Literature DB >> 21337011

hNUDT16: a universal decapping enzyme for small nucleolar RNA and cytoplasmic mRNA.

Guangwen Lu1, Jie Zhang, Yan Li, Zhixin Li, Na Zhang, Xiang Xu, Tingting Wang, Zhenhong Guan, George F Gao, Jinghua Yan.   

Abstract

Human NUDT16 (hNUDT16) is a decapping enzyme initially identified as the human homolog to the Xenopus laevis X29. As a metalloenzyme, hNUDT16 relies on divalent cations for its cap-hydrolysis activity to remove m⁷GDP and m²²⁷GDP from RNAs. Metal also determines substrate specificity of the enzyme. So far, only U8 small nucleolar RNA (snoRNA) has been identified as the substrate of hNUDT16 in the presence of Mg²(+). Here we demonstrate that besides U8, hNUDT16 can also actively cleave the m⁷GDP cap from mRNAs in the presence of Mg²(+) or Mn²(+). We further show that hNUDT16 does not preferentially recognize U8 or mRNA substrates by our cross-inhibition and quantitative decapping assays. In addition, our mutagenesis analysis identifies several key residues involved in hydrolysis and confirms the key role of the REXXEE motif in catalysis. Finally an investigation into the subcellular localization of hNUDT16 revealed its abundance in both cytoplasm and nucleus. These findings extend the substrate spectrum of hNUDT16 beyond snoRNAs to also include mRNA, demonstrating the pleiotropic decapping activity of hNUDT16.

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Year:  2011        PMID: 21337011      PMCID: PMC4875290          DOI: 10.1007/s13238-011-1009-2

Source DB:  PubMed          Journal:  Protein Cell        ISSN: 1674-800X            Impact factor:   14.870


  46 in total

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Journal:  Structure       Date:  2006-02       Impact factor: 5.006

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Authors:  Melissa J Taylor; Brenda A Peculis
Journal:  Nucleic Acids Res       Date:  2008-09-27       Impact factor: 16.971

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6.  Substrate ambiguity among the nudix hydrolases: biologically significant, evolutionary remnant, or both?

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Journal:  Cell Mol Life Sci       Date:  2012-11-27       Impact factor: 9.261

7.  mRNAs containing the histone 3' stem-loop are degraded primarily by decapping mediated by oligouridylation of the 3' end.

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9.  An octamer of enolase from Streptococcus suis.

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Journal:  Protein Cell       Date:  2012-10-11       Impact factor: 14.870

10.  Mechanism of 53BP1 activity regulation by RNA-binding TIRR and a designer protein.

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Journal:  Nat Struct Mol Biol       Date:  2018-07-02       Impact factor: 15.369

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