Selenoprotein synthesis in E. coli
Open Access
- 1 June 1992
- journal article
- Published by Wiley in European Journal of Biochemistry
- Vol. 206 (3) , 767-773
- https://doi.org/10.1111/j.1432-1033.1992.tb16983.x
Abstract
The product of the selD gene from Escherichia coli catalyses the formation of an activated selenium compound which is required for the synthesis of Sec‐tRNA (Sec, selenocysteine) from Ser‐tRNA and for the formation of the unusual nucleoside 5‐methylaminomethyl‐2‐selenouridine in several tRNA species. selD was overexpressed in a T7 promoter/polymerase system and purified to apparent homogeneity. Purified SELD protein is a monomer of 37 kDa in its native state and catalyses a selenium‐dependent ATP‐cleavage reaction delivering AMP and releasing the β‐phosphate as orthophosphate. The γ‐phosphate group of ATP was not liberated in a form able to form a complex with molybdate. It was precluded that any putative covalent or non‐covalent ligand of SELD not removed during purification participated in the reaction. In a double‐labelling experiment employing [75Se]selenite plus dithiothreitol and [γ‐32P]ATP the 75Se and 32P radioactivities co‐chromatographed on a poly(ethyleneimine)‐cellulose column. No radioactivity originating from ATP eluted in this position when [α‐32P]ATP or [β‐32P]ATP or [14C]ATP were offered as substrates. The results support the speculation that the product of SELD is a phosphoselenoate with the phosphate moiety derived phosphoselenoate from the γ‐phosphate group of ATP. The α,β cleavage of ATP is also supported by the finding that neither adenosine 5′‐[α,β‐methylene]triphosphate nor adenosine 5′‐[β,γ‐methylene]triphosphate served as substrates in the reaction.Keywords
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