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Iron-Dependent RNA-Binding Activity of Mycobacterium tuberculosis Aconitase
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ABSTRACT
Cellular iron levels are closely monitored by iron regulatory and sensor proteins of
Mycobacterium tuberculosis
for survival inside macrophages. One such class of proteins systematically studied in eukaryotes and reported in a few prokaryotes are the iron-responsive proteins (IRPs). These IRPs bind to iron-responsive elements (IREs) present at untranslated regions (UTRs) of mRNAs and are responsible for posttranscriptional regulation of the expression of proteins involved in iron homeostasis. Amino acid sequence analysis of
M. tuberculosis
aconitase (Acn), a tricarboxylic acid (TCA) cycle enzyme, showed the presence of the conserved residues of the IRP class of proteins. We demonstrate that
M. tuberculosis
Acn is bifunctional. It is a monomeric protein that is enzymatically active in converting isocitrate to
cis
-aconitate at a broad pH range of 7 to 10 (optimum, pH 8). As evident from gel retardation assays,
M. tuberculosis
Acn also behaves like an IRP by binding to known mammalian IRE-like sequences and to predicted IRE-like sequences present at the 3′ UTR of thioredoxin (
trxC
) and the 5′ UTR of the iron-dependent repressor and activator (
ideR
) of
M. tuberculosis. M. tuberculosis
Acn when reactivated with Fe
2+
functions as a TCA cycle enzyme, but upon iron depletion by a specific iron chelator, it behaves like an IRP, binding to the selected IREs in vitro. Since iron is required for the Acn activity and inhibits the RNA-binding activity of Acn, the two activities of
M. tuberculosis
Acn are mutually exclusive. Our results demonstrate the bifunctional nature of
M. tuberculosis
Acn, pointing to its likely role in iron homeostasis.
American Society for Microbiology
Title: Iron-Dependent RNA-Binding Activity of
Mycobacterium tuberculosis
Aconitase
Description:
ABSTRACT
Cellular iron levels are closely monitored by iron regulatory and sensor proteins of
Mycobacterium tuberculosis
for survival inside macrophages.
One such class of proteins systematically studied in eukaryotes and reported in a few prokaryotes are the iron-responsive proteins (IRPs).
These IRPs bind to iron-responsive elements (IREs) present at untranslated regions (UTRs) of mRNAs and are responsible for posttranscriptional regulation of the expression of proteins involved in iron homeostasis.
Amino acid sequence analysis of
M.
tuberculosis
aconitase (Acn), a tricarboxylic acid (TCA) cycle enzyme, showed the presence of the conserved residues of the IRP class of proteins.
We demonstrate that
M.
tuberculosis
Acn is bifunctional.
It is a monomeric protein that is enzymatically active in converting isocitrate to
cis
-aconitate at a broad pH range of 7 to 10 (optimum, pH 8).
As evident from gel retardation assays,
M.
tuberculosis
Acn also behaves like an IRP by binding to known mammalian IRE-like sequences and to predicted IRE-like sequences present at the 3′ UTR of thioredoxin (
trxC
) and the 5′ UTR of the iron-dependent repressor and activator (
ideR
) of
M.
tuberculosis.
M.
tuberculosis
Acn when reactivated with Fe
2+
functions as a TCA cycle enzyme, but upon iron depletion by a specific iron chelator, it behaves like an IRP, binding to the selected IREs in vitro.
Since iron is required for the Acn activity and inhibits the RNA-binding activity of Acn, the two activities of
M.
tuberculosis
Acn are mutually exclusive.
Our results demonstrate the bifunctional nature of
M.
tuberculosis
Acn, pointing to its likely role in iron homeostasis.
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