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PDBsum entry 2nqr
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Biosynthetic protein
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PDB id
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2nqr
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References listed in PDB file
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Key reference
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Title
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Mutational analysis of escherichia coli moea: two functional activities map to the active site cleft.
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Authors
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J.D.Nichols,
S.Xiang,
H.Schindelin,
K.V.Rajagopalan.
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Ref.
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Biochemistry, 2007,
46,
78-86.
[DOI no: ]
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PubMed id
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Abstract
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The molybdenum cofactor is ubiquitous in nature, and the pathway for Moco
biosynthesis is conserved in all three domains of life. Recent work has helped
to illuminate one of the most enigmatic steps in Moco biosynthesis, ligation of
metal to molybdopterin (the organic component of the cofactor) to form the
active cofactor. In Escherichia coli, the MoeA protein mediates ligation of Mo
to molybdopterin while the MogA protein enhances this process in an
ATP-dependent manner. The X-ray crystal structures for both proteins have been
previously described as well as two essential MogA residues, Asp49 and Asp82.
Here we describe a detailed mutational analysis of the MoeA protein. Variants of
conserved residues at the putative active site of MoeA were analyzed for a loss
of function in two different, previously described assays, one employing moeA-
crude extracts and the other utilizing a defined system. Oddly, no correlation
was observed between the activity in the two assays. In fact, our results showed
a general trend toward an inverse relationship between the activity in each
assay. Moco binding studies indicated a strong correlation between a variant's
ability to bind Moco and its activity in the purified component assay. Crystal
structures of the functionally characterized MoeA variants revealed no major
structural changes, indicating that the functional differences observed are not
due to disruption of the protein structure. On the basis of these results, two
different functional areas were assigned to regions at or near the MoeA active
site cleft.
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