A mild and quantitative procedure for the removal of nucleoside alkoxycarbonyl groups using pig liver esterase or Candida antarctica B lipase

A set of eight mono-, di-, tri- and tetraalkoxycarbonylated nucleosides was tested in order to assess their enzymatic hydrolysis. All the alkoxycarbonyl groups of the assayed substrates, from both carbonate and carbamate functions, were quantitatively hydrolysed using pig liver esterase (PLE) at pH...

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Bibliographic Details
Main Authors: Capello, M., González, M., Rodríguez, S.D., Iglesias, L.E., Iribarren, A.M.
Format: Journal/Newspaper
Language:unknown
Subjects:
Carbamates
Carbonates
Deprotection
Hydrolases
Nucleosides
Enzymes
Hydrolysis
Substrates
Synthesis (chemical)
carbamic acid
carbonic acid
carbonyl derivative
esterase
liver enzyme
nucleoside derivative
triacylglycerol lipase
article
Candida antarctica
carbonylation
catalyst
controlled study
hydrolysis kinetics
nonhuman
pH measurement
quantitative analysis
temperature dependence
Sus scrofa
Antarc*
Antarctica
Carbonic acid
Online Access:https://hdl.handle.net/20.500.12110/paper_13811177_v36_n1-6_p36_Capello
Description
Summary:A set of eight mono-, di-, tri- and tetraalkoxycarbonylated nucleosides was tested in order to assess their enzymatic hydrolysis. All the alkoxycarbonyl groups of the assayed substrates, from both carbonate and carbamate functions, were quantitatively hydrolysed using pig liver esterase (PLE) at pH 7 and 60°C, regardless of the nucleoside base. Quantitative full alkoxycarbonyl groups removal was also reached by Candida antarctica B lipase (CAL B) under mild conditions, but in this case, longer reaction times were required. Thus, PLE appears as an useful catalyst for the mild and quantitative deprotection of nucleoside carbonates and carbamates in the synthesis of modified nucleosides. © 2005 Elsevier B.V. All rights reserved.

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