Concentration-Dependent Dual Role of Thrombin in Protection of Cultured Rat Cortical Neurons

Thrombin’s role in the nervous system is not well understood. Under conditions of blood–brain barrier compromise (e.g., neurosurgery or stroke), thrombin can result in neuroapoptosis and the formation of glial scars. Despite this, preconditioning with thrombin has been found to be neuroprotective in...

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Published in:Neurochemical research Vol. 40; no. 11; pp. 2220 - 2229
Main Authors: García, Paul S., Ciavatta, Vincent T., Fidler, Jonathan A., Woodbury, Anna, Levy, Jerrold H., Tyor, William R.
Format: Journal Article
Language:English
Published: New York Springer US 01-11-2015
Springer Nature B.V
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Abstract Thrombin’s role in the nervous system is not well understood. Under conditions of blood–brain barrier compromise (e.g., neurosurgery or stroke), thrombin can result in neuroapoptosis and the formation of glial scars. Despite this, preconditioning with thrombin has been found to be neuroprotective in models of cerebral ischemia and intracerebral hemorrhage. We investigated the effects of physiologically relevant concentrations of thrombin on cortical neurons using two culture-based assays. We examined thrombin’s effect on neurites by quantitative analysis of fluorescently labeled neurons. To characterize thrombin’s effects on neuron survival, we spectrophotometrically measured changes in enzymatic activity. Using receptor agonists and thrombin inhibitors, we separately examined the role of thrombin and its receptor in neuroprotection. We found that low concentrations of thrombin (1 nM) enhances neurite growth and branching, neuron viability, and protects against excitotoxic damage. In contrast, higher concentrations of thrombin (100 nM) are potentially detrimental to neuronal health as evidenced by inhibition of neurite growth. Lower concentrations of thrombin resulted in equivalent neuroprotection as the antifibrinolytic, aprotinin, and the direct thrombin inhibitor, argatroban. Interestingly, exogenous application of the species-specific thrombin inhibitor, antithrombin III, was detrimental to neuronal health; suggesting that some endogenous thrombin is necessary for optimal neuron health in our culture system. Activation of the thrombin receptor, protease-activated receptor-1 (PAR-1), via micromolar concentrations of the thrombin receptor agonist peptide, TRAP, did not adversely affect neuronal viability. An optimal concentration of thrombin exists to enhance neuronal health. Neurotoxic effects of thrombin do not involve activation of PAR receptors and thus separate pharmacologic manipulation of thrombin’s receptor in the setting of direct thrombin inhibitors could be a potential neuroprotective strategy.
AbstractList Thrombin's role in the nervous system is not well understood. Under conditions of blood-brain barrier compromise (e.g., neurosurgery or stroke), thrombin can result in neuroapoptosis and the formation of glial scars. Despite this, preconditioning with thrombin has been found to be neuroprotective in models of cerebral ischemia and intracerebral hemorrhage. We investigated the effects of physiologically relevant concentrations of thrombin on cortical neurons using two culture-based assays. We examined thrombin's effect on neurites by quantitative analysis of fluorescently labeled neurons. To characterize thrombin's effects on neuron survival, we spectrophotometrically measured changes in enzymatic activity. Using receptor agonists and thrombin inhibitors, we separately examined the role of thrombin and its receptor in neuroprotection. We found that low concentrations of thrombin (1 nM) enhances neurite growth and branching, neuron viability, and protects against excitotoxic damage. In contrast, higher concentrations of thrombin (100 nM) are potentially detrimental to neuronal health as evidenced by inhibition of neurite growth. Lower concentrations of thrombin resulted in equivalent neuroprotection as the antifibrinolytic, aprotinin, and the direct thrombin inhibitor, argatroban. Interestingly, exogenous application of the species-specific thrombin inhibitor, antithrombin III, was detrimental to neuronal health; suggesting that some endogenous thrombin is necessary for optimal neuron health in our culture system. Activation of the thrombin receptor, protease-activated receptor-1 (PAR-1), via micromolar concentrations of the thrombin receptor agonist peptide, TRAP, did not adversely affect neuronal viability. An optimal concentration of thrombin exists to enhance neuronal health. Neurotoxic effects of thrombin do not involve activation of PAR receptors and thus separate pharmacologic manipulation of thrombin's receptor in the setting of direct thrombin inhibitors could be a potential neuroprotective strategy.
Thrombin’s role in the nervous system is not well understood. Under conditions of blood–brain barrier compromise (e.g., neurosurgery or stroke), thrombin can result in neuroapoptosis and the formation of glial scars. Despite this, preconditioning with thrombin has been found to be neuroprotective in models of cerebral ischemia and intracerebral hemorrhage. We investigated the effects of physiologically relevant concentrations of thrombin on cortical neurons using two culture-based assays. We examined thrombin’s effect on neurites by quantitative analysis of fluorescently labeled neurons. To characterize thrombin’s effects on neuron survival, we spectrophotometrically measured changes in enzymatic activity. Using receptor agonists and thrombin inhibitors, we separately examined the role of thrombin and its receptor in neuroprotection. We found that low concentrations of thrombin (1 nM) enhances neurite growth and branching, neuron viability, and protects against excitotoxic damage. In contrast, higher concentrations of thrombin (100 nM) are potentially detrimental to neuronal health as evidenced by inhibition of neurite growth. Lower concentrations of thrombin resulted in equivalent neuroprotection as the antifibrinolytic, aprotinin, and the direct thrombin inhibitor, argatroban. Interestingly, exogenous application of the species-specific thrombin inhibitor, antithrombin III, was detrimental to neuronal health; suggesting that some endogenous thrombin is necessary for optimal neuron health in our culture system. Activation of the thrombin receptor, protease-activated receptor-1 (PAR-1), via micromolar concentrations of the thrombin receptor agonist peptide, TRAP, did not adversely affect neuronal viability. An optimal concentration of thrombin exists to enhance neuronal health. Neurotoxic effects of thrombin do not involve activation of PAR receptors and thus separate pharmacologic manipulation of thrombin’s receptor in the setting of direct thrombin inhibitors could be a potential neuroprotective strategy.
Author García, Paul S.
Fidler, Jonathan A.
Woodbury, Anna
Tyor, William R.
Levy, Jerrold H.
Ciavatta, Vincent T.
AuthorAffiliation Graduate Student, Department of Neurology, Emory University School of Medicine
Medical Student, Cardiothoracic ICU, Deparment of Anesthesiology, Duke University
Professor, Department of Neurology, Emory University School of Medicine, Research Division, Atlanta VA Medical Center, Atlanta, Georgia
Research Specialist, Cardiothoracic ICU, Deparment of Anesthesiology, Duke University
Assistant Professor, Department of Anesthesiology, Emory University School of Medicine, Research Division, Atlanta VA Medical Center, Atlanta, Georgia
Professor of Anesthesiology, Co-Director, Cardiothoracic ICU, Deparment of Anesthesiology, Duke University
AuthorAffiliation_xml – name: Research Specialist, Cardiothoracic ICU, Deparment of Anesthesiology, Duke University
– name: Graduate Student, Department of Neurology, Emory University School of Medicine
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– name: Professor of Anesthesiology, Co-Director, Cardiothoracic ICU, Deparment of Anesthesiology, Duke University
– name: Assistant Professor, Department of Anesthesiology, Emory University School of Medicine, Research Division, Atlanta VA Medical Center, Atlanta, Georgia
– name: Medical Student, Cardiothoracic ICU, Deparment of Anesthesiology, Duke University
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  givenname: William R.
  surname: Tyor
  fullname: Tyor, William R.
  organization: Research Division, Atlanta VA Medical Center, Department of Neurology, Emory University School of Medicine
BackLink https://www.ncbi.nlm.nih.gov/pubmed/26342829$$D View this record in MEDLINE/PubMed
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Snippet Thrombin’s role in the nervous system is not well understood. Under conditions of blood–brain barrier compromise (e.g., neurosurgery or stroke), thrombin can...
Thrombin's role in the nervous system is not well understood. Under conditions of blood-brain barrier compromise (e.g., neurosurgery or stroke), thrombin can...
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springer
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Publisher
StartPage 2220
SubjectTerms Animals
Antithrombin III - pharmacology
Aprotinin - pharmacology
Biochemistry
Biomedical and Life Sciences
Biomedicine
Cell Biology
Cell Survival - drug effects
Cells, Cultured
Cerebral Cortex - cytology
Cerebral Cortex - drug effects
Neurites - drug effects
Neurochemistry
Neurology
Neurons - drug effects
Neuroprotective Agents - pharmacology
Neurosciences
Original Paper
Peptide Fragments - pharmacology
Pipecolic Acids - pharmacology
Rats
Rats, Sprague-Dawley
Receptor, PAR-1 - agonists
Receptors, Thrombin - drug effects
Thrombin - antagonists & inhibitors
Thrombin - pharmacology
Title Concentration-Dependent Dual Role of Thrombin in Protection of Cultured Rat Cortical Neurons
URI https://link.springer.com/article/10.1007/s11064-015-1711-1
https://www.ncbi.nlm.nih.gov/pubmed/26342829
https://www.proquest.com/docview/1732536560
https://search.proquest.com/docview/1733188753
https://search.proquest.com/docview/1751217030
https://pubmed.ncbi.nlm.nih.gov/PMC4644093
Volume 40
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