Any feedback?
Please rate this page
(search_result.php)
(0/150)

BRENDA support

Refine search

Search Protein Variants

show results
Don't show organism specific information (fast!)
Search organism in taxonomic tree (slow, choose "exact" as search mode, e.g. "mammalia" for rat,human,monkey,...)
(Not possible to combine with the first option)
Refine your search

Search term:

<< < Results 11 - 17 of 17
download as CSV
download all results as CSV
EC Number Protein Variants Commentary Reference
Show all pathways known for 2.9.1.2Display the word mapDisplay the reaction diagram Show all sequences 2.9.1.2R72A the mutant enzyme is significantly less active in L-selenocysteinyl-tRNASec formation in vivo and Cys-tRNASec formation in vitro. The mutant enzyme is unable to form L-selenocysteinyl-tRNASec in vitro 694428
Show all pathways known for 2.9.1.2Display the word mapDisplay the reaction diagram Show all sequences 2.9.1.2R75A mutant is inactive in vivo 695136
Show all pathways known for 2.9.1.2Display the word mapDisplay the reaction diagram Show all sequences 2.9.1.2R97A in vivo activity of the mutant is indistinguishable from that of the wild-type enzyme 695136
Show all pathways known for 2.9.1.2Display the word mapDisplay the reaction diagram Show all sequences 2.9.1.2R97Q in vivo activity of the mutant is indistinguishable from that of the wild-type enzyme 695136
Show all pathways known for 2.9.1.2Display the word mapDisplay the reaction diagram Show all sequences 2.9.1.2T325S naturally occurring mutation and site-directed mutagenesis, the mutation does not affect the binding affinity of the SepSecS-tRNA complex. The mutant does not form a complex with GroEL. Residue Thr325 is located in helix alpha12 and about 15 A away from the active site. The Thr325 to Ser replacement does not cause any changes in the tetrameric structure of SepSecS. Tetramers of T325S adopt the same structure as wild-type SepSecS. The pathogenic mutation Thr325Ser does not alter the three-dimensional structure of the SepSecS tetramer 762417
Show all pathways known for 2.9.1.2Display the word mapDisplay the reaction diagram Show all sequences 2.9.1.2Y334C naturally occurring mutation and site-directed mutagenesis, the mutation does not affect the binding affinity of the SepSecS-tRNA complex. The mutant forms a stable complex with GroEL. The side chain of Tyr334 is in helix alpha13 near the active-site pocket. Its hydroxyl group forms a hydrogen bond with the backbone carbonyl of Asn285, and this interaction may help stabilize a loop that carries Lys284 and the covalently attached PLP cofactor. In the Y334C crystal, the side chain of Cys334 coordinates two water molecules, which interact with the backbone carbonyl of Asn285 in the same fashion as the Tyr side chain in the wild-type enzyme. Tetramers of Y334C adopt the same structure as wild-type SepSecS. The pathogenic mutation Tyr334Cys does not alter the three-dimensional structure of the SepSecS tetramer 762417
Show all pathways known for 2.9.1.2Display the word mapDisplay the reaction diagram Show all sequences 2.9.1.2Y429* naturally occurring nonsense mutation and site-directed mutagenesis. Y429* expresses at low levels and as insoluble protein regardless of the incubation temperature, induction point, or the growth media used. Tyr429 is located before strand beta14. Premature abortion of protein synthesis yields a truncated enzyme devoid of strand beta14, loop beta14-alpha15, and the C-terminal helix alpha15. Loop beta14-alpha15 establishes a side of the catalytic groove, and helix alpha15 provides residues that bind the 5'-end of tRNASec. The Y429* variant is not be capable of promoting selenocysteine synthesis 762417
<< < Results 11 - 17 of 17
download as CSV
download all results as CSV