A hypomorphic BMPR1B mutation causes du Pan acromesomelic dysplasia

The proposita was a 38 year-old woman who presented to the genetics clinic because of short stature and limb anomalies. She is the 11^th child (of 11) born to first cousin parents originating from Morocco (Fig. 1a). One of her sisters and two of her brothers are similarly affected; they live in a remote area of Morocco with very limited access to medical care and no detailed clinical information, skeletal radiographs or DNA were available from them. The parents were unaffected; maternal height was 160 cm and paternal height 180 cm.

The proposita had disproportionate short stature with a height of 148 cm (− 2.7 SD) and mild acromesomelic limb shortening. The fibulae were not palpable. She had short fingers and abnormal finger joints with deviations (Fig. 1b). Fingers II and V were most severely affected. Finger nails were normal. The toes were hypoplastic, in particular toes III to V, with broad and short toe nails (Fig. 1b). Radiological examination for the hands revealed proximal symphalangism and dysplastic middle phalanges (absence of the middle phalanx in the index finger, hypoplasia of the middle phalanges with narrow proximal phalangeal joints in the middle and ring fingers, and absence of the middle phalanx and long proximal phalanx in the little finger), shortening of the first metacarpal and a single long phalanx in the thumb, short proximal phalanx of the index finger and narrow carpal joint spaces (Fig. 1c). Radiographs of the feet showed similar findings, including a single misshapen phalanx in the great toe, hypoplasia of the middle phalanx in the second toe, absence of the middle phalanges in the third, fourth, and fifth toes, and calcaneocuboid fusion (Fig. 1c). The ankle joints were mal-aligned. The fibula was totally missing (Fig. 1c).

The proposita reported normal puberty with menarche at 13 years and regular menstrual cycles. Abdominal ultrasound was normal with the presence of a uterus and ovaries of normal size and shape. There was no hypergonadotropic hypogonadism with normal LH, FSH, estradiol and progesterone.

Because the clinical presentation was compatible with du Pan dysplasia we first sequenced the coding region and exon-intron boundaries of GDF5 and identified no mutation. Upon sequencing of BMPR1B we detected a homozygous c.91C>T (p.Arg31Cys) variant (Fig. 1d). No DNA from other affected and unaffected family members was available to test for co-segregation with du Pan dysplasia. Consistent with BMPR1B being located in an autozygous region, genotyping of two highly polymorphic BMPR1B intragenic STRs showed homozygosity and SNP array genotyping confirmed a large (20.2 Mb) homozygous region at the BMPR1B locus in the proposita, defined by the flanking SNPs rs2131361 and rs17278473 (data not shown). Residue Arg31 is moderately conserved in BMPR1B orthologs. It is conserved e.g., in mouse, rat, cat, dog, and platypus; it is replaced with a histidine in e.g., green monkey, panda and hedgehog, and with a glutamine in e.g., opossum and turtles. None of the >60 species included in the UCSC multiple species alignment has a cysteine at the corresponding position. While the ExAC browser (http://​exac.​broadinstitute.​org/​) lists a p.Arg31His substitution (rs200035802) with an allele frequency of 18/121.162, p.Arg31Cys was only identified in 1/121.150 alleles, compatible with p.Arg31Cys being disease causing. Consistently, PolyPhen-2 [16] predicts p.Arg31Cys as “possibly damaging” and p.Arg31His as “benign” (both variants are predicted “not tolerated” by SIFT [17]). Finally, no variant predicting p.Arg31Cys was identified in exome sequences from 30 Moroccan patients with unrelated disorders (Jaber Lyahyai, personal communication) and no p.Arg31Cys homozygotes or heterozygotes were present in the 5,718 exomes included in the Institut Imagine (Paris) in-house database, which is enriched for exomes of Maghrebian individuals, and contains a very conservatively estimated number of Moroccan exomes of 33.

Arg31 is located at the beginning of the BMPR1B ligand binding domain (LBD), suggesting that the p.Arg31Cys mutation may interfere with GDF5 binding. We modeled p.Arg31Cys using the structure of human BMPR1B bound to human GDF5 [13]. Residue 31 shares no direct contact with the ligand GDF5 and is more than 10 Å remote (Fig. 2a). Thus, a direct impact on the GDF5-receptor binding by loss of direct van der Waals interactions seems unlikely. In our in silico models the exchange of Arg31 by cysteine however places an unpaired thiol group in close proximity to Cys32, Cys47, Cys53, and Cys71 (Fig. 2b) thereby possibly allowing for an alternate disulfide network. The model of such a rearranged disulfide bond network suggested that it will not necessarily destroy the BMP receptor’s three-finger toxin fold, but may introduce conformational changes in the disulfide-bond connected loops in particular of the β1β2-loop (Fig. 2c). As this loop is engaged in contacts with GDF5 and has been implicated in ligand recognition and binding (Fig. 2a) [13] even such smaller changes may affect ligand-receptor interaction. The effects of p.Arg31His seem subtler as those predicted for p.Arg31Cys (Fig. 2d).

We performed a luciferase reporter gene assay using the SMAD dependent BRE reporter to determine the signal transduction capacity of the BMPR1B variant Arg31Cys, which is associated with ACD du Pan type in our patient (Fig. 3a). We compared its activity to the previously described BMPR1B mutation Cys53Arg, which is associated with ACD Grebe type and to Arg31His, another allele listed in genomic databases [9]. The WT receptor induced the luciferase expression approximately 8-fold compared to a control vector and was strongly stimulated by the presence of recombinant GDF5. BMPR1B Arg31Cys showed only moderate activity when no ligand was used for stimulation (less than 2-fold). Arg31His induced the SMAD signaling pathway approximately 5-fold, but remained significantly less active than the WT receptor. SMAD1/5/8 activation via the BMPR1B variants Arg31His and Arg31Cys was significantly increased upon ligand stimulation. However, BMPR1B Arg31Cys still could not accomplish the level of BMPR1B Arg31His or BMPR1B WT, pointing to a partial loss of function. In line with previous findings BMPR1B Cys53Arg exhibited no SMAD activity and could not be stimulated by GDF5 either. Confocal microscopy showed that all investigated BMPR1B variants are translocated to the cell surface (Fig. 3b).