Metabolism - Clinical and Experimental
Volume 59, Issue 8 , Pages 1106-1114, August 2010

Adipose tissue lamin A/C messenger RNA expression in women

  • Mélanie Nadeau

      Affiliations

    • Molecular Endocrinology and Genomics Center, Laval University Medical Research Center, Quebec City, Quebec, Canada G1V 4G2
  • ,
  • Suzanne Noël

      Affiliations

    • Gynecology Unit, Laval University Medical Research Center, Quebec City, Quebec, Canada G1V 4G2
  • ,
  • Philippe Y. Laberge

      Affiliations

    • Gynecology Unit, Laval University Medical Research Center, Quebec City, Quebec, Canada G1V 4G2
  • ,
  • Johanne Hurtubise

      Affiliations

    • Gynecology Unit, Laval University Medical Research Center, Quebec City, Quebec, Canada G1V 4G2
  • ,
  • André Tchernof

      Affiliations

    • Molecular Endocrinology and Genomics Center, Laval University Medical Research Center, Quebec City, Quebec, Canada G1V 4G2
    • Department of Nutrition, Laval University, Quebec City, Quebec, Canada G1V 0A6
    • Corresponding Author InformationCorresponding author. Endocrinology and Genomics and Department of Nutrition, Laval University Medical Research Center, and Laval University, Québec City, Québec, Canada G1V 4G2. Tel.: +1 418 654 2296; fax: +1 418 654 2761.

Received 28 April 2008; accepted 9 September 2009. published online 04 January 2010.

Abstract 

Mutations in the lamin A/C gene (LMNA) cause lipodystrophy. However, little data are available on lamin A/C expression in various fat depots in women. We recruited 34 women scheduled for gynecologic surgery. Blood samples were collected on the morning of surgery to obtain a detailed lipid profile. Radiological examinations were performed to measure total body fat mass and abdominal fat accumulation. Fat samples were taken from the subcutaneous (SC) fat depot and from the greater omentum (OM) during the surgical procedure. Whole adipose tissue samples were used for total messenger RNA (mRNA) extraction and real-time polymerase chain reaction quantification of the LMNA transcript. No association was observed between lamin A/C mRNA expression, either in SC or OM fat tissue, and adiposity measures. Women with low SC lamin A/C expression, identified on the basis of the median value of SC lamin A/C mRNA expression, had a significantly altered lipid profile including lower levels of high-density lipoprotein (HDL) cholesterol and HDL2 cholesterol and reduced HDL2 cholesterol to HDL3 cholesterol ratio (P < .05 for all). These women were also characterized by higher cholesterol to HDL cholesterol, low-density lipoprotein–triglycerides, very low-density lipoprotein–apolipoprotein B, and low-density lipoprotein cholesterol to HDL cholesterol (P < .05 for all). Low SC lamin A/C mRNA expression levels were also associated with significantly increased lipolysis in isolated fat cells from this fat depot. Specifically, the response to lipolytic agent isoproterenol was significantly increased at doses ranging from 10−5 to 10−10 mol/L (P < .05). A similar trend was observed in OM fat cells but did not reach significance. In conclusion, low lamin A/C expression in SC adipose tissue is associated with significant alterations in the lipid profile and increased fat cell lipolysis, independent of the level of total or abdominal adiposity.

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PII: S0026-0495(09)00477-6

doi:10.1016/j.metabol.2009.09.034

Metabolism - Clinical and Experimental
Volume 59, Issue 8 , Pages 1106-1114, August 2010