Nuclear retention of full-length HTT RNA is mediated by splicing factors MBNL1 and U2AF65

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作者
Xin Sun
Pan P. Li
Shanshan Zhu
Rachael Cohen
Leonard O. Marque
Christopher A. Ross
Stefan M. Pulst
Ho Yin Edwin Chan
Russell L. Margolis
Dobrila D. Rudnicki
机构
[1] Johns Hopkins University School of Medicine,Department of Psychiatry and Behavioral Sciences, Division of Neurobiology
[2] Johns Hopkins University School of Medicine,Department of Neurology
[3] Johns Hopkins University School of Medicine,Department of Neuroscience
[4] Program of Cellular and Molecular Medicine,Department of Neurology
[5] Johns Hopkins University School of Medicine,undefined
[6] University of Utah,undefined
[7] Laboratory of Drosophila Research,undefined
[8] School of Life Sciences,undefined
[9] Faculty of Science,undefined
[10] The Chinese University of Hong Kong,undefined
[11] Guangdong-Hong Kong-Macau Institute of CNS Regeneration,undefined
[12] Jinan University,undefined
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摘要
Huntington’s disease (HD) is caused by a CAG repeat expansion in the huntingtin (HTT) gene. Recent evidence suggests that HD is a consequence of multimodal, non-mutually exclusive mechanisms of pathogenesis that involve both HTT protein- and HTT RNA-triggered mechanisms. Here we provide further evidence for the role of expanded HTT (expHTT) RNA in HD by demonstrating that a fragment of expHTT is cytotoxic in the absence of any translation and that the extent of cytotoxicity is similar to the cytotoxicity of an expHTT protein fragment encoded by a transcript of similar length and with a similar repeat size. In addition, full-length (FL) expHTT is retained in the nucleus. Overexpression of the splicing factor muscleblind-like 1 (MBNL1) increases nuclear retention of expHTT and decreases the expression of expHTT protein in the cytosol. The splicing and nuclear export factor U2AF65 has the opposite effect, decreasing expHTT nuclear retention and increasing expression of expHTT protein. This suggests that MBNL1 and U2AF65 play a role in nuclear export of expHTT RNA.
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