4.6 Article

Blood sphingolipidomics in healthy humans: impact of sample collection methodology

期刊

JOURNAL OF LIPID RESEARCH
卷 51, 期 10, 页码 3074-3087

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ELSEVIER
DOI: 10.1194/jlr.D008532

关键词

sphingolipid metabolome; sphingomyelin; ceramide; sphingosine

资金

  1. National Institutes of Health [HL-079274, R0-1HL079274-04S1]
  2. Southeastern Clinical and Translational Research Institute
  3. South Carolina Center of Biomedical Research Excellence (COBRE) in Lipidomics and Pathobiology
  4. National Center for Research Resources (NCCR) [P20 RR17677, CO6RR018823]
  5. Department of Veterans Affairs

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We used a HPLC-MS/MS methodology for determination of a basic metabolomic profile (18:1,18:0 sphingoid backbone, C-14-C-26 N-acyl part) of normal sphingolipid levels in human serum and plasma. Blood was collected from healthy males and nonpregnant females under fasting and nonfasting conditions with and without anticoagulants. Sphingolipids analyzed included sphingoid bases, sphingosine and dihydrosphingosine, their 1-phosphates (S1P and dhS1P), molecular species (C-n-) of ceramide (Cer), sphingomyelin (SM), hexosylceramide (HexCer), lactosylceramide (LacCer), and Cer 1-phosphate (Cer1P). SM, LacCer, HexCer, Cer, and Cer1P constituted 87.7, 5.8, 3.4, 2.8, and 0.15% of total sphingolipids, respectively. The abundant circulating SM was C-16-SM (64.0 mu M), and it increased with fasting (100 mu M). The abundant LacCer was C-16-LacCer (10.0 mu M) and the abundant HexCer was C-24-HexCer (2.5 mu M). The abundant Cer, C-24-Cer (4.0 mu M), was not influenced by fasting; however, levels of C-16-C-20 Cers were decreased in response to fasting. S1P levels were higher in serum than plasma (0.68 mu M vs. 0.32 mu M). We also determined levels of sphingoid bases and SM species in isolated lipoprotein classes. HDL3 was the major carrier of S1P, dhS1P, and Sph, and LDL was the major carrier of Cer and dhSph. Per particle, VLDL contained the highest levels of SM, Cer, and S1P. HPLC-MS/MS should provide a tool for clinical testing of circulating bioactive sphingolipids in human blood.-Hammad, S. M., J. S. Pierce, F. Soodavar, K. J. Smith, M. M. Al Gadban, B. Rembiesa, R. L. Klein, Y. A. Hannun, J. Bielawski, and A. Bielawska. Blood sphingolipidomics in healthy humans:impact of sample collection methodology. J. Lipid Res. 2010. 51: 3074-3087.

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