Abstract:Domain swapping is a widespread oligomerization process that is observed in a large variety of protein families. In the large superfamily of substrate-binding proteins, non-monomeric members have rarely been reported. The arginine-binding protein from Thermotoga maritima (TmArgBP), a protein endowed with a number of unusual properties, presents a domain-swapped structure in its dimeric native state in which the two polypeptide chains mutually exchange their C-terminal helices. It has previously been shown that… Show more
“…The structure of cs-TmArgBP ΔCTH refers to the structure of closed-state conformation of TmArgBP without the CTH (PDB: 6GGV). Recently, the crystal structure of a monomeric version of the protein in the closed-state conformation complexed with arginine has also been solved (PDB: 6SVF, which is referred as cs-TmArgBP CTH ) ( Smaldone et al, 2019 ). In this structure a proline residue occurring prior to CTH is mutated (P215GK).…”
Section: Methodsmentioning
confidence: 99%
“…Recently, a monomeric version of the arginine-bound closed-state conformation of TmArgBP has been solved. In this structure more flexibility is introduced in the loop prior to CTH by mutating PRO-215 with GLY(2 1 5)-LYS(2 1 6) enabling the CTH to fold against the same chain ( Smaldone et al, 2019 ). Fig.…”
Section: Introductionmentioning
confidence: 99%
“…Biophysical investigations suggested this truncated version to be a better scaffold for arginine sensing while imposing a destabilization effect on the ligand-bound closed-state. In another attempt to generate the monomer a single proline residue prior to CTH was mutated and the crystal structure of this mutant was solved in a closed-state conformation bound to arginine ( Smaldone et al, 2019 ).…”
“…The structure of cs-TmArgBP ΔCTH refers to the structure of closed-state conformation of TmArgBP without the CTH (PDB: 6GGV). Recently, the crystal structure of a monomeric version of the protein in the closed-state conformation complexed with arginine has also been solved (PDB: 6SVF, which is referred as cs-TmArgBP CTH ) ( Smaldone et al, 2019 ). In this structure a proline residue occurring prior to CTH is mutated (P215GK).…”
Section: Methodsmentioning
confidence: 99%
“…Recently, a monomeric version of the arginine-bound closed-state conformation of TmArgBP has been solved. In this structure more flexibility is introduced in the loop prior to CTH by mutating PRO-215 with GLY(2 1 5)-LYS(2 1 6) enabling the CTH to fold against the same chain ( Smaldone et al, 2019 ). Fig.…”
Section: Introductionmentioning
confidence: 99%
“…Biophysical investigations suggested this truncated version to be a better scaffold for arginine sensing while imposing a destabilization effect on the ligand-bound closed-state. In another attempt to generate the monomer a single proline residue prior to CTH was mutated and the crystal structure of this mutant was solved in a closed-state conformation bound to arginine ( Smaldone et al, 2019 ).…”
“…This protein presents a number of distinctive/unique features in the large class of SBP. Although substrate-binding proteins are generally monomeric, TmArgBP is essentially dimeric, with the concomitant presence, as minor components, of higher oligomerization states [ 14 , 15 , 16 ]. The crystallographic structure of the protein has highlighted that its dimer is stabilized by swapping of the terminal C -terminal helix [ 9 ] ( Figure 1 ).…”
Section: Introductionmentioning
confidence: 99%
“…We have exploited the extraordinary stability of TmArgBP to effectively manipulate the protein through mutation, truncation and dissection of its native structure [ 10 , 13 , 14 ]. In particular, we have shown that a stable monomeric form may be obtained either though site-directed mutagenesis [ 15 ] or through the deletion of the C -terminal end, the swapping element in the protein binding [ 10 ]. TmArgBP can be further manipulated by dissecting it into its constitutive D1 and D2 domains ( Figure 1 ).…”
Arginine is one of the most important nutrients of living organisms as it plays a major role in important biological pathways. However, the accumulation of arginine as consequence of metabolic defects causes hyperargininemia, an autosomal recessive disorder. Therefore, the efficient detection of the arginine is a field of relevant biomedical/biotechnological interest. Here, we developed protein variants suitable for arginine sensing by mutating and dissecting the multimeric and multidomain structure of Thermotoga maritima arginine-binding protein (TmArgBP). Indeed, previous studies have shown that TmArgBP domain-swapped structure can be manipulated to generate simplified monomeric and single domain scaffolds. On both these stable scaffolds, to measure tryptophan fluorescence variations associated with the arginine binding, a Phe residue of the ligand binding pocket was mutated to Trp. Upon arginine binding, both mutants displayed a clear variation of the Trp fluorescence. Notably, the single domain scaffold variant exhibited a good affinity (~3 µM) for the ligand. Moreover, the arginine binding to this variant could be easily reverted under very mild conditions. Atomic-level data on the recognition process between the scaffold and the arginine were obtained through the determination of the crystal structure of the adduct. Collectively, present data indicate that TmArgBP scaffolds represent promising candidates for developing arginine biosensors.
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