Effect of fumonisin B1 on phosphatidylethanolamine biosynthesis in Chinese hamster ovary cells

Ketan Badiani, David M. Byers, Harold W. Cook, Neale D. Ridgway

Producción científica: Contribución a una revistaArtículorevisión exhaustiva

17 Citas (Scopus)

Resumen

Fumonisin B1 has been shown to inhibit dihydroceramide synthesis and elevate cellular sphinganine levels in several cultured cell lines. In Chinese hamster ovary (CHO)-K1 cells, 20 μM fumonisin B1 inhibited sphingomyelin synthesis by 75% after 5 h, but stimulated [3H]serine incorporation into PtdEtn by 5- to 7-fold. Fumonisin caused a 10-20% increase in [3H]serine labelling of PtdSer. While fumonisin (20 μM) caused sustained inhibition of sphingomyelin synthesis, PtdEtn labelling peaked at 7-fold above controls at 12 h and declined to 4-fold by 24 h. Fumonisin treatment for 12 h increased the in vitro activity of PtdSer synthase by 62% and inhibited PtdSer decarboxylase by 35%, suggesting that increased PtdEtn labelling by [3H]serine is not by this pathway. An ethanolamine 'trap' experiment was performed to assess the contribution of phosphoethanolamine from sphinganine degradation for PtdEtn labelling. Stimulation of [3H]serine incorporation into PtdEtn by fumonisin could be reduced by 60% with the inclusion of 50 μM unlabelled ethanolamine in the culture medium. The ethanolamine-mediated reduction in [3H]serine incorporation into PtdEtn was accompanied by 4-fold increase in cellular [3H]phosphoethanolamine. In control cells labelled with [3H]serine, 50 μM ethanolamine did not cause [3H]phosphoethanolamine to accumulate. Consistent with elevated phosphoethanolamine production in fumonisin-treated cells, [3H]ethanolamine incorporation into PtdEtn was inhibited by 75% after 12 h. The degradation of endogenous long-chain bases to phosphoethanolamine and entry into the CDP-ethanolamine pathway appears to be a major pathway for PtdEtn synthesis in fumonisin-treated CHO-K1 cells.

Idioma originalEnglish
Páginas (desde-hasta)190-196
Número de páginas7
PublicaciónBiochimica et Biophysica Acta - Lipids and Lipid Metabolism
Volumen1304
N.º3
DOI
EstadoPublished - dic. 13 1996

Nota bibliográfica

Funding Information:
Thanks to Robert Zwicker and Gladys Keddy for their assistancew ith cell culture. This work was supported by a program granftr om the Medical Research Council of Canada (PG-11476) and a Scholarship to N.D.R.K.B. is a Heart and Stroke Foundationo f CanadaR esearchF ellow.

ASJC Scopus Subject Areas

  • Biophysics
  • Biochemistry
  • Endocrinology

PubMed: MeSH publication types

  • Journal Article
  • Research Support, Non-U.S. Gov't

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