Specific recognition between YTHDF3 and m⁶A‐modified RNA: An all‐atom molecular dynamics simulation study

Abstract: The YTH domain of YTHDF3 belongs to a class of protein "readers" recognizing the N6-methyladenosine (m 6 A) modification in mRNA. Although static crystal structure reveals m 6 A recognition by a conserved aromatic cage, the dynamic process in recognition and importance of aromatic cage residues are not completely clear. Here, molecular dynamics (MD) simulations are performed to explore the issues and negative selectivity of YTHDF3 toward unmethylated substrate. Our results reveal that there exist conformation … Show more

“…Although these binding experiments with the wild-type protein sequences demonstrate the selectivity of the human YTH proteins and–more specifically–their domains for m 6 A, the key regions responsible for this selectivity needed to be determined. To elucidate the protein features responsible for the selective recognition of m 6 A containing transcripts, crystal structures were resolved in tandem with binding characterization efforts for all human YTH domains [39] , [40] , [41] , [42] , [43] , [45] , [55] , [56] , [57] , [58] , [59] , [60] .…”

“…In addition to the work that has been performed to identify interacting proteins with m 6 A modified RNAs, similar mass spectrometry techniques have been used to identify proteins interacting with m 1 A [28] , m 5 C [29] , and 8-oxoG [30] ( Table 2 , [5] , [7] , [11] , [17] , [21] , [28] , [29] , [30] , [37] , [39] , [40] , [45] , [56] , [58] , [59] , [62] , [76] , [77] , [78] , [79] , [80] , [81] , [82] , [83] ). Stable isotope labeling by amino acid in cell culture (SILAC) [84] has been used to identify proteins interacting with m 1 A with a 34-mer RNA probe designed to carry a portion of the SOX18 gene known to be modified in vivo [28] , [36] , [85] .…”

Characterization of epitranscriptome reader proteins experimentally and in silico: Current knowledge and future perspectives beyond the YTH domain

“…Although these binding experiments with the wild-type protein sequences demonstrate the selectivity of the human YTH proteins and–more specifically–their domains for m 6 A, the key regions responsible for this selectivity needed to be determined. To elucidate the protein features responsible for the selective recognition of m 6 A containing transcripts, crystal structures were resolved in tandem with binding characterization efforts for all human YTH domains [39] , [40] , [41] , [42] , [43] , [45] , [55] , [56] , [57] , [58] , [59] , [60] .…”

“…In addition to the work that has been performed to identify interacting proteins with m 6 A modified RNAs, similar mass spectrometry techniques have been used to identify proteins interacting with m 1 A [28] , m 5 C [29] , and 8-oxoG [30] ( Table 2 , [5] , [7] , [11] , [17] , [21] , [28] , [29] , [30] , [37] , [39] , [40] , [45] , [56] , [58] , [59] , [62] , [76] , [77] , [78] , [79] , [80] , [81] , [82] , [83] ). Stable isotope labeling by amino acid in cell culture (SILAC) [84] has been used to identify proteins interacting with m 1 A with a 34-mer RNA probe designed to carry a portion of the SOX18 gene known to be modified in vivo [28] , [36] , [85] .…”

Characterization of epitranscriptome reader proteins experimentally and in silico: Current knowledge and future perspectives beyond the YTH domain

Molecular Dynamics Simulations of Chemically Modified Ribonucleotides

Molecular Simulations to Investigate the Impact of N6-Methylation in RNA Recognition: Improving Accuracy and Precision of Binding Free Energy Prediction