Familial neurohypophyseal diabetes insipidus (FNDI) is a rare single-gene disorder caused by mutations of the arginine vasopressin-neurophysin II (AVP-NPII) gene. These changes impair the release of vasopressin from the posterior pituitary gland. In the present study, the AVP-NPII gene of a Chinese adult patient with central diabetes insipidus, the patient's symptomatic mother and an asymptomatic sister of the patient was sequenced. Examination of the family history revealed cases of FNDI across four generations. Gene sequencing analysis revealed a novel heterozygous mutation, c.268A>T (p.Lys90Ter), in exon 2 of the AVP-NPII gene, in the patient and the patient's mother, which led to the loss of 6 cysteine residues and aberrant disulfide bonds, which is predicted to alter the mature protein structure. The present study identified a novel heterozygous nonsense mutation of the AVP-NPII gene associated with FNDI, which broadens the spectrum of known mutations associated with this disorder and contributes to the understanding of its molecular basis.
Neurohypopheseal diabetes insipidus is a disorder caused by increased urine production and volume depletion due to vasopressin (AVP) deficiency. Most cases are linked with structural damage of the hypothalamus, pituitary stalk or posterior pituitary gland (1). Familial neurohypophyseal diabetes insipidus (FNDI) is a rare inherited disease that accounts for only 1% of central diabetes insipidus cases (2). The disorder usually presents in early childhood with polyuria and polydipsia, and follow-up evaluation frequently reveals loss of the posterior pituitary bright spot on T1-weighted magnetic resonance imaging (MRI) (3–5). FNDI is caused by mutations of the arginine vasopressin-neurophysin II (AVP-NPII) gene (GenBank ID, NM_000490.4), which is located on chromosome 20 and encodes a preproprotein that is proteolytically processed to generate multiple products, including AVP, neurophysin II and copeptin (6). Biosynthesis of AVP is tightly regulated by translation and post-translational processes, including enzymatic cleavage of the AVP-neurophysin II prohormone and appropriate secretion of AVP into the circulation upon various stimuli (7,8). Since the publication of the first genetic study on FNDI (9), ~70 mutations have been described and all are located within the 2.5 kb-long AVP-NPII gene. The proposed pathogenic mechanisms include aberrant preprohormone processing leading to the gradual destruction of AVP-secreting cells (10) and mutations that alter the amino acid structure of the mature AVP hormone (11).
The present study reports on a female patient with autosomal dominant FNDI linked to a novel nonsense mutation of AVP-NPII gene and her extended family. The clinical, biochemical and radiological characteristics of the patient were investigated. The novel nonsense mutation was also identified in another affected family member.
Patients and methodsPatients
A 46-year-old Chinese woman was referred to Peking Union Medical College Hospital (Beijing, China) for evaluation of acute urinary retention. A urinary catheter was placed to alleviate severe bladder distension. She reported having polyuria and polydipsia since age 13, but had not sought any medical care, as she always had access to water. The patient was born at term without any complications and had a normal pubescence. A total of 12 additional family members spanning four generations, including the patient's mother and younger brother, also had teenage-onset of polyuria and polydipsia. Daily urine volumes varied from 6.0 to 15.0 liters. No mental retardation or delay in puberty had been identified. The average final body height was 160.1 cm for females and 175.2 cm for male members of the family. The pedigree of the family is presented in Fig. 1.
Clinical, laboratory and radiological assessments
Clinical data were collected in accordance with the Declaration of Helsinki. Written informed consent was obtained from the patient (IV-8), the patient's mother (III-7) and an asymptomatic sister of the patient (IV-7). A water deprivation test followed by the administration of vasopressin was performed to diagnose central diabetes insipidus as described previously (12). Enhanced MRI of the hypothalamo-hypophyseal area and pelvis was performed. The residual urine volume was measured by performing an ultrasound scan of the bladder.
Genomic DNA extraction, amplification and sequencing of the AVP-NPII gene
The AVP-NPII gene was analyzed by direct sequencing from genomic DNA extracted from leucocytes of peripheral blood with the QIAamp DNA Mini kit (Qiagen GmbH). In brief, PCR was performed in a 40-µl reaction volume containing 100 ng genomic DNA, 20 µl 2X GC PCR buffer, 0.1 µM of each dNTP, 0.1 µM of each primer and 2.5 units of rTaq polymerase (Takara Bio, Inc.) in a thermocycler (ABI 9700; Applied Biosystems; Thermo Fisher Scientific, Inc.). All genomic DNA was denatured at 94°C for 10 min and amplified with 35 cycles. For exon 1, the cycles were programmed as 94°C for 30 sec, 60°C for 30 sec and 72°C for 40 sec. The cycling conditions for exons 2 and 3 were programmed as follows: Module 1 was 94°C for 5 min, 65°C for 5 min and 74°C for 5 min (1 cycle); module 2 was 94°C for 1 min, 65°C for 1 min and 74°C for 4 min (35 cycles); module 3 was 74°C for 10 min; module 4 was a hold at 4°C. Primers for amplification and sequencing of the AVP-NPII gene are provided in Table I. Amplified products were detected by agarose gel electrophoresis and sequenced using an ABI 3730 DNA analyzer (Applied Biosystems; Thermo Fisher Scientific, Inc.).
Three-dimensional structural models of the predicted wild-type and mutant proteins were generated and comparisons between the proteins were performed using the PHYRE2 Protein Fold Recognition Server database (http://wwwsbg.bio.ic.ac.uk/phyre2) and the SWISS-MODEL protein structure homology-modelling server (http://swissmodel.expasy.org) as reported previously (5).
ResultsClinical and MRI assessments
Diabetes insipidus was confirmed via a standard water deprivation test. After 8 h of water deprivation, the plasma osmolality rose from 301 to 315 mOsm/kg and the urine osmolality rose from 50 to 65 mOsm/kg. 4 U vasopressin was subsequently injected intramuscularly. Following 2 h, the plasma osmolality decreased from 315 to 302 mOsm/kg and the urine osmolality increased from 65 to 587 mOsm/kg. As presented in Fig. 2A, the cranial MRI revealed a high signal region in the posterior lobe of the pituitary gland. Serum cortisol, thyroid function, growth hormone levels, insulin-like growth factor 1 and estrogen were all within normal ranges. Pelvic MRI revealed a significantly enlarged urinary bladder (Fig. 2B). The daily urine output decreased from 15 l to 2 l after 1 week of treatment with 100 µg 1-deamino-8-D-arginine-vasopressin three times per day. The dosage was then tapered to 50 µg, which was administered 3 times per day and maintained thereafter. The residual urine volume decreased from 1,250 to 4 ml and the urinary catheter was removed.
PCR and sequencing
The AVP-NPII genes were sequenced from the patient, the patient's mother and a sister of the patient. Sequence analyses of the patient's entire AVP-NPII coding region revealed a novel heterogeneous nonsense mutation at codon 268 (c.268A>T), which results in a substitution in exon 2 of Lys (AAG) with a stop codon (TAG) and corresponds to lysine 90 of the NPII moiety (p.Lys90Ter) (Fig. 3A). The same mutation was identified in the patient's mother (Fig. 3B), but not in the patient's sister, who had a normal phenotype (Fig. 3C). The 3-D structures of the wild-type and mutant (p.Lys90Ter) AVP-NPII proteins were modeled using the above-mentioned computational servers. As presented in Fig. 4, the Lys90Ter mutation is located in the middle of NPII and leads to the loss of 74 amino acids, including 6 cysteine residues. The loss of cysteine residues results in aberrant disulfide bonds, which is expected to alter the protein structure.
Discussion
The present study reports on a novel p.Lys90Ter mutation identified in exon 2 of the AVP-NPII gene that is linked with FNDI. The pedigree examined included cases spanning four generations, with no apparent gender preponderance among affected individuals. Similar to the observations of previously published studies on FNDI, the affected individuals in the present study were normal at birth and gradually developed symptoms of vasopressin deficiency beginning in childhood or adolescence (13). None of the subjects had any mental deficits or impaired pubescent development.
FNDI is a rare, single-gene disorder caused by mutations in the 2.5-kb AVP-NPII gene located in chromosome region 20p13 (14,15). The AVP-NPII gene has three exons: Exon 1 encodes a signal peptide, AVP, and the NH2-terminal portion of neurophysin II, exon 2 encodes the central region of neurophysin II and exon 3 encodes the COOH-terminal region of neurophysin II and copeptin. AVP is synthesized in the supraoptic nucleus and paraventricular nucleus of the hypothalamus and then packaged into neurosecretory vesicles along with its carrier protein neurophysin II. It is then transported axonally to the neurohypophysis. Most of the mutations reported to be associated with FNDI are located in the region encoding the NPII moiety, which is the intracellular binding protein for AVP. Several mutations are localized to the coding region for signaling peptide or AVP per se. The mutant NPII is assumed to interfere with axonal transport of intracellular AVP proteolysis (16,17).
A total of 7 mutations spanning all 3 exons of the AVP-NPII gene have been previously described in Chinese populations (Table II) (18–20), including 3 missense mutations in exon 2. To the best of our knowledge, the present study is the first to report on a nonsense mutation in exon 2 of the AVP-NPII gene in Chinese individuals. The mutation results in a preterm stop codon and thus a truncated NPII moiety. Wild-type pro-vasopressin has 164 amino acids and 7 disulfide bonds between all 14 cysteine residues (21). The mutant NPII loses 6 of these cysteine residues and the resultant aberrant disulfide bonds cause misfolding of the prohormone. As a result, the prohormone is likely retained within the endoplasmic reticulum and exceeds its capacity to tolerate the ‘unfolded protein response’, causing stress that may trigger apoptosis (22,23). However, further investigations are required to verify the molecular mechanisms underlying FNDI. It may be hypothesized that FNDI follows a pattern of autosomal dominant inheritance, which is consistent in the present pedigree.
Previous studies have described the MRI presentation of subjects with FNDI. In one study, the presence of a bright spot in the posterior lobe appeared to vary between members of the same family (5). In another case series, such a spot was entirely absent from all 13 patients (24). The MRI of the patient in the current study revealed a bright spot on the posterior lobe of pituitary gland. More serious urological complications are uncommon in these patients, as they retain a limited capacity to secrete AVP during severe dehydration.
In conclusion, the present study identified a novel nonsense mutation in the AVP-NPII gene linked with NDI in a Chinese patient whose family members shared a history of polyuria and polydipsia across four generations. This heterogeneous Lys90Ter mutation is located in the middle of NPII and leads to loss of 6 cysteine residues and aberrant disulfide bonds, which is expected to alter the mature protein structure. Although a number of studies have described variant mutations of NPII in FNDI, further elucidation of the molecular mechanisms underlying specific mutant interference with the axonal transport of intracellular AVP proteolysis are required.
Acknowledgements
Not applicable.
Funding
This work was supported by the Special Research Fund for Central Universities, Peking Union Medical College (grant no. 2017PT31004) and the CAMS Innovation Fund for Medical Science (grant no. CAMS-2016-I2M-1-002□2016-I2M-1-008).
Availability of data and materials
The datasets used and/or analyzed during the current study are available from the corresponding author on reasonable request.
Authors' contributions
HY analyzed and interpreted the patient data and wrote the primary manuscript. KY performed the PCR experiments. LW collected the blood samples of the patient and the patient's relatives and analyzed the gene sequencing data. FG supervised the experiments and data analysis. ZJ helped to interpret the patient's clinical data. HZ revised the primary manuscript and was a major contributor in writing the manuscript.
Ethics approval and consent to participate
The present study was approved by the ethics committee of Peking Union Medical College Hospital (Beijing, China).
Patient consent for publication
Written informed consent was obtained from the patient, the patient's mother and an asymptomatic sister prior to genetic testing and the publication of data and images in the present study.
Competing interests
The authors declare that they have no competing interests.
AbbreviationsAVP-NPII
arginine vasopressin-neurophysin II
FNDI
familial neurohypophyseal diabetes insipidus
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Pedigree of the family. The patient with diabetes insipidus is indicated by a solid symbol and an arrow. Family members with symptoms of polyuria and polydipsia are indicated by a filling of diagonal lines. Family members whose conditions were unknown are indicated with question marks. Squares indicate male and circles female subjects. Symbols that are crossed indicate deceased subjects.
MRI of the pituitary gland and pelvis. (A) Sagittal MRI of the pituitary gland. A high-signal region at the posterior lobe was present. (B) MRI of the pelvis revealed a significantly enlarged urinary bladder. MRI, magnetic resonance image.
Automated sequencing of the AVP-NPII gene in the patient, the patient's mother and the patient's asymptomatic sister. Sequencing of the coding region within Exon 2 of the AVP-NPII gene in (A) the patient and (B) the patient's mother revealed a heterozygous missense mutation (c.268A>T), as indicated by the arrow, which causes the substitution of AAG (Lys) by stop codon UAG. (C) No mutation was found in the patient's asymptomatic sister. AVP-NPII, arginine vasopressin-neurophysin II.
Three-dimensional protein structure prediction of (A) wild-type and (B) mutant (p.Lys90Ter) arginine vasopressin-NPII. The Lys90Ter mutation is located in the middle of NPII and leads to loss of 6 cysteine residues and aberrant disulfide bonds, which is likely to lead to an altered protein structure. NPII, neurophysin II.
Primer sequences for PCR of the arginine vasopressin-neurophysin II gene.
Exon/direction
Sequences (5′-3′)
1
Forward
ATGATCCCCTGCACAGACAG
Reverse
CTGCCCAGCCATGCCATG
2
Forward
TCGCTGCGTTCCCCTCCAACCCCTCGACTC
Reverse
CGCCCCCCCCCAGGCCCGCCCCCGCCGCGC
3
Forward
CCCAGGCGCCCGTGCTCACACGTCCTCCCG
Reverse
CCTCTCTCCCCTTCCCTCTTCCCGCCAGAG
Arginine vasopressin-neurophysin II gene mutations in familial neurohypophyseal diabetes insipidus reported in the Chinese population.