Structures of permuted halves of a modern ribose binding protein
Florian Michel, Sooruban Shanmugaratnam, Sergio Romero-Romero, Birte Höcker [1]
Molecular Tour
Periplasmic binding proteins (PBPs) are responsible for the cellular detection, binding, and transport of soluble ligands. Generally, the PBP-like fold consists of two opposing lobes, each consisting of a central, five-stranded parallel β-sheet with five α-helices flanking its sides. The ligand is bound in the resulting cleft between the two lobes.
The orientation of the two lobes to each other changes upon ligand binding, with a transition from a ligand-free open conformation to a ligand-bound closed one. This change in structure is often detected by associated receptor proteins and initiates specific downstream signaling processes. Among the diverse PBPs found in nature, the ribose binding protein (RBP) from Thermotoga maritima is a typical representative of the PBP-like type I fold and acts as a component for ribose transport.
Despite diversity in the sequences of different PBP types, a shared common ancestry has been proposed. The structural symmetry of the two lobes has long led to the hypothesis that the PBP-like folds originated from a single-lobed ancestor protein, with a flavodoxin-like fold topology.
To try and isolate a structural entity resembling the progenitor protein, we generated permuted halves of the N- and C-terminal lobes of RBP from T. maritima, purified, characterized, and solved their structures via X-ray crystallography. The obtained structures differ somewhat from the expected conformation, highlighting the inherent adaptability of this class of protein. This non-native structural rearrangement offers interesting clues for an evolutionary path for this protein fold. Tracing the mechanism of duplication of the single-lobed precursor, its adaptation to a bilobal form and their variations on a structural level can help us understand how this fold came about.
Image 1: Canonical topology of both the parental RBP and the two halves investigated in this study. We observed an alternative arrangement of the halves compared to the one expected from the PBP-architecture.
Depiction of the crystal structures of both and RBP-CPN. Differences in the topology are highlighted by comparison of the parental structure (salmon) with the solved crystal structures of RBP-CPC (c, yellow) and RBP-CPN (d, blue). Interestingly, the non-native conformation observed in RBP-CPN resembles the sequence of other types of PBPs found in nature.
References
- ↑ Michel F, Shanmugaratnam S, Romero-Romero S, Hocker B. Structures of permuted halves of a modern ribose-binding protein. Acta Crystallogr D Struct Biol. 2023 Jan 1;79(Pt 1):40-49. doi: , 10.1107/S205979832201186X. Epub 2023 Jan 1. PMID:36601806 doi:http://dx.doi.org/10.1107/S205979832201186X
