 |
PDBsum entry 2eeu
|
|
|
|
References listed in PDB file
|
 |
|
Key reference
|
|
|
Title
|
|
Mutational analysis of the purine riboswitch aptamer domain.
|
|
|
Authors
|
|
S.D.Gilbert,
C.E.Love,
A.L.Edwards,
R.T.Batey.
|
|
|
Ref.
|
|
Biochemistry, 2007,
46,
13297-13309.
|
|
|
PubMed id
|
|
|
|
|
|
Abstract
|
|
|
The purine riboswitch is one of a number of mRNA elements commonly found in the
5'-untranslated region capable of controlling expression in a cis-fashion via
its ability to directly bind small-molecule metabolites. Extensive biochemical
and structural analysis of the nucleobase-binding domain of the riboswitch,
referred to as the aptamer domain, has revealed that the mRNA recognizes its
cognate ligand using an intricately folded three-way junction motif that
completely encapsulates the ligand. High-affinity binding of the purine
nucleobase is facilitated by a distal loop-loop interaction that is conserved
between both the adenine and guanine riboswitches. To understand the
contribution of conserved nucleotides in both the three-way junction and the
loop-loop interaction of this RNA, we performed a detailed mutagenic survey of
these elements in the context of an adenine-responsive variant of the xpt-pbuX
guanine riboswitch from Bacillus subtilis. The varying ability of these mutants
to bind ligand as measured by isothermal titration calorimetry uncovered the
conserved nucleotides whose identity is required for purine binding.
Crystallographic analysis of the bound form of five mutants and chemical probing
of their free state demonstrate that the identity of several universally
conserved nucleotides is not essential for formation of the RNA-ligand complex
but rather for maintaining a binding-competent form of the free RNA. These data
show that conservation patterns in riboswitches arise from a combination of
formation of the ligand-bound complex, promoting an open form of the free RNA,
and participating in the secondary structural switch with the expression
platform.
|
|
|
|
|
|
|
|
Headers
|
|
|
|
|
|
