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Pediatric Endocrinology Diabetes and Metabolism
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SCImago Journal & Country Rank
4/2021
vol. 27
 
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Opis przypadku

Umiarkowana postać wrodzonego przerostu nadnerczy u dwóch dziewcząt zdiagnozowanych w przesiewie noworodkowym

Magdalena Banaszak-Ziemska
1
,
Elżbieta Małecka
1
,
Katarzyna Łacna
2
,
Maria Ginalska-Malinowska
3
,
Marek Niedziela
1, 4

  1. Karol Jonscher’s Clinical Hospital, Poznan University of Medical Sciences, Poznan, Poland
  2. Center of Medical Genetics GENESIS, Poznan, Poland
  3. Screening and Metabolic Diseases Department, Institute of Mother and Child, Warsaw, Poland
  4. Department of Pediatric Endocrinology and Rheumatology, Institute of Pediatrics, Poznan University of Medical Sciences, Poznan, Poland
Pediatr Endocrinol Diabetes Metab 2021; 27 (4): 291–297
Data publikacji online: 2021/12/30
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Introduction

Congenital adrenal hyperplasia (CAH) is one of the most common hereditary autosomal recessive diseases in humans and is associated with defects in steroid biosynthesis. Deficiency of 21-hydroxylase activity is most common and is estimated to account for 90-95% of all CAH cases, whereas 5–8% of cases are associated with the deficiency of 11β-hydroxylase. Deficiency of other steroidogenesis enzymes such as 3β-hydroxysteroid dehydrogenase, 17α-hydroxylase and Steroidogenic Acute Regulatory Protein (STaR) are very rare. The range of symptoms in CAH vary widely from the mild form with acne, hirsutism, and problems with fertility that manifest later in life to the severe form with ambiguous genitalia, which is associated with an excess of sex steroids in females and deficiency of sex steroids in males, precocious puberty, delayed puberty, hypokalemic hypertension and ultimately life-threatening salt-loss syndrome. CAH due to deficiency of 21-hydroxylase may be manifested in the following clinical forms: classic form with salt-wasting (SW-CAH), classic form with simple virilization (SV-CAH) and a milder nonclassic form (NC-CAH) characterizes with late onset. Clinical severity is correlated with the type CYP21A2 gene mutation. Approximately 75% of classic form CAH cases suffer from aldosterone deficiency with failure to thrive, feeding problems, salt-wasting syndrome leading to life-threatening hypovolemia and shock. Newborns typically present with these symptoms in the 2nd-3rd week of life [1]. In Europe, the frequency of the occurrence of homozygotes with the classic form CAH ranges from 1:5000 to 1:12000, and the frequency of the nonclassic form is 1:1000. According to information from the first years of neonatal Polish screening, the frequency of CAH occurrence in Poland is 1:14781 [2, 3]. The carrier of the classic form is noted in 1:40 individuals in the European population, and nonclassic form is noted in 1:9 [46].

Neonatal screening

Pang et al. were the first to introduce neonatal screening based on 17-OHP measurements from filter paper in 1977 [7]. Worldwide guidelines from the Endocrine Society and European Society for Paediatric Endocrinology recommend to incorporate screening for 21-hydroxylase deficiency into all newborn screening programs [1]. Screening markedly reduces the time from birth to diagnosis [5, 810]. Patients with nonclassic CAH could also be recognized in screening, especially after incorporating genetic analysis into the screening [11, 12]. Affected infants ascertained through screening have less severe hyponatremia [10, 13]. The delay in the appropriate sex assignment of severely virilized females is also markedly reduced [6, 10]. Evaluation of 17-OHP concentration is the first step of neonatal screening in all countries, but further steps may differ. Equally important is determining which parameter is used as a reference for 17-OHP concentration. The concentration of 17-OHP is more correlated with gestational age, but the determination of gestational age might be less reliable than birth weight [14]. In Wielkopolska, newborn screening for CAH was introduced in September 2016. Until the end of 2016, all of Poland was involved in this program [2]. The first step of the screening is to evaluate 17-OHP concentration from dried blood spots from filter paper taken on the 3rd day of life using the fluoroimmunoassay (FIA) method in regional screening laboratories. In the Polish screening program, 17-OHP is assessed based on gestational age and day of sampling. Elevated results are verified by blood steroid profile by tandem mass spectrometry (LC/MS/MS) at the Institute of Mother and Child in Warsaw using samples on filter paper obtained on the 3rd day of life and sent for screening for inborn metabolic defects. The following steroids are assessed in the blood steroid profile: 17-OHP, cortisol, 21-deoxycortisol, 11-deoxycortisol and androstenedione. Evaluation of the (17-OHP+androstenedione)/cortisol ratio and (17-OHP+21-deoxycortisol)/cortisol) ratio are also included in the LC/MS/MS screening results. Both of these ratios improve the specificity of the screening [2, 15]. In preterm newborns, a retest of the 2nd filter paper is necessary. Borderline and equivocal results of 17-OHP (FIA) and steroid profiles are also verified in the 2nd filter paper. After that, the regional consultant for pediatric endocrinology is informed about the child suspected for CAH. The newborn is subsequently admitted to the endocrine ward, and diagnosis is verified. The last step of the neonatal screening is the genetic analysis of the CYP21A2 gene at the Institute of Mother and Child in Warsaw.

Patients’ report

We present two diagnostically difficult CAH female patients investigated in the first months of the neonatal screening in the Wielkopolska region, Poland.

Patient 1 was born as a 2nd child (older brother is unaffected) to nonconsanguineous parents at the 40th week of gestation with the birth weight of 3520 g and the birth length of 56 cm. The patient scored 9-10 points on the Apgar scale. A girl was discharged from the neonatal department without any suspicion of disease. The screening filter paper was sampled twice on the 3rd day of life and again on the 14th day of life (blood steroid profiles in Warsaw were performed on the 11th and the 25th day of life, respectively). For both filter papers, 17-OHP (FIA) concentrations were slightly elevated (Table II). In blood steroid profiles (LC/MS/MS), 17-OHP concentrations were in the normal range, and androstenedione levels were reduced. The 21-deoxycortisol concentration was slightly elevated in the first LC/MS/MS and was normalized in the second LC/MS/MS analysis. The cortisol level was low and decreased over time. Therefore, the (17-OHP+androstendione/cortisol) ratio and the (17-OHP+21-deoxycortisol/cortisol) ratio were increased, especially in the second steroid profile (Table I). Given the inconclusive results, the child was urgently called to the endocrine ward. Upon admission (28th day of life), the weight was 3970 g. Based on the patient’s history, the girl was less active and required awakening for feeding. Upon physical examination, her state of nutrition was satisfactory, and there were no signs of dehydration. A tendency for marbling skin color was noted with hyperpigmentation of external genitalia and nipples. Only a small virilization was noticed, which was graded as the 1st stage based on the Prader scale. At admission, the electrolyte concentrations were as follows: 132 mmol/l Na (normal range 132–145) and 5,31 K mmol/l (normal range 3.1–5.1). We observed an insufficient increase in cortisol and an abnormal increase in 17-OHP concentration in the short-Synacthen test (36 ug/kg) (Table II). Concentrations of ACTH, androstenedione, testosterone, and DHEA-S were greater than the upper limits (Table II). The steroid profile in the 24-hr urine collection was assessed by GC-MS and confirmed the diagnosis of 21-hydroxylase deficiency (Table III). On the 30th day of life, hydrocortisone (HC) treatment was started. HC was initially administered intravenously. After three days, the patient was switched to an oral regimen. Given that the sodium concentration was in the lower limit, fludrocortisone was also added. We diagnosed a classic form of simple virilizing/moderate congenital adrenal hyperplasia due to 21-hydroxylase deficiency. Karyotype was 46,XX. Genetic evaluation by MLPA (MRC-Holland: SALSA MLPA Probemix P050 CAH) detected two mutations in the CYP21A2 gene: heterozygous intron 2 splice variant I2G (HGVS nomenclature: NM_000500.7: c.293-13C>G) and heterozygous mutation p.I172N (HGVS nomenclature: NM_000500.7: c.515T>A; NP_000491.4: p.I172N).

Table I

17-OHP (FIA) concentration and steroid profile from neonatal screening in both patients

Parameters from neonatal screening Below standard (persons) Below standard (persons) Standard (persons) Above standard (persons)
17-OHP (FIA) (nmol/l)45.9562.0261.710.1–33
17-OHP MS/MS (nmol/l)3.581130.40.1–14.8
Cortisol MS/MS (nmol/l)2.40.119.911–4569
21-deoxycortisol MS/MS (nmol/l)16.83.8243.85.9
11-deoxycortisol MS/MS (nmol/l)1.550.580.7685.2
Androstenedione MS/MS (nmol/l)0.570.034.061.75–32.65
(17-OHP+androstenedione)/cortisol ratio MS/MS2.03110.291.730.1–1.95
(17-OHP+21-deoxycortisol)/cortisol ratio MS/MS9.99148.23.730.1–1.95

[i] 17-OHP – 17-hydroxyprogesterone; FIA – fluoroimmunoassay method; MS-MS – tandem mass spectometry

Table II

Concentration of hormones in plasma/serum

Parameters Patient 1 Patient 2
Cortisol in Synacthen test
0’ min (ng/ml)
2116
Cortisol in Synacthen test 30’ min (ng/ml)2827
Cortisol in Synacthen test 60’ min (ng/ml)2938
17-OHP in Synacthen test 0’ min (ng/ml)33.433.9
17-OHP in Synacthen test 30’ min (ng/ml)36.437.1
17-OHP in Synacthen test 60’ min (ng/ml)34.838.68
Androstenedione (ng/ml)
3.47
(0.06–0.78)
9.55
(0.06–0.78)
DHEA-S (μmol/l)15.24 (0.14–1)12.2 (0.14–1)
Testosterone (nmol/l)1.85 (0.03–0.17)2.57 (0.03–0.17)
ACTH (pg/ml)110.5 (10–60)420.9 (10–60)
PRA (ng/ml/h)5.5 (4–37)

[i] 17-OHP – 17-hydroxyprogesterone; DHEA-S – dehydroepiandrosteronesulphate; PRA – plasma renin activity

Table III

Steroid profile by GC/MS in 24th hour urine collection analyzed in The Children's Memorial Health Institute Warsaw

Hormone/metabolite Patient 1
(μg/24 h)
Normal range Patient 2
(μg/24 h)
Normal range
AN (androsterone)32.92–2025.21–10
ET (etiocholanolone)2.20–31.11–5
11-OAN/ET (11-cetoandrosterone/etiocholanolone)15.40.5–6.530.05–20
11-OHAN (11-hydroxy-androsterone)109.13–2444.02–20
11-OHET (11-hydroxy-etiocholanolone)0.00–30.90–3
ET/AN0.10.0
DHA (dehydroepiandrosterone)2.20–311.31–10
5-AND (5-androstenediol)1.80–121.71–10
16α-OHDHA (16 α-hydroxy-DHA)467.57–230744.2135–500
An-3-ol (5-androstenetriol)129.615–150128.340–600
5-PT (5-pregnenetriol)38.90–2640.32–20
16-OHPN (16α-hydroxy-pregnenolone)884.70–1401010.6110–495
17-OHPN (5β) (17-hydroxy-pregnanolone)165.31–16123.64–19
17-OHPN (5α) (17-hydroxy-pregnanolone)134.50.5–972.10.5–9
PT (pregnanetriol)312.33–28121.85–21
PTN (pregnanetriolone)1087.10.2–10427.70–5
PD (pregnanediol)32.80.2–10172–20
E1 (estrone)0.00.0
E2 (estradiol)0.00.0
E3 (estriol)0.00.0
THS (tetrahydro-11-deoxycortisol)4.01–116.71–3
THDOC (tetrahydro-11-deoxycorticosterone)0.00–10.00–1
THA (tetrahydro-11-dehydrocorticosterone)0.05–500.05–30
Allo-THA (allo-tetrahydro-11-dehydrocorticosterone)0.010–600.015–90
THB (tetrahydro-corticosterone)0.00–80.00–8
Allo-THB (allo-tetrahydro-corticosterone)0.00–400.00–40
THaldo (tetrahydro-aldosterone)6.74–253.14–12
THE (tetrahydro-cortisone)94.4150–40072.938–408
THF (tetrahydro-cortisol)8.83–686.8
Allo-THF (allo-tetrahydrocortisol)17.27–26015.6
THF/alloTHF0.50.4
THF+alloTHF/THE0.3< 0.80.3
Hormone/metabolitePatient 1
(μg/24 h)
Normal rangePatient 2
(μg/24 h)
Normal range
α-CTN (α-cortolone)22.820–13017.820–100
β-CTN (β-cortolone)57.925–15551.520–100
β-CT (β-cortol)27.05–4019.55–10
α-CT (α-cortol)52.14–4220.05–20
E (free cortisone)12.65–4511.75–20
F (free cortisol)10.52–1625.13–20
F/E0.80.3–0.752.2
6β-OHF (6β-hydrocortisol)0.00.0
20α-DHF (20α/β-dihydrocortisol)0.00.0

Patient 2 was born as an only child to nonconsanguineous parents at the 40th week of gestation with the birth weight of 3670 g and the birth length of 56 cm. The patient scored 10 points on the Apgar scale. The girl was discharged from the neonatal department without any suspicion of disease. Filter paper obtained on the 3rd day of life reached the Poznan screening laboratory 6 days later (the 9th day of life) and the Warsaw screening laboratory in the next 5 days (the 14th day of life). Elevated concentration of 17-OHP (61.71 nmol/l) suggested CAH. In the blood steroid profile, 17-OHP and 21-deoxycortisol concentrations were elevated, whereas the cortisol concentration was at the lower limit of the normal range. The androstenedione concentration and the 11-deoxycortisol and (17-OHP+androstendione/cortisol) ratio were in the normal range, and only the (17-OHP+21-deoxycortisol)/cortisol ratio was slightly elevated (Table I). The child was urgently called to the endocrine ward. At admission (24th day of life), weight was 4000 g. Physical examination revealed the following: eutrophic newborn, no signs of dehydration, active, hyperpigmentation of external genitalia and nipples, and 2nd stage virilization based on Prader scale. At admission, the electrolyte concentration (134 mmol/l Na and 5,07 mmol/l K) were normal. We performed a short-Synacthen test (36 µg/kg). We observed an insufficient increase in cortisol and an abnormal increase in 17-OHP concentration (Table II). Basal concentrations of ACTH, androstenedione, testosterone, and DHEA-S were significantly elevated (Table II). The steroid profile in the 24-hr urine collection (GC-MS) confirmed the diagnosis of 21-hydroxylase deficiency (Table III). On the 25th day of life, hydrocortisone (HC) treatment was started. HC was initially administered intravenously and then switched to an oral regimen after three days. Given that the sodium concentration was in the lower normal limit, fludrocortisone was added. We diagnosed a classic form of simple virilizing/moderate congenital adrenal hyperplasia due to 21-hydroxylase deficiency. Karyotype was 46,XX. Genetic evaluation by MLPA (MRC-Holland: SALSA MLPA Probemix P050 CAH) detected two abnormalities: heterozygous deletion of the exon 4 in the CYP21A2 gene and heterozygous duplication of the exon 4 in CYP21A1P pseudogene.

Discussion

The introduction of a new screening method for the population offers new benefits. We would such as to highlight that both patients described in this paper were discharged from neonatal departments without any suspicion of disease although the symptoms of virilization were described a few weeks later and expressed to a greater degree in patient 2. The question arises as to whether virilization was present at birth but missed by neonatologists or developed over time. The first option is more likely compared with its development in such a short period, i.e., from birth until the 28th and 24th day in the two patients, separately. Some previous reports have demonstrated that greater than 50% of females had an incorrect clinical evaluation of the virilization features [10, 12-13]. In Poland, in 5 of 31 female cases identified in the first three years of neonatal CAH screening, there were no data about virilization in the newborn hospital documentation [3]. In all these 5 cases, initially small abnormalities found in the first filter paper were worsened in time with each subsequent studies. Afterward, clinical and laboratory verification in the endocrine department allowed the diagnosis of moderate CAH in these girls. Eventually, virilization (the 1st to 3rd Prader stage) was identified despite not being noticed in neonatal unit earlier [3].

As a standard, a single 17-OHP (FIA) called ‘singlet’ is performed. Increased values are retested in the next working day as a doublet. When 17-OHP (FIA) elevation is confirmed again, a steroid profile (LC/MS/MS) is performed. If the screening laboratory has information about virilization, both investigations, namely 17-OHP (FIA) in a triplet and steroid profile (LC/MS/MS), are performed simultaneously to confirm or exclude CAH as soon as possible. To fulfill the neonatal screening function, the time between filter paper sampling and diagnosis of the disease should be as short as possible. In the study by Thil’en, et al., the median age at diagnosis was 11 days (range, 6-127 days), and the median age of detection was eight days for SW-CAH vs. 24 days for SV-CAH (10). In the Swedish population, the time between sampling and the time for recall decreased from 7 days (median) at the beginning of the study to 4 days (median) after 1991 [10]. Additionally, at the beginning of the screening program in Poland, we often noted an increase in time between filter paper sampling and delivery to the screening laboratory that was associated with the use of regular mail [3]. The use of regular mail explained the delay in analyses in our patients. The first filter paper of patient 1 was recorded in the Poznan Regional Screening Laboratory after four days and in Warsaw one day later. However, the 2nd filter paper sample obtained on the 14th day of life was recorded in Warsaw after ten days. Regarding patient 2, the filter paper arrived at the regional laboratory after 6 days and to Warsaw after 11 days. Therefore, in the first patient, we received information about the suspicion of CAH within 26 days of the newborn’s life. This information was received within 16 days of life for the second patient. Since last year, the filter papers have been sent via courier mail from neonatal departments to the screening laboratories. Therefore, such delays are no longer observed.

Findings from both our patients indicate that CAH is occasionally difficult to diagnose based on screening. In the first patient, results obtained from the first filter paper were not obvious. The diagnosis was complicated by the fact that in a phone call with the neonatal department any virilization was excluded. The slight increase in 17-OHP (FIA) concentration and increased 21-deoxycortisol levels with normal androgen levels in the first steroid profile needed to be repeated. Eventually, increased 17-OHP (FIA) concentrations in the second filter paper, significantly decreased cortisol levels in LC/MS/MS, and significantly increased steroid ratios in LC/MS/MS suggested 21-hydroxylase deficiency in this neonate (Table I). Further evaluation of androgen concentrations in plasma and the study of steroid profiles in 24-h urine collection facilitated the diagnosis of SV-CAH (Tables II and III). In this case, the urinary steroid profile analysis was the most helpful in establishing a correct diagnosis. Genetic analysis confirmed the diagnosis definitively. Unclear results in the first patient were associated with SV-CAH. Lack of information about virilization on the first filter paper extended the time of analysis, which caused a delay in the diagnosis. Approximately 70% of CYP21A2 disease-causing mutations are pseudogene-derived variants due to gene conversion, involving the transfer of deleterious mutations from pseudogene to the active CYP21A2 gene [17]. Most patients with CAH are compound heterozygotes carrying two different disease-causing mutations. The phenotype is defined by the mutation retaining the most enzyme activity [18]. Similar to that noted in patient 1, SV-CAH occurs in approximately 76% of patients with CAH who carry the p.I172N mutation on one allele and a severe mutation on the other, whereas 23% of these patients present with SW-CAH. The intron 2G variant primarily results in SW-CAH. However, 20% of patients have an SV phenotype [18]. Genetic analysis in patient 2 revealed a carrier state. Nevertheless, clinical evaluation, the insufficient increase in cortisol levels, and an abnormal increase in the 17-OHP concentration in the Synacthen test allowed the diagnosis of SV-CAH. These results suggested the presence of an additional mutation that has not been detected by the given method to date. Incorporating the molecular analysis of the CYP21A2 gene into neonatal screening can improve screening specificity and may also aid in the clinical management of the disease [5, 19]. Such analysis helps to discriminate between real cases and false positives and to clarify borderline cases, including NC-CAH patients with persistent elevated 17-OHP concentrations. The analysis can also be used to diagnose carriers of NC-CAH [5, 12, 19].

In summary, we report two girls with SV-CAH who received a substantial benefit from neonatal screening. They were discharged from the neonatal department without any suspicion of CAH despite mild virilization. During verification, CAH testing with Synacthen revealed a decreased response in cortisol synthesis, so these patients manifest adrenal insufficiency in challenging situations. Early diagnosis allowed the administration of more rapid treatment to prevent further virilization and development of precocious puberty.

Conclusions

As we demonstrate, a milder form of CAH may experience great benefit from this screening, especially when these cases present with mild virilization that could be missed. However, this condition should not be missed. Careful evaluation of external genitals in neonatological departments is critical. In female newborns, physicians should be focused on the even smallest signs of the virilization. The Screening Regional Laboratory should be informed about each case with even mild virilization of external genitals or with skin hyperpigmentation to perform a complete screening immediately decreasing significantly the time between taking the paper sample and the final diagnosis.

Conflict of interests

none declared.

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