Sumangala P. Shetty scite author profile

Background: Selenocysteine incorporation into selenoprotein P (SEPP1), which contains 10 Sec residues, is unique. Results: Processive Sec incorporation can be reconstituted in vitro, independently of the conserved non-SECIS portions of the 3Ј-UTR. Conclusion: Processivity is intrinsic, but efficiency is governed by selenium levels. Significance: SEPP1 synthesis is essential for male fertility and proper neurologic function.

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The molecular biology of selenocysteine

González-Flores¹,

Shetty²,

Dubey³

et al. 2013

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Selenium is an essential trace element that is incorporated into 25 human proteins as the amino acid selenocysteine (Sec). The incorporation of this amino acid turns out to be a fascinating problem in molecular biology because Sec is encoded by a stop codon, UGA. Layered on top of the canonical translation elongation machinery is a set of factors that exist solely to incorporate this important amino acid. The mechanism by which this process occurs, put into the context of selenoprotein biology, is the focus of this review.

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Multiple RNA structures affect translation initiation and UGA redefinition efficiency during synthesis of selenoprotein P

Mariotti

Shetty

Baird

et al. 2017

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Gene-specific expansion of the genetic code allows for UGA codons to specify the amino acid selenocysteine (Sec). A striking example of UGA redefinition occurs during translation of the mRNA coding for the selenium transport protein, selenoprotein P (SELENOP), which in vertebrates may contain up to 22 in-frame UGA codons. Sec incorporation at the first and downstream UGA codons occurs with variable efficiencies to control synthesis of full-length and truncated SELENOP isoforms. To address how the Selenop mRNA can direct dynamic codon redefinition in different regions of the same mRNA, we undertook a comprehensive search for phylogenetically conserved RNA structures and examined the function of these structures using cell-based assays, in vitro translation systems, and in vivo ribosome profiling of liver tissue from mice carrying genomic deletions of 3′ UTR selenocysteine-insertion-sequences (SECIS1 and SECIS2). The data support a novel RNA structure near the start codon that impacts translation initiation, structures located adjacent to UGA codons, additional coding sequence regions necessary for efficient production of full-length SELENOP, and distinct roles for SECIS1 and SECIS2 at UGA codons. Our results uncover a remarkable diversity of RNA elements conducting multiple occurrences of UGA redefinition to control the synthesis of full-length and truncated SELENOP isoforms.

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