Abstract
Novel mouse models were developed in which the hepatic selenoprotein population was targeted for removal by disrupting the selenocysteine (Sec) tRNA([Ser]Sec) gene (trsp), and selenoprotein expression was then restored by introducing wild type or mutant trsp transgenes. The selenoprotein population was partially replaced in liver with mutant transgenes encoding mutations at either position 34 (34T-->A) or 37 (37A-->G) in tRNA([Ser]Sec). The A34 transgene product lacked the highly modified 5-methoxycarbonylmethyl-2'-O-methyluridine, and its mutant base A was converted to I34. The G37 transgene product lacked the highly modified N(6)-isopentenyladenosine. Both mutant tRNAs lacked the 2'-methylribose at position 34 (Um34), and both supported expression of housekeeping selenoproteins (e.g. thioredoxin reductase 1) in liver but not stress-related proteins (e.g. glutathione peroxidase 1). Thus, Um34 is responsible for synthesis of a select group of selenoproteins rather than the entire selenoprotein population. The ICA anticodon in the A34 mutant tRNA decoded Cys codons, UGU and UGC, as well as the Sec codon, UGA. However, metabolic labeling of A34 transgenic mice with (75)Se revealed that selenoproteins incorporated the label from the A34 mutant tRNA, whereas other proteins did not. These results suggest that the A34 mutant tRNA did not randomly insert Sec in place of Cys, but specifically targeted selected selenoproteins. High copy numbers of A34 transgene, but not G37 transgene, were not tolerated in the absence of wild type trsp, further suggesting insertion of Sec in place of Cys in selenoproteins.
Highlights
1st breeding trspϩ/ϩ ϫ trspfl/ϩ-AlbCreϩ/ϩ trspt/t ϫ trspfl/ϩ-AlbCreϩ/ϩ trspϩ/ϩ-A34t/t ϫ trspfl/ϩ-AlbCreϩ/ϩ trspϩ/ϩ-G37t/t ϫ trspfl/ϩ-AlbCreϩ/ϩ trspfl/f ϫ trspfl/ϩ-AlbCreϩ/ϩ
⌬trsp a Matings to obtain each mouse line used in this study are shown in the table. b Both wild type mice, designated trsp in the text, and wild type selenoprotein replacement mice, designated trspt in the text, were used as control mice. c Genotype designations denote the following: trspϩ, trspfl; trspt (Sec tRNASerSec transgene); ⌬trsp; AlbCre; A34 (A34 mutant transgene); and G37 (G37 mutant transgene)
The selenoprotein-labeled population in kidney appeared to be similar in the four tRNA[Ser]Sec-defective mouse lines with the possible exceptions of a reduced level of GPx1 in the high copy G37 transgene line (Fig. 6) and the elevated levels of GPx1 and -4 in ⌬trsp
Summary
Materials—[75Se]Selenium (specific activity 1000 Ci/mmol) was obtained from the Research Reactor Facility, University of Missouri, Columbia; [3H]serine (specific activity 29 Ci/mmol) was from GE Healthcare, and [␣-32P]dCTP (specific activity ϳ6000 Ci/mmol) was from PerkinElmer Life Sciences. Protein extracts were prepared from liver and kidney and electrophoresed on NuPAGE 10% polyacrylamide gels. Proteins were transferred to polyvinylidene difluoride membranes as described previously with the exception that 40 g of each protein extract were loaded onto gels [21,22,23, 27] and immunoblotted with antibodies against GPx1 (1:1000 dilution), GPx4 (1:2000), SelR (1:1000), and SelT (1:400). Nirenberg or were prepared as described [29]
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