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Vitamin K-dependent carboxylation of the carboxylase
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Vitamin K-dependent (VKD) proteins require modification by the VKD-γ-glutamyl carboxylase, an enzyme that converts clusters of glus to glas in a reaction that requires vitamin K hydroquinone, for their activity. We have discovered that the carboxylase also carboxylates itself in a reaction dependent on vitamin K. When pure human recombinant carboxylase was incubated
in vitro
with
14
CO
2
and then analyzed after SDS/PAGE, a radiolabeled band corresponding to the size of the carboxylase was observed. Subsequent gla analysis of
in vitro
-modified carboxylase by base hydrolysis and HPLC showed that all of the radioactivity could be attributed to gla residues. Quantitation of gla, asp, and glu residues indicated 3 mol gla/mol carboxylase. Radiolabeled gla was acid-labile, confirming its identity, and was not observed if vitamin K was not included in the
in vitro
reaction. Carboxylase carboxylation also was detected in baculovirus(carboxylase)-infected insect cells but not in mock-infected insect cells, which do not express endogenous VKD proteins or carboxylase. Finally, we showed that the carboxylase was carboxylated
in vivo
. Carboxylase was purified from recombinant carboxylase BHK cells cultured in the presence or absence of vitamin K and analyzed for gla residues. Carboxylation of the carboxylase only was observed with carboxylase isolated from BHK cells cultured in vitamin K, and 3 mol gla/mol carboxylase were detected. Analyses of carboxylase and factor IX carboxylation
in vitro
suggest a possible role for carboxylase carboxylation in factor IX turnover, and
in vivo
studies suggest a potential role in carboxylase stability. The discovery of carboxylase carboxylation has broad implications for the mechanism of VKD protein carboxylation and Warfarin-based anti-coagulant therapies that need to be considered both retrospectively and in the future.
Proceedings of the National Academy of Sciences
Title: Vitamin K-dependent carboxylation of the carboxylase
Description:
Vitamin K-dependent (VKD) proteins require modification by the VKD-γ-glutamyl carboxylase, an enzyme that converts clusters of glus to glas in a reaction that requires vitamin K hydroquinone, for their activity.
We have discovered that the carboxylase also carboxylates itself in a reaction dependent on vitamin K.
When pure human recombinant carboxylase was incubated
in vitro
with
14
CO
2
and then analyzed after SDS/PAGE, a radiolabeled band corresponding to the size of the carboxylase was observed.
Subsequent gla analysis of
in vitro
-modified carboxylase by base hydrolysis and HPLC showed that all of the radioactivity could be attributed to gla residues.
Quantitation of gla, asp, and glu residues indicated 3 mol gla/mol carboxylase.
Radiolabeled gla was acid-labile, confirming its identity, and was not observed if vitamin K was not included in the
in vitro
reaction.
Carboxylase carboxylation also was detected in baculovirus(carboxylase)-infected insect cells but not in mock-infected insect cells, which do not express endogenous VKD proteins or carboxylase.
Finally, we showed that the carboxylase was carboxylated
in vivo
.
Carboxylase was purified from recombinant carboxylase BHK cells cultured in the presence or absence of vitamin K and analyzed for gla residues.
Carboxylation of the carboxylase only was observed with carboxylase isolated from BHK cells cultured in vitamin K, and 3 mol gla/mol carboxylase were detected.
Analyses of carboxylase and factor IX carboxylation
in vitro
suggest a possible role for carboxylase carboxylation in factor IX turnover, and
in vivo
studies suggest a potential role in carboxylase stability.
The discovery of carboxylase carboxylation has broad implications for the mechanism of VKD protein carboxylation and Warfarin-based anti-coagulant therapies that need to be considered both retrospectively and in the future.
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