AUTHOR=Zou Minjing , Guven Ayla , BinEssa Huda A. , Al-Rijjal Roua A. , Meyer Brian F. , Alzahrani Ali S. , Shi Yufei 

TITLE=Molecular Analysis of CYP27B1 Mutations in Vitamin D-Dependent Rickets Type 1A: c.590G > A (p.G197D) Missense Mutation Causes a RNA Splicing Error

JOURNAL=Frontiers in Genetics

VOLUME=11

YEAR=2020

URL=https://www.frontiersin.org/journals/genetics/articles/10.3389/fgene.2020.607517

DOI=10.3389/fgene.2020.607517

ISSN=1664-8021

ABSTRACT=<sec><title>Context</title><p>Vitamin D-dependent rickets type 1A (VDDR1A) is a rare autosomal recessively inherited disorder due to loss-of-function mutations in the <italic>CYP27B1</italic> gene. <italic>CYP27B1</italic> encodes an enzyme of 25-hydroxyvitamin D-1α-hydroxylase for converting inactive 25-OHD to biologically active 1,25-(OH)<sub>2</sub>D.</p></sec><sec><title>Objective</title><p>To identify underlying genetic defects in patients with VDDR1A.</p></sec><sec><title>Methods</title><p>Twelve patients from 7 Turkish and 2 Saudi families were investigated. The coding exons and intron-exon boundaries of the <italic>CYP27B1</italic> gene were amplified by Polymerase Chain Reaction (PCR) from peripheral lymphocyte DNA. PCR products were directly sequenced. The consequences of c.590G &gt; A mutation were analyzed by <italic>in silico</italic> and functional analysis.</p></sec><sec><title>Results</title><p><italic>CYP27B1</italic> mutations were identified in all the patients. Two novel mutations were identified in two separate families: c.171delG (family 7) and c.398_400dupAAT (family 8). The intra-exon deletion of c.171delG resulted in a frameshift and premature stop codon 20 amino acids downstream from the mutation (p.L58Cfs<sup>∗</sup>20). The intra-exon duplication of c.398_400dupAAT generated a premature stop codon at the mutation site (p.W134<sup>∗</sup>). A missense c.590G &gt; A (p.G197D) mutation was found in a patient from family 4 and caused a defect in pre-mRNA splicing. As a result, two populations of transcripts were detected: the majority of them with intron 3 retention (83%), and the minority (17%) being properly spliced transcripts with about 16% of wild-type enzymatic activity. The remaining nine patients from six families carried a previously reported c.1319_1325dupCCCACCC (F443Pfs<sup>∗</sup>24) mutation. Clinically, all the patients need continued calcitriol treatment, which was consistent with inactivation of 25-hydroxy vitamin D1α-hydroxylase activity.</p></sec><sec><title>Conclusion</title><p>Two novel frameshift <italic>CYP27B1</italic> mutations were identified and predicted to inactivate 25-hydroxyvitamin D-1α-hydroxylase. The loss of enzymatic activity by c.590G &gt; A missense mutation was mainly caused by aberrant pre-mRNA splicing.</p></sec>