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The structure and catalytic mechanism of new cellular and viral HDV ribozymes
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ABSTRACT
We have determined the molecular structure and investigated the catalytic mechanism of two new ribozymes of the Hepatitis delta virus family, found in the nematode
Caenorhabditis briggsae
and virus
Ackermannviridae
. Crystal structures of both conform to the double-pseudoknot architecture adopted by the viral HDV ribozyme. The
C. briggsae
ribozyme has been determined both pre- and post-cleavage. In the former both nucleotides flanking the scissile phosphate are observed, along with a metal ion, and cytosine 75 N3 bound to the O5’ leaving group. The pH dependence of cleavage rate reveals a p
K
a
of 6.6 and together with the inactivity of a C75U mutant provides evidence for its role as general acid. In contrast to other nucleolytic ribozymes that use catalytic metal ions, reaction rate does not depend on the p
K
a
of the divalent metal ion. Limited adjustment of structure of the active center is consistent with direct bonding of the metal ion to the O2’ and non-bridging O, suggesting that the ion acts as a Lewis acid to activate nucleophilic attack. This mechanism appears to be general for the HDV ribozyme class, and distinguishes it from the majority of nucleolytic ribozymes that use general base catalysis.
Title: The structure and catalytic mechanism of new cellular and viral HDV ribozymes
Description:
ABSTRACT
We have determined the molecular structure and investigated the catalytic mechanism of two new ribozymes of the Hepatitis delta virus family, found in the nematode
Caenorhabditis briggsae
and virus
Ackermannviridae
.
Crystal structures of both conform to the double-pseudoknot architecture adopted by the viral HDV ribozyme.
The
C.
briggsae
ribozyme has been determined both pre- and post-cleavage.
In the former both nucleotides flanking the scissile phosphate are observed, along with a metal ion, and cytosine 75 N3 bound to the O5’ leaving group.
The pH dependence of cleavage rate reveals a p
K
a
of 6.
6 and together with the inactivity of a C75U mutant provides evidence for its role as general acid.
In contrast to other nucleolytic ribozymes that use catalytic metal ions, reaction rate does not depend on the p
K
a
of the divalent metal ion.
Limited adjustment of structure of the active center is consistent with direct bonding of the metal ion to the O2’ and non-bridging O, suggesting that the ion acts as a Lewis acid to activate nucleophilic attack.
This mechanism appears to be general for the HDV ribozyme class, and distinguishes it from the majority of nucleolytic ribozymes that use general base catalysis.
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