Case Report Open Access
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World J Clin Cases. Nov 26, 2022; 10(33): 12440-12446
Published online Nov 26, 2022. doi: 10.12998/wjcc.v10.i33.12440
Novel TINF2 gene mutation in dyskeratosis congenita with extremely short telomeres: A case report
Verónica Judith Picos-Cárdenas, Laboratorio de Genética, Facultad de Medicina, Universidad Autónoma de Sinaloa, Culiacán 80018, Sinaloa, Mexico
Saúl Armando Beltrán-Ontiveros, Centro de Investigación y Docencia en Ciencias de la Salud, Hospital Civil de Culiacán, Universidad Autónoma de Sinaloa, Culiacán 80030, Sinaloa, Mexico
José Alfonso Cruz-Ramos, Departamento de Clínicas Médicas, Centro Universitario de Ciencias de la Salud, Universidad de Guadalajara, Guadalajara 44340, Jalisco, Mexico
José Alfredo Contreras-Gutiérrez, Facultad de Medicina, Universidad Autónoma de Sinaloa, Culiacán 80018, Sinaloa, Mexico
Eliakym Arámbula-Meraz, Emir Adolfo Leal-León, Dora María Cedano-Prieto, Laboratorio de Genética y Biología Molecular, Facultad de Ciencias Químico-Biológicas, Universidad Autónoma de Sinaloa, Culiacán 80010, Sinaloa, Mexico
Carla Angulo-Rojo, Laboratorio de Neurociencias, Facultad de Medicina, Universidad Autónoma de Sinaloa, Culiacán 80018, Sinaloa, Mexico
Alma Marlene Guadrón-Llanos, Laboratorio de Diabetes y Comorbilidades, Facultad de Medicina, Universidad Autónoma de Sinaloa, Culiacán 80018, Sinaloa, Mexico
Juan Pablo Meza-Espinoza, Facultad de Medicina, Universidad Autónoma de Tamaulipas, Matamoros 87349, Tamaulipas, Mexico
ORCID number: Verónica Judith Picos-Cárdenas (0000-0002-4320-9619); Saúl Armando Beltrán-Ontiveros (0000-0002-8411-0957); José Alfonso Cruz-Ramos (0000-0002-5791-612X); José Alfredo Contreras-Gutiérrez (0000-0003-3774-1278); Eliakym Arámbula-Meraz (0000-0003-1026-7430); Carla Angulo-Rojo (0000-0002-5097-2444); Alma Marlene Guadrón-Llanos (0000-0003-4782-6398); Emir Adolfo Leal-León (0000-0001-9927-5917); Dora María Cedano-Prieto (0000-0002-4204-2175); Juan Pablo Meza-Espinoza (0000-0003-2621-7649).
Author contributions: Picos-Cárdenas VJ conceptualization, data collection, and manuscript preparation; Beltrán-Ontiveros SA, Contreras-Gutiérrez JA, Arámbula-Meraz E, and Angulo-Rojo C performed clinical examination and data analysis; Cruz-Ramos JA telomere study and critical review; Guadrón-Llanos AM, Leal-León EA, Cedano-Prieto DM collection of samples and interpretation of molecular studies; Meza-Espinoza JP supervision, drafting, reviewing, and editing. All the authors approved the final version of the manuscript.
Informed consent statement: Written consent was obtained from the patient’s parents for the publication of this case and the accompanying images.
Conflict-of-interest statement: All the authors indicated no conflicts of interest.
CARE Checklist (2016) statement: The authors have read the CARE Checklist (2016). The manuscript was prepared and revised according to the CARE Checklist (2016).
Open-Access: This article is an open-access article that was selected by an in-house editor and fully peer-reviewed by external reviewers. It is distributed in accordance with the Creative Commons Attribution NonCommercial (CC BY-NC 4.0) license, which permits others to distribute, remix, adapt, build upon this work non-commercially, and license their derivative works on different terms, provided the original work is properly cited and the use is non-commercial. See: https://creativecommons.org/Licenses/by-nc/4.0/
Corresponding author: Juan Pablo Meza-Espinoza, PhD, Researcher, Facultad de Medicina, Universidad Autónoma de Tamaulipas, Sendero Nacional km 3, Matamoros 87349, Tamaulipas, Mexico. sirol1073@yahoo.com.mx
Received: September 13, 2022
Peer-review started: September 13, 2022
First decision: September 26, 2022
Revised: October 13, 2022
Accepted: October 20, 2022
Article in press: October 20, 2022
Published online: November 26, 2022

Abstract
BACKGROUND

Dyskeratosis congenita is a rare disease characterized by bone marrow failure and a clinical triad of oral leukoplakia, nail dystrophy, and abnormal skin pigmentation. The genetics of dyskeratosis congenita include mutations in genes involved in telomere maintenance, including TINF2.

CASE SUMMARY

Here, we report a female patient who presented thrombocytopenia, anemia, reticulate hyperpigmentation, dystrophy in fingernails and toenails, and leukoplakia on the tongue. A histopathological study of the skin showed dyskeratocytes; however, a bone marrow biopsy revealed normal cell morphology. The patient was diagnosed with dyskeratosis congenita, but her family history did not reveal significant antecedents. Whole-exome sequencing showed a novel heterozygous punctual mutation in exon 6 from the TINF2 gene, namely, NM_001099274.1:c.854delp.(Val285Alafs*32). An analysis of telomere length showed short telomeres relative to the patient’s age.

CONCLUSION

The disease in this patient was caused by a germline novel mutation of TINF2 in one of her parents.

Key Words: Dyskeratosis congenita, TINF2, Germline mutation, Novel mutation, Short telomeres, Case report

Core Tip: Dyskeratosis congenita, characterized by a clinical triad of oral leukoplakia, nail dystrophy, and abnormal skin pigmentation, is a rare disease caused by mutations in genes governing telomere maintenance, including TINF2. We performed whole-exome sequencing in a female pediatric patient who presented with dyskeratosis congenita, and subsequently, a novel heterozygous mutation in exon 6 of the TINF2 gene was detected: NM_001099274.1:c.854delp.(Val285Alafs*32). An analysis of telomere length demonstrated short telomeres relative to the girl’s age. Patients with TINF2 mutations have more severe disease, so their detection is necessary to provide timely treatment.



INTRODUCTION

Dyskeratosis congenita is a rare genetic disease whose prevalence in the general population has been estimated at nearly 1/1000000[1]. This disorder is characterized by bone marrow failure and a typical clinical triad comprised of oral leukoplakia, nail dystrophy, and abnormal skin pigmentation. The risk of aplastic anemia, myelodysplastic syndrome, and leukemia is elevated in patients with this condition[2,3]. Other clinical findings in dyskeratosis congenita include pulmonary fibrosis, liver cirrhosis, and premature hair graying[4]. The genetics of dyskeratosis congenita involve mutations in genes that govern the maintenance of telomeres; therefore, this disorder is marked, molecularly, by a progressive shortening of telomeres[5,6]. The genes associated with dyskeratosis congenita are DKC1, TERC, TERT, TINF2, RTEL1, PARN, ACD, NOP10, NHP2, TERT, USB1, and WRAP53[2,3,7] (Table 1). Pathogenic variants in any of these genes have been identified in most individuals who meet diagnostic criteria for dyskeratosis congenita[3]. Because of this locus heterogeneity, there is a wide clinical variation among patients with this syndrome[8]. Here, we report the case of a girl with dyskeratosis congenita who carries a previously undescribed germline mutation in the TINF2 gene and an extremely short telomere length.

Table 1 Genetic spectrum of dyskeratosis congenita[1,3].
Gene
Chromosome
Inheritence pattern
Frequency, %
Main mutation types
DKC1Xq28XLRApproximately 25Missense
TINF214q12ADApproximately 12Missense
TERC3q26ADApproximately 5Point and deletions
TERT5p15AD, ARApproximately 5Missense
USB116q21ARApproximately 2Frameshift and nonsense
RTEL120q13AR, ADApproximately 2Missense
CTC117p13ARApproximately 1Missense and frameshift
NHP25q35AR< 1Missense
NOP1015q14AR< 1Missense
WRAP5317p13AR< 1Missense
ACD16q22AD, AR< 1Missense and frameshift
PARN16p13AR, AD< 1Frameshift
CASE PRESENTATION
Chief complaints

A 13-year-old Mexican female patient, height 151.0 cm and weight 48.0 kg, was found to have thrombocytopenia, anemia, abnormal skin pigmentation, dystrophic nails, and leukoplakia on the tongue.

History of present illness

The patient was the product of the second pregnancy of healthy nonconsanguineous parents (both parents were 31 years old at the time of birth). At the age of 5 years, she was detected to have thrombocytopenia and anemia (platelets 26000/mm3 and hemoglobin 9.0 g/dL); peripheral blood cell smears showed normal morphology and no evidence of blasts. She was thought to have primary immune thrombocytopenia. Prednisone (1 mg/kg/d) was administered as therapy for 21 d. After the administration of prednisone, platelet and hemoglobin counts have fluctuated from 32000/mm3 to 110000/mm3 and 9.5 g/dL to 11.7 g/dL, respectively.

When the patient was 9 years old, she was suspected to have systemic lupus erythematosus and mixed connective tissue disease due to her nail dystrophy and neck pigmentation abnormalities, but an antinuclear antibody test was negative. Methotrexate was administered as prophylaxis regardless. Around this time, an esophagogram was performed due to her difficulty swallowing since childhood; this revealed esophageal stenosis requiring two endoscopies for dilation. At the age of 11, dyskeratosis congenita was suspected due to the progression of reticulate pigmentation to the entire upper trunk, the presence of leucoplakia on the tongue, and the evolution of fingernails and toenails dystrophy; a molecular study was subsequently performed.

History of past illness

The patient had no history of other significant diseases.

Personal and family history

The patient had a healthy older brother, and family history did not indicate any significant morbidities.

Physical examination

At the age of 6, the patient presented with microcephaly, reticulate pigmentation in the neck, neckline, and axillae, dystrophic nails on hands and feet (Figure 1A and B), and lacrimal obstruction in the right eye. At the age of 11, she showed leukoplakia on the tongue (Figure 1C), and her reticulate pigmentation progressed to the entire upper trunk (Figure 1D).

Figure 1
Figure 1 Clinical findings in the patient. A: Dystrophic fingernails; B: Dystrophic toenails; C: White patches on the tongue representing leukoplakia; D: Upper trunk showing reticulate skin pigmentation.
Laboratory examinations

A histopathological study of the skin showed dyskeratocytes (Figure 2). Although previous peripheral blood smears showed normal leukocyte counts and the absence of blasts throughout the disease, a bone marrow biopsy was performed, which revealed normal cellularity.

Figure 2
Figure 2 Histopathological study. A and B: Skin biopsy images showing dyskeratocytes. The arrows point to these abnormal cells.
Whole-exome sequencing

Whole-exome sequencing analysis was performed according to the manufacturer’s protocol. DNA was enzymatically fragmented and hybridized with CentoXomeTM (CENTOGENE, Rostock, Germany). Libraries were generated with Illumina-compatible adapters and sequenced on the Illumina platform (Illumina, Inc., San Diego, CA, United States). Sequenced readings were aligned to the hg19 version of the human genome (Genome Reference Consortium GRCh37) using validated software (Rostock, Germany). All variants reported in the Human Gene Mutation Database (HGMD®), ClinVar, and CentoMD, as well as those in which the frequency of the least common allele was less than 1% in the Single Nucleotide Polymorphism database (dbSNP) and the Genome Aggregation Database (gnomAD) were considered. After analysis, a novel mutation, Chr14(GRCh37):g.24709832del NM_001099274.1:c.854delp.(Val285Alafs*32), was identified in exon 6 of the TINF2 gene. This mutation was verified by Sanger sequencing. Bidirectional sequencing and comparison to the coding sequence of TINF2 was performed (Figure 3). The reference sequence was NM_001099274.1.

Figure 3
Figure 3 Sequencing study. Plot showing the identification of the mutation in the TINF2 gene (deletion of the T in the position 250; shaded area). Courtesy of Centogene AG, Rostock, Germany.
Telomere analysis

To assess telomere length, genomic DNA was extracted from peripheral blood leukocytes using the Flexigene DNA kit (QIAGEN, Hilden, Germany) and qPCR was performed using the Absolute Human Telomere Length and Mitochondrial DNA Copy Number Dual Quantification qPCR kit (ScienCell Research Laboratories, San Diego, CA, United States) on a CFX96 Touch Real-Time PCR Detection System (Bio-Rad, Hercules, CA, United States) according to the supplier’s recommendations. The analysis showed an absolute telomere length of 2.80 ± 0.09 kb.

FINAL DIAGNOSIS

Based on clinical features and molecular analysis, the patient was diagnosed with dyskeratosis congenita.

TREATMENT

Prednisone (1 mg/kg/d) is administered as therapy for 21 d, whenever platelet count drops by nearly 30000/mm3.

OUTCOME AND FOLLOW-UP

Hopefully, the patient has had a favorable evolution, as she has not developed aplastic anemia or bone marrow failure, although she is currently off medication.

DISCUSSION

Dyskeratosis congenita is caused more than 99% of the time by a germline mutation in one of the parents[9], as was the case of our patient, who presented with the typical triad of this disease: Dystrophy in fingernails and toenails, leukokeratosis plaques on the tongue, and reticulate skin pigmentation. Mutations in the TINF2 gene (which encodes the TIN2 protein, a component of the shelterin telomere protection complex)[2] represent the second most common cause of dyskeratosis congenita, accounting for approximately 12% of the cases, only after mutations in the DKC1 gene (approximately 25%)[1]. It is well known that patients with a mutation in the TINF2 gene have a more severe course and a higher risk of developing aplastic anemia before the age of 10 years[6]. To date, there are more than 200 punctual variations in the TINF2 gene recorded in the ClinVar database. Most of them result in missense mutations, eight in nonsense, and almost twenty are frameshift mutations (Table 2), although some are associated with Revesz syndrome, a more severe variant of dyskeratosis congenita. Most pathogenic mutations occur in exon 6, principally between codons 280 and 288[10]. The mutation detected in this patient was a deletion of a nucleotide (frameshift), which also occurred in exon 6, codon 285, and caused an amino acid change at position 285 and a stop codon 31 amino acids later.

Table 2 Frameshift mutations in TINF2 causing dyskeratosis congenita[10].
Location (GRCh37)
Mutation
Protein change
Chr14:24709067NM_001099274.3(TINF2):c.1292del (p.Pro431fs)P431fs
Chr14:24709132NM_001099274.3(TINF2):c.1227del (p.Leu410fs)L410fs
Chr14:24709288-24709289NM_001099274.3(TINF2):c.1202dup (p.Asn401fs)N401fs
Chr14:24709507-24709508NM_001099274.3(TINF2):c.1090dup (p.Leu364fs)L364fs
Chr14:24709627-24709628NM_001099274.3(TINF2):c.1058dup (p.Glu354fs)E354fs
Chr14:24709676NM_001099274.3(TINF2):c.1010del (p.Gly337fs)G337fs
Chr14:24709794NM_001099274.3(TINF2):c.892del (p.Gln298fs)Q298fs
Chr14:24709836-24709837NM_001099274.3(TINF2):c.849dup (p.Thr284fs)T284fs
Chr14:24709860NM_001099274.3(TINF2):c.826del (p.Arg276fs)R276fs
Chr14:24710080NM_001099274.3(TINF2):c.606del (p.Glu202fs)E202fs
Chr14:24710937-24710938NM_001099274.3(TINF2):c.342_343del (p.Phe114fs)F114fs
Chr14:24711135-24711136NM_001099274.3(TINF2):c.257_258del (p.His86fs)H86fs
Chr14:24711394-24711395NM_001099274.3(TINF2):c.144_145insTT (p.Val49fs)V49fs

While telomere shortening is a molecular feature of dyskeratosis congenita[5], this is dramatic in patients with TINF2 mutations[11], as their telomere lengths are significantly shorter than those of patients with DKC1 mutations[6]. Our case showed an absolute telomere length of 2.80 ± 0.09 kb, which is considered very short relative to the patient's age. As a reference, a study performed on healthy young women aged 18 to 30 years showed an absolute telomere length of 4.59 ± 0.24 kb[12]. TIN2 is important for telomere protection, and TIN2 deficiency increases the risk of telomeric DNA damage and consequent telomere shortening[13-15]. Short telomeres are known to cause premature aging and increase the risk of developing cancer[16]. Accordingly, patients with dyskeratosis congenita have a higher risk of developing bone marrow failure, acute leukemia, myelodysplastic syndrome, and squamous cell carcinoma of the head and neck[3]. However, despite her extremely short telomere length, our patient has had a favorable evolution, as she has not developed aplastic anemia or bone marrow failure, although she is currently off medication.

CONCLUSION

Since patients with mutations in the TINF2 gene have a more severe course and a higher risk of developing aplastic anemia[6], it is important to detect patients with such mutations to follow them more frequently, mainly through blood cytometry, and, if necessary, to provide some treatment, as has been done in this patient. In the meantime, she and her parents are hoping for an orphan or experimental drug that will impede the progression of the disease.

The strength of this case report is that it was approached with a clinical, genetic, and pathological focus. The main limitation is that it is a single case.

ACKNOWLEDGEMENTS

We thank the proband and her parents for their collaboration and support for the publication of this case. We also thank the biomedicine and genomic biotechnology students, Liliana Itzel Patrón Baro (fellowship PROFAPI-UAS-2022, Pro_A3_031) and Lucero García Hernández, respectively, for the technical and samples collection support. Special thanks to Centogene AG, Germany for its support for the whole-exome sequencing analysis.

Footnotes

Provenance and peer review: Unsolicited article; Externally peer reviewed.

Peer-review model: Single blind

Specialty type: Dermatology

Country/Territory of origin: Mexico

Peer-review report’s scientific quality classification

Grade A (Excellent): 0

Grade B (Very good): B

Grade C (Good): C, C

Grade D (Fair): 0

Grade E (Poor): 0

P-Reviewer: Ishida T, Japan; Vyshka G, Albania S-Editor: Liu JH L-Editor: A P-Editor: Liu JH

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