Novel aggrecan variant, p. Gln2364Pro, causes severe familial nonsyndromic adult short stature and poor growth hormone response in Chinese children

This study was approved by the Hospital Ethics Committee of the Children’s Hospital of Fudan University. Three children from the same large family, comprising 90 members, were recruited. Two of the children (Fig. 1. IV:23 and IV:44) were initially referred to us due to their short statures, according to the growth charts for Chinese children and adolescents aged 0 to 18 years [13]. Normal GH secretion in both children was confirmed by a peak of GH ≥10 ng/mL in insulin or arginine provocative tests. After evident physical deformities and organic etiologies were excluded, the primary diagnosis of ISS was made according to the diagnosis consensus [3]. The third child, for whom an initial height record was lacking, had height (Fig. 1. III:21) -0.88 standard deviation score (SDS) from the same family and had received 1 year of GH therapy before being referred to our clinic. We initiated GH therapy in these three children at a dose between 40 and 60 μg/kg/d and titrated to maintain serum IGF-1 levels between the average and + 2 standard deviations (SDs) of the reference [3]. All three children showed a poor response to GH treatment according to the criterion of SDS < 0.5 proposed by Patel and Clayton [14]. Therefore, the three children and their family members were offered genetic testing. Among the 90 family members, 62 subjects were available.

Whole exome sequencing was performed with genomic DNA extracted (QIAamp DNA Blood Mini kit, Qiagen, Germany) from subjects’ blood samples. Exomes were enriched with Illumina’s SureSelect Human All Exon kit V4, targeting 50 Mb of sequence from exons and flanking regions. Sequencing was performed with the Illumina HiSeq 2000 platform. Reads with adaptors, reads with > 10% of unknown bases (Ns), and low-quality reads with > 50% of low-quality bases (i.e., bases with a sequencing quality of 5 or less) were discarded from the raw data to generate clean reads, 90-bp paired-end and with at least 100-fold average sequencing depth. Clean reads were aligned to the reference human genome (UCSC hg19) by using the Burrows-Wheeler Aligner (BWA) (v.0.5.9-r16). Subsequent processing steps of sorting, merging, and removing duplicates for the BAM files were performed by using SAMtools and Picard (http://​broadinstitute.​github.​io/​picard/​). Mutation calls, which differed from the reference sequence, were obtained with the use of GATK. Mutations were annotated by ANNOVAR and VEP software [15, 16]. Mutations with suboptimal quality scores were removed from consideration. The remaining mutations were compared computationally with the list of reported mutations from the Human Gene Mutation Database (HGMD, professional version). Mutations in this database with minor allele frequency < 5% according to either the 1000 Genomes Project or ExAC data of The Exome Aggregation Consortium (http://​exac.​broadinstitute.​org/​) were retained. For changes that were not represented in the HGMD, synonymous mutations, intronic mutations that were > 15 bp from exon boundaries (which are unlikely to affect messenger RNA splicing), and common mutations (minor allele frequency > 1%) were discarded [15, 16].

To assess the effects of the variant, we conducted analyses using SIFT, PolyPhen-2, and MutationTaster software, to predict possible deleterious effects [17‐19]. In addition, we performed conservation analysis, using the PhyloP score embedded in the USCS genome browser [20]. Three-dimensional models of aggrecan protein were produced by SWISS-MODEL SERVER [21].

After the identification of an ACAN variant in family members, we performed Sanger sequencing on PCR products containing the variant (in exon 14). The purified DNA was used as template for PCR amplification. The reaction mixture (20 μL) contained 50 ng DNA; 1 U Taq DNA polymerase (Promega, USA); 1.5 mM MgCl₂; 0.25 mM each dNTP; and 0.5 μM primers. The primers for the amplification of ACAN were as follows: ACAN-Forward: CATCTGCCATCCCCTGGT, ACAN-Reverse: CCTACACCGCCACTCTCCTC. The thermal cycling conditions for the PCR reactions consisted of an initial denaturation step at 95 °C for 5 min; 35 cycles of denaturation at 95 °C for 30 s, primer annealing at 58 °C for 30 s, and extension at 72 °C for 30 s; and a final step at 72 °C for 7 min. The PCR products were sequenced in an ABI sequencer 3500 xL GA (Applied Biosystems). The sequence data were evaluated using Mutation Surveyor software and compared with the reference sequence of ACAN (NM_001135).

After identification of ACAN variant in the three children who came to our clinic, we invited all family members to participate in our study; the pedigree is shown in Fig. 1. Genotyping and collection of basic information (height, age, and history of bone disorders) in the adult family members were conducted after obtaining informed consent from the subjects. For persons younger than 18 y, informed consent was obtained from the parents.

During GH treatment of the three children, we measured the levels of serum IGF-1 and IGF-binding protein 3 (IGFBP3) every three or six months by solid-phase, two-site chemiluminescent immunometric assay via an automated MMULITE 1000 immunoassay system (Siemens, Munich, Germany).

Whole exome sequencing to a median of 150× 125.47 (125.47~ 165.65) coverage in the index patients identified 825,823 genetic variants of which 119 were not found in dbSNP137, ExAC, the 1000 Genomes database, or in internal database at 0.5% allele frequency. Further analysis showed that only one variant, c.7465 T > C (p. Gln2364Pro), was consistent with the phenotype of the index and shared by the three affected children in this family. Subsequent Sanger sequencing detected the same variant (p. Gln2364Pro) totally in 19 of 62 blood samples available which was not present in the HGMD or GNOMAD databases. These 19 subjects (10 females and 9 males) ranged in age from 4.1 to 60.6 y and included 7 children (< 18 y; 3 females, 4 males) and 12 adults (7 females, 5 males). The missense variant was predicted by in silico tools to be deleterious (Table 1). Amino acid conservation analysis showed that the affected site was highly conserved in at least fifteen species, including humans (Additional file 1: Figure S1). The three-dimensional models for aggrecan protein with the variant, produced by SWISS-MODEL SERVER (Fig. 2), showed significant anomalies in the formation of normal dimensional structure.

Among the 31 adult family members (15 females, 16 males), there were 12 adult variant carriers (7 females, 5 males). All of the adults with the ACAN mutation had severe short stature (height < − 2 SD, Table 2), and the difference in height between members with and without the ACAN variant was significant in both genders (p < 0.001, Table 2).

The major characteristics of the three children who received GH treatment are shown in Table 1. The proband (Fig. 1, III:44) was a boy born with normal birth length and weight. However, his father’s height was 153 cm (− 5.36 SDS) and his mother’s height was 140 cm (− 2.33 SDS). He was referred to us at the age of 6.4 y with height 100.5 cm (− 3.74 SDS). After GH therapy, 60 μg/kg/d for 8 years, his height was − 3.75 SD below average, at latest evaluation (age 14.1 y, Fig. 3c).

The affected relative 1 in the family was a girl (Fig. 1. IV:23), born full term, with normal birth length and weight. She was referred to our clinic at the age of 5.6 y with height 104.5 cm (− 2.09 SDS) and bone age (BA) 6.5 y. Her father’s height was 170 cm (− 0.44 SDS), and her mother’s height was 138 cm (− 4.19 SDS). Radiographs showed slight abnormalities of her spine, including cervical-vertebral clefts and apophyses in the upper and lower thoracic vertebrae (Additional file 2: Figure S2). We started GH treatment at dose 40 μg/kg/d, and she received GnRHa for pubertal management at age 7. Her height was − 1.07 SDS at her latest visit (age 9.5 y, Fig. 3a).

Relative 2 (Fig. 1. IV:21) was a boy born with normal birth length and weight at full term. He visited our department at the age of 7.8 y with height 122.5 cm (− 0.88SDS). His father’s height was 150 cm (− 3.72 SDS), and his mother’s height was 160 cm (− 0.11 SDS). His bone age (BA) was 9.5 y at his first visit. He received GH therapy, 50 μg/kg/d (Fig. 3b). He received GnRHa at 12.2 y due to his pubertal development. His latest height was − 0.31 SD (at age 12.8 y, Fig. 3b).

In addition to reporting on our current cases, we reviewed the two other available studies on children with an ACAN variant, which involved 18 patients. The characteristics of these patients and their responses to GH treatment are shown in Table 3. The change in height SDS during the first year of treatment ranged from − 0.5 SDS to 0.8 SDS, and the overall yearly height change during GH treatment was − 0.5 SDS to 0.9 SDS. Among these children, there was a general trend of a gradual reduction in yearly height SDS growth over the course of GH treatment (Fig. 4).