Excitotoxicity

(Redirected from Excitotoxic)

In excitotoxicity, nerve cells suffer damage or death when the levels of otherwise necessary and safe neurotransmitters such as glutamate become pathologically high, resulting in excessive stimulation of receptors. For example, when glutamate receptors such as the NMDA receptor or AMPA receptor encounter excessive levels of the excitatory neurotransmitter, glutamate, significant neuronal damage might ensue. Excess glutamate allows high levels of calcium ions (Ca2+) to enter the cell. Ca2+ influx into cells activates a number of enzymes, including phospholipases, endonucleases, and proteases such as calpain. These enzymes go on to damage cell structures such as components of the cytoskeleton, membrane, and DNA.[1][2] In evolved, complex adaptive systems such as biological life it must be understood that mechanisms are rarely, if ever, simplistically direct. For example, NMDA in subtoxic amounts induces neuronal survival of otherwise toxic levels of glutamate.[3][4]

Low Ca2+ buffering and excitotoxicity under physiological stress and pathophysiological conditions in motor neuron (MNs). Low Ca2+ buffering in amyotrophic lateral sclerosis (ALS) vulnerable hypoglossal MNs exposes mitochondria to higher Ca2+ loads compared to highly buffered cells. Under normal physiological conditions, the neurotransmitter opens glutamate, NMDA and AMPA receptor channels, and voltage dependent Ca2+ channels (VDCC) with high glutamate release, which is taken up again by EAAT1 and EAAT2. This results in a small rise in intracellular calcium that can be buffered in the cell. In ALS, a disorder in the glutamate receptor channels leads to high calcium conductivity, resulting in high Ca2+ loads and increased risk for mitochondrial damage. This triggers the mitochondrial production of reactive oxygen species (ROS), which then inhibit glial EAAT2 function. This leads to further increases in the glutamate concentration at the synapse and further rises in postsynaptic calcium levels, contributing to the selective vulnerability of MNs in ALS. Jaiswal et al., 2009.[1]

Excitotoxicity may be involved in cancers, spinal cord injury, stroke, traumatic brain injury, hearing loss (through noise overexposure or ototoxicity), and in neurodegenerative diseases of the central nervous system such as multiple sclerosis, Alzheimer's disease, amyotrophic lateral sclerosis (ALS), Parkinson's disease, alcoholism, alcohol withdrawal or hyperammonemia and especially over-rapid benzodiazepine withdrawal, and also Huntington's disease.[5][6] Other common conditions that cause excessive glutamate concentrations around neurons are hypoglycemia. Blood sugars are the primary glutamate removal method from inter-synaptic spaces at the NMDA and AMPA receptor site. Persons in excitotoxic shock must never fall into hypoglycemia. Patients should be given 5% glucose (dextrose) IV drip during excitotoxic shock to avoid a dangerous build up of glutamate around NMDA and AMPA neurons.[citation needed] When 5% glucose (dextrose) IV drip is not available high levels of fructose are given orally. Treatment is administered during the acute stages of excitotoxic shock along with glutamate antagonists. Dehydration should be avoided as this also contributes to the concentrations of glutamate in the inter-synaptic cleft[7] and "status epilepticus can also be triggered by a build up of glutamate around inter-synaptic neurons."[8]

History

edit

The harmful effects of glutamate on the central nervous system were first observed in 1954 by T. Hayashi, a Japanese scientist who stated that direct application of glutamate caused seizure activity,[9] though this report went unnoticed for several years.[citation needed] D. R. Lucas and J. P. Newhouse, after noting that "single doses of [20–30 grams of sodium glutamate in humans] have ... been administered intravenously without permanent ill-effects", observed in 1957 that a subcutaneous dose described as "a little less than lethal", destroyed the neurons in the inner layers of the retina in newborn mice.[10] In 1969, John Olney discovered that the phenomenon was not restricted to the retina, but occurred throughout the brain, and coined the term excitotoxicity. He also assessed that cell death was restricted to postsynaptic neurons, that glutamate agonists were as neurotoxic as their efficiency to activate glutamate receptors, and that glutamate antagonists could stop the neurotoxicity.[11]

In 2002, Hilmar Bading and co-workers found that excitotoxicity is caused by the activation of NMDA receptors located outside synaptic contacts.[12] The molecular basis for toxic extrasynaptic NMDA receptor signaling was uncovered in 2020 when Hilmar Bading and co-workers described a death signaling complex that consists of extrasynaptic NMDA receptor and TRPM4.[13] Disruption of this complex using NMDAR/TRPM4 interface inhibitors (also known as ‚interface inhibitors‘) renders extrasynaptic NMDA receptor non-toxic.[citation needed]

Pathophysiology

edit

Excitotoxicity can occur from substances produced within the body (endogenous excitotoxins). Glutamate is a prime example of an excitotoxin in the brain, and it is also the major excitatory neurotransmitter in the central nervous system of mammals.[14] During normal conditions, glutamate concentration can be increased up to 1mM in the synaptic cleft, which is rapidly decreased in the lapse of milliseconds.[15] When the glutamate concentration around the synaptic cleft cannot be decreased or reaches higher levels, the neuron kills itself by a process called apoptosis.[16][17]

This pathologic phenomenon can also occur after brain injury and spinal cord injury. Within minutes after spinal cord injury, damaged neural cells within the lesion site spill glutamate into the extracellular space where glutamate can stimulate presynaptic glutamate receptors to enhance the release of additional glutamate.[18] Brain trauma or stroke can cause ischemia, in which blood flow is reduced to inadequate levels. Ischemia is followed by accumulation of glutamate and aspartate in the extracellular fluid, causing cell death, which is aggravated by lack of oxygen and glucose. The biochemical cascade resulting from ischemia and involving excitotoxicity is called the ischemic cascade. Because of the events resulting from ischemia and glutamate receptor activation, a deep chemical coma may be induced in patients with brain injury to reduce the metabolic rate of the brain (its need for oxygen and glucose) and save energy to be used to remove glutamate actively. (The main aim in induced comas is to reduce the intracranial pressure, not brain metabolism).[citation needed]

Increased extracellular glutamate levels leads to the activation of Ca2+ permeable NMDA receptors on myelin sheaths and oligodendrocytes, leaving oligodendrocytes susceptible to Ca2+ influxes and subsequent excitotoxicity.[19][20] One of the damaging results of excess calcium in the cytosol is initiating apoptosis through cleaved caspase processing.[20] Another damaging result of excess calcium in the cytosol is the opening of the mitochondrial permeability transition pore, a pore in the membranes of mitochondria that opens when the organelles absorb too much calcium. Opening of the pore may cause mitochondria to swell and release reactive oxygen species and other proteins that can lead to apoptosis. The pore can also cause mitochondria to release more calcium. In addition, production of adenosine triphosphate (ATP) may be stopped, and ATP synthase may in fact begin hydrolysing ATP instead of producing it,[21] which is suggested to be involved in depression.[22]

Inadequate ATP production resulting from brain trauma can eliminate electrochemical gradients of certain ions. Glutamate transporters require the maintenance of these ion gradients to remove glutamate from the extracellular space. The loss of ion gradients results in not only the halting of glutamate uptake, but also in the reversal of the transporters. The Na+-glutamate transporters on neurons and astrocytes can reverse their glutamate transport and start secreting glutamate at a concentration capable of inducing excitotoxicity.[23] This results in a buildup of glutamate and further damaging activation of glutamate receptors.[24]

On the molecular level, calcium influx is not the only factor responsible for apoptosis induced by excitoxicity. Recently,[25] it has been noted that extrasynaptic NMDA receptor activation, triggered by both glutamate exposure or hypoxic/ischemic conditions, activate a CREB (cAMP response element binding) protein shut-off, which in turn caused loss of mitochondrial membrane potential and apoptosis. On the other hand, activation of synaptic NMDA receptors activated only the CREB pathway, which activates BDNF (brain-derived neurotrophic factor), not activating apoptosis.[25][26]

Exogenous excitotoxins

edit

Exogenous excitotoxins refer to neurotoxins that also act at postsynaptic cells but are not normally found in the body. These toxins may enter the body of an organism from the environment through wounds, food intake, aerial dispersion etc.[27] Common excitotoxins include glutamate analogs that mimic the action of glutamate at glutamate receptors, including AMPA and NMDA receptors.[28]

BMAA

edit

The L-alanine derivative β-methylamino-L-alanine (BMAA) has long been identified as a neurotoxin which was first associated with the amyotrophic lateral sclerosis/parkinsonismdementia complex (Lytico-bodig disease) in the Chamorro people of Guam.[29] The widespread occurrence of BMAA can be attributed to cyanobacteria which produce BMAA as a result of complex reactions under nitrogen stress.[30] Following research, excitotoxicity appears to be the likely mode of action for BMAA which acts as a glutamate agonist, activating AMPA and NMDA receptors and causing damage to cells even at relatively low concentrations of 10 μM.[31] The subsequent uncontrolled influx of Ca2+ then leads to the pathophysiology described above. Further evidence of the role of BMAA as an excitotoxin is rooted in the ability of NMDA antagonists like MK801 to block the action of BMAA.[29] More recently, evidence has been found that BMAA is misincorporated in place of L-serine in human proteins.[32][33] A considerable portion of the research relating to the toxicity of BMAA has been conducted on rodents. A study published in 2016 with vervets (Chlorocebus sabaeus) in St. Kitts, which are homozygous for the apoE4 (APOE-ε4) allele (a condition which in humans is a risk factor for Alzheimer's disease), found that vervets orally administered BMAA developed hallmark histopathology features of Alzheimer's Disease including amyloid beta plaques and neurofibrillary tangle accumulation. Vervets in the trial fed smaller doses of BMAA were found to have correlative decreases in these pathology features. This study demonstrates that BMAA, an environmental toxin, can trigger neurodegenerative disease as a result of a gene/environment interaction.[34] While BMAA has been detected in brain tissue of deceased ALS/PDC patients, further insight is required to trace neurodegenerative pathology in humans to BMAA.[citation needed]

See also

edit

References

edit
  1. ^ a b Jaiswal MK, Zech WD, Goos M, Leutbecher C, Ferri A, Zippelius A, et al. (June 2009). "Impairment of mitochondrial calcium handling in a mtSOD1 cell culture model of motoneuron disease". BMC Neuroscience. 10: 64. doi:10.1186/1471-2202-10-64. PMC 2716351. PMID 19545440.
  2. ^ Manev H, Favaron M, Guidotti A, Costa E (July 1989). "Delayed increase of Ca2+ influx elicited by glutamate: role in neuronal death". Molecular Pharmacology. 36 (1): 106–112. PMID 2568579.
  3. ^ Zheng S, Eacker SM, Hong SJ, Gronostajski RM, Dawson TM, Dawson VL (July 2010). "NMDA-induced neuronal survival is mediated through nuclear factor I-A in mice". The Journal of Clinical Investigation. 120 (7): 2446–2456. doi:10.1172/JCI33144. PMC 2898580. PMID 20516644.
  4. ^ Chuang DM, Gao XM, Paul SM (August 1992). "N-methyl-D-aspartate exposure blocks glutamate toxicity in cultured cerebellar granule cells". Molecular Pharmacology. 42 (2): 210–216. PMID 1355259.
  5. ^ Kim AH, Kerchner GA, and Choi DW. Blocking Excitotoxicity or Glutamatergic Storm. Chapter 1 in CNS Neuroprotection. Marcoux FW and Choi DW, editors. Springer, New York. 2002. Pages 3-36
  6. ^ Hughes JR (June 2009). "Alcohol withdrawal seizures". Epilepsy & Behavior. 15 (2): 92–97. doi:10.1016/j.yebeh.2009.02.037. PMID 19249388. S2CID 20197292.
  7. ^ Camacho A, Massieu L (January 2006). "Role of glutamate transporters in the clearance and release of glutamate during ischemia and its relation to neuronal death". Archives of Medical Research. 37 (1): 11–18. doi:10.1016/j.arcmed.2005.05.014. PMID 16314180.
  8. ^ Fujikawa DG (December 2005). "Prolonged seizures and cellular injury: understanding the connection". Epilepsy & Behavior. 7 (Suppl 3): S3-11. doi:10.1016/j.yebeh.2005.08.003. PMID 16278099. S2CID 27515308.
  9. ^ Watkins JC, Jane DE (January 2006). "The glutamate story". British Journal of Pharmacology. 147 (Suppl 1): S100–S108. doi:10.1038/sj.bjp.0706444. PMC 1760733. PMID 16402093.
  10. ^ Lucas DR, Newhouse JP (August 1957). "The toxic effect of sodium L-glutamate on the inner layers of the retina". A.M.A. Archives of Ophthalmology. 58 (2): 193–201. doi:10.1001/archopht.1957.00940010205006. PMID 13443577.
  11. ^ Olney JW (May 1969). "Brain lesions, obesity, and other disturbances in mice treated with monosodium glutamate". Science. 164 (3880): 719–721. Bibcode:1969Sci...164..719O. doi:10.1126/science.164.3880.719. hdl:10217/207298. PMID 5778021. S2CID 46248201.
  12. ^ Hardingham GE, Fukunaga Y, Bading H (May 2002). "Extrasynaptic NMDARs oppose synaptic NMDARs by triggering CREB shut-off and cell death pathways". Nature Neuroscience. 5 (5): 405–414. doi:10.1038/nn835. PMID 11953750. S2CID 659716.
  13. ^ Yan J, Bengtson CP, Buchthal B, Hagenston AM, Bading H (October 2020). "Coupling of NMDA receptors and TRPM4 guides discovery of unconventional neuroprotectants". Science. 370 (6513): eaay3302. doi:10.1126/science.aay3302. PMID 33033186. S2CID 222210921.
  14. ^ Temple MD, O'Leary DM, and Faden AI. The role of glutamate receptors in the pathophysiology of traumatic CNS injury. Chapter 4 in Head Trauma: Basic, Preclinical, and Clinical Directions. Miller LP and Hayes RL, editors. Co-edited by Newcomb JK. John Wiley and Sons, Inc. New York. 2001. Pages 87-113.
  15. ^ Clements JD, Lester RA, Tong G, Jahr CE, Westbrook GL (November 1992). "The time course of glutamate in the synaptic cleft". Science. 258 (5087): 1498–1501. Bibcode:1992Sci...258.1498C. doi:10.1126/science.1359647. PMID 1359647.
  16. ^ Yang DD, Kuan CY, Whitmarsh AJ, Rincón M, Zheng TS, Davis RJ, et al. (October 1997). "Absence of excitotoxicity-induced apoptosis in the hippocampus of mice lacking the Jnk3 gene". Nature. 389 (6653): 865–870. Bibcode:1997Natur.389..865Y. doi:10.1038/39899. PMID 9349820. S2CID 4430535.
  17. ^ Ankarcrona M, Dypbukt JM, Bonfoco E, Zhivotovsky B, Orrenius S, Lipton SA, Nicotera P (October 1995). "Glutamate-induced neuronal death: a succession of necrosis or apoptosis depending on mitochondrial function". Neuron. 15 (4): 961–973. doi:10.1016/0896-6273(95)90186-8. PMID 7576644.
  18. ^ Hulsebosch CE, Hains BC, Crown ED, Carlton SM (April 2009). "Mechanisms of chronic central neuropathic pain after spinal cord injury". Brain Research Reviews. 60 (1): 202–213. doi:10.1016/j.brainresrev.2008.12.010. PMC 2796975. PMID 19154757.
  19. ^ Nakamura T, Cieplak P, Cho DH, Godzik A, Lipton SA (August 2010). "S-nitrosylation of Drp1 links excessive mitochondrial fission to neuronal injury in neurodegeneration". Mitochondrion. 10 (5): 573–578. doi:10.1016/j.mito.2010.04.007. PMC 2918703. PMID 20447471.
  20. ^ a b Dutta R, Trapp BD (January 2011). "Mechanisms of neuronal dysfunction and degeneration in multiple sclerosis". Progress in Neurobiology. 93 (1): 1–12. doi:10.1016/j.pneurobio.2010.09.005. PMC 3030928. PMID 20946934.
  21. ^ Stavrovskaya IG, Kristal BS (March 2005). "The powerhouse takes control of the cell: is the mitochondrial permeability transition a viable therapeutic _target against neuronal dysfunction and death?". Free Radical Biology & Medicine. 38 (6): 687–697. doi:10.1016/j.freeradbiomed.2004.11.032. PMID 15721979.
  22. ^ Allen J, Romay-Tallon R, Brymer KJ, Caruncho HJ, Kalynchuk LE (2018). "Mitochondria and Mood: Mitochondrial Dysfunction as a Key Player in the Manifestation of Depression". Frontiers in Neuroscience. 12: 386. doi:10.3389/fnins.2018.00386. PMC 5997778. PMID 29928190.
  23. ^ Li S, Stys PK (2001). "Na(+)-K(+)-ATPase inhibition and depolarization induce glutamate release via reverse Na(+)-dependent transport in spinal cord white matter". Neuroscience. 107 (4): 675–683. doi:10.1016/s0306-4522(01)00385-2. PMID 11720790. S2CID 25693141.
  24. ^ Siegel, G J, Agranoff, BW, Albers RW, Fisher SK, Uhler MD, eds. (1999). "Glutamate". Basic Neurochemistry: Molecular, Cellular, and Medical Aspects (6th ed.). Philadelphia: Lippincott, Williams & Wilkins. p. 287. ISBN 9780080472072.
  25. ^ a b Hardingham GE, Fukunaga Y, Bading H (May 2002). "Extrasynaptic NMDARs oppose synaptic NMDARs by triggering CREB shut-off and cell death pathways". Nature Neuroscience. 5 (5): 405–414. doi:10.1038/nn835. PMID 11953750. S2CID 659716.
  26. ^ Hardingham GE, Bading H (October 2010). "Synaptic versus extrasynaptic NMDA receptor signalling: implications for neurodegenerative disorders". Nature Reviews. Neuroscience. 11 (10): 682–696. doi:10.1038/nrn2911. PMC 2948541. PMID 20842175.
  27. ^ Brand LE (2009). "Human exposure to cyanobacteria and BMAA". Amyotrophic Lateral Sclerosis. 10 (Suppl 2): 85–95. doi:10.3109/17482960903273585. PMID 19929739. S2CID 37986519.
  28. ^ Vyas KJ, Weiss JH (2009). "BMAA--an unusual cyanobacterial neurotoxin". Amyotrophic Lateral Sclerosis. 10 (Suppl 2): 50–55. doi:10.3109/17482960903268742. PMID 19929732. S2CID 22391321.
  29. ^ a b Chiu AS, Gehringer MM, Braidy N, Guillemin GJ, Welch JH, Neilan BA (November 2012). "Excitotoxic potential of the cyanotoxin β-methyl-amino-L-alanine (BMAA) in primary human neurons". Toxicon. 60 (6): 1159–1165. Bibcode:2012Txcn...60.1159C. doi:10.1016/j.toxicon.2012.07.169. PMID 22885173.
  30. ^ Papapetropoulos S (June 2007). "Is there a role for naturally occurring cyanobacterial toxins in neurodegeneration? The beta-N-methylamino-L-alanine (BMAA) paradigm". Neurochemistry International. 50 (7–8): 998–1003. doi:10.1016/j.neuint.2006.12.011. PMID 17296249. S2CID 24476846.
  31. ^ Team Nord (2007). Analysis, occurrence and toxicity of BMAA. Denmark: Nordic. pp. 46–47. ISBN 9789289315418.
  32. ^ Dunlop RA, Cox PA, Banack SA, Rodgers KJ (2013). "The non-protein amino acid BMAA is misincorporated into human proteins in place of L-serine causing protein misfolding and aggregation". PLOS ONE. 8 (9): e75376. Bibcode:2013PLoSO...875376D. doi:10.1371/journal.pone.0075376. PMC 3783393. PMID 24086518.
  33. ^ Holtcamp W (March 2012). "The emerging science of BMAA: do cyanobacteria contribute to neurodegenerative disease?". Environmental Health Perspectives. 120 (3): A110–A116. doi:10.1289/ehp.120-a110. PMC 3295368. PMID 22382274.
  34. ^ Cox PA, Davis DA, Mash DC, Metcalf JS, Banack SA (January 2016). "Dietary exposure to an environmental toxin triggers neurofibrillary tangles and amyloid deposits in the brain". Proceedings. Biological Sciences. 283 (1823): 20152397. doi:10.1098/rspb.2015.2397. PMC 4795023. PMID 26791617.

Further reading

edit
  NODES
HOME 1
Intern 1
languages 1
mac 4
Note 2
os 64