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AbstractAbstract
[en] Unsealed inside-out and right-side out vesicles were prepared from human red cells. The vesicles were incubated with D-glucose [14C(U)] and sodium cyanoborohydride in phosphate buffer, pH 7.4. After incubation, lipids were extracted with 1-butanol and non-lipid contaminants removed by Sephadex G-25 chromatography. Phosphatidylethanolamine-sorbitol was purified by chromatography on columns of silicic acid and phenylboronate agarose gel. Phospholipase C (B. cereus) liberated phosphoethanolamine-sorbitol (I) which comigrated on TLC with synthetic I prepared by reductive condensation of phosphoethanolamine and D-glucose and also with the product of phospholipase C (B. cereus) hydrolysis of reference phosphatidylethanolamine-sorbitol. Exposure of I to alkaline phosphatase (E. coli) gave P/sub i/ and ethanolamine-sorbitol (II) which comigrated on TLC with synthetic II prepared by reductive condensation of ethanolamine and D-glucose or by phospholipase D hydrolysis of reference phosphatidylethanolamine-sorbitol. These studies demonstrate that vesicular phosphatidylethanolamine can be reductively glycated and illustrate the applicability of both phospholipase C and phospholipase D in characterizing glycated phosphoglycerides
Primary Subject
Source
76. annual meeting of the Federation of American Society for Experimental Biology; Washington, DC (USA); 8-12 Jun 1986; CONF-8606151--
Record Type
Journal Article
Literature Type
Conference
Journal
Federation Proceedings. Federation of American Societies for Experimental Biology; ISSN 0014-9446;
; CODEN FEPRA; v. 45(6); p. 1838

Country of publication
ALDEHYDES, ANIMALS, BIOLOGICAL MATERIALS, BLOOD, BLOOD CELLS, BODY FLUIDS, CARBOHYDRATES, CARBON COMPOUNDS, CARBOXYLESTERASES, ENZYMES, ESTERASES, ESTERS, HEXOSES, HYDROLASES, ISOTOPE APPLICATIONS, LIPIDS, MAMMALS, MATERIALS, MONOSACCHARIDES, ORGANIC COMPOUNDS, ORGANIC PHOSPHORUS COMPOUNDS, PHOSPHATASES, PRIMATES, SACCHARIDES, SEPARATION PROCESSES, VERTEBRATES
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