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This Article IMMEDIATE FREE ACCESS ARTICLE OA Abstract Full Text (PDF) Supplementary Table 1 OA All Versions of this Article: EJE-09-0615v1 161/5/731    most recent Alert me when this article is cited Alert me if a correction is posted Services Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Google Scholar Articles by Kapoor, R. R Articles by Hussain, K. PubMed PubMed Citation Articles by Kapoor, R. R Articles by Hussain, K.

Hyperinsulinism–hyperammonaemia syndrome: novel mutations in the GLUD1 gene and genotype–phenotype correlations

Developmental Endocrinology Research Group, Molecular Genetics Unit, London Centre for Paediatric Endocrinology and Metabolism, Great Ormond Street Hospital for Children NHS Trust, and The Institute of Child Health, University College London, 30 Guilford Street, London WC1N 1EH, UK¹ Institute of Biomedical and Clinical Science, Peninsula Medical School, Exeter EX2 5DW, UK² Department of Inherited Metabolic Disorders, Birmingham Children's Hospital, Birmingham B4 6NH, UK³ Metabolic Biochemistry, Hôpital Necker – Enfants Malades, Université Paris Descartes, Paris, France⁴ Clinical and Metabolic Genetics, Department of Pediatrics, Hamad Medical Corporation and Weil-Cornell Medical College, Doha, Qatar⁵ Department of Paediatric Endocrinology, Royal Manchester Children's Hospital and Alder Hey Children's Hospital, Manchester M27 4HA, UK⁶ Department of Child Health, Bristol Royal Hospital for Children, Bristol BS2 8BJ, UK

(Correspondence should be addressed to K Hussain; Email: k.hussain{at}ich.ucl.ac.uk)

This is an Open Access article distributed under the terms of the European Journal of Endocrinology's Re-use Licence which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

	Abstract

Top Abstract Introduction Research design and methods Results Discussion Conclusion Declaration of interest References

 
Background: Activating mutations in the GLUD1 gene (which encodes for the intra-mitochondrial enzyme glutamate dehydrogenase, GDH) cause the hyperinsulinism–hyperammonaemia (HI/HA) syndrome. Patients present with HA and leucine-sensitive hypoglycaemia. GDH is regulated by another intra-mitochondrial enzyme sirtuin 4 (SIRT4). Sirt4 knockout mice demonstrate activation of GDH with increased amino acid-stimulated insulin secretion.

Objectives: To study the genotype–phenotype correlations in patients with GLUD1 mutations. To report the phenotype and functional analysis of a novel mutation (P436L) in the GLUD1 gene associated with the absence of HA.

Patients and methods: Twenty patients with HI from 16 families had mutational analysis of the GLUD1 gene in view of HA (n=19) or leucine sensitivity (n=1). Patients negative for a GLUD1 mutation had sequence analysis of the SIRT4 gene. Functional analysis of the novel P436L GLUD1 mutation was performed.

Results: Heterozygous missense mutations were detected in 15 patients with HI/HA, 2 of which are novel (N410D and D451V). In addition, a patient with a normal serum ammonia concentration (21 µmol/l) was heterozygous for a novel missense mutation P436L. Functional analysis of this mutation confirms that it is associated with a loss of GTP inhibition. Seizure disorder was common (43%) in our cohort of patients with a GLUD1 mutation. No mutations in the SIRT4 gene were identified.

Conclusion: Patients with HI due to mutations in the GLUD1 gene may have normal serum ammonia concentrations. Hence, GLUD1 mutational analysis may be indicated in patients with leucine sensitivity; even in the absence of HA. A high frequency of epilepsy (43%) was observed in our patients with GLUD1 mutations.

	Introduction

Top Abstract Introduction Research design and methods Results Discussion Conclusion Declaration of interest References

 
The hyperinsulinism/hyperammonaemia (HI/HA) syndrome is a form of congenital HI (CHI) in which affected children have recurrent symptomatic hypoglycaemia together with a persistently elevated serum ammonia concentration. It has been shown that this disorder is caused by activating mutations in the GLUD1 gene that encodes for the intra-mitochondrial enzyme, glutamate dehydrogenase (GDH) (1). GDH is highly expressed in the liver, pancreatic β-cells, kidney and the brain (2). It catalyses the oxidative deamination of glutamate to -ketoglutarate and ammonia. In the pancreatic β-cells, -ketoglutarate enters the tricarboxylic acid cycle and leads to insulin exocytosis.

GDH is allosterically activated by leucine and inhibited by GTP (3). Activating mutations in the GLUD1 gene reduce the sensitivity of the enzyme to allosteric inhibition by GTP and ATP (4). The loss of inhibition by GTP leads to increased leucine-induced glutamate oxidation to -ketoglutarate. Hence, leucine sensitivity is manifested by postprandial hypoglycaemia (following protein-rich meals), which is a classical feature of this condition (5). The mechanism of the persistent HA, a striking and consistent feature of this condition, is not completely understood.

GDH is also inhibited by sirtuin 4 (SIRT4), an intra-mitochondrial enzyme (6) that is highly expressed in the pancreatic islets (6, 7). Hence, SIRT4 would be an ideal candidate gene to analyse in patients with HI/HA syndrome, where no mutations in the GLUD1 gene are found.

In this study, we report the phenotype and genotype of 20 patients with HI/HA syndrome. We also report a novel GLUD1 mutation in a patient with severe leucine sensitivity but a completely normal serum ammonia concentration. We highlight the high risk of epilepsy in patients with GLUD1 mutations and we discuss our findings of the SIRT4 gene analysis in a cohort of patients with HI/HA syndrome, where no mutations are identified in the GLUD1 gene.

	Research design and methods

Top Abstract Introduction Research design and methods Results Discussion Conclusion Declaration of interest References

 
We studied 20 patients with HI who were referred for mutational analysis of the GLUD1 gene either in view of HA (n=19) or leucine sensitivity (n=1). Sixteen patients were unrelated and four were related demonstrating vertical transmission of disease consistent with a dominant pattern of inheritance. The diagnosis of HI was based on diagnostic criteria described previously, i.e. inappropriately elevated insulin concentrations at the time of hypoglycaemia with corresponding low concentrations of plasma β-hydroxybutyrate and fatty acids. Clinical information (birth weight, age of presentation, treatment details, seizure history and family history) was collected from case notes and the referring clinicians. The clinical characteristics are presented as means and summarised in Table 1.

Molecular genetics

DNA was extracted from peripheral leukocytes using standard procedures. The exons of the GLUD1 gene, which encode the catalytic and allosteric domains of GDH (exons 6, 7, 10, 11 and 12), were amplified by PCR (for primer sequences see Supplementary Table 1, which can be viewed online at http://www.eje-online.org/supplemental/) and sequenced using BigDye Terminator v3.1 (Applied Biosystems, Warrington, UK). Sequencing reactions were analysed on the ABI 3730 (Applied Biosystems) and compared with the published sequence (M37154 [GenBank] ) using Mutation Surveyor software (SoftGenetics, Philadelphia, PA, USA). Mutation testing was performed on parental samples and microsatellite analysis of six markers on chromosome 20 was undertaken to confirm family relationships when a novel de novo mutation was identified (primers available on request).

When no GLUD1 mutation was identified, exons 1–3 of the SIRT4 gene were analysed. All exons were amplified by PCR using a single set of primers with the exception of exon 1, which was amplified in two overlapping fragments (for primer sequences see Supplementary Table 1). PCR products were sequenced and compared with the published sequence (NM_012240.1) using Mutation Surveyor software (SoftGenetics).

Functional analysis of GDH activity

Lymphocytes were isolated from peripheral blood of the patient with the novel P436L mutation and transformed with Epstein–Barr virus to establish lymphoblast cultures. The activity of GDH in lymphoblast homogenates and the effect of added GTP were determined spectrophotometrically by the oxidation of NADH at 25 °C in Tris–0.01 M acetate buffer, pH 8, containing 10 µM EDTA according to the protocol of de Lonlay et al. (8). Protein was measured according to the method of Lowry et al. (9).

	Results

Top Abstract Introduction Research design and methods Results Discussion Conclusion Declaration of interest References

 
Molecular genetics

Seven different heterozygous mutations in the GLUD1 gene were identified in 13 out of 17 screened probands (76%; see Table 1). Three mutations were novel: N410D, D451V and P436L. These mutations were not present in the probands' unaffected parents and affected residues were conserved across species. Mutations at residue N410 have previously been reported in patients with HI/HA, including one patient within this cohort, suggesting that N410 is a functionally important residue.

Two mutations, S445L and R269H, were each identified in three unrelated families. All other mutations were identified in a single proband. Testing of unaffected parents demonstrated that the mutation had arisen de novo in 11 out of 13 probands. For one patient, with a S445L mutation, a spontaneous mutation could not be confirmed as DNA was unavailable from the unaffected father. In a second patient, the R269H mutation was inherited by the proband from their affected mother. Testing of further family members demonstrated that the R269H mutation was also present in the proband's maternal uncle and grandmother, all of whom have HI/HA.

Sequencing of SIRT4 in the four patients referred with HI/HA and negative for a GLUD1 mutation did not reveal any mutations. The mean serum ammonia concentration of this group of patients was 66.7 µmol/l (50–87 µmol/l). All four patients had diazoxide-responsive HI with no clinical symptoms suggestive of protein/leucine sensitivity.

Clinical characteristics of patients with GLUD1 mutation

The clinical characteristics of the 16 patients with a GLUD1 mutation are summarised in Table 1. The mean birth weight of our cohort with a mutation was 3133 g at a mean gestational age of 38.6 weeks. Macrosomia was not a common feature with birth weight >90th centile in only three patients. The age of presentation was delayed (mean of 23.4 weeks) in comparison with the patients with CHI due to K_ATP channel mutations, with only three presenting in the neonatal period. Two patients were successfully managed with manipulation of diet alone; all others required treatment with diazoxide. None of our patients required a pancreatectomy.

Patient 12 presented at 1 year of age with a tonic–clonic seizure associated with HI (insulin 9.6 mU/l and blood glucose 1.7 mmol/l). She had a normal serum ammonia concentration (21 µmol/l) on presentation and on repeated measurements (30 and 41 µmol/l) during childhood. She responded to diazoxide and demonstrated a normal fasting tolerance on a moderate dose of diazoxide (12–15 mg/kg per day). However, she continued to experience intermittent hypoglycaemic episodes in the postprandial period even on a high dose of diazoxide (15–17 mg/kg per day). She was hence evaluated for leucine sensitivity at 13 years of age by an oral leucine tolerance test. Following a fast of 4 h, an oral dose of 0.15 g/kg L-leucine was administered (10). Blood glucose and plasma insulin levels were then measured at –30, 0, 30, 60, 90 and 120 min. Diazoxide was not discontinued for the purpose of the test. The test was stopped at 60 min following the oral leucine load as she developed symptomatic (sweating, disordered consciousness and blurred vision) hypoglycaemia with a blood glucose concentration of 2.2 mmol/l and simultaneous plasma insulin concentration of 69.5 mU/l. Sequencing of the GLUD1 gene was requested in view of the severe leucine sensitivity. At the age of 13.7 years, she has mild learning difficulties with memory skills and emotional functioning being the areas of most concern.

There was a high incidence of seizures in our cohort of patients with a GLUD1 mutation. Out of 16 patients, 15 presented with seizures and 7 (43%) of them have developed epilepsy. All of the patients who developed epilepsy had generalised seizures. Out of seven patients with epilepsy, six had mutations in exons 6 and 7. All three patients with the mutation S445L developed epilepsy.

GDH activity in lymphoblasts

The activity and allosteric response of GDH in lymphoblasts from patient 12 were measured. She had normal basal GDH activities, but the half-maximal inhibitory concentration of GTP expressed in nmol/l (IC50) was 470% higher than that of controls (n=20) consistent with an excessive activity of GDH.

	Discussion

Top Abstract Introduction Research design and methods Results Discussion Conclusion Declaration of interest References

 
The phenotype of CHI due to mutations in the GLUD1 gene is well characterised. It is reported to be milder, not usually associated with macrosomia at birth and tends to escape recognition till later in infancy (4, 5, 11). This was confirmed in our study where the mean age of presentation was 23.4 weeks with only 3 out of 17 patients presenting in the neonatal period. Interestingly, only three patients had a birth weight of >90th centile and all three had the S445L mutation. This may indicate that this mutation causes more severe foetal HI than the other mutations identified in our cohort.

Epilepsy has been frequently reported in association with HI/HA syndrome (12, 13). The increased frequency of epilepsy is thought to be either the result of a) hypoglycaemic brain injury due to recurrent hypoglycaemia or b) chronic HA or c) decreased concentrations of glutamine and the neurotransmitter -aminobutyric acid in the brain due to raised GDH activity (13). Our study confirms that a high risk of epilepsy is associated with HI due to mutations in the GLUD1 gene, as 7 out of 16 (43%) of our patients developed epilepsy. Six out of the seven patients had mutations in exons 6 and 7; this was consistent with the study by Bahi-Buisson et al. (14), which reported that epilepsy is associated more frequently with mutations in exons 6 and 7. The mechanism of this genotype–phenotype association according to the location of the mutations is as yet unclear.

The most consistent feature of the HI due to mutations in GLUD1 is the persistent HA, and hence the term ‘HI/HA syndrome’ is used synonymously with CHI due to GLUD1 mutations (4, 8, 15). It is proposed that HA is the result of excessive GDH activity in the hepatocytes leading to an increase in the production of ammonia from glutamate and/or depletion of glutamate with reduction in the production of N-acetylglutamate, an allosteric activator essential for the first step of ammonia detoxification (16). The second mechanism is supported by the reduction in the concentration of blood ammonia on administration of N-carbamylglutamate (an analogue of N-acetylglutamate) (17, 18). There has been one other report of two patients (father and son) with HI due to the R269H mutation in the GLUD1 gene and normal serum ammonia concentrations (35 and 28 µmol/l) (19). Our patient with the novel P436L mutation had a completely normal serum ammonia concentration (highest being 41 µmol/l) that led to a delay in establishing the molecular diagnosis. If the origin of the HA is in the liver, it is possible that our patient is mosaic for the mutation with the mutation being absent or at <50% in the hepatic tissues. And hence this absence of HA may not be genotype specific. However, we cannot prove or disprove this possibility without a liver/pancreatic biopsy. Similarly, mosaicism may be the underlying mechanism in our four patients with HI/HA syndrome and no GLUD1 mutation with the mutation affecting the liver and pancreas, but not blood.

Enzymatic analysis of the lymphoblastic GDH from our patient with the P436L mutation showed a loss of GTP inhibition with the half-maximal inhibitory concentration of GTP being 470% higher than that of controls. Loss of GTP inhibition is known to increase glutamate oxidation in the presence of leucine causing leucine-sensitive HI, a classical feature of HI/HA syndrome. This was clinically evident in our patient with this novel P436L mutation and was confirmed by the oral leucine tolerance test. The confirmation of leucine sensitivity prompted us to sequence the GLUD1 gene and led to the molecular diagnosis. This suggests that analysis of the GLUD1 gene must be considered in all patients with leucine sensitivity even in the absence of HA.

This study also reports two other novel mutations (N410D and D451V) in the GLUD1 gene. N410 is located in the antenna-like structure connecting to the pivot helix of the GDH structure. A mutation (N410T) previously described at the same residue is known to cause HI/HA (20). D451 is located in the allosteric domain of the GLUD1 gene, a common site for mutations causing HI/HA syndrome and hence likely to be pathogenic by interfering with the allosteric binding sites. Conservation data suggest that these residues are functionally important as they are both well conserved among species.

SIRT4 has been shown to regulate insulin secretion by repressing the activity of GDH (6). Sirt4 knockout mice have increased glucose-stimulated and amino acid-stimulated insulin secretion in comparison with wild-type mice along with fasting hypoglycaemia in the male knockout mice. We hypothesised that a loss of function mutation of SIRT4 will cause a phenotype similar to gain of function GLUD1 mutations, i.e. HI/HA syndrome. However, our cohort of HI/HA patients with no known genetic aetiology is small, and hence the negative findings of our study are not enough to exclude a putative role of this gene in HI/HA syndrome.

	Conclusion

Top Abstract Introduction Research design and methods Results Discussion Conclusion Declaration of interest References

 
Mutations in the GLUD1 gene are not always associated with HA; hence mutational analysis of the GLUD1 gene may be indicated in patients with HI with evidence of leucine sensitivity even in the absence of HA. GLUD1 gene mutations cause a mild form of CHI associated with normal birth weight, delayed age at presentation and a high risk of epilepsy.

	Declaration of interest

Top Abstract Introduction Research design and methods Results Discussion Conclusion Declaration of interest References

 
The authors declare that there is no conflict of interest that would prejudice the impartiality of this scientific work.

	Funding

 
This work was funded by the Wellcome Trust (081188/A/06/Z).

	Acknowledgements

 
The authors would like to thank Michael Day and Kevin Colclough for their technical assistance. This study was funded by the Wellcome Trust (081188/A/06/Z). S E Flanagan is the Sir Graham Wilkins Peninsula Medical School Research Fellow and S Ellard was funded by the Royal Devon and Exeter NHS Foundation Trust Research and Development Directorate. The authors would also like to thank the clinicians who provided clinical information, including Dr Ariane Spitaels from Department of Paediatric and Adolescent Endocrinology, Groote Schuur and Red Cross Children's Hospitals, University of Cape Town, Cape Town, South Africa.

	References

Top Abstract Introduction Research design and methods Results Discussion Conclusion Declaration of interest References

 

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This Article IMMEDIATE FREE ACCESS ARTICLE OA Abstract Full Text (PDF) Supplementary Table 1 OA All Versions of this Article: EJE-09-0615v1 161/5/731    most recent Alert me when this article is cited Alert me if a correction is posted Services Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Google Scholar Articles by Kapoor, R. R Articles by Hussain, K. PubMed PubMed Citation Articles by Kapoor, R. R Articles by Hussain, K.