CUG Start Codon Generates Thioredoxin/Glutathione Reductase Isoforms in Mouse Testes

Male 570 Molecular Sequence Data Biophysics Codon, Initiator In Vitro Techniques Biochemistry Cell Line Mice 03 medical and health sciences Other Biochemistry Multienzyme Complexes Chlorocebus aethiops Animals Humans NADH, NADPH Oxidoreductases Amino Acid Sequence 0303 health sciences Life Sciences Immunohistochemistry Rats Isoenzymes Mice, Inbred C57BL Seminiferous Epithelium COS Cells and Structural Biology NIH 3T3 Cells Electrophoresis, Polyacrylamide Gel Biotechnology
DOI: 10.1074/jbc.m109.070532 Publication Date: 2009-12-15T02:05:44Z
ABSTRACT
Mammalian cytosolic and mitochondrial thioredoxin reductases are essential selenocysteine-containing enzymes that control thioredoxin functions. Thioredoxin/glutathione reductase (TGR) is a third member of this enzyme family. It has an additional glutaredoxin domain and shows highest expression in testes. Herein, we found that human and several other mammalian TGR genes lack any AUG codons that could function in translation initiation. Although mouse and rat TGRs have such codons, we detected protein sequences upstream of them by immunoblot assays and direct proteomic analyses. Further gene engineering and expression analyses demonstrated that a CUG codon, located upstream of the sequences previously thought to initiate translation, is the actual start codon in mouse TGR. The use of this codon relies on the Kozak consensus sequence and ribosome-scanning mechanism. However, CUG serves as an inefficient start codon that allows downstream initiation, thus generating two isoforms of the enzyme in vivo and in vitro. The use of CUG evolved in mammalian TGRs, and in some of these organisms, GUG is used instead. The newly discovered longer TGR form shows cytosolic localization in cultured cells and is expressed in spermatids in mouse testes. This study shows that CUG codon is used as an inefficient start codon to generate protein isoforms in mouse.
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