Novel pathogenic OCRL mutations and genotype–phenotype analysis of Chinese children affected by oculocerebrorenal syndrome: two cases and a literature review

Background Oculocerebrorenal syndrome of Lowe is a rare X-linked disorder characterized by congenital cataracts, mental retardation, and proximal tubulopathy. This condition is caused by a mutation of OCRL gene (located at chromosome Xq26.1), which encodes an inositol polyphosphate 5-phosphatase. Case presentation We identified two novel OCRL mutations in two unrelated Chinese boys, each with a severe phenotype of Lowe syndrome. A novel de novo deletion (hemizygous c.659_662delAGGG, p.E220Vfs*29) was present in patient 1 and a novel splicing mutation (hemizygous c.2257-2A > T) that was maternally inherited was present in patient 2. A renal biopsy in patient 2 indicated mild mesangial proliferative glomerulonephritis, mild focal mononuclear cells infiltration, and interstitial focal fibrosis. Moreover, renal expression of OCRL-1 protein in patient 2 was significantly reduced compared to a control patient with thin basement membrane disease. Conclusions This study reports two novel OCRL variants associated with severe ocular and neurologic deficiency, despite only mild renal dysfunction. Based on our two patients and a literature review, the genotype–phenotype correlation of OCRL mutations with this severe phenotype of Lowe syndrome suggest a possible clustering of missense, deletion, and nonsense mutations in the 5-phosphatase domain and Rho-GAP domain in the Chinese population.


Background
Oculocerebrorenal syndrome of Lowe (OCRL; OMIM #309000), also known as Lowe syndrome, is an X-linked recessive multisystem disorder in which patients present with major abnormalities of the eyes (congenital cataracts), the kidneys (renal tubular acidosis, Fanconi syndrome, renal rickets), and the central nervous system (hypotonia, areflexia, and mental retardation) [1,2].
It is a rare disease with an estimated prevalence of about 1/500,000 in the general population. The manifestations of tubular dysfunction at onset vary among patients, and disease severity tends to increase with age. Proteinuria with low molecular weight (LMW) proteins is invariably present and aminoaciduria, hyperphosphaturia, bicarbonaturia, and hypercalciuria are frequently present. Progressive proximal tubulopathy ultimately leads to renal failure [2,3].
This disease results from mutations of the OCRL gene (chromosome Xq26.1), which contains 24 exons and encodes a 105-kD phosphatidylinositol (4,5) biphosphate (PI(4,5)P2) 5-phosphatase [4,5]. This protein is primarily located in the trans-Golgi network, endosomes, and endocytic clathrin-coated pits. A deficiency of this protein leads to dysregulation of vesicular transport, which may be decisive for the development of organ dysfunction that is typical of Lowe syndrome [6]. Most pathogenic mutations are deletions, frame-shifts, or premature termination codons; missense mutations and splice-site mutations are less frequent [7]. Here, we report two novel pathogenic DNA variations, a hemizygous deletion mutation c.659_662delAGGG and a hemizygous splicing mutation c.2257-2A > T, in two boys from China who had proximal tubulopathy and congenital cataracts due to Lowe syndrome, and discuss the genotype-phenotype correlations of this disease.

Case 1
A 5-year-old boy was referred to our department with proteinuria, delayed motor milestones, hypotonia, congenital cataract, and failure to thrive. His past medical history indicated he was born at full term after a normal pregnancy, received surgery for congenital cataracts at the age of 3 months, and experienced several limb fractures. He was the first child of a nonconsanguineous marriage, and detailed pedigree analysis indicated no family history of congenital disorders. At birth, his weight was 3200 g (-1SD-Median) and length was 51 cm (Median-+ 1SD). The boy lifted his head at 8 months, sat up at 12 months, walked unassisted at 30 months, and talked at 3 years.
The physical examination at presentation indicated his body weight was 13.3 kg (< -3SD) and length of 96 cm (< -3SD). He presented with slight frontal bossing, deepset eyes, chubby cheeks, low-set ears, sparse hair, funnel chest, simian line, joint hypermobility, decreased muscle tone, and hyporeflexia. The laboratory findings indicated occasionally positive urine glucose, hypercalciuria, phosphaturia, mild proteinuria, β2-microglobulinuria, metabolic acidosis, and occasional elevations of creatinine kinase and lactate dehydrogenase ( Table 1). The estimated glomerular filtration rate (eGFR), calculated using the Schwartz formula, was 162.6 mL/min/1.73 m 2 . Renal size and shape were normal based on an ultrasound examination. Magnetic resonance imaging (MRI) of the brain indicated mild ventriculomegaly, lacunar lesions in the bilateral white matter consistent with periventricular leukomalacia, and multiple gliotic lesions, which were hypointense on T1-weighted and hyperintense on T2-weighted analyses (Fig. 1). An electroencephalography examination indicated no abnormalities. He was attending a school for children with special needs because his IQ was 55 and he had serious sensory integrative dysfunction.
Whole-exome sequencing, with validation by Sanger sequencing, indicated a de novo hemizygous pathogenetic c.659_662delAGGG mutation in exon 8 of the OCRL gene (NM_000276.3; Fig. 2a), confirming the diagnosis. This deletion caused a frame shift from protein position 220 (between the PH and 5-phosphatase domains) leading to an insertion of 28 aberrant amino acids and a premature termination codon, resulting in a truncated protein of 247 out of 901 amino acids (p.E220Vfs*29; Fig. 2b) with an altered three-dimensional structure (Fig. 2c).
To date, he is receiving treatment with an angiotensin converting enzyme inhibitor (ACEI) for proteinuria, hydrochlorothiazide for hypercalciuria, a citrate mixture for metabolic acidosis, and rehabilitation training.

Case 2
The boy, 7 months old, was the first baby of a healthy nonconsanguineous couple. The pregnancy was uneventful, the baby had spontaneous vaginal delivery, and his birth weight was 3450 g (Median-+ 1SD). The boy had bilateral cataracts since birth, and underwent surgery at the age of 3 months, but his visual acuity remained poor. At the age of 7 months, he could not roll over or crawl, and could not sit without support. He was admitted to our hospital with proteinuria. At admission, physical examination indicated his weight was 11 kg (+ 2SD-+ 3SD), height was 76 cm (+ 2SD-+ 3SD), and that he had sparse hair, chubby cheeks, bilateral nystagmus, visual impairment,   size and shape of the kidneys were normal (left kidney: 6.5 × 2.5 cm, right kidney: 6.0 × 2.5 cm). MRI of the brain indicated severe ventriculomegaly, white matter shrinkage, leukoaraiosis, cerebellar hypoplasia, and a large cistern magna cyst (Fig. 3a). The electroencephalography results were normal. He could not complete the evaluation of psychomotor development because of poor vision. Histological examination of a renal biopsy sample indicated mild mesangial proliferation, mild infiltration of focal mononuclear cells, and interstitial focal fibrosis (Fig. 3b). Tubular lesions, including atrophy, necrosis, dilatation, and protein casts, were not detected.
To confirm the clinical diagnosis of Lowe syndrome, we analyzed the OCRL gene. Whole-exome sequencing, with Sanger sequencing validation, indicated a hemizygous c.2257-2A > T DNA variant in OCRL intron 20  Fig. 4a), a novel splicing variant. We then designed two pairs of primers for reverse transcription PCR of exon 8 and exon 12, but this yielded no transcriptional products. Therefore, we speculated that the mutated transcript was removed by nonsense mediated degradation (NMD) of the mRNA. We only detected the expression of OCRL-1 protein in renal tissues by immunohistochemistry using an anti-OCRL polyclonal antibody against the C-terminus of the human OCRL-1 protein (Proteintech Group, USA). This patient had a markedly reduced content of OCRL-1 in kidney tissue compared with a control patient with thin membrane basement disease (Fig. 4b).
Thus, this splicing mutation in the OCRL gene led to almost no expression of the wild-type protein. The patient's mother was heterozygous for the c.2257-2A > T mutation, but had no proximal tubulopathy, and refused an ophthalmologic examination.
We treated this patient with ACEI for proteinuria, a citrate mixture for metabolic acidosis, hydrochlorothiazide for hypercalciuria, intraocular lens implantation, and rehabilitation training to improve his motor and sensory integrative function.

Discussion and conclusion
The clinical diagnosis of Lowe syndrome is based on specific ophthalmologic, renal and neurologic abnormalities [8]. Bilateral cataract is a hallmark finding among all clinical features. A history of cataract surgery during the early infantile period provided an important clue for the diagnosis of Lowe syndrome in the patients. The neurological features of Lowe syndrome are muscle hypotonia, areflexia, intellectual disability, seizures, behavioral abnormalities (e.g., stubbornness, aggression, irritability, temper tantrums, complex repetitive purposeless movements, etc.), and abnormal findings in neuroimaging, such as brain atrophy, delayed myelination, mild ventriculomegaly, and hyperintense cerebral white matter on MRI T2-weighted images [9]. The two patients described here had the common clinical manifestations of muscle hypotonia, areflexia, and intellectual disability.
An MRI scan showed mild ventriculomegaly, bilateral periventricular leukomalacia, and multiple gliotic lesions in patient 1, and brain atrophy, leukoaraiosis, and ventriculomegaly in patient 2. Previous studies of affected patients reported the renal phenotype included LMW proteinuria, aminoaciduria, macroalbuminuria, hyperphosphaturia, hypercalciuria, glycosuria, metabolic acidosis, and progressive renal failure [7,8]. Renal tubular dysfunction is not always present at birth, but usually manifests within the first few weeks to months of life. The onset of renal tubulopathy can be asymptomatic, but can also manifest as Fanconi syndrome or even chronic renal failure, and disease severity tends to increase with age. LWM proteinuria is a prominent finding and occurs in all patients, although aminoaciduria, bicarbonaturia, and hypercalciuria are also frequently present [6]. Both of our patients had incomplete Fanconi syndrome. Thus, tubular proteinuria, hypercalciuria, phosphaturia, metabolic acidosis, and focal interstitial fibrosis were present, but other renal tubular functions were normal. We therefore consider our patients to have a severe phenotype of Lowe syndrome.
Clinical findings are considered adequate for the diagnosis of Lowe syndrome, but gene analysis is necessary for genetic counseling and analysis of genotype-phenotype correlation. According to the Human Gene Mutation Database (http:// www. hgmd. cf. ac. uk/ ac/ index. php), there are approximately 250 pathogenic DNA variations of OCRL, and more than 90% are in exon 10-18 and exon 19-23. Our patient 1 had a c.659_662delAGGG mutation in exon 8, which caused a frameshift and a premature termination codon at aa 248. Patient 2 had one splice-site mutation in intron 20, which presumably led to abnormal splicing of the RNA precursor and degradation of the mutated transcript by NMD. The two mutations identified here were not previously reported in any other , which was inherited from his mother. The IVS20 sequencing result for the mother indicated a heterozygous mutation. b Renal immunohistochemical staining of OCRL-1 in patient 2 and a control patient with thin basement membrane disease. Patient 2 had a significantly reduced OCRL-1 protein level compared to the control patients with Lowe syndrome, and these two mutations seem related to a severe phenotype of Lowe syndrome.
To date, 30 OCRL mutations have been identified in Chinese patients with Lowe syndrome, including the two patients identified here (Table 2) [10][11][12][13][14][15][16][17][18][19][20][21][22][23][24][25][26]. Frameshift, splicing, or nonsense mutations leading to truncated proteins account for 67% of these mutations, missense mutations account for 27%, and genomic deletions account for 6%. Forty percent of these mutations occur in exons 9-16 (which encode the 5-phosphatase domain) and most of these mutations are single base pair missense changes. Another 40% of these mutations occur in exons 18-23 (which encode the RhoGAP-like domain in C terminus) and most of them cause truncated proteins. There was only one reported deletion mutation in exon 5 (which partially encodes the PH domain) and two reported mutations in exon 8 (which encodes the linkage domain between the PH and 5-phosphatase domains) that led to truncated proteins. Thus, based on literature review and our data, the genotype-phenotype correlation of OCRL mutations with the severe phenotype indicated clustering of frame-shifts and splicing mutations in or near the 5-phosphatase domain and the RhoGAP-like domain.
In summary, we identified two patients with novel OCRL variants who had severe ocular and neurologic deficiency, although only mild renal dysfunction. This study also emphasizes that a genotype-phenotype correlation of OCRL mutations with a severe phenotype of Lowe syndrome due to clustering of missense, deletion, and nonsense mutations in the 5-phosphatase domain and the Rho-GAP domain in the Chinese population.