Abstract
In this study it could be shown that in rat the normally occurring N-acetyl neuraminic acid can be modified in its N-acyl moiety by in vivo administration of the chemically synthesized N-propanoyl precursors, N-propanoyl-D-glucosamine or N-propanoyl-D-mannosamine. It could be shown that each of these nonphysiological amino sugar analogues was incorporated into both membrane and serum glycoproteins. After treatment of rats with radiolabeled N-[acyl-1-14C]D-mannosamine, radioactivity could be removed from serum glycoprotein fractions by incubation with neuraminidase from Clostridium perfringens or from Arthrobacter ureafaciens. Mild acid hydrolysis removed 98% of the radioactivity after in vivo labeling with N-[acetyl-1-14C]D-mannosamine and 86% after labeling with N-[propanoyl-1-14C]D-mannosamine. Chromatographic analysis yielded two compounds, i.e. N-acetyl neuraminic acid and N-propanoyl neuraminic acid, the latter being identified by gas liquid chromatography/mass spectrometry studies. Measurement of protein-bound radioactivity in different rat organs revealed a different organotropy of the natural and the nonphysiological neuraminic acid precursor. Of the glucosamine derivatives, N-acetyl-D-glucosamine showed the higher rate of uptake and incorporation in most organs (except in the submandibulary gland), and especially in kidney cortex and Morris hepatoma 7777. Natural and the unphysiological mannosamine derivatives were incorporated at similar rates, except in liver, where N-acetyl-D-mannosamine was taken up and metabolized more effectively. This finding indicates that it is possible to modify the acyl group of N-acetyl neuraminic acid in vivo by the introduction of an N-propanoyl group and possibly other homologous N-acyl groups. This procedure may provide a tool for a further characterization of the biological function of sialic acids.
Highlights
RESULTSDifferent Rat Organs-After labeling rats with N-[acetyl-114C]D-glucosamine, N-[a~etyl-l-'~C]mannosarnineN,-[proparation were found in kidney (4.2 X lo3cpm/mg protein) and Morris hepatoma 7777 (5.0 X lo3cpm/mg protein)
Glycoprotein fractions by incubation with neuramini- inhibition of terminal glycosylation or metabolic replacement dase from Clostridium perfringens or from Arthroobfatch-e physiological terminal sugar by a modified sugar anater ureafaciens
This finding indicatesthat itis pos- Chemicals and solutes were of analytical grade and were obtained sible tomodify the acyl groupof N-acetyl neuraminic acid in vivo by the introduction of a n N-propanoyl group and possibly other homologous N-acyl groups
Summary
Different Rat Organs-After labeling rats with N-[acetyl-114C]D-glucosamine, N-[a~etyl-l-'~C]mannosarnineN,-[proparation were found in kidney (4.2 X lo3cpm/mg protein) and Morris hepatoma 7777 (5.0 X lo3cpm/mg protein). No incorn~y~-~-'~C]D-glucosarnionre,N-[pr~panoyl-l-'~C]D-mannop-oration into membrane glycoproteins could be detected in samine, radioactivity was found in liver, kidney, lung, brain, submandibulary gland, andMorrishepatoma 7777 inthe range of 1 x 10' cpm/g to 1 x lo cpm/g (Fig. 1).In kidney and Morris hepatoma 7777, especially high radioactivity was detected after labeling with N-[a~etyl-l-'~C]D-glucosarni(n4e X lo cpm/g). Surprisingly,we found a low incorporation of N-[propanoyll-'4C]D-glucosamine into kidney membrane glycoproteins, relatively high amounts of radioactivity were taken up by this organ. This may be due to renal secretion of the applied radioactivity.
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