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dc.contributor.author Fülöp László
dc.contributor.author Rajki Anikó
dc.contributor.author Katona Dávid
dc.contributor.author Szanda Gergő
dc.contributor.author Spät András
dc.date.accessioned 2017-01-20T11:12:33Z
dc.date.available 2017-01-20T11:12:33Z
dc.date.issued 2013
dc.identifier 84882741152
dc.identifier.citation pagination=70-79; journalVolume=381; journalIssueNumber=1-2; journalTitle=MOLECULAR AND CELLULAR ENDOCRINOLOGY;
dc.identifier.uri http://repo.lib.semmelweis.hu//handle/123456789/2629
dc.identifier.uri doi:10.1016/j.mce.2013.07.021
dc.description.abstract We have previously described that silencing of the mitochondrial protein OPA1 enhances mitochondrial Ca2+ signaling and aldosterone production in H295R adrenocortical cells. Since extramitochondrial OPA1 (emOPA1) was reported to facilitate cAMP-induced lipolysis, we hypothesized that emOPA1, via the enhanced hydrolysis of cholesterol esters, augments aldosterone production in H295R cells. A few OPA1 immunopositive spots were detected in approximately 40% of the cells. In cell fractionation studies OPA1/COX IV (mitochondrial marker) ratio in the post-mitochondrial fractions was an order of magnitude higher than that in the mitochondrial fraction. The ratio of long to short OPA1 isoforms was lower in post-mitochondrial than in mitochondrial fractions. Knockdown of OPA1 failed to reduce db-cAMP-induced phosphorylation of hormone-sensitive lipase (HSL), Ca2+ signaling and aldosterone secretion. In conclusion, OPA1 could be detected in the post-mitochondrial fractions, nevertheless, OPA1 did not interfere with the cAMP - PKA - HSL mediated activation of aldosterone secretion.
dc.relation.ispartof urn:issn:0303-7207
dc.title Extramitochondrial OPA1 and adrenocortical function.
dc.type Journal Article
dc.date.updated 2015-11-24T10:44:51Z
dc.language.rfc3066 en
dc.identifier.mtmt 2402208
dc.identifier.wos 000327568200009
dc.identifier.pubmed 23906536
dc.contributor.department SE/AOK/I/Élettani Intézet
dc.contributor.institution Semmelweis Egyetem


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