A Novel FECH Mutation Causes Erythropoietic Protoporphyria with Severe Liver Dysfunction

authors:

avatar Fang Xu 1 , avatar Xiaomei Wang 1 , avatar Xiumei Chi 1 , avatar Xiuting He 1 , avatar Yue Qi 1 , avatar Huijuan Peng 1 , avatar Junqi Niu 1 , avatar Yanjun Cai 1 , * , avatar Pujun Gao 1 , **

The First Hospital of Jilin University, Changchun, China
Corresponding Authors:
Hepatitis Monthly: Vol.18, issue 11; e80767
published online: September 26, 2018
article type: Research Article
received: June 13, 2018
revised: August 8, 2018
accepted: September 14, 2018
DOI: https://doi.org/10.5812/hepatmon.80767

how to cite: Xu F , Wang X , Chi X , He X , Qi Y , et al. A Novel FECH Mutation Causes Erythropoietic Protoporphyria with Severe Liver Dysfunction. Hepat Mon. 2018;18(11):e80767. https://doi.org/10.5812/hepatmon.80767.

Abstract

Background:

Erythropoietic protoporphyria (EPP) is a rare autosomal dominant disease that is caused by partial ferrochelatase (FECH) deficiency because of a genetic mutation in the FECH gene.

Objectives:

The aim of this study was to investigate the genetic mechanism of EPP in a Chinese family.

Methods:

Clinical physical examination, laboratory testing, and medical history tracking were performed for phenotyping. The FECH gene was sequenced for genotyping.

Results:

The proband presented EPP with severe liver dysfunction. A novel nonsense mutation of c.910 C>T in the FECH gene, resulting in p.Arg304Ter, was identified in the proband as well as her symptomatic mother, aunt, and asymptomatic male cousin. The proband and her living family members, except the asymptomatic male cousin, carried the alleles IVS 3-48C and IVS 1-23T on the FECH gene. The mutation of c.910 C>T in the FECH gene presented its heterozygous autosomal dominant inherent clinical manifestations, only in the presence of the heterozygous alleles IVS 3-48C and IVS 1-23T. The frequencies of the alleles IVS 3-48C and IVS 1-23T were 30.8% and 27.9% in a northeast Chinese Han population, respectively.

Conclusions:

A new nonsense mutation of c.910 C>T was identified in the FECH gene, which expressed EPP with severe liver dysfunction when it was co-inherited with the heterozygous alleles IVS 3-48C and IVS 1-23T, in a Chinese family.

1. Background

Erythropoietic protoporphyria (EPP) is a relatively rare inherited disorder that is characterized by photosensitivity of skin exposed to sunlight. It is caused by partial deficiency of ferrochelatase (FECH), which is the terminal enzyme of heme synthesis, leading to accumulation of free protoporphyrin IX in erythrocytes, other tissues (skin and liver), and biological fluids (bile and feces). The most common clinical manifestation of EPP is cutaneous photosensitivity in sun-exposed skin, including edema, erythema, itching, and burning (1-4). Scars form on the face and skin, particularly over the joints on the backs of the hands, become thick and waxy, and in rare cases, palmar keratoderma can occur in chronic patients (5-7). In addition to skin problems, 10% to 20% of EPP patients suffer from liver dysfunction. Moreover, protoporphyrin can form gallstones, resulting in an increased risk of cholelithiasis (1). Approximately 2% of patients with EPP develop fatal liver failure, and some patients need to be treated with liver transplantation (5, 8-13).

The mode of inheritance of EPP is complex. Among 190 mutations identified in the FECH gene in patients with EPP throughout the world (14), most are autosomal dominant with a low penetrance. Fewer than 10% of mutation carriers develop overt clinical symptoms (9). The activity of FECH is only 10% to 30% of the normal value in symptomatic EPP patients, and approximately 50% of the normal value in asymptomatic carriers (15). The phenotypic expression of EPP is generally the result of the coinheritance of a low-expressed wild-type allele and a mutant allele (16-18). The mechanism responsible for the low expression of the wild-type allele of FECH is the single nucleotide polymorphism IVS 3-48T/C (2, 19). The single nucleotide polymorphism IVS 3-48 T>C in the FECH gene modulates the use of a constitutive aberrant acceptor splice site, which is located 63 bp upstream of the normal one (17). The aberrantly spliced mRNA is degraded by a nonsense-mediated decay mechanism, leading to a decreased steady-state level of mRNA and additional FECH enzyme deficiency, necessary for EPP phenotypic expression. In western countries and Japan, ferrochelatase IVS 3-48T/C accounts for 85% to 90% of cases of EPP (2). The frequency of the low-expression allele, IVS 3-48C, varies widely in different ethnic groups (19-21). The allele IVS 3-48C is distributed in an east-west gradient in China: from 41.35% in Shanghai, 28.9% in Beijing, 28% in Hong Kong, to putatively less than 1% in Xi’an (22-24). Carriers of null-allele mutations in the FECH gene, which lead to the formation of a shorter mRNA and a truncated protein, are more likely to develop liver disease than carriers of missense mutations (25, 26).

Furthermore, EPP cases have been reported in Europe, United States, and Japan (27-31). However, only 16 EPP patients with detailed genetic information have been reported in a Chinese population (14, 22-24, 32-37). In the present study, one new mutation was identified in the FECH gene to cause EPP in a Chinese family, and the frequencies of the IVS 3-48C and IVS 1-23T polymorphisms were further assessed in a northeast Chinese Han population.

2. Methods

2.1. Subjects

This study was approved by the Ethics Committee of the First Hospital of Jilin University, Jilin, China. Each procedure in this study was performed after written consents were provided by the participants.

A total of 60 individuals were investigated in this study, including a family with EPP and 52 healthy individuals from a northeast Chinese Han population. In the family with EPP, except for the proband’s grandfather, grandmother, and uncle, who had died, eight individuals, including the proband, her father, her mother, her aunt, her aunt’s daughter and son, her uncle’s wife, and her uncle’s daughter, were tested.

2.2. Genetic Analyses

Phenotypic analyses were performed through clinical examination and laboratory testing for the living individuals; for individuals, who had died, their medical history was tracked. For genotyping, peripheral blood samples (approximately 5 mL) were taken from the proband, the proband’s family members, and healthy participants, using ethylene diamine tetraacetic acid-coated tubes, and sent to BGI Diagnosis Co., Shenzhen, Guangdong province, China (certified with ISO 15189), for next-generation sequencing. Genomic DNA was isolated from peripheral blood samples, using a QIAamp DNA Blood Midi Kit (Qiagen, Hilden, Germany), then sheared by Covaris LE220 (Woburn, MA, USA) to generate a paired-end library (200 to 250 bp). The library was enriched by array hybridization, followed by elution and post-capture amplification. The products were subjected to analysis by an Agilent 2100 Bioanalyzer (Agilent, CA, USA) and ABI StepOne (Thermo Fisher Scientific, Waltham, MA, USA) to estimate the magnitude of enrichment. After quality control, captured library sequencing was carried out on Illumina HiSeq2500 Analyzers (Illumina, San Diego, CA, USA) for 90 cycles per read to generate paired-end reads. Image analysis, error estimation, and base calling were carried out using the Illumina Pipeline software (version 1.3.4; Illumina, San Diego, CA, USA) to generate raw data. Previously published filtering criteria were used to generate “clean reads” for further analysis (38).

The “clean reads” (with a length of 90 bp), derived from targeted sequencing and filtering, were then aligned to the human genome reference (hg19), using the Burrows Wheeler Aligner Multi-Vision software package (39). The SOAPsnp software (40) and Samtools (41) were used to detect single-nucleotide variants and insertion/deletions. The single-nucleotide variants and insertions/deletions were filtered and estimated through multiple databases, including NCBI dbSNP, HapMap, 1000 human genome dataset (42), and a database of 100 Chinese healthy adults. The Human Gene Mutation Database (43) was used to screen mutations reported in published studies. To validate the mutation, the FECH region, harboring the mutation, was screened using the Sanger method. The ALAS2, CPOX, HMBS, UROS, ALAD, PPOX, and UROD genes of the proband were also sequenced.

3. Results

3.1. Characteristics of the Patients and Family Members

The proband was a 16-year-old Han female, living in Jilin province, who was admitted to the First Hospital of Jilin University in 2017. Since her childhood, when she was exposed to sunlight, painful erythema and edema would immediately present on the palmar and dorsal aspects of her hands. The painful photosensitivity became severe during the summer and autumn. The skin over the joints on the dorsal aspects of her hands had become thick and waxy for several years. She took diphenhydramine as a treatment. One month prior to admission, she complained of jaundice, abdominal distension, severe abdominal pain, constipation, nausea, vomiting, neuralgia of all four limbs, and headache. Her family members, including her grandmother, mother, aunt, and uncle also had painful photosensitivity, and lived in Jilin Province. Her grandmother had died due to other reasons at the age of 72 years old, and her uncle had died from liver failure for an unknown reason at the age of 31 years old (Table 1).

Table 1.

Clinical Manifestations and Genetic Test Results of the EPP Family

SubjectsAgeEthnicityClinical SymptomsC.910 C>TIVS 1-23C>TIVS 3-48T>C
Proband16HanSkin, liverC/TC/TC/T
Grandmother72HanSkin---
Mother42HanSkinC/TC/TC/T
Father47HanNoneC/CC/TC/T
Aunt52HanSkinC/TC/TC/T
Aunt’s son30HanNoneC/TC/CT/T
Aunt’s daughter29HanNoneC/CC/TC/T
Uncle31HanSkin, liver---
Uncle’s wife52HanNoneC/CT/TC/C
Uncle’s daughter24HanNoneC/CT/TC/C

Physical examination revealed marked jaundice and thickening of the skin over the joints on the backs of her hands. Her liver function test results (Table 2) showed that she had high levels of aspartate transaminase (AST), alanine aminotransferase (ALT), r-glutamyl-transpeptidase (r-GGT), alkaline phosphatase (ALP), and total bilirubin (TBIL). Routine blood tests showed normocytic anemia and an elevated reticulocyte percentage (Table 2). Her anti-nuclear antibody test and extractable nuclear antigen levels had not increased. Her blood tests for hepatitis A, B, C, and E viruses were negative, and her blood test for ceruloplasmin was normal. Urine porphyrins were normal. Free protoporphyrin in her erythrocytes was elevated (Table 2). Therefore, a diagnosis of EPP was made. Genetic testing was performed to confirm the diagnosis. She died due to liver failure one month after admission.

Table 2.

Laboratory Test Results of the Proband

ParameterValueNormal Reference
Aspartate transaminase (AST)385 U/L15 - 40 U/L
Alanine aminotransferase (ALT)345 U/L9 - 50 U/L
r-glutamyl-transpeptidase (r-GGT)1032.4 U/L10 - 60 U/L
Alkaline phosphatase (ALP)446 U/L45 - 125 U/L
Total bilirubin (TBIL)390.6 μmol/L6.8 - 30 μmol/L
Direct bilirubin (DBIL)244.6 μmol/L0 - 8.6 μmol/L
Hemoglobin88 g/L115 - 150 g/L
Reticulocyte6.31%0.59 - 2.07%
Antinuclear antibodyNormal
Extractable nuclear antigenNormal
Hepatitis A, B, C, and E virusesNegative
Protoporphyrin80.1 µg/gHb0 - 4.7 μg/gHb

The proband’s father, mother, aunt, aunt’s daughter and son, uncle’s wife, and uncle’s daughter showed normal routine blood test results as well as liver and renal function.

3.2. Genotyping

Genetic screening showed that there were no variations or deletions in the sequences of ALAS2, CPOX, HMBS, UROS, ALAD, PPOX, and UROD of the proband. A heterozygous nucleotide change (c.910 C>T) and two heterozygous nucleotide polymorphism variations (IVS 1-23 C>T and IVS 3-48 T>C) were detected in the FECH gene of the proband, her mother, and her aunt. The heterozygous nucleotide change (c.910 C>T) in the FECH gene was also detected in her aunt’s son (Figures 1 and 2), who was asymptomatic. No nucleotide polymorphism variations (IVS 1-23 C>T and IVS 3-48 T>C) were detected in the FECH gene of the proband’s male cousin (Figures 1 and 2). The c.910 C>T mutation resulting in p.Arg304Ter is a null mutation (Table 1).

Pedigree of the Chinese family with erythropoietic protoporphyria analyzed in this study.
Pedigree of the Chinese family with erythropoietic protoporphyria analyzed in this study.
Figure 1.

Pedigree of the Chinese family with erythropoietic protoporphyria analyzed in this study.

C > T transition at FECH c.910 . ↓, shows the C > T mutation at FECH c.910 , which caused the change of the arginine codon to a premature stop codon. The sequence shown in the figure is of the negative strand.
C > T transition at FECH c.910 . ↓, shows the C > T mutation at FECH c.910 , which caused the change of the arginine codon to a premature stop codon. The sequence shown in the figure is of the negative strand.
Figure 2.

C > T transition at FECH c.910 . ↓, shows the C > T mutation at FECH c.910 , which caused the change of the arginine codon to a premature stop codon. The sequence shown in the figure is of the negative strand.

3.3. Allele Frequency of the IVS 1-23 C/T and IVS 3-48 T/C Polymorphisms

The allele frequencies of the IVS 1-23 C/T and IVS 3-48 T/C polymorphisms in the northeast Chinese Han population were assessed by genotyping 52 healthy individuals without porphyria, liver, or skin disease. There were 25 females and 27 males; the average age was 42 ± 9.9 years old. They were all of Han ethnicity, living in Jilin province (Table 3). It was found that for allele IVS 1-23, 28 individuals had the C/C genotype, 19 had the C/T genotype, and five had the T/T genotype, resulting in an IVS 1-23T allele frequency of 27.9% in the northeast Chinese Han population. It was also found that for IVS 3-48, 26 individuals had the T/T genotype, 20 had the C/T genotype, and six had the C/C genotype, resulting in an IVS 3-48C allele frequency of 30.8% in the northeast Chinese Han population (Table 4).

Table 3.

Demographic Features of the Healthy Controls

Controls
Gender (female/male)25/27
Age (y)42 ± 9.9
EthnicityHan
Residential locationJilin province in northeast China
Table 4.

Number of Subjects with Genotypic and Allelic Frequencies of the IVS 1-23C/T and IVS 3-48T/C Shift in 52 Northeast Chinese Han controls

No. of Subjects with GenotypeAllelic Frequency
C/CC/TT/TTC
IVS 1-23281950.2790.921
IVS 3-48620260.6920.308

5. Discussion

In the present study, the proband presented clinical manifestations of photosensitivity, thick and waxy skin, and severe liver dysfunction, which are typical symptoms of EPP (1-7) accompanied with liver dysfunction (5, 8-13). Different degrees of severity of liver disease, include cholelithiasis, mild increased levels of aminotransferase, jaundice, and progressive end-stage liver disease. Furthermore, FECH deficiency causes accumulation of protoporphyrin in hepatocytes and bile canaliculi, leading to oxidative stress, cell damage, cytolysis, cholestasis, and further protoporphyrin retention (1, 44).

The presence of the same symptoms in her grandmother, mother, aunt, and uncle indicated that the proband might have had a genetic disease, which was further confirmed by the presence of the mutation of c.910 C>T in the FECH gene of the proband, her mother, her aunt, and a male cousin.

The mutation of c.910 C>T in the FECH gene found in this Chinese family is not among the 190 mutations identified in the FECH gene of patients with EPP throughout the world, indicating that this mutation has not been identified previously (43). The mutation corresponds to a C>T substitution, resulting in the exchange of an arginine codon to a premature stop codon at codon 304, and leading to loss of a domain containing one section of the active-site pocket, six α-helices (α12-α17), two β-sheets (β7-β8), and part of the binding motif for the (2Fe-2S) cluster in the FECH protein (45). The null mutation mediated clinical manifestations of severe liver dysfunction in the proband, which is consistent with the observations that carriers of null-allele mutations in the FECH gene are more likely to develop liver disease than are carriers of missense mutations (25, 26). Although it was difficult to determine whether the mutation was autosomal dominant or autosomal recessive, based on the phenotype and the pedigree, genetic screening indicated that the proband, her symptomatic mother, and her aunt were c.910 T mutation heterozygous. The clinical manifestations were only expressed in the proband, her mother, and her aunt, who had a heterozygous c.910 T mutation, a heterozygous IVS 1-23 C>T mutation, and a heterozygous IVS 3-48 T>C mutation; while they were not expressed in the proband’s male cousin, who had a heterozygous c.910 T mutation in the absence of a heterozygous IVS 1-23 C>T or IVS 3-48 T>C mutation, indicating that the phenotypic expression of the c.910 T mutation needs the co-existence of the c.910 T mutation with the heterozygous IVS 1-23 C>T mutation or the IVS 3-48 T>C mutation (14, 22-24, 32-37). Thus, the findings support the observation that the phenotypic expression of EPP results from the coinheritance of a low-expressed wild-type allele and a mutant allele (16, 17). Although the proband, her mother, and her aunt had the same genotype, only the proband had severe liver disease, suggesting that there might be other risk factors involved in the pathogenesis of EPP, such as epigenetic changes (31). Future studies are required for further clarification.

The observed IVS 3-48C allele frequency was 30.8% in the northeast Chinese Han population, which supports that there is an east-west distribution gradient of the IVS 3-48C allele in China (22-24). The IVS 1-23T allele frequency was found to be 27.9% in the northeast Chinese Han population, which is higher than that found in France (16). The relatively high frequencies of the IVS 3-48C allele and the IVS 1-23T allele in the northeast Chinese Han population implicate that it is not rare for mutations in the FECH gene to come together with alleles of IVS 3-48C and IVS 1-23T through the reproductive recombination process, as observed in the Chinese family in the present study.

One limitations of the present study was its small sample size. Since EPP is a rare inherited disorder, only a very small number of patients and control subjects were included in this study. However, the definite pedigree relationship among the patients and other members of the same family helped elucidate the inheritance pattern of the disease.

In conclusion, a new nonsense mutation of c.910 C>T was identified in the FECH gene, which expressed EPP with severe liver dysfunction when a heterozygous allele of the mutation was co-inherited with heterozygous IVS 3-48C and IVS 1-23T, in a Chinese family.

Acknowledgements

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