4.5 Article

Role of purα in targeting mRNA to sites of translation in hippocampal neuronal dendrites

Journal

JOURNAL OF NEUROSCIENCE RESEARCH
Volume 83, Issue 6, Pages 929-943

Publisher

WILEY
DOI: 10.1002/jnr.20806

Keywords

BC1; Map2; FMRP; Staufen; Map1B; Ankyrin G

Categories

Funding

  1. NCI NIH HHS [1 R24 CA095823] Funding Source: Medline
  2. NINDS NIH HHS [NS43970, NS-35000] Funding Source: Medline

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Using genetic inactivation in the mouse, PURA, encoding Pur alpha, is demonstrated to be essential for developmentally-timed dendrite formation in the cerebellum and hippocampus. Comparison of RNA species bound by Pur alpha prompts the hypothesis that Pur alpha functions with non-coding RNA in transport of certain mRNA molecules to sites of translation in dendrites. Pur alpha binds to human BC200 RNA, implicated in dendritic targeting, and this has homologies to 7SL RNA, implicated in compartmentalized translation. Results using hippocampal rat neurons in situ show that Pur alpha binds to BC1 RNA, implicated in dendritic targeting as a mouse counterpart of BC200, and to mRNA molecules translated in dendrites; Pur alpha: is specifically located in dendrites, where it is colocalized with Map2, but not in axons, where it fails to colocalize with Ankyrin G. Pur alpha and Staufen are colocalized at dendritic sites of mRNA translation. Microtubule disruptors inhibit Pur alpha dendritic targeting and allow its mislocalization to axons. Using mouse brain, double-RNA immuno-precipitation places Pur alpha together with Staufen or FMRP on BC1 RNA and specific mRNA species in vivo. These results help define a mechanism by which Pura. targets specific mRNA molecules to sites of dendritic translation. (c) 2006 wiley-Liss,inc.

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