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Nitrile Reductase QueF

SBKB [doi:10.3942/psi_sgkb/fm_2011_3]
Featured System - March 2011
Short description: Nature uses exotic chemistry to build its diverse collection of molecules.

Nature uses exotic chemistry to build its diverse collection of molecules. Some of the oddest reactions are performed on transfer RNA. Most often, these changes are made by enzymes that capture a tRNA and then make modifications, adding additional groups or swapping out a few atoms for others with different properties. These chemical changes modify the interactions of tRNA with mRNA or ribosomes, making small adjustments that refine its function as the translator of genetic information.

Unique Reduction

The bacterial nitrile reductase QueF is a key enzyme in the biosynthesis of queuosine, a modified base used in the wobble anticodon position in several types of tRNA. QueF is unusual in two respects. First, it makes its modification on a free base, instead of the normal process of modifying a nucleotide that has already been built into a tRNA chain. The new group, after a few additional modifications, is then swapped onto the tRNA anticodon by another enzyme. Second, QueF performs a unique reaction, never before observed in nature, reducing a nitrile group to a primary amine.

Tools of Reduction

QueF uses several chemical tricks to perform its exotic reaction. NADPH, a carrier of hydride groups, provides the reductive power. Two molecules of NADPH are needed to perform the full reaction, which poses a potential problem: the reaction must be performed in two steps. Unfortunately, the intermediate form, created after the first NADPH has performed its half of the reduction, is reactive and would easily be destroyed by water. The enzyme solves this problem by using a cysteine amino acid to hold the intermediate, forming a covalent bond with it and protecting it from the surrounding water.

QueF Revealed

The structure of QueF, recently solved by PSI researchers at MCSG and available in PDB entry 3bp1, reveals much of this process, and leaves some mysteries. Two subunits of the enzyme form an elongated groove. In the crystal structure, two molecules of guanine were found at either end of this groove (shown here in green), and a pyrophosphate bound right in the center (red and yellow). The little loop of protein that carries the active site cysteine is disordered and cannot be seen in the structure. Presumably it folds over the top of the groove to perform the reaction when NADPH binds.

QueF in Action

To gain more insight into the reaction, PSI researchers performed computational simulations to explore the binding of NADPH and the nucleotide base that is modified. In the final model, NADPH is stretched out in the groove, and displaces one of the guanine bases observed in the crystal structure. To take a closer look at this model, the JSmol tab below displays an interactive JSmol image.

The JSmol tab below displays an interactive JSmol

A2A Adenine Receptor (PDB entries 3qak and 3eml)

Binding of adenosine shifts the structure of the receptor to the active form. Use the buttons to flip between the active agonist-bound form and the inactive antagonist-bound form and see the motion of the receptor. There is also a button to show just the adenosine portion of the agonist ligand. In each structure, the adenine portion of the molecule is colored green, and the ribose portion is colored magenta.

References

  1. Kim, Y. et al. High resolution structure of the nitrile reductase QueF combined with molecular simulations provide insight into enzyme mechanism. J. Mol. Biol. 404, 127-137 (2010).

  2. Iwata-Reuyl, D. An embarrassment of riches: the enzymology of RNA modification. Curr. Op. Chem. Biol. 12, 126-133 (2008).

Structural Biology Knowledgebase ISSN: 1758-1338
Funded by a grant from the National Institute of General Medical Sciences of the National Institutes of Health