Kinetic and mutational studies of the adenosine diphosphate ribose hydrolase from Mycobacterium tuberculosis
Abstract
Mycobacterium tuberculosis represents one
of the world’s most devastating infectious agents – with one third of
the world’s population infected and 1.5 million people dying each year
from this deadly pathogen. As part of an effort to identify targets for
therapeutic intervention, we carried out the kinetic characterization of
the product of gene rv1700 of M. tuberculosis. Based on
its sequence and its structure, the protein had been tentatively
identified as a pyrophosphohydrolase specific for adenosine diphosphate
ribose (ADPR), a compound involved in various pathways including
oxidative stress response and tellurite resistance. In this work we
carry out a kinetic, mutational and structural investigation of the
enzyme, which provides a full characterization of this Mt-ADPRase. Optimal catalytic rates were achieved at alkaline pH (7.5–8.5) with either 0.5–1 mM Mg2+ or 0.02–1 mM Mn2+. K
m
and k
cat values for hydrolysis of ADPR with Mg2+ ions are 200 ± 19 μM and 14.4 ± 0.4 s−1, and with Mn2+ ions are 554 ± 64 μM and 28.9 ± 1.4 s−1.
Four residues proposed to be important in the catalytic mechanism of
the enzyme were individually mutated and the kinetics of the mutant
enzymes were characterized. In the four cases, the K
m
increased only slightly (2- to 3-fold) but the k
cat decreased significantly (300- to
1900-fold), confirming the participation of these residues in catalysis.
An analysis of the sequence and structure conservation patterns in
Nudix ADPRases permits an unambiguous identification of members of the
family and provides insight into residues involved in catalysis and
their participation in substrate recognition in the Mt-ADPRase.
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