Plant evolution: A promiscuous intermediate underlies the evolution of the transcription factor LEAFY

Gene duplication is a general and widely accepted mechanism for the acquisition of new gene functions. Some genes, however, are under selective pressure to remain single-copy genes, and their evolution cannot be explained by the gene duplication paradigm. Sayou et al. tackle this question using the LEAFY (LFY) gene of plants as the evolutionary model {1}, carrying out a wide range of experimental and computational analyses. The authors propose a molecular evolutionary mechanism where an ortholog – intermediate in the evolutionary history of plants – innovates new DNA binding specificities while preserving the original specificity and, later in evolution, diverges to retain the binding specificity for only one particular DNA binding motif.

The LFY gene encodes a transcription factor (TF) that is essential for reproduction and cell division and mostly exists as a single-copy gene in land plants. Previous experiments suggested that DNA binding specificity might have changed during land plant evolution {1}. Sayou et al. expand the evolutionary history of this gene {1} by orthology detection in algal species. Phylogenetic analysis is combined with SELEX experiments and reveals three different DNA binding motifs that correspond to the described evolutionary transitions. Representative LFY orthologs are found to preferentially bind one particular DNA binding motif, thus demonstrating that LFY specificity has changed during plant evolution. X-ray crystallography, protein modeling, mutagenesis and DNA binding assays reveal that LFY specificity can be defined using only three residues. Two of these residues are found to determine the half-sequence identity, while the remaining residue influences the dimerization mode and the requirement for a spacer between half-sites.

The discovery of an evolutionary intermediate ortholog, capable of binding all three types of DNA binding motifs, suggests a molecular evolutionary mechanism that explains how LFY has evolved to capture different specificities without the need of gene duplication. This very much goes along the lines of the innovation-amplification-divergence (IAD) model in the sense that innovation of new gene functions precedes gene duplication events {2}.

References

1. The floral regulator LEAFY evolves by substitutions in the DNA binding domain. Maizel A, Busch MA, Tanahashi T, Perkovic J, Kato M, Hasebe M, Weigel D. Science 2005 Apr 8; 308(5719):260-3

2. Evolution of new gene functions: simulation and analysis of the amplification model. Pettersson ME, Sun S, Andersson DI, Berg OG. Genetica 2009 Apr; 135(3):309-24

Engineering ligand-binding proteins with high affinity and selectivity

Protein design aims to rationally design proteins that fold into particular target structures capable of performing new desired functions. Such an approach will undoubtedly have a huge impact in medicine and biotechnology in the future. However, and despite important recent advances in the field, efforts have had limited success in designing proteins with high affinity and selectivity for small ligands.

Baker and colleagues describe a novel computational method to design ligand-binding proteins, which is combined with directed-evolution experiments. The described computational protocol mimics properties of naturally occurring binding sites: specific hydrogen-bonding and van der Waals interactions with the ligand, shape complementarity and structural organization in the unbound state.

As a result, the designed protein is able to bind the target ligand with picomolar affinity. X-ray crystallography confirms the computer-designed ligand-binding mode. Specificity assays show that related ligands bind less tightly to the designed protein. Furthermore, fine tuning the hydrogen-bonding interactions at the designed binding site permits control of affinities over related ligands.Computational design of ligand-binding proteins is likely to have a strong influence on future protein design attempts and, as the authors state, “should provide an increasingly powerful approach to creating small molecule receptors for synthetic biology, therapeutic scavengers for toxic compounds, and robust binding domains for diagnostic devices”.

A joint effort to elucidate the structure of the mature HIV-1 capsid

This paper describes a major breakthrough in the structural biology of the mature HIV-1 virus, and it is a good example on how computational modeling can expand the knowledge provided by experimental methods.

This work combines cryo-electron microscopy (cryo-EM) of HIV-1 tubular assembly and cryo-electron tomography of HIV-1 cores isolated from virions, along with previously published crystal structures of the HIV-1 capsid protein. For this, molecular modeling and all-atom molecular dynamics flexible fitting are applied, and, as a result, a complete capsid model is shown at pseudo-atomic resolution.The obtained results highlight a three-helix bundle in the carboxy term of the capsid protein, which is essential for viral assembly, stability and infectivity. Thus, this work suggests a direction for future pharmacological studies.