPK. There is a positive feedback loop that
results from a simultaneous input of signals from PF-CF and increases
DAG and Ca2+ in Purkinje dendritic spines. Calcium and DAG
activate conventional PKC (cPKC), which then activates MAPKKK and the
rest of the MAPK cascade. Activated MAPK and Ca2+ activate
PLA2, AA and cPKC creating a positive feedback loop. Induced cPKC
phosphorylates AMPA receptors and are eventually removed form the
postsynaptic membrane via endocytosis. The timescale is for this process
is approximately 40 minutes. overall, the magnitude of the LTD
correlates with AMPAR phosphorylation.
Striatum
The mechanisms of LTD differ in the two subregions of the striatum. LTD is induced at corticostriatal medium spiny neuron synapses in the dorsal striatum by a high frequency stimulus coupled with postsynaptic depolarization, coactivation of dopamine D1 and D2 receptors and group I mGlu receptors, lack of NMDA receptor activation, and endocannabinoid activation.
In the prelimbic cortex of the striatum, three forms or LTD have been established. The mechanism of the first is similar to CA1-LTD: a low frequency stimulus induces LTD by activation of NMDA receptors, with postsynaptic depolarization and increased postsynaptic calcium influx. The second is initiated by a high frequency stimulus and is arbitrated by presynaptic mGlu receptor 2 or 3, resulting in a long term reduction in the involvement of P/Q-type calcium channels in glutamate release. The third form of LTD requires endocannabinoids, activation of mGlu receptors and repetitive stimulation of glutamatergic fibers (13 Hz for ten minutes), resulting in a long term decrease in presynaptic glutamate release. It is proposed that LTD in GABAergic striatal neurons leads to a long term decrease in inhibitory effects on the basal ganglia, influencing the storage of motor skills.
Visual cortex
Long-term depression has also been observed in the visual cortex, and it is proposed to be involved in ocular dominance. Recurring low-frequency stimulation of layer IV of the visual cortex or the white matter of the visual cortex causes LTD in layer III. In this form of LTD, low-frequency stimulation of one pathway results in LTD only for that input, making it homosynaptic. This type of LTD is similar to that found in the hippocampus, because it is triggered by a small elevation in postsynaptic calcium ions and activation of phosphatases. LTD has also been found to occur in this fashion in layer II.[1] A different mechanism is at work in the LTD that occurs in layer V. In layer V, LTD requires low frequency stimulation, endocannabinoid signaling, and activation of presynaptic NR2B-containing NMDA receptors.
It has been found that paired-pulse stimulation (PPS) induces a form of homosynaptic LTD in the superficial layers of the visual cortex when the synapse is exposed to carbachol (CCh) and norepinephrine (NE).
The magnitude of this LTD is comparable to that which results
from low frequency stimulation, but with fewer stimulation pulses (40
PPS for 900 low frequency stimulations). It is suggested that the effect of NE is to control the gain of NMDA receptor-dependent homosynaptic LTD. Like norepinephrine, acetylcholine
is proposed to control the gain of NMDA receptor-dependent homosynaptic
LTD, but it is likely to be a promoter of additional LTD mechanisms as
well.
Prefrontal cortex
The neurotransmitter serotonin is involved in LTD induction in the prefrontal cortex (PFC).
The serotonin system in the PFC plays an important role in regulating
cognition and emotion. Serotonin, in cooperation with a group I
metabotropic glutamate receptor (mGluR) agonist, facilitates LTD
induction through augmentation of AMPA receptor internalization. This
mechanism possibly underlies serotonin's role in the control of
cognitive and emotional processes that synaptic plasticity in PFC
neurons mediates.
Perirhinal cortex
Computational models predict that LTD creates a gain in recognition memory storage capacity over that of LTP in the perirhinal cortex, and this prediction is confirmed by neurotransmitter receptor blocking experiments. It is proposed that there are multiple memory mechanisms in the perirhinal cortex.
The exact mechanisms are not completely understood, however pieces of
the mechanisms have been deciphered. Studies suggest that one perirhinal cortex LTD mechanism involves NMDA receptors and group I and II mGlu receptors 24 hours after the stimulus. The other LTD mechanism involves acetylcholine receptors and kainate receptors at a much earlier time, about 20 to 30 minutes after stimulus.
Role of endocannabinoids
Endocannabinoids
affect long-lasting plasticity processes in various parts of the brain,
serving both as regulators of pathways and necessary retrograde
messengers in specific forms of LTD. In regard to retrograde signaling,
cannabinoid receptors
function widely throughout the brain in presynaptic inhibition.
Endocannabinoid retrograde signaling has been shown to effect LTD at corticostriatal synapses and glutamatergic synapses in the prelimbic cortex of the nucleus accumbens (NAc), and it is also involved in spike-timing-dependent LTD in the visual cortex. Endocannabinoids are implicated in LTD of inhibitory inputs (LTDi) within the basolateral nucleus of the amygdala (BLA)
as well as in the stratum radiatum of the hippocampus. Additionally,
endocannabinoids play an important role in regulating various forms of
synaptic plasticity. They are involved in inhibition of LTD at parallel
fiber Purkinje neuron synapses in the cerebellum and NMDA
receptor-dependent LTD in the hippocampus.
Spike timing-dependent plasticity
Spike timing-dependent plasticity (STDP) refers to the timing of presynaptic and postsynaptic action potentials. STDP is a form of neuroplasticity
in which a millisecond-scale change in the timing of presynaptic and
postsynaptic spikes will cause differences in postsynaptic Ca2+ signals, inducing either LTP or LTD. LTD occurs when postsynaptic spikes precede presynaptic spikes by up to 20-50 ms. Whole-cell patch clamp experiments "in vivo" indicate that post-leading-pre spike delays elicit synaptic depression.
LTP is induced when neurotransmitter release occurs 5-15 ms before a back-propagating action potential, whereas LTD is induced when the stimulus occurs 5-15 ms after the back-propagating action potential.
There is a plasticity window: if the presynaptic and postsynaptic
spikes are too far apart (i.e., more than 15 ms apart), there is little
chance of plasticity. The possible window for LTD is wider than that for LTP – although it is important to note that this threshold depends on synaptic history.
When postsynaptic action potential firing occurs prior to
presynaptic afferent firing, both presynaptic endocannabinoid (CB1)
receptors and NMDA receptors are stimulated at the same time.
Postsynaptic spiking alleviates the Mg2+ block on NMDA receptors. The postsynaptic depolarization will subside by the time an EPSP occurs, enabling Mg2+ to return to its inhibitory binding site. Thus, the influx of Ca2+ in the postsynaptic cell is reduced. CB1 receptors detect postsynaptic activity levels via retrograde endocannabinoid release.
STDP selectively enhances and consolidates specific synaptic
modifications (signals), while depressing global ones (noise). This
results in a sharpened signal-to-noise ratio in human cortical networks that facilitates the detection of relevant signals during information processing in humans.
Motor learning and memory
Long-term depression has long been hypothesized to be an important mechanism behind motor learning and memory.
Cerebellar LTD is thought to lead to motor learning, and hippocampal
LTD is thought to contribute to the decay of memory. However, recent
studies have found that hippocampal LTD may not act as the reverse of
LTP, but may instead contribute to spatial memory formation.
Although LTD is now well characterized, these hypotheses about its
contribution to motor learning and memory remain controversial.
Studies have connected deficient cerebellar LTD with impaired motor learning. In one study, metabotropic glutamate receptor 1 mutant mice maintained a normal cerebellar anatomy but had weak LTD and consequently impaired motor learning.
However the relationship between cerebellar LTD and motor learning has
been seriously challenged. A study on rats and mice proved that normal
motor learning occurs while LTD of Purkinje cells is prevented by (1R-1-benzo thiophen-5-yl-2[2-diethylamino)-ethoxy] ethanol hydrochloride (T-588).
Likewise, LTD in mice was disrupted using several experimental
techniques with no observable deficits in motor learning or performance. These taken together suggest that the correlation between cerebellar LTD and motor learning may have been illusory.
Studies on rats have made a connection between LTD in the hippocampus and memory. In one study, rats were exposed to a novel environment, and homosynaptic plasticity (LTD) in CA1 was observed.
After the rats were brought back to their initial environment, LTD
activity was lost. It was found that if the rats were exposed to
novelty, the electrical stimulation required to depress synaptic
transmission was of lower frequency than without novelty. When the rat was put in a novel environment, acetylcholine was released in the hippocampus from the medial septum fiber, resulting in LTD in CA1. Therefore, it has been concluded that acetylcholine facilitates LTD in CA1.
LTD has been correlated with spatial learning in rats, and it is crucial in forming a complete spatial map. It suggested that LTD and LTP work together to encode different aspects of spatial memory.
New evidence suggests that LTP works to encode space, whereas LTD works to encode the features of space.
Specifically, it is accepted that encoding of experience takes place
on a hierarchy. Encoding of new space is the priority of LTP, while
information about orientation in space could be encoded by LTD in the dentate gyrus, and the finer details of space could be encoded by LTD in the CA1.
Cocaine as a model of LTD in drug addiction
The addictive property of cocaine is believed to occur in the nucleus accumbens (NAc). After chronic cocaine use, the amount of AMPA receptors relative to NMDA receptors decreases in the medium spiny neurons in the NAc shell. This decrease in AMPA receptors
is thought to occur through the same mechanism as NMDR-dependent LTD,
because this form of plasticity is reduced after cocaine use. During the period of cocaine use, the mechanisms of LTD artificially occur in the NAc. As a consequence, the amount of AMPA receptors is ramped up in the NAc neurons during withdrawal. This is possibly due to homeostatic synaptic scaling. This increase in AMPA receptors causes a hyperexcitability in the NAc neurons. The effect of this hyperexcitability is thought to be an increase in the amount of GABA release from the NAc on the ventral tegmental area (VTA), making the dopaminergic neurons in the VTA less likely to fire, and thus resulting in the symptoms of withdrawal.
Current research
Research on the role of LTD in neurological disorders such as Alzheimer's disease (AD)
is ongoing. It has been suggested that a reduction in NMDAR-dependent
LTD may be due to changes not only in postsynaptic AMPARs but also in
NMDARs, and these changes are perhaps present in early and mild forms of
Alzheimer-type dementia.
Additionally, researchers have recently discovered a new mechanism (which involves LTD) linking soluble amyloid beta protein (Aβ)
with the synaptic injury and memory loss related to AD. While Aβ's
role in LTD regulation has not been clearly understood, it has been
found that soluble Aβ facilitates hippocampal LTD and is mediated by a
decrease in glutamate
recycling at hippocampal synapses. Excess glutamate is a proposed
contributor to the progressive neuronal loss involved in AD. Evidence
that soluble Aβ enhances LTD through a mechanism involving altered
glutamate uptake at hippocampal synapses has important implications for
the initiation of synaptic failure in AD and in types of age-related Aβ
accumulation. This research provides a novel understanding of the
development of AD and proposes potential therapeutic targets for the
disease. Further research is needed to understand how soluble amyloid
beta protein specifically interferes with glutamate transporters.
The mechanism of long-term depression has been well characterized
in limited parts of the brain. However, the way in which LTD affects motor learning and memory is still not well understood. Determining this relationship is presently one of the major focuses of LTD research.
Neurodegeneration
Neurodegenerative
diseases research remains inconclusive as to the mechanisms that
triggers the degeneration in the brain. New evidence demonstrates there
are similarities between the apoptotic pathway and LTD which involves
the phosphorylation/activation of GSK3β. NMDAR-LTD(A)
contributes to the elimination of excess synapses during development.
This process is downregulated after synapses have stabilized, and is
regulated by GSK3β. During neurodegeneration, there is the possibility
that there is deregulation of GSK3β resulting in 'synaptic pruning'.
If there is excess removal of synapses, this illustrates early signs of
neurodegeration and a link between apoptosis and neurodegeneration
diseases.
