Efficiency of Mammalian Selenocysteine Incorporation

Mehta, Anupama; Rebsch, Cheryl M; Kinzy, Scott A.; Fletcher, Julia E.; Copeland, Paul R.

doi:10.1074/jbc.m404639200

Cited by 82 publications

(104 citation statements)

References 24 publications

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“…This assay, which is widely used in the field, has been validated to be specific for selenocysteine incorporation. 33,34 As shown in Figure 1B, maximal luciferase activity was obtained using 80 nM purified bacterially expressed SBP2-CT, which is comparable to reports in the literature that range from 40-300 nM. [35][36][37][38][39] In contrast, 0.4 nM in vitro translated SBP2-CT generates an equivalent signal to 40 nM of recombinant protein (compare Figs.…”

Section: Resultssupporting

confidence: 64%

“…The luciferase reporter constructs luc/UGA 258 /PhGPx and luc/UGA 258 /Dio1 have been previously described. 26,33 The phospholipid hydroperoxide glutathione peroxidase (PHGPx), glutathione peroxidase 1 (GPx1), and deiodinase 2 (Dio2) SECIS probe sequences were also previously described. 26,53 DNA sequences The sequences used in the multiple alignment of SBP2-RBD were obtained primarily from GenBank and Ensembl databases.…”

Section: Reagentsmentioning

confidence: 99%

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Characterization of the UGA-recoding and SECIS-binding activities of SECIS-binding protein 2

2014

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Selenium, a micronutrient, is primarily incorporated into human physiology as selenocysteine (Sec). The 25 Seccontaining proteins in humans are known as selenoproteins. Their synthesis depends on the translational recoding of the UGA stop codon to allow Sec insertion. This requires a stem-loop structure in the 3' untranslated region of eukaryotic mRNAs known as the Selenocysteine Insertion Sequence (SECIS). The SECIS is recognized by SECIS-binding protein 2 (SBP2) and this RNA:protein interaction is essential for UGA recoding to occur. Genetic mutations cause SBP2 deficiency in humans, resulting in a broad set of symptoms due to differential effects on individual selenoproteins. Progress on understanding the different phenotypes requires developing robust tools to investigate SBP2 structure and function. In this study we demonstrate that SBP2 protein produced by in vitro translation discriminates among SECIS elements in a competitive UGA recoding assay and has a much higher specific activity than bacterially expressed protein. We also show that a purified recombinant protein encompassing amino acids 517-777 of SBP2 binds to SECIS elements with high affinity and selectivity. The affinity of the SBP2:SECIS interaction correlated with the ability of a SECIS to compete for UGA recoding activity in vitro. The identification of a 250 amino acid sequence that mediates specific, selective SECIS-binding will facilitate future structural studies of the SBP2:SECIS complex. Finally, we identify an evolutionarily conserved core cysteine signature in SBP2 sequences from the vertebrate lineage. Mutation of multiple, but not single, cysteines impaired SECIS-binding but did not affect protein localization in cells.

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Section: Resultssupporting

confidence: 64%

Section: Reagentsmentioning

confidence: 99%

Characterization of the UGA-recoding and SECIS-binding activities of SECIS-binding protein 2

2014

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“…The addition of recombinant His-tagged eEFSec to rabbit reticulocyte lysate, a system limiting for SBP2, did not increase Sec incorporation activity (13). Efforts to deplete eEFSec from reticulocyte lysate by immunoprecipitation have also been unsuccessful (data not shown).…”

Section: Resultsmentioning

confidence: 99%

“…1A). This method has been demonstrated to faithfully indicate Sec incorporation because the production of full-length and active luciferase is strictly SECIS-and SBP2-dependent (13).…”

Section: Resultsmentioning

confidence: 99%

“…In Vitro Translation and Sec Incorporation Assay-Sec incorporation activity in cell-free extracts was measured with a luciferase mRNA reporter containing a UGA-Sec codon at position 258 of the coding region and the rat GPX4 SECIS element at the 3Ј untranslated region (13). The luciferase reporter was also used to measure the translation activity by having an UGU-Cys codon instead of the UGA-Sec codon.…”

Section: Methodsmentioning

confidence: 99%

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The Selenocysteine-specific Elongation Factor Contains a Novel and Multi-functional Domain

González-Flores¹,

Gupta²,

DeMong³

et al. 2012

Journal of Biological Chemistry

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Background: Selenocysteine (Sec) incorporation requires the function of a unique translation elongation factor, eEFSec. Results: The novel Domain IV of eEFSec is required for at least three functions. Conclusion: Domain IV of eEFSec is the key site for dictating specificity in the conversion of the UGA stop codon into a Sec codon. Significance: Understanding elongation factor function is critical to deciphering the mechanism of Sec incorporation.

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