Literature DB >> 25267995

Renal sulfatides: sphingoid base-dependent localization and region-specific compensation of CerS2-dysfunction.

Christian Marsching1, Mariona Rabionet2, Daniel Mathow3, Richard Jennemann3, Christiane Kremser4, Stefan Porubsky5, Christian Bolenz6, Klaus Willecke4, Hermann-Josef Gröne7, Carsten Hopf8, Roger Sandhoff9.   

Abstract

Mammalian kidneys are rich in sulfatides. Papillary sulfatides, especially, contribute to renal adaptation to chronic metabolic acidosis. Due to differences in their cer-amide (Cer) anchors, the structural diversity of renal sulfatides is large. However, the underling biological function of this complexity is not understood. As a compound's function and its tissue location are intimately connected, we analyzed individual renal sulfatide distributions of control and Cer synthase 2 (CerS)2-deficient mice by imaging MS (IMS) and by LC-MS(2) (in controls for the cortex, medulla, and papillae separately). To explain locally different structures, we compared our lipid data with regional mRNA levels of corresponding anabolic enzymes. The combination of IMS and in source decay-LC-MS(2) analyses revealed exclusive expression of C20-sphingosine-containing sulfatides within the renal papillae, whereas conventional C18-sphingosine-containing compounds were predominant in the medulla, and sulfatides with a C18-phytosphingosine were restricted to special cortical structures. CerS2 deletion resulted in bulk loss of sulfatides with C23/C24-acyl chains, but did not lead to decreased urinary pH, as previously observed in sulfatide-depleted kidneys. The reasons may be the almost unchanged C22-sulfatide levels and constant total renal sulfatide levels due to compensation with C16- to C20-acyl chain-containing compounds. Intriguingly, CerS2-deficient kidneys were completely depleted of phytosphingosine-containing cortical sulfatides without any compensation.
Copyright © 2014 by the American Society for Biochemistry and Molecular Biology, Inc.

Entities:  

Keywords:  ceramide synthase 2; cortex; electrospray ionization-mass spectrometry; galactosylceramide I3-sulfate; imaging mass spectrometry; in source decay; knockout; lactosylceramide II3-sulfate; liquid chromatography; matrix-assisted laser desorption/ionization-time-of-flight; medulla; papillae; serine palmitoyl-coenzyme A transferase small subunits; sphingosine; tandem mass spectrometry

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Year:  2014        PMID: 25267995      PMCID: PMC4617137          DOI: 10.1194/jlr.M051839

Source DB:  PubMed          Journal:  J Lipid Res        ISSN: 0022-2275            Impact factor:   5.922


  50 in total

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