Cleavage of an Amide Bond by a Ribozyme

13 January 1995

journal article
Published by American Association for the Advancement of Science (AAAS) in Science

Vol. 267 (5195) , 237-240
https://doi.org/10.1126/science.7809628

Abstract

A variant form of a group I ribozyme, optimized by in vitro evolution for its ability to catalyze magnesium-dependent phosphoester transfer reactions involving DNA substrates, also catalyzes the cleavage of an unactivated alkyl amide when that linkage is presented in the context of an oligodeoxynucleotide analog. Substrates containing an amide bond that joins either two DNA oligos, or a DNA oligo and a short peptide, are cleaved in a magnesium-dependent fashion to generate the expected products. The first-order rate constant, kcat, is 0.1 x 10(-5) min-1 to 1 x 10(-5) min-1 for the DNA-flanked substrates, which corresponds to a rate acceleration of more than 10(3) as compared with the uncatalyzed reaction.

Keywords

This publication has 33 references indexed in Scilit:

Inventing and improving ribozyme function: Rational design versus iterative selection methods
Trends in Biotechnology, 1994
In vitro selection of catalytic RNAs
Current Opinion in Structural Biology, 1994
RNA substrate binding site in the catalytic core of the Tetrahymena ribozyme
Nature, 1992
Unusual Resistance of Peptidyl Transferase to Protein Extraction Procedures
Science, 1992
Comparison of binding of mixed ribose-deoxyribose analogs of CUCU to a ribozyme and to GGAGAA by equilibrium dialysis: evidence for ribozyme specific interactions with 2'-hydroxy groups
Biochemistry, 1991
Drugs and the RNA world
Nature, 1991
DNA cleavage catalysed by the ribozyme from Tetrahymena
Nature, 1990
RNA evolution and the origins of life
Nature, 1989
Hydrolysis of a peptide bond in neutral water
Journal of the American Chemical Society, 1988
Studies on the Stability of Amides. I. Hydrolysis Mechanism of N-Substituted Aliphatic Amides
CHEMICAL & PHARMACEUTICAL BULLETIN, 1972