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Archives of Endocrinology and Metabolism

Print version ISSN 2359-3997On-line version ISSN 2359-4292

Arch. Endocrinol. Metab. vol.64 no.1 São Paulo Jan./Feb. 2020  Epub Sep 30, 2019

http://dx.doi.org/10.20945/2359-3997000000173 

original article

MODY probability calculator for GCK and HNF1A screening in a multiethnic background population

Roberta Magalhães Tarantino1 
http://orcid.org/0000-0001-7759-1564

Gabriella de Medeiros Abreu2 
http://orcid.org/0000-0002-0434-3815

Ana Carolina Proença de Fonseca2 
http://orcid.org/0000-0001-6123-0481

Rosane Kupfer3 
http://orcid.org/0000-0002-4073-0038

Maria de Fátima Carvalho Pereira4 
http://orcid.org/0000-0003-3932-6481

Mario Campos Júnior2 
http://orcid.org/0000-0002-7121-0748

Lenita Zajdenverg1 
http://orcid.org/0000-0002-1579-3299

Melanie Rodacki1 
http://orcid.org/0000-0002-9007-1325

1Seção de Diabetes e Nutrologia, Departamento de Medicina Interna, Universidade Federal do Rio de Janeiro (UFRJ), Rio de Janeiro, RJ, Brasil

2Laboratório de Genética Humana, Instituto Oswaldo Cruz, Fundação Oswaldo Cruz, Rio de Janeiro, RJ, Brasil

3Seção de Diabetes, Instituto Estadual de Diabetes e Endocrinologia do Rio de Janeiro, Rio de Janeiro, RJ, Brasil

4Departamento de Patologia Clínica da Universidade Federal do Rio de Janeiro, Rio de Janeiro, RJ, Brasil


ABSTRACT

Objective

We aimed to identify the frequency of monogenic diabetes, which is poorly studied in multiethnic populations, due to GCK or HNF1A mutations in patients with suggestive clinical characteristics from the Brazilian population, as well as investigate if the MODY probability calculator (MPC) could help patients with their selection.

Subjects and methods

Inclusion criteria were patients with DM diagnosed before 35 years; body mass index < 30 kg/m2; negative autoantibodies; and family history of DM in two or more generations. We sequenced HNF1A in 27 patients and GCK in seven subjects with asymptomatic mild fasting hyperglycemia. In addition, we calculated MODY probability with MPC.

Results

We identified 11 mutations in 34 patients (32.3%). We found three novel mutations. In the GCK group, six cases had mutations (85.7%), and their MODY probability on MPC was higher than 50%. In the HNF1A group, five of 27 individuals had mutations (18.5%). The MPC was higher than 75% in 11 subjects (including all five cases with HNF1A mutations).

Conclusion

Approximately one third of the studied patients have GCK or HNF1A mutations. Inclusion criteria included efficiency in detecting patients with GCK mutations but not for HNF1A mutations (< 20%). MPC was helpful in narrowing the number of candidates for HNF1A screening.

Key words: GCK; HNF1A; MODY; monogenic diabetes

INTRODUCTION

The frequency of monogenic diabetes mellitus (DM) has been underestimated in various populations (1). Most cases are caused by mutations in GCK [glucokinase gene] (GCK MODY [maturity onset diabetes of the young]) or HNF1A [hepatocyte nuclear factor 1-alpha gene] (HNF1A MODY) (2). Their molecular diagnosis is expensive but promotes the improvement of genetic counseling and treatment (3). Strategies to select the ideal subjects to screen for monogenic DM (MDM) in different populations are necessary to establish cost-effective diagnostic algorithms.

Different authors have developed clinical criteria for MODY screening based on age, family history and clinical characteristics (4,5). Although their use appears to be cost-effective (6), there is a concern that the screening based on clinical criteria would either miss part of the affected patients or still result in an excessive number of genetic tests (7). Therefore, authors have pursued optimal strategies for selecting patients. Shields and cols. developed a clinical prediction model that generates a probability of MODY (8) and shows good discrimination between MDM and type 1 (T1DM) or type 2 DM (T2DM) in European patients diagnosed under 35 years. The performance of this calculator in non-Caucasians is unknown.

The Brazilian population is very diverse and comprises individuals from multiple ethnic backgrounds, especially Caucasoid and Afro-descendants. There are scarce data about the prevalence of MDM and its optimal screening strategy in this setting. Our aim in this study was to estimate the frequency of MDM due to GCK or HNF1A mutations in patients with suggestive clinical characteristics and to investigate if the MODY probability calculator (MPC) could improve patient detection in this population (8,9).

SUBJECTS AND METHODS

In this cross-sectional observational study, we selected patients clinically defined with monogenic diabetes from two specialized centers in Rio de Janeiro, between March 2012 and June 2015. MODY screening is not part of the routine laboratory panel of either center. We analyzed thirty-four unrelated probands from Brazilian families for mutations in GCK and HNF1A.

The inclusion criteria were age of DM diagnosis ≤ 35 years, body mass index (BMI) ≤ 30 kg/m2 or 95th percentile at onset, negative anti-glutamic decarboxylase antibody (anti-GAD) and anti-islet antigen 2 antibody (anti-IA2) antibodies and family history of diabetes in at least two generations, excluding the generation of the index case, and/or two or more first-degree relatives at the same side of the family. We excluded patients with T1DM; past diabetic ketoacidosis; clinical signs of insulin resistance (acanthosis nigricans, increased abdominal circumference and obesity); and secondary causes of diabetes.

The Ethics and Research Committee of the Clementino Fraga Filho University Hospital and State institute of Diabetes and Endocrinology of Rio de Janeiro approved this study protocol. We informed all participants about the aim of this study and provided verbal and written consent.

We calculated the positive predictive value (PPV) for MODY based on the MPC for each patient (8) and divided the patients into two groups. The GCK group included patients with fasting hyperglycemia (100-154 mg/dL); increased glycaemia after 75 g anhydrous dextrose <54 mg/dL and HbA1c < 7.5% (58 mmol/mol); and evolutionarily stable disease (even without antidiabetic drugs), most often asymptomatic and with hyperglycemia since birth (10). The HNF1A group included all other cases that met the inclusion criteria and that did not have the profile for the GCK group.

We isolated genomic DNA from peripheral blood leukocytes using QIAamp DNA Blood Mini Kit (Qiagen, Hilden, Germany). Also, we purified PCR products using Clean Sweep PCR Purification Reagent (Applied Biosystems, Vilnius, Lithuania). Then, we performed screening of the entire coding sequence of GCK and HNF1A genes through bidirectional Sanger sequencing using the Big Dye Terminator Kit v3.1 (Applied Biosystems, Austin, TX, USA), conducted on an ABI 3130 Automatic Genetic Analyzer (Applied Biosystems). Primers sequences are available upon request. We confirmed all mutations by bidirectional sequencing of a second PCR reaction. Then, we estimated the serum levels of anti-GAD and anti-IA2 antibodies by means of an enzyme-linked immunosorbent assay method (ELISA) using a EUROIMMUN kit.

We checked the variants identified against public Databases PubMed, Clinvar, dbSNP (https://www.ncbi.nlm.nih.gov/), Human Genome Mutation Database (HGMD®) (http://www.hgmd.cf.ac.uk/ac/), ExAC Browser (http://exac.broadinstitute.org), GnomAD (http://gnomad.broadinstitute.org/) and 1000 Genomes project database (http://www.internationalgenome.org/) to investigate their previous identification in the literature. We performed functional analyses using Mutation Taster (http://www.mutationtaster.org) (11-13).

We evaluated the differences between patients with mutations and others with Student’s t-test and chi-square tests. In addition, we performed statistical analysis using SPSS software (version 22.0).

RESULTS

Characteristics of the study group

We included 34 individuals (61.7% females) with a mean age of DM diagnosis and a duration of 19.8 ± 8.8 and 14.6 ± 9.9 years, respectively, as well as a mean BMI of 22.8 ± 3.2 kg/m2. 55.8% used insulin, and 41.2% used oral antidiabetic drugs (OAD). Their previous DM classifications included the following: non-classified in 38.2%, T1DM in 35.3%, T2DM in 23.5% and gestational diabetes (GDM) in 3%. Patients in the GCK (n = 7) and HNF1A (n = 27) groups had similar age at onset (16.1 ± 7.8 vs 20.8 ± 9.0 years; p = 0.286), diabetes duration (9.88.8 vs 15.4 ± 10.1 years; p = 0.82) or BMI (20.6 ± 4.0 vs 23.3 ± 2.8; p = 0.143).

None of the patients in the GCK group used insulin, and one used OAD. Most patients (70.3%) in the HNFA group used insulin (mean dose: 0.9 ± 0.4 UI/kg/day), and 48.1% used OAD.

Genetic tests

We found MODY mutations (GCK or HNF1A) in 11 patients (32.3%). Fifty per cent of patients with non-classified DM had mutations in GCK or HNF1A. We fond mutations in 16.6% of those previously classified as T1DM and in none classified as T2DM. The only patient classified as GDM had a GCK mutation.

In the GCK-suspicious group, six cases had mutations (85.7%): Five were missense mutations: p.Tyr61Asp (c.181T>G; novel); p.Arg191Trp (c.571C>T); p.Thr228Met (c.683C>T); p.Ala384Val (c.1151C>T); p.Gly227Asp (c.680G>A); and one in-frame deletion p.Phe150del (c.449_451delTCT). We tested the patient in this group without the GCK mutation for HNF1A, and we found no mutations.

In the MODY-HNF1A-suspicious group, we found five mutations (5/27-18.5%); three missense substitutions: p.Gly31Asp (c.92G>A), p.Val133Glu (c.398T>A; novel) and p.Trp165Arg (c.493T>C); one nonsense mutation: p.Arg171Ter (c.511C>T); and one frameshift insertion: p.Thr433Hisfs*116 (c.1296_1297insC; (novel). Patients with HNF1A mutations used insulin less frequently than others. Those who used insulin reported a lower insulin dose/kg (Table 1). Other characteristics of those with or without HNF1A mutations are shown in Table 1.

Table 1 Clinical characteristics of patients according to mutations in the HNF1A gene 

Mutation p

Present (n = 5) Absent (n = 22)
Sex
Female 1 (20%) 15 (68.2%) 0.048
Male 4 (80%) 7 (31.8%)
Age of diagnosis (years) 17.6 ± 6.8 21.5 ± 9.4 0.237
BMI* (kg/m2) 22.08 ± 3.73 23.6 ± 2.6 0.154
Insulin use 1 (20%) 18 (81.8%) 0.006
OAD** use 3 (60%) 10 (45.4%) 0.557
Affected generations
1 0 5 (22.7%) 0.054
2 or more 5 (100%) 17 (77.3%)
Age of diagnosis/grade
Childhood 0 3 (13.6%) 0.323
Adolescence 3 (60%) 6 (27.3%)
Adult 2 (40%) 13 (59.1%)
Diabetes presentation 0.583
Insidious 1 (20%) 3 (13.6%)
Abrupt# 4 (80%) 19 (82.6%)
Diabetes Duration (years) 8.6 ± 7.06 16.95 ± 10.13 0.432
MODY probability (PPV) 75.5 ± 0.0 35.7 ± 30.9 < 0.001
Mean insulin dose per kg of weight (units/kg) 0.37 0.9 ± 0.37 -

Note: Quantitative variables are presented as mean and standard deviation. Categorical variables are presented as total number (n) and percentage (%). The age groups used included the following: childhood, 0-9 years, adolescence, 10-19 years and adult, over 20 years (17).

* BMI: body mass index; ** OAD: oral anti diabetic drug; # Symptoms of insulinopenia such as polyuria, polydipsia and weight loss.

Among the 11 mutations, eight had already been described, and three were novel mutations. The mutation p.Tyr61Asp (c.181T>G), found in exon 2 of the GCK gene of one patient, is a missense mutation classified as pathogenic. The other two novel mutations occurred in the HNF1A gene (exons 2 and 6). We considered the missense mutation p.Val133Glu (c.398T>A) and the frameshift insertion p.Thr433Hisfs*116 (c.1296_1297insC) pathogenic because they alter the codon reading frame due to the insertion of a nucleotide (Table 2).

Table 2 Mutations identified in this study 

Gene Exon Patient Change in protein Change in DNA Consequence SIFT prediction SIFT score Polyphen Mutation Taster prob. ClinVar Reference
GCK 2 P40 p.Tyr61Asp c.181T>G Missense Deleterious 0 Probably harmful 0.999999998323156 NA This study, novel
4 P1 p.Phe150del c.449_451delTCT In-frame deletion NA NA NA 0.999999999980624 NA Massa and cols., 2001
5 P7 p.Arg191Trp c.571C>T Missense Deleterious 0 Probably harmful 0.999999947468603 Pathogenic Ellard and cols., 2000
7 P29 p.Gly227Asp c.680G>A Missense Deleterious 0 Probably damaging 0.999999999998095 NA Domínguez-López and cols., 2013
7 P9 p.Thr228Met c.683C>T Missense Deleterious 0 Possibly harmful 0.99999999999911 Pathogenic Stoffel and cols., 1992
9 P32 p.Ala384Val c.1151C>T Missense Tolerated 0.06 Possibly harmful 0.999999998673333 Uncertain meaning Costantini and cols., 2014
HNF1A 1 P4 p.Gly31Asp c.92G>A Missense Tolerated 0.29 Possibly harmful 0.995035768629034 Pathogenic Chèvre and cols., 1998
2 P28 p.Val133Glu c.398T>A Missense Deleterious 0 Possibly harmful 0.999999999738075 NA This study, novel
2 P13 p.Trp165Arg c.493T>C Missense Deleterious 0 Possibly harmful 0.999999998737327 NA Tatsi and cols., 2013
2 P37 p.Arg171Ter c.511C>T Nonsense NA NA NA 1 Pathogenic Vaxillaire and cols., 1999
6 P5 p.Thr433Hisfs*116 c.1296_1297insC Frameshift-insertion NA NA NA 1 NA This study, novel

NA: not applicable; prob: probability of causing disease.

We recruited the family of all three probands with novel mutations, as presented in the pedigrees (Figure 1). We recruited four family members of the patient with the p.Tyr61Asp mutation in GCK. Then, we tested all four individuals with diabetes. The brother and sister had the same p.Tyr61Asp mutation, and we observed that it was inherited from the mother with diabetes. The father with recent onset DM (after 50 years of age) did not have the mutation. We recruited the mother with DM of the patient with the mutation p.Thr433Hisfs*116. She also had the same mutation. Four family members of the patient (three sisters and the mother) with the mutation p.Val133Glu in HNF1A were recruited. The only sister with diabetes also had the same mutation of the patient, and they inherited the mutation from their healthy mother. We believe it may be a case of incomplete penetrance uncommon with HNF1A mutations but already observed by other authors (14,15). In addition, the mutation p.Val133Glu was absent in the two healthy sisters.

Figure 1 Pedigree and genotype of novel mutations. (A) Family 40 with the GCK p.Tyr61Asp (c.181T>G) in heterozygous state. K: allele T or G. (B) Family 5 showing the novel insertion HNF1A p.Thr433Hisfs*116 (c.1296_1297insC). The blue arrow indicates where the insertion occurs. (C) Family 28 presenting the HNF1A p.Val133Glu (c.398T>A). W: allele T or A. Filled symbols and empty symbols represent subjects with diabetes and healthy individuals, respectively. The present age of the individuals is show below the symbols in years, followed by age of diagnosis (AOD) in years and genotype interpretation. Genotypes are expressed by normal allele (N) and mutated allele (M); NT: Not tested. An arrow indicates the index case. 

MODY probability calculator

In the sample as a whole, 61.8% of patients (n = 21) had PPV > 50%, and 50% (n = 17) had PPV > 75%, according to the MPC. In those with PPV > 50%, 47.6% had mutations, and in those with PPV > 75%, 52.9% had mutations.

HNF1A group

The probability of MODY, according to MPC, was ≥ 50% in 14 patients (51.8%) and ≥ 75% in 11 patients (40.7%). All five patients in the HNF1A group with mutations had PPV for MODY ≥75% (Table 1). We found a mutation in 5/11 (45%) patients with PPV ≥75% and in 5/14 (35.71%) of those with PPV ≥ 50%.

GCK group

Six patients had PPV ≥ 75%, and 1 had PPV between 50 and 75%. We detected GCK mutations in 5 patients with PPV ≥ 75% and in patients with PPV between 50 and 75%, but not in 1 individual with PPV ≥75%.

DISCUSSION

In this study, we identified patients with phenotypes suggestive of MDM and performed mutation screening for GCK and HNF1A genes. We found mutations in 32.3%. Although a high frequency of mutations in these two genes have been reported in individuals with a clinical diagnosis of MDM from several populations, especially from Northern Europe (16,17), others (including Southern Europeans, Asians and Brazilians) have found a lower frequency of mutations, as true with our findings (18-21). In some populations, other types of diabetes might share clinical features with MDM more frequently than others. Alternatively, other genes implicated in the pathogenesis of MODY could be more frequent in these groups, such as HNF4A, insulin promoter factor-1 (IPF-1), HNF1B, NeuroD1 and others. In the other two studies with Brazilian cohorts (20,21), approximately 60% of patients with clinical suspicion of MDM did not have mutations in HNF1A, GCK or HNF4A genes, but we did not test other MODY genes.

In those with mild fasting hyperglycemia, we found GCK mutations in 85.7%, which suggests a high sensitivity for the clinical criteria. The frequency of GCK mutations in this study was slightly higher than previously reported for most populations (42.4 to 61%), including Brazilians (21-23). We found mutations in HNF1A, the most common gene for non-GCK MDM, in 18.5%, which was much like the data obtained by Santana and coworkers in the Brazilian population but lower than reported in other populations (16-19,24). Therefore, the clinical criteria for the selection of patients for GCK testing seem to be adequate in most populations, including ours. Surprisingly, we found the opposite for non-GCK MODY. This suggests that an improvement in the clinical criteria to adequately select patients for screening is necessary or that, alternatively, other genes should also be investigated.

We have evaluated if MPC (8) could help identify a group of patients that would be more suitable for screening. All patients with HNF1A mutations had PPV > 75%. If we had selected only subjects above this cutoff, 60% of the patients would not have been tested. This strategy would make the screening more cost-effective. However, the frequency of mutations in other genes in patients with a clinical diagnosis of non-GCK MODY is still not known for our population. It is possible that patients without HNF1A mutations could have alterations in other MODY genes, which would be overlooked with this strategy.

In this study, a cutoff for MODY probability of > 75% and >62%, based on MPC, was found in all patients with HNF1A and GCK mutations, respectively. Although in UK the current pick-up rate for MODY testing is PPV > 25% (9), other authors have found a good specificity and negative predictive value in higher cutoff values (> 62.5%) for detecting MODY in non-Caucasian population (25). Our findings suggest that higher cutoff values should be considered for MODY screening in non-Caucasian populations.

This study has some limitations. First, we included a limited number of patients. Secondly, we tested only two MODY genes for financial reasons. Additionally, we used only one methodology (Sanger sequencing) to investigate mutations. This method is unable to detect copy number variations, large deletions and duplications that can represent up to 3% of all genetic alterations of the GCK, HNF1A and HNF4A (26). Another concern is related to the absence of a control group. The selection of the studied population was done in a pragmatic way when the patient did not present clinical criteria of T1 or T2 DM. An additional potential limitation is the lack of C-peptide measurement as a screening tool for MODY. The strengths of our study included finding three novel mutations not previously reported and providing new information about the screening of monogenic diabetes in individuals with multiethnic backgrounds. For future studies, we aim to bypass these limitations and to perform functional genomic studies to confirm novel mutations as pathogenic ones.

In conclusion, we investigated MODY mutations in patients with clinical features suggestive of MDM from a multiethnic background. Approximately one third of patients with clinical features suggestive of MDM from a multiethnic background had GCK or HNF1A mutations. While clinical criteria were efficient for detecting patients with GCK mutations, we found HNF1A mutations in less than 20% of the cases. Although MPC has not been validated for non-Caucasians, its use as a screening tool for selecting patients to test for HNF1A mutations, using a cutoff of 75%, would reduce the number of tests in 60% and increase the percentage of positive cases to 45%. These data suggest that the use of the MPC could be a cost-effective strategy for selecting patients to screening for non-GCK MODY mutations, but it is important to consider the possible role of non-HNF1A mutations in non-Caucasian populations such as ours.

Acknowledgements

Professor Tânia Maria Ruffoni Ortiga, from the Laboratory of Translational Endocrinology of the Biophysics Institute Carlos Chagas Filho, and professor Márcia Mattos Gonçalves Pimentel, head of the Human Genetics Service of State University of Rio de Janeiro, who assisted in the initial phases of the research.

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Funding: this work was supported by National Council for Scientific and Technological Development (CNPq) and Oswaldo Cruz Institute (IOC).

Received: February 25, 2019; Accepted: June 19, 2019

Correspondence to: Roberta M. Tarantino. Rua Rodolpho Paulo Rocco, 255, Ilha do Fundão 21941-590 – Rio de Janeiro, RJ, Brasil drarobertatarantino@gmail.com

Contributions: RMT was the physician responsible for recruiting patients in the study, gathering and analyzing the data and writing the manuscript. GMA was responsible for the molecular genetics and bioinformatic analysis. ACPF contributed to statistical analysis of the data. RK reviewed the manuscript. FC reviewed the manuscript. MC reviewed and edited the manuscript. LZ contributed to the discussion. MR reviewed and edited the manuscript and contributed to the discussion. The authors are grateful to the patients and their families, as well as to all the authors who approved the final version of this article.

Disclosure: RMT has been a Novo Nordisk employee (i.e., regional medical advisor) since July 2017 but started the monogenic diabetes research project in 2012 and judges that it could not inappropriately influence (bias) this work. The other authors have no declarations of interest.

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