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dc.contributor.authorTan, Paul
dc.contributor.authorPepin, Émilie
dc.contributor.authorLavoie, Julie
dc.date.accessioned2022-10-31T12:51:25Z
dc.date.availableNO_RESTRICTIONfr
dc.date.available2022-10-31T12:51:25Z
dc.date.issued2018-01-31
dc.identifier.urihttp://hdl.handle.net/1866/26995
dc.publisherMyJove Corporationfr
dc.titleMouse adipose tissue collection and processing for RNA analysisfr
dc.typeArticlefr
dc.contributor.affiliationUniversité de Montréal. Faculté de médecine. École de kinésiologie et des sciences de l'activité physiquefr
dc.contributor.affiliationAutrefr
dc.identifier.doi10.3791/57026
dcterms.abstractCompared to other tissues, white adipose tissue has a considerably less RNA and protein content for downstream applications such as real-time PCR and Western Blot, since it mostly contains lipids. RNA isolation from adipose tissue samples is also challenging as extra steps are required to avoid these lipids. Here, we present a procedure to collect three anatomically different white adipose tissues from mice, to process these samples and perform RNA isolation. We further describe the synthesis of cDNA and gene expression experiments using real-time PCR. The hereby described protocol allows the reduction of contamination from the animal's hair and blood on fat pads as well as cross-contamination between different fat pads during tissue collection. It has also been optimized to ensure adequate quantity and quality of the RNA extracted. This protocol can be widely applied to any mouse model where adipose tissue samples are required for routine experiments such as real-time PCR but is not intended for isolation from primary adipocytes cell culture.fr
dcterms.isPartOfurn:ISSN:1940-087Xfr
dcterms.languageengfr
UdeM.ReferenceFournieParDeposanthttps://doi.org/10.3791/57026fr
UdeM.VersionRioxxVersion publiée / Version of Recordfr
oaire.citationTitleJournal of visualized experimentsfr
oaire.citationIssue131fr


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