Unlike the other amino acids, no free pool of selenocysteine exists in the cell. Its high reactivity would cause damage to cells. Instead, cells store selenium in the less reactive oxidized form, selenocystine, or in methylated form, selenomethionine.
Production Selenocysteine synthesis occurs on a specialized
tRNA, which also functions to incorporate it into nascent polypeptides. The primary and secondary structure of selenocysteine-specific tRNA, tRNASec, differ from those of standard tRNAs in several respects, most notably in having an 8-base-pair (bacteria) or 10-base-pair (eukaryotes) acceptor stem, a long variable region arm, and substitutions at several well-conserved base positions. The selenocysteine tRNAs are initially charged with serine by
seryl-tRNA ligase, but the resulting Ser-tRNASec is not used for translation because it is not recognised by the normal translation elongation factor (
EF-Tu in bacteria,
eEF1A in eukaryotes). Rather, the tRNA-bound seryl residue is converted to a selenocysteine residue by the
pyridoxal phosphate-containing enzyme
selenocysteine synthase. In eukaryotes and archaea, two enzymes are required to convert tRNA-bound seryl residue into tRNA selenocysteinyl residue: PSTK (
O-phosphoseryl-tRNA[Ser]Sec kinase) and selenocysteine synthase. Finally, the resulting Sec-tRNASecis specifically bound to an alternative translational elongation factor (SelB or mSelB (or eEFSec)), which delivers it in a targeted manner to the ribosomes translating mRNAs for selenoproteins. The specificity of this delivery mechanism is brought about by the presence of an extra protein domain (in bacteria, SelB) or an extra subunit (
SBP2 for eukaryotic mSelB/eEFSec) which bind to the corresponding RNA secondary structures formed by the SECIS elements in selenoprotein mRNAs.
Selenoproteins Selenocysteine has a lower
reduction potential than cysteine. These properties make it very suitable in proteins that are involved in
antioxidant activity. Although it is found in the
three domains of life, it is not universal in all organisms. Unlike other amino acids present in biological
proteins, selenocysteine is not coded for directly in the
genetic code. Instead, it is encoded in a special way by a UGA
codon, which is normally the "opal"
stop codon. Such a mechanism is called translational
recoding and its efficiency depends on the selenoprotein being synthesized and on translation
initiation factors. When cells are grown in the absence of selenium, translation of selenoproteins terminates at the UGA codon, resulting in a truncated, nonfunctional enzyme. The UGA codon is made to encode selenocysteine by the presence of a
selenocysteine insertion sequence (SECIS) in the
mRNA. The SECIS element is defined by characteristic nucleotide sequences and secondary structure base-pairing patterns. In
bacteria, the SECIS element is typically located immediately following the UGA codon within the reading frame for the selenoprotein. In
Archaea and in
eukaryotes, the SECIS element is in the
3′ untranslated region (3′ UTR) of the mRNA and can direct multiple UGA codons to encode selenocysteine residues. , 136 human proteins (in 37 families) are known to contain selenocysteine (selenoproteins).
Breakdown Selenocysteine is decomposed by the enzyme
selenocysteine lyase into L-
alanine and selenide. This probably helps with the safe recycling of Sec during degradation of selenoproteins.
Toxicity Just as selenomethionine can be randomly incorporated into proteins, selenocystine can also be mistakenly attached to tRNACys by cysteinyl-tRNA synthetase and incorporated into proteins in lieu of
cystine. This causes considerable toxicity. A variant synthase that can distinguish between Cys and Sec helps reduce toxicity.
Derivatives Selenocysteine derivatives γ-glutamyl-
Se-methylselenocysteine and
Se-methylselenocysteine occur naturally in plants of the genera
Allium and
Brassica. == Applications ==