Comprehensive genetic diagnosis of Japanese patients with severe proteinuria

Numerous disease-causing gene mutations have been identified in proteinuric diseases, such as nephrotic syndrome and glomerulosclerosis. This report describes the results of comprehensive genetic diagnosis of Japanese patients with severe proteinuria. In addition, the report describes the clinical characteristics of patients with monogenic disease-causing mutations. We conducted comprehensive gene screening of patients who had either congenital nephrotic syndrome, infantile nephrotic syndrome, steroid-resistant nephrotic syndrome, or focal segmental glomerular sclerosis. Using targeted next-generation sequencing, 60 podocyte-related genes were screened in 230 unrelated patients with proteinuria. A retrospective review of clinical data was conducted for these patients. We detected monogenic disease-causing mutations in 30% (69 of 230) of patients among 19 of the screened genes. Common genes with disease-causing mutations were WT1 (25%), NPHS1 (12%), INF2 (12%), TRPC6 (10%), and LAMB2 (9%). With various immunosuppressive or renoprotective therapies, remission of proteinuria in patients with unknown causative mutations was observed in 26% of patients, whereas only 5% of patients with monogenic disease-causing mutations exhibited complete remission. We assessed the genetic backgrounds of Japanese patients with severe proteinuria. The proportion of patients with gene defects was similar to that of other reports, but the disease-causing gene mutation frequency was considerably different.

Studies of Western and Chinese cohorts of paediatric SRNS patients showed that the results of genetic analyses vary among ethnicities 8,9 . Following the advent of NGS, the discovery of proteinuric disease-causing gene mutations in patients has grown rapidly, although the exact incidence remains unclear. Until now, there have been no large-scale mutation screening studies of Japanese patients with nephrotic syndrome.
In this study, we used targeted NGS for simultaneous sequencing of 60 podocyte-related genes and aimed to clarify the clinical characteristics of Japanese patients with one of the following diseases: CNS, INS, SRNS, FSGS, or asymptomatic proteinuria with likely genetic disease.

Results
Mutations. We collected samples from facilities throughout Japan ( Supplementary Fig. S1). A total of 230 unrelated patients (132 men/boys and 98 women/girls) were included. Their median age at disease onset was 3 years (range, 1 day to 65 years). Of these 230 patients, 10 were diagnosed with CNS, 14 were diagnosed with INS, 101 were diagnosed with SRNS, and 105 were diagnosed with FSGS or asymptomatic proteinuria. We detected disease-causing gene mutations in 69 of 230 unrelated patients (30%). The coverage depths of detected genes are shown in Supplementary Table S1. One of the 69 patients was from a consanguineous family, whereas 15 patients had a positive family history of proteinuria, and 15 patients had a positive family history of renal failure (Table 1). In the 25 patients harbouring autosomal recessive disease-causing mutations, four homozygous and 21 compound heterozygous mutations were found ( Table 2).
We detected the disease-causing gene mutation in 85% of patients with CNS, 53% of patients with INS, 26% of patients with onset age of 1-3 years, 17% of patients with onset age of 4-6 years, 31% of patients with onset age of 7-12 years, 20% of patients with onset age of 13-18 years, and 20% of patients with onset age of 19 years or older ( Supplementary Fig. S2). WT1 gene variants were most common, detected in 17 patients; variants in NPHS1 and INF2 were detected in eight patients, variants in TRPC6 were detected in seven patients, and variants in LAMB2 were detected in six patients (Table 3).
Genes with disease-causing mutations within the first 1 year of life were as follows: 37% of mutations in WT1, 26% of mutations in NPHS1, 26% of mutations in LAMB2, and 11% of mutations in other genes. WT1 was also the most frequent gene mutated in individuals with onset of SRNS after the age of 1 year. In 27 (12%) patients, one or several extra-renal abnormalities were reported; these included symptoms suggestive of Denys-Drash syndrome (caused by WT1 gene mutation and characterised by nephropathy, Wilms tumour, and genital abnormalities) and Pierson syndrome (caused by LAMB2 gene mutation and characterised by the occurrence of congenital nephrotic syndrome and ocular anomalies in combination with microcoria).

Discussion
In this study, we found that 30% (69 of 230) of the patients had a single gene defect in one of 60 currently known podocyte-related genes in the Japanese population. In a previous study 8 , genetic diagnoses were established in 526 patients from 183 families (detection rate of 29.5%); four genes were identified as major SRNS genes: NPHS2 (9.93%), NPHS1 (7.34%), WT1 (4.77%), and PLCE1 (2.17%). The highest rate of mutation detection (69.4%) was recorded in the youngest group of patients (0-3 months); this proportion decreased with age. In the PodoNet study 15 , genetic disease was identified in 23.6% of patients; the most common mutated genes were NPHS2, WT1, and NPHS1. In that report, the proportion of patients with gene mutations also decreased with age; it was 66% in patients with CNS, whereas it decreased to 15-16% in older children. In the PodoNet study, the distribution of causative genes in patients with CNS was as follows: 40% had mutations in NPHS1, 10.6% had mutations in NPHS2, 8.5% had mutations in WT1, 5.5% had mutations in LAMB2, and 4.7% had mutations in all other genes (combined). In the present study, genetic diagnoses were established in 69 of 230 unrelated patients (30%); the mutation detection rate was similar. Furthermore, common genes were WT1 (25%), NPHS1 (12%), INF2 (12%), TRPC6 (10%), and LAMB2 (9%). In the present study, the distribution of causative genes in patients with CNS was as follows: 36% had mutations in NPHS1, 36% had mutations in LAMB2, and 18% had mutations in WT1. No NPHS2 mutations were detected in our study, which was consistent with the results of a study of Korean children  Neph139 with SRNS (patients with CNS were excluded from that study) 16 . In China, the most common mutated genes were ADCK4 (6.67%), NPHS1 (5.83%), WT1 (5.83%), and NPHS2 (3.33%) 9 . The results of these studies show that there are differences in the types and frequencies of mutations among ethnicities and regions. The Child Welfare Law, passed in 1961 in Japan, mandated urinary screening for preschool children, typically at 3 years of age. The purpose of urinary screening for preschool children was to prevent progression to ESRD or to improve the quality of life of children who were expected to develop ESRD. This first urinalysis is performed by using dip-and-reagent strips. In our study, we detected the disease-causing gene mutation in 41% of patients at the age of 3 years; this high detection rate was likely because of the mandatory urine screening for preschool children, which helped to detect the presence of proteinuria and could increase the likelihood that genetic analyses were conducted in affected children.
The treatment of SRNS is a challenging task for nephrologists because of its poor response to immunosuppressive drugs. High-dose steroids, cyclophosphamide, calcineurin inhibitors, mycophenolate mofetil, and rituximab have been used with variable success rates in children. However, complete remission of non-genetic SRNS was observed in 78% of patients during calcineurin inhibitor therapy 17 . In contrast, genetic SRNS was associated with a high rate of ESRD development: one patient with genetic SRNS experienced complete remission and 16% of patients with genetic SRNS experienced partial remission after calcineurin inhibitor therapy 17 . In our study, complete remission of SRNS without mutations was observed in 26% of patients during immunosuppressive therapy. However, this proportion does not reflect the natural clinical course of SRNS because most patients with SRNS who do not have mutations will be treated with immunosuppressants, such as repeated steroid pulses or rituximab treatment after genetic analyses, and there is insufficient long-term follow-up data for these types of patients. Complete remission of nephrotic syndrome in patients with mutations was observed in 5% (2/37) of patients during treatment with immunosuppressive therapies and in one patient during treatment with angiotensin-converting enzyme inhibitors. Notably, angiotensin-converting enzyme inhibitors and angiotensin receptor blockers may cause urinary protein reduction and have renoprotective effects. However, a previous study Neph19 www.nature.com/scientificreports www.nature.com/scientificreports/ showed that more patients reached ESRD when using calcineurin inhibitors; the investigators concluded that calcineurin inhibitors may cause proteinuria reduction, but may negatively influence kidney function 17 . Most patients with nephrotic syndrome who have mutations do not respond to immunosuppressive therapy; however, patients with disease-causing mutations in PLCE1 18 and TRPC6 19 at least partially respond to therapy. Thus far, there are insufficient data to determine whether this proteinuria reduction has a renoprotective effect, and further studies of extended cohorts are needed.
The identification of gene mutations is important for decision-making in terms of future treatment strategies and predicting prognosis. However, it is not yet feasible to perform genetic testing in all patients with proteinuria. Therefore, it is necessary to consider which patients should undergo genetic testing. In previous reports of patients with SRNS, the likelihood of identifying a genetic mutation was inversely related to age at disease onset and was increased in patients with positive family history and in those with extra-renal manifestations 7 . In our study, we compared patients with and without known causative mutations, among all patients. The results showed that risk factors of genetic disease were younger age, family history, absence of oedema, and absence of remission. Importantly, absence of remission was strongly associated with genetic disease in this study. In a previous report of adult-onset FSGS, secondary FSGS (i.e., resistance to immunosuppression and atypical primary FSGS) was considered for genetic evaluation 20 ; our results concur with those of the prior report.  This study had several limitations. First, this was a cross-sectional retrospective study with a small study population, which limits the generalisability of the findings. Second, the examinations of individual patients relied entirely on the attending clinicians' decisions, due to the retrospective nature of the study. Finally, treatment details were not accessible for some patients, which limited our ability to make inferences regarding their disease characteristics.     Table 6. Comparison of clinical phenotype between patients with and without mutations in the analysed genes in Japanese patients. *Median (interquartile range).
www.nature.com/scientificreports www.nature.com/scientificreports/ In conclusion, we found pathogenic disease-causing gene mutations in Japanese patients with severe proteinuria. Detection of these mutations in podocyte-related genes will be helpful in treatment and prediction of renal outcome.

patients. This study protocol was approved by the Institutional Review Board of Kobe University Graduate
School of Medicine (IRB approval number 301). Informed consent was obtained from the patients or their family members in this study. The patients were recruited between January 2016 and December 2018. Inclusion in the study was based on fulfilment of one of the following criteria: (i) diagnosis of CNS, which presents within the first 3 months of life; (ii) diagnosis of INS, which presents between 3-12 months of age; (iii) diagnosis of SRNS, which is defined by persistent proteinuria after 4 weeks of daily treatment with 60 mg/m 2 prednisone; (iv) diagnosis of FSGS or asymptomatic proteinuria. Asymptomatic proteinuria was defined as the absence of who extra-renal symptoms or the presence of proteinuria and microhaematuria. (Supplementary Table S2). Details regarding family history and other clinical features were obtained from the referring clinician or the patient's hospital records. eGFR was calculated for ages 3 month to 18 years using the creatinine based eGFR formula in Japanese child 21,22 . For the patients aged <3 month, eGFR was calculated using the original Schwartz formula 23 as follows: k × body length (cm)/serum Cr level (mg/dL). For this study, the k values was set as 0.45.

Genetic analysis.
As we previously reported 24 , genomic DNA was isolated from peripheral blood leukocytes from patients and their family members using the Quick Gene Mini 80 system (Wako Pure Chemical Industries, Ltd., Tokyo, Japan), in accordance with the manufacturer's instructions. Targeted sequencing using NGS was conducted for genes that are associated with inherited glomerular diseases (Supplementary Table S3). NGS samples were prepared using a HaloPlex target enrichment system kit (Agilent Technologies, Santa Clara, CA, USA), in accordance with the manufacturer's instructions. All indexed DNA samples were amplified by polymerase chain reaction and sequenced using the MiSeq platform (Illumina, San Diego, CA, USA). Resulting sequence data were analysed (from alignment to categorisation of mutations) using SureCall software (version 4.0, Agilent Technologies). As we previously reported 24 , pair analysis by SureCall was used to determine copy number changes in experimental samples relative to a reference sample without a copy number change. We conducted an additional custom array comparative genomic hybridisation when the identified exons (more than two exons) in a single patient exhibited deletions that were all consistent with the clinical presentation of the patient. custom array comparative genomic hybridisation. As we previously reported 25 , we conducted custom array comparative genomic hybridisation for one patient. We selected the COQ6 gene and constructed probes for it and the regions surrounding it. We used a custom HD-comparative genomic hybridisation microarray, 8 × 15 K (Agilent Technologies), in accordance with the manufacturer's instructions. We used Agilent CytoGenomics software (Agilent Technologies) to analyse chromosomal patterns within the microarray profiles.

Statistical analysis.
Results are presented as median and interquartile range (IQR). The chi-squared test or Fisher's exact test was used to compare variables between two groups. The Mann-Whitney U test was used to compare median differences between two experimental groups. Multivariate logistic regression analysis was performed to calculate odds ratios (ORs) and 95% confidence intervals (95% CIs) after controlling for potential confounders. Statistical analysis was performed using standard statistical software (JMP version 10 for Windows; SAS Institute, Cary, NC, USA). In all tests, p < 0.05 was considered statistically significant.

Data availability
The data are not available for public access because of patient privacy concerns, but are available from the corresponding author on reasonable request.  Table 7. Multivariate logistic regression analysis of risk factors for patients with mutations.