Mapping of CaM, S100A1 and PIP2-Binding Epitopes in the Intracellular N- and C-Termini of TRPM4

Abstract: Molecular determinants of the binding of various endogenous modulators to transient receptor potential (TRP) channels are crucial for the understanding of necessary cellular pathways, as well as new paths for rational drug designs. The aim of this study was to characterise interactions between the TRP cation channel subfamily melastatin member 4 (TRPM4) and endogenous intracellular modulators—calcium-binding proteins (calmodulin (CaM) and S100A1) and phosphatidylinositol 4, 5-bisphosphate (PIP2). We have found… Show more

“…TRPM7np (see Material and Methods) contains aromatic and hydrophobic amino acids (Y524–Y528–F533) arranged in 1-5-10 CaM-binding motif, and five interspaced basic amino acids (R525, R530, K531, R532 and R534). Due to the known shared binding epitopes of CaM and S100A1 at e.g., ryanodine (RyR) or TRP receptors [ 22 , 25 , 37 , 37 , 38 ], we also decided to investigate binding site of S100A1 at TRPM7np. The position of TRPM7np in the TRPM7 structure (PDB: 5ZXZ) proves the accessibility of the binding region to intracellular environment and the basic amino acid residues of TRPM7np are exposed out of the TRPM7 structure backbone which suggest suitable condition for complex formation with the ligands ( Figure 2 A–C).…”

“…The S100A1 and CaM binding regions often overlap, and S100A1/CaM can compete for the same binding site on the target protein [ 22 , 39 ]. Based on our previous experience of shared CaM binding regions with S100A1 [ 25 , 37 , 37 , 38 , 39 ] we also investigated the possible binding of S100A1 to the identified CaM-binding epitope to TRPM7np ( Figure 3 A). The interaction of S100A1 with TRPM7np was confirmed by steady state fluorescence anisotropy similar to that described above for CaM binding experiments.…”

“…The multiple sequence alignment analysis of TRPM binding regions revealed consensus sequences of basic amino acid residues (RxxxxR/K, where x is any amino acid) in analysed regions ( Figure 4 ) suggested the importance of R525, R530, K531, R532 and R534 in TRPM7np. This analysis of multiple TRPM sequences was performed from in vitro experimentally characterized TRPM binding regions for CaM and S100A1 [ 25 , 37 , 38 , 40 , 41 ].

Figure 4 Multiple alignment of selected CaM binding regions in TRPM channels.

…”

“…The multiple sequence alignment analysis of TRPM binding regions revealed consensus sequences of basic amino acid residues (RxxxxR/K, where x is any amino acid) in analysed regions (Figure 4) suggested the importance of R525, R530, K531, R532 and R534 in TRPM7np. This analysis of multiple TRPM sequences was [15,25,37,38,40,41]. The sequence alignment shows a first perfect match (indicated by an asterisk) of arginine residues and second almost accurate match (indicated by dots) of basic residues across the TRPM sequences.…”

“…The number on the right side of the sequence marks its amino acid length. performed from in vitro experimentally characterized TRPM binding regions for CaM and S100A1 [25,37,38,40,41].…”

TRPM7 N-terminal region forms complexes with calcium binding proteins CaM and S100A1

“…TRPM7np (see Material and Methods) contains aromatic and hydrophobic amino acids (Y524–Y528–F533) arranged in 1-5-10 CaM-binding motif, and five interspaced basic amino acids (R525, R530, K531, R532 and R534). Due to the known shared binding epitopes of CaM and S100A1 at e.g., ryanodine (RyR) or TRP receptors [ 22 , 25 , 37 , 37 , 38 ], we also decided to investigate binding site of S100A1 at TRPM7np. The position of TRPM7np in the TRPM7 structure (PDB: 5ZXZ) proves the accessibility of the binding region to intracellular environment and the basic amino acid residues of TRPM7np are exposed out of the TRPM7 structure backbone which suggest suitable condition for complex formation with the ligands ( Figure 2 A–C).…”

“…The S100A1 and CaM binding regions often overlap, and S100A1/CaM can compete for the same binding site on the target protein [ 22 , 39 ]. Based on our previous experience of shared CaM binding regions with S100A1 [ 25 , 37 , 37 , 38 , 39 ] we also investigated the possible binding of S100A1 to the identified CaM-binding epitope to TRPM7np ( Figure 3 A). The interaction of S100A1 with TRPM7np was confirmed by steady state fluorescence anisotropy similar to that described above for CaM binding experiments.…”

“…The multiple sequence alignment analysis of TRPM binding regions revealed consensus sequences of basic amino acid residues (RxxxxR/K, where x is any amino acid) in analysed regions ( Figure 4 ) suggested the importance of R525, R530, K531, R532 and R534 in TRPM7np. This analysis of multiple TRPM sequences was performed from in vitro experimentally characterized TRPM binding regions for CaM and S100A1 [ 25 , 37 , 38 , 40 , 41 ].

Figure 4 Multiple alignment of selected CaM binding regions in TRPM channels.

…”

“…The multiple sequence alignment analysis of TRPM binding regions revealed consensus sequences of basic amino acid residues (RxxxxR/K, where x is any amino acid) in analysed regions (Figure 4) suggested the importance of R525, R530, K531, R532 and R534 in TRPM7np. This analysis of multiple TRPM sequences was [15,25,37,38,40,41]. The sequence alignment shows a first perfect match (indicated by an asterisk) of arginine residues and second almost accurate match (indicated by dots) of basic residues across the TRPM sequences.…”

“…The number on the right side of the sequence marks its amino acid length. performed from in vitro experimentally characterized TRPM binding regions for CaM and S100A1 [25,37,38,40,41].…”

TRPM7 N-terminal region forms complexes with calcium binding proteins CaM and S100A1

TRPM5 Channel Binds Calcium-Binding Proteins Calmodulin and S100A1

Structural and accessibility studies highlight the differential binding of clemizole to TRPC5 and TRPC6