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Splicing analysis of SLC40A1 missense variations and contribution to hemochromatosis type 4 phenotypes

外显子 RNA剪接 错义突变 选择性拼接 血色病 遗传学 生物 外显子跳跃 小基因 表型 基因 遗传性血色病 突变 外显子剪接增强剂 核糖核酸
作者
Marlène Le Tertre,Chandran Ka,Loann Raud,Isabelle Berlivet,Isabelle Gourlaouen,Gaëlle Richard,Kévin Uguen,Jian‐Min Chen,Claude Férec,Yann Fichou,Gérald Le Gac
出处
期刊:Blood Cells Molecules and Diseases [Elsevier BV]
卷期号:87: 102527-102527 被引量:7
标识
DOI:10.1016/j.bcmd.2020.102527
摘要

Hemochromatosis type 4, or ferroportin disease, is considered as the second leading cause of primary iron overload after HFE-related hemochromatosis. The disease, which is predominantly associated with missense variations in the SLC40A1 gene, is characterized by wide clinical heterogeneity. We tested the possibility that some of the reported missense mutations, despite their positions within exons, cause splicing defects. Fifty-eight genetic variants were selected from the literature based on two criteria: a precise description of the nucleotide change and individual evidence of iron overload. The selected variants were investigated by different in silico prediction tools and prioritized for midigene splicing assays. Of the 15 variations tested in vitro, only two were associated with splicing changes. We confirm that the c.1402G>A transition (p.Gly468Ser) disrupts the exon 7 donor site, leading to the use of an exonic cryptic splicing site and the generation of a truncated reading frame. We observed, for the first time, that the p.Gly468Ser substitution has no effect on the ferroportin iron export function. We demonstrate alternative splicing of exon 5 in different cell lines and show that the c.430A>G (p.Asn144Asp) variant promotes exon 5 inclusion. This could be part of a gain-of-function mechanism. We conclude that splicing mutations rarely contribute to hemochromatosis type 4 phenotypes. An in-depth investigation of exon 5 auxiliary splicing sequences may help to elucidate the mechanism by which splicing regulatory proteins regulate the production of the full length SLC40A1 transcript and to clarify its physiological importance.
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