The branched-chain aminotransferase proteins: novel redox chaperones for protein disulfide isomerase--implications in Alzheimer's disease

The human branched-chain aminotransferase proteins (hBCATm and hBCATc) are regulated through oxidation and S-nitrosation. However, it remains unknown whether they share common redox characteristics to enzymes such as protein disulfide isomerase (PDI) in terms of regulating cellular repair and protei...

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Veröffentlicht in:	Antioxidants & redox signaling 2014-06, Vol.20 (16), p.2497-2513
Hauptverfasser:	El Hindy, Maya, Hezwani, Mohammed, Corry, David, Hull, Jonathon, El Amraoui, Farah, Harris, Matthew, Lee, Christopher, Forshaw, Thomas, Wilson, Andrew, Mansbridge, Abbe, Hassler, Martin, Patel, Vinood B, Kehoe, Patrick Gavin, Love, Seth, Conway, Myra Elizabeth
Format:	Artikel
Sprache:	eng
Schlagworte:	Alzheimer Disease - enzymology Alzheimer Disease - metabolism Alzheimer Disease - pathology Cell Line Humans Original Research Communications Oxidation-Reduction Oxidative Stress Protein Disulfide-Isomerases - metabolism Transaminases - metabolism
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container_title	Antioxidants & redox signaling
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creator	El Hindy, Maya Hezwani, Mohammed Corry, David Hull, Jonathon El Amraoui, Farah Harris, Matthew Lee, Christopher Forshaw, Thomas Wilson, Andrew Mansbridge, Abbe Hassler, Martin Patel, Vinood B Kehoe, Patrick Gavin Love, Seth Conway, Myra Elizabeth
description	The human branched-chain aminotransferase proteins (hBCATm and hBCATc) are regulated through oxidation and S-nitrosation. However, it remains unknown whether they share common redox characteristics to enzymes such as protein disulfide isomerase (PDI) in terms of regulating cellular repair and protein misfolding. Here, similar to PDI, the hBCAT proteins showed dithiol-disulfide isomerase activity that was mediated through an S-glutathionylated mechanism. Site-directed mutagenesis of the active thiols of the CXXC motif demonstrates that they are fundamental to optimal protein folding. Far Western analysis indicated that both hBCAT proteins can associate with PDI. Co-immunoprecipitation studies demonstrated that hBCATm directly binds to PDI in IMR-32 cells and the human brain. Electron and confocal microscopy validated the expression of PDI in mitochondria (using Mia40 as a mitochondrial control), where both PDI and Mia40 were found to be co-localized with hBCATm. Under conditions of oxidative stress, this interaction is decreased, suggesting that the proposed chaperone role for hBCATm may be perturbed. Moreover, immunohistochemistry studies show that PDI and hBCAT are expressed in the same neuronal and endothelial cells of the vasculature of the human brain, supporting a physiological role for this binding. This study identifies a novel redox role for hBCAT and confirms that hBCATm differentially binds to PDI under cellular stress. These studies indicate that hBCAT may play a role in the stress response of the cell as a novel redox chaperone, which, if compromised, may result in protein misfolding, creating aggregates as a key feature in neurodegenerative conditions such as Alzheimer's disease.
doi_str_mv	10.1089/ars.2012.4869
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Moreover, immunohistochemistry studies show that PDI and hBCAT are expressed in the same neuronal and endothelial cells of the vasculature of the human brain, supporting a physiological role for this binding. This study identifies a novel redox role for hBCAT and confirms that hBCATm differentially binds to PDI under cellular stress. 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However, it remains unknown whether they share common redox characteristics to enzymes such as protein disulfide isomerase (PDI) in terms of regulating cellular repair and protein misfolding. Here, similar to PDI, the hBCAT proteins showed dithiol-disulfide isomerase activity that was mediated through an S-glutathionylated mechanism. Site-directed mutagenesis of the active thiols of the CXXC motif demonstrates that they are fundamental to optimal protein folding. Far Western analysis indicated that both hBCAT proteins can associate with PDI. Co-immunoprecipitation studies demonstrated that hBCATm directly binds to PDI in IMR-32 cells and the human brain. Electron and confocal microscopy validated the expression of PDI in mitochondria (using Mia40 as a mitochondrial control), where both PDI and Mia40 were found to be co-localized with hBCATm. Under conditions of oxidative stress, this interaction is decreased, suggesting that the proposed chaperone role for hBCATm may be perturbed. Moreover, immunohistochemistry studies show that PDI and hBCAT are expressed in the same neuronal and endothelial cells of the vasculature of the human brain, supporting a physiological role for this binding. This study identifies a novel redox role for hBCAT and confirms that hBCATm differentially binds to PDI under cellular stress. These studies indicate that hBCAT may play a role in the stress response of the cell as a novel redox chaperone, which, if compromised, may result in protein misfolding, creating aggregates as a key feature in neurodegenerative conditions such as Alzheimer's disease.</description><subject>Alzheimer Disease - enzymology</subject><subject>Alzheimer Disease - metabolism</subject><subject>Alzheimer Disease - pathology</subject><subject>Cell Line</subject><subject>Humans</subject><subject>Original Research Communications</subject><subject>Oxidation-Reduction</subject><subject>Oxidative Stress</subject><subject>Protein Disulfide-Isomerases - metabolism</subject><subject>Transaminases - metabolism</subject><issn>1523-0864</issn><issn>1557-7716</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2014</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNpVkctu1jAQRi1ERW8s2SLvYOMf32InLJCqigJSpW7ateXYE2KU2MHOXwFv0LfGoRfRlS9z_HlGB6E3jO4YbbsPNpcdp4zvZKu6F-iINY0mWjP1cttzQWir5CE6LuUHpZQzRl-hQy5pJ6loj9Dd9Qi4zza6ETxxow0R2znEtNa7MkC2BfCS0wohlo84pluYcAaffuEKL5BThIKHlB8h7EPZT0PwgENJ878AQsK8TMHZNaRYcIXOpj8jhFp9V7YHUKFTdDDYqcDrh_UE3Vx8vj7_Si6vvnw7P7skTnK6EilBNpKClLzToHurXMuhV6IRgnvFG1mPlimr-4FxTQdte-W87QevhfJUnKBP97nLvp_BO4h11MksOcw2_zbJBvO8EsNovqdbIylXnIka8P4hIKefeyirmUNxME02QtoXw7RUbac5bSpK7lGXUykZhqdvGDWbPlP1mU2f2fRV_u3_vT3Rj77EXytkmt8</recordid><startdate>20140601</startdate><enddate>20140601</enddate><creator>El Hindy, Maya</creator><creator>Hezwani, Mohammed</creator><creator>Corry, David</creator><creator>Hull, Jonathon</creator><creator>El Amraoui, Farah</creator><creator>Harris, Matthew</creator><creator>Lee, Christopher</creator><creator>Forshaw, Thomas</creator><creator>Wilson, Andrew</creator><creator>Mansbridge, Abbe</creator><creator>Hassler, Martin</creator><creator>Patel, Vinood B</creator><creator>Kehoe, Patrick Gavin</creator><creator>Love, Seth</creator><creator>Conway, Myra Elizabeth</creator><general>Mary Ann Liebert, Inc</general><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>AAYXX</scope><scope>CITATION</scope><scope>7TK</scope><scope>5PM</scope></search><sort><creationdate>20140601</creationdate><title>The branched-chain aminotransferase proteins: novel redox chaperones for protein disulfide isomerase--implications in Alzheimer's disease</title><author>El Hindy, Maya ; 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However, it remains unknown whether they share common redox characteristics to enzymes such as protein disulfide isomerase (PDI) in terms of regulating cellular repair and protein misfolding. Here, similar to PDI, the hBCAT proteins showed dithiol-disulfide isomerase activity that was mediated through an S-glutathionylated mechanism. Site-directed mutagenesis of the active thiols of the CXXC motif demonstrates that they are fundamental to optimal protein folding. Far Western analysis indicated that both hBCAT proteins can associate with PDI. Co-immunoprecipitation studies demonstrated that hBCATm directly binds to PDI in IMR-32 cells and the human brain. Electron and confocal microscopy validated the expression of PDI in mitochondria (using Mia40 as a mitochondrial control), where both PDI and Mia40 were found to be co-localized with hBCATm. Under conditions of oxidative stress, this interaction is decreased, suggesting that the proposed chaperone role for hBCATm may be perturbed. Moreover, immunohistochemistry studies show that PDI and hBCAT are expressed in the same neuronal and endothelial cells of the vasculature of the human brain, supporting a physiological role for this binding. This study identifies a novel redox role for hBCAT and confirms that hBCATm differentially binds to PDI under cellular stress. These studies indicate that hBCAT may play a role in the stress response of the cell as a novel redox chaperone, which, if compromised, may result in protein misfolding, creating aggregates as a key feature in neurodegenerative conditions such as Alzheimer's disease.</abstract><cop>United States</cop><pub>Mary Ann Liebert, Inc</pub><pmid>24094038</pmid><doi>10.1089/ars.2012.4869</doi><tpages>17</tpages><oa>free_for_read</oa></addata></record>
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subjects	Alzheimer Disease - enzymology Alzheimer Disease - metabolism Alzheimer Disease - pathology Cell Line Humans Original Research Communications Oxidation-Reduction Oxidative Stress Protein Disulfide-Isomerases - metabolism Transaminases - metabolism
title	The branched-chain aminotransferase proteins: novel redox chaperones for protein disulfide isomerase--implications in Alzheimer's disease
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