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J. Biol. Chem., Vol. 259, Issue 17, 10764-10770, 09, 1984
WA Dunn, G Rettura, E Seifter and S Englard
The production of carnitine from peptide-bound 6-N-trimethyl-L-lysine
(Lys(Me3)) or 4-N-trimethyl-aminobutyrate(gamma-butyrobetaine) perfused
through isolated guinea pig livers was investigated. [Methyl-3H]
Lys(Me3)-labeled agalacto-orosomucoid (AGOR) and asialofetuin were rapidly
taken up and degraded by the perfused liver. Most of the free Lys(Me3)
derived from Lys(Me3)-AGOR was released unmodified into the perfusion
medium. However, Lys(Me3), arising from Lys(Me3)-asialofetuin was converted
mostly to gamma-butyrobetaine and carnitine. gamma- Butyrobetaine added to
the perfusion medium was hydroxylated to carnitine by the liver at a rate
of 2.3 mumol/h. Guinea pigs maintained on an ascorbate-free diet for 17-60
days showed lowered ascorbate contents in all tissues measured and,
coincidentally, a sharp reduction in carnitine levels in kidney, liver, and
cardiac, and skeletal muscle. Carnitine production from
[1,2,3,4-14C]gamma-butyrobetaine and [methyl- 3H]Lys(Me3)-asialofetuin was
reduced in perfused livers obtained from ascorbate-deficient guinea pigs.
Although hydroxylation of gamma- butyrobetaine to carnitine was effectively
depressed in the perfused isolated livers from ascorbate-deficient animals,
hydroxylation of [methyl-3H]Lys(Me3) (derived from asialofetuin) to
[methyl-3H]3-hydroxy- 6-N-trimethyl-L-lysine was unaffected. Prior
administration of ascorbate to the medium perfusing the isolated livers
caused carnitine biosynthesis from all precursors examined to return to
control values.
Carnitine biosynthesis from gamma-butyrobetaine and from exogenous protein-bound 6-N-trimethyl-L-lysine by the perfused guinea pig liver. Effect of ascorbate deficiency on the in situ activity of gamma- butyrobetaine hydroxylase
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