Skip to main content

CASE REPORT article

Front. Genet., 05 October 2021
Sec. Genetics of Common and Rare Diseases
This article is part of the Research Topic Improving Medical Diagnosis in Rare Diseases View all 24 articles

Molecular Diagnosis and Prenatal Phenotype Analysis of Eight Fetuses With Ciliopathies

Yuefang Liu&#x;Yuefang Liu1Hui Wang,&#x;Hui Wang2,3Xin JinXin Jin1Qixiang Shao,,
Qixiang Shao2,3,4*Qiong Pan
Qiong Pan1*
  • 1Department of Clinical Genetics, Huai’an Maternity and Child Clinical College of Xuzhou Medical University, Huai’an, China
  • 2Reproductive Sciences Institute, Jiangsu University, Zhenjiang, China
  • 3Department of Immunology, Jiangsu Key Laboratory of Medical Science and Laboratory Medicine, School of Medicine, Zhenjiang, China
  • 4Jiangsu College of Nursing, School of Medical Science and Laboratory Medicine, Huai’an, China

Human ciliopathies are hereditary conditions caused by variants in ciliary-associated genes. Ciliopathies are often characterized by multiple system defects. However, it is not easy to make a definite diagnosis in the prenatal period only based on the imageology. In this report, eight new prenatal cases from five unrelated families diagnosed with ciliopathies were systematically examined. The clinical manifestations of these fetuses showed such prenatal diagnostic features as occipital encephalocele, and polydactyly and polycystic kidneys. Situs inversus caused by CPLANE1 variant was first reported. In Family 1 and Family 3, homozygous variants of CPLANE1 and NPHP4 caused by consanguineous marriage and uniparental disomy were detected by whole-exome sequencing, respectively. In Family 2, Family 4 and Family 5, compound heterozygotes of TMEM67 and DYNC2H1 including two novel missense variants and one novel nonsense variant were identified. The distribution of pathogenic missense variants along TMEM67 gene mainly clustered in the extracellular cysteine rich region, extracellular area with unknown structure, and the transmembrane regions. Genotype-phenotype relationship between CPLANE1 and TMEM67 genes was concluded. This report describes new clinical manifestations and novel variants in CPLANE1, TMEM67, NPHP4, and DYNC2H1.

Introduction

Primary cilia are highly conserved organelles located on the surface of almost all polar cells, which play important roles in tissue morphogenesis, and chemical and mechanical signal transduction (Hirokawa et al., 2006; Copeland, 2020). Genetic variants affecting the structure or function of primary cilia can lead to a broad range of developmental diseases known as ciliopathies. The whole-exome sequencing (WES) has been widely used in the clinical molecular diagnosis of ciliopathies in adults and children. Presently, approximately 187 established ciliopathy-related genes have been identified in humans, variants in which can be associated with 35 ciliopathy syndromes (Reiter and Leroux, 2017; McConnachie et al., 2021). It has been clarified that variant in CPLANE1 causes Joubert syndrome (JBS; MIM#614615), which is characterized by a unique cerebellar and brainstem malformation, also known as molar tooth sign (MTS). Moreover, TMEM67-related ciliopathies are mainly JBS and Meckel syndrome (MKS; MIM#607361). While MKS is a lethal disorder with typical renal cystic dysplasia, polydactyly, and occipital encephalocele. Variants in NPHP4 cause nephronophthisis (NPH; MIM#606966) characterized by end-stage renal disease in the first 2 decades of life. In addition, the typical feature of short-rib thoracic dysplasia (SRTD; MIM#613091) caused by DYNC2H1 variants is skeletal dysplasia. However, the different etiology of ciliopathies and the wide range of genetic variations lead to phenotypic variability. It is challenging to choose appropriate molecular testing in the prenatal period. Therefore, it is important to have a comprehensive understanding of the prenatal phenotypes of different ciliopathy syndromes before the WES testing.

Here we report the typical and atypical features of eight fetuses with pathogenic variants in CPLANE1, TMEM67, NPHP4, and DYNC2H1 found via WES. New clinical manifestations and the discovery of novel genetic variants are helpful for the prenatal diagnosis of ciliopathies.

Patients and Methods

Patients

Eight fetuses from five unrelated families diagnosed with ciliopathies were collected. Informed consents for research investigations were obtained from the relatives of the fetuses. The research protocol was approved by the local ethics committee of Jiangsu Huai’an Maternity and Child Healthcare Hospital (2019036).

Whole-Exome Sequencing

The whole exomes were captured by using Agilent’s SureSelect Whole Exome Gene Detection Kit. High-throughput sequencing was performed by using the Novoseq sequencer from Illumina. The obtained sequence was aligned on the human genome GRCh37/hg19 reference sequence by BWA (Burrows-Wheeler Aligner) software. A BAM (binary sequence alignment map format) file was produced via Picard software. GATK4 (Genome Analysis Toolkit) Realigner Target Creator software and Haplotype Caller software were used to adjust the sequence, extract variants, and generate VCF (Variant Call Format) files. The Annovar software was used to filter and annotate the variant.

Analysis of Variants

All nonsense, frameshift, and canonical splice site variants were considered to be deleterious. The pathogenic potential of missense variants was predicted by PolyPhen2, SIFT, PROVEAN, and Mutation Taster. The frequency of putative variants was obtained from the Human Gene Mutation Database (HGMD), Genome Aggregation Database (gnomAD), and the 1000 Genomes (1000G) database. Conservation of mutated amino acid residues in different species was compared by UCSC. SpliceAI was used to evaluate a destroyed splice site. The deleteriousness of variants was assessed according to American College of Medical Genetics (ACMG) standards and guidelines.

Sanger Sequencing

Sanger sequencing was performed to confirm suspected variant segregation within probands’ family, and the authenticity of variants identified by WES. Primer 5 was used for primer designs. Target DNA of the fetus and its parents was amplified by PCR. Sanger sequencing results were compared with standard sequence in GenBank by SeqMan software.

Case Presentation

Family 1

Family 1 was a consanguineous marriage with a healthy girl and five adverse obstetric outcomes. In addition to two early miscarriages, the third time was due to a widened posterior fossa and vermis hypoplasia at the 27th week of pregnancy without genetic detection. Case 1 was the fifth pregnancy, whose prenatal ultrasound in 18+4th week of pregnancy showed absence of cerebellar vermis, dandy-walker malformation, hydrocephalus, dextrocardia, situs inversus, ventricular septal defect (0.3 cm), and double outlet of fetal right ventricle with pulmonary artery stenosis (Table 1). Pregnancy was terminated at the 23rd week and no obvious abnormality in appearance was observed (Figure 1A). The sixth pregnancy (case 2) showed recurrence of malformations by prenatal ultrasound at the 20th week of fetal development including occipital encephalocele (1.3 × 0.8 cm) (Figure 2A) and intra-uterine growth restriction (Table 1) (Figures 1B,C).

TABLE 1
www.frontiersin.org

TABLE 1. Clinical phenotype and related genetic variants in eight fetuses with ciliopathies from five unrelated families.

FIGURE 1
www.frontiersin.org

FIGURE 1. Phenotypes of ciliary diseases {Family 1 [(A): case 1; (B,C): case 2], Family 4 [(D): case 6], Family 5 [(E,F): case 8], occipital encephalocele (C), polydactyly of hands and feet (D–F), short limb and ribs (D,E)}.

FIGURE 2
www.frontiersin.org

FIGURE 2. Imaging examination of ciliary diseases {Family 1 [(A): case 2], Family 3 [(B): case 5], Family 4 [(C): case 6], Family 5 [(D): case 8], occipital encephalocele (A), increased echogenicity in both renal cortexes (B), fetal X-ray showing bilateral shortened curved femora and disproportionately shortened tibiae (C), bone dysplasia and narrow chest (D)}.

WES revealed case 1 with a novel homozygous frame shift variant of c.7939delC (p.H2647IfsTer51) in CPLANE1 (NM_023073.3). Sanger sequencing confirmed homozygosity in the proband and the heterozygosity in each parent (Table 1). Case 2 was also confirmed with same variant in case 1. The c.7939delC was not present in HGMD, gnomAD, or 1000G databases.

Family 2

Case 3 and case 4 were affected siblings conceived of unrelated healthy parents with two early unexplained miscarriages. Prenatal ultrasound in 23+4rd week of case 3 showed separation of left lateral ventricles (0.9 cm), abnormality of the cerebellum, low amniotic fluid volume (amniotic fluid index 1.5 cm, maximum depth 1.0 cm), pericardial effusion (0.3 cm), and enlarged echogenic kidneys (left kidney 5.7 × 2.8 cm, right kidney 5.4 × 2.8 cm) with renal cysts (Table 1). Case 4 was found with congenital balkes pouch, cystic kidneys, polydactyly, and occipital encephalocele (Table 1). The pregnancy was terminated at the 24th week of gestation. Because prenatal detection and labor induction were performed in another hospital, we only obtained DNA of the two cases without ultrasound images and postnatal fetus examination.

WES was selected by Family 2 and the result showed that case 4 had compound heterozygous variants in TMEM67 gene (NM_153704.6): a missense variant at c.1175C > G (p.P392R) and a synonymous variant at c.2439G > T (p.A813A), which were inherited from the parents, respectively (Table 1). The c.1175C > G, not reported previously, was predicted as damaging by PolyPhen2, SIFT, PROVEAN, and Mutation Taster. Total population frequency of this variant is 3.23185e-05. The c. 2439G > T variant is located at the last base of exon 23 and was classified as a disease-causing variant in HGMD. It might abolish the donor splice site following in silico analysis via SpliceAI. The predicted score of a donor site loss via SpliceAI was 0.64. After this, the DNA of case 3 was subjected to molecular analysis by Sanger sequencing. The result revealed the c.1175C > G and c.2439G > T variants in the TMEM67 gene in case 3.

Family 3

Case 5 was the first pregnancy of unrelated healthy parents. Prenatal diagnosis was performed in the 20th week of pregnancy due to a 12 Mb deletion in chromosome 1 as indicated by noninvasive prenatal testing (NIPT). The Affymetrix CytoScan 750K SNP array was used for chromosomal microarray analysis (CMA) and the result showed a region of homozygosity in 1p36.33-p36.13 (arr[hg19] 1p36.33p36.13 (888,658_18,337,268) x2 hmz) involving no established imprinted genes. In 26+4th week, missing nasal bone, delayed growth and development, and increased echogenicity in both renal cortexes were indicated by ultrasound (Figure 2B and Table 1). Prenatal trio-WES was chosen for further detection. A homozygous variant of c.3730C > T (p.Q1244X) (chr1:5,925,248) in NPHP4 (NM_001184.3) (Table 1) was detected. This variant, occurring in the region of homozygosity, was inherited from the father. These results indicated that a segmental uniparental disomy at 1p36.33-p36.13 inherited from the father caused the autosomal recessive NPH.

Family 4

Case 6 and case 7 were affected sibling fetuses from a non-consanguineous family with a healthy 6-year-old daughter. Ultrasound imaging of case 6 revealed abdominal circumference (10.3 cm), a femur length of 1.3 cm (<5th percentile), a humerus length of 1.0 cm (<5th percentile), and polydactyly. The pregnancy was subsequently terminated at the 18th week of gestation (Figure 1D). Fetal X-ray (Figure 2C) showed bilateral shortened curved femora and disproportionately shortened tibiae. Metaphyseal flaring of femora, tibiae, and fibulae were indicated. Ultrasound imaging of case 7 at the 28th week of gestation from this family exhibited similar sonographic features including small short femur (1.2 cm), narrow chest, light band separation in double kidney collection system (0.8 and 0.9 cm), peritoneal effusion (deepest 0.5 cm), and polydactyly. We only obtained DNA of case 7 but failed to perform postnatal fetus observation.

WES of case 6 revealed the compound heterozygous variants of DYNC2H1 (NM_001377.3): c.152T > G (p.L51R) in exon 1 and c.988C > T (p.R330C) in exon 6. Sanger sequencing confirmed that the c.152T > G was present in the mother, and the c.988C > T in the father (Table 1). Case 7 was also confirmed with variants as case 6 through Sanger sequencing (Table 1). The c.988C > T has been reported as a pathogenic variant (El Hokayem et al., 2012; Schmidts et al., 2013). The c.152T > G was not present in HGMD, gnomAD, or 1000G databases, and was predicted as deleterious following in silico analysis. In addition, the c.152T > G is localized to the region of nucleotide-binding site of the DYNC2H1 gene, which is highly conserved in mouse, rat, and dog orthologs of DYNC2H1 gene.

Family 5

Prenatal ultrasound of case 8 (the first fetus from non-relative parents) in the 12th week of pregnancy showed abnormal NT (4.4 mm). Recheck in the 17th week showed multiple malformations with large abdominal circumference (12.1 cm), ventricular septal defect (0.08 cm), left ventricular dysplasia, valve thickening, and transposition of the great arteries (Table 1). Besides, increased bowel and kidney echo, and bone dysplasia (femur = 1.3 cm, humerus = 0.9 cm, narrow chest) (Figure 2D) were detected. Examination of the aborted fetus showed low-set ears, polydactyly, a swollen abdomen, and short limbs (Figures 1E,F). Compound heterozygous variants of c.4267C > T (p.R1423C) and c.7858C > T (p.R2620X) in DYNC2H1 (NM_001377.3) were identified. We confirmed a heterozygosity in each parent by Sanger sequencing (Table 1). The c.4267C > T was a pathogenic variant in short-rib polydactyly syndromes (SRPS) (Zhang et al., 2018). The c.7858C > T was a novel nonsense variant causing a truncated protein.

Genotypes–Phenotypes Analysis

Since CPLANE1 and TMEM67 variants show significant clinical overlap, genotype-phenotype relationship analysis between them could help discriminate related disorders.

CPLANE1 was identified as causative of OFD6 (orofaciodigital syndrome VI) and JBS. More than 60 pathogenic variants in the CPLANE1 gene have been identified (Srour et al., 2012; Lopez et al., 2014; Vilboux et al., 2017; Bonnard et al., 2018) and 66% of cases carried biallelic truncating variants (Bonnard et al., 2018). Penetrance of common organ systems involving brain, skeleton, and kidney diseases in CPLANE1 patients were compared (Table 2) (Lopez et al., 2014; Vilboux et al., 2017; Bonnard et al., 2018). MTS was nearly 100% detected in both JBS and OFD6. Polydactyly was with higher penetrance (100%) in OFD6 than JBS. The penetrance of occipital encephalocele in both JBS and OFD6 was estimated to be about 20%. However, cystic kidneys, short limbs, and congenital heart disease (CHD) were rarely observed.

TABLE 2
www.frontiersin.org

TABLE 2. The comparison of clinical phenotypes between CPLANE1 and TMEM67.

TMEM67 was identified as causative of JBS and MKS. A genotype-phenotype correlation analysis based on a literature review shows that combination of two truncating variants in TMEM67 gene is more common in lethal MKS than milder JBS (Iannicelli et al., 2010; Szymanska et al., 2012; Bachmann-Gagescu et al., 2015; Vilboux et al., 2017), which suggests that severity of variant changes disease outcomes. Thus, it is reasonable to presume that missense variant of TMEM67 identified in MKS might bring more severe damage to protein function. There were about 58 (likely) pathogenic missense variants in TMEM67 identified thus far including 37 in JBS, 15 in MKS, and 6 in both (Baala et al., 2007; Consugar et al., 2007; Khaddour et al., 2007; Brancati et al., 2009; Doherty et al., 2010; Iannicelli et al., 2010; Suzuki et al., 2016; Vilboux et al., 2017; Radhakrishnan et al., 2019) (Supplemental Table S1). Analysis of the topology of human TMEM67 suggests the presence of a signal peptide (1–36 aa), a cysteine-rich region (50–187 aa), an extracellular area with unknown structure (188–526 aa), seven transmembrane regions (527–967 aa), and a short cytoplasmic tail (968–995 aa) (Figure 3) (Smith et al., 2006). Pathogenic missense variants of TMEM67 mainly fall in the extracellular cysteine rich region, extracellular area with unknown structure, and the seven transmembrane regions (Figure 3). No pathogenic missense variant in the signal peptide and cytoplasmic tail has been reported (Figure 3). The comparison of their distribution along the gene in MKS versus JBS showed no obvious difference.

FIGURE 3
www.frontiersin.org

FIGURE 3. Missense variants of the TMEM67 gene in MKS and JBS. There were about 58 (likely) pathogenic missense variants in the TMEM67 gene identified thus far including 37 in JBS (green), 15 in MKS (red), and 6 in both (blue). The topology of TMEM67: a signal peptide (1–36 aa), a cysteine-rich region (50–187 aa), an extracellular area with unknown structure (188–526 aa), seven transmembrane regions (527–967 aa), and a short cytoplasmic tail (968–995 aa).

Two studies with larger TMEM67 gene mutated cases were reviewed to analyze the characteristic of clinical phenotypes (Table 2) (Brancati et al., 2009; Szymanska et al., 2012; Vilboux et al., 2017). Incidence of liver and kidney diseases caused by TMEM67 variants was high in both JBS and MKS. The prevalence of occipital encephalocele in MKS was higher than in JBS.

Discussion and Conclusion

A clinical diagnosis of JBS can be made by brain imaging showing MTS. However, prenatal diagnosis of JBS has been proved to be difficult because of the relatively non-specific prenatal ultrasound findings. The clinical phenotypes of CPLANE1 mutated cases in this report were highly heterogeneous, with intrafamilial variability. Meanwhile, case 1 and case 2 had no obvious MTS. Consistent with the absence of MTS in our fetuses, Doherty et al. described a JBS fetus with no obvious MTS phenotype instead of a deepening of the interpedullary fossa on MRI (Doherty et al., 2005). Zhu et al. reported a prenatal JBS case with lemon sign and encephalocele (Zhu et al., 2021). Situs inversus, a specific feature in some MKS cases resulted from MKS1 variants (Khaddour et al., 2007), was reported for the first time in our JBS case.

MKS is a perinatally lethal autosomal recessive condition characterized by central nervous system anomalies, hepatic defects, polycystic kidneys, and polydactyly (Radhakrishnan et al., 2019). Hepatic phenotype in the prenatal period could be detected at about the 15th to 26th week (Consugar et al., 2007). MKS fetuses in Family 2 were found with abnormal nervous system, polycystic kidneys, polydactyly but not hepatic defects at the 23rd and 24th weeks of pregnancy.

NPH is a major cause of pediatric end-stage renal disease and the phenotypes were mostly observed in children (Konig et al., 2017). It may be limited to the kidneys or can be associated with extrarenal organ. A study including 250 NPH patients showed that only 6/250 patients (2.4%) were detected with homozygous or compound heterozygous variants of the NPHP4 gene (Hoefele et al., 2005). The prenatal diagnosis is one of the effective ways to avoid the birth of NPH children. However, prenatal NPH cases are rarely described. An NPH fetus with NPHP1 variants manifested bilateral polycystic renal dysplasia and oligohydramnios at 16+th gestational week (Wu et al., 2020). As for the fetus in this study, antenatal ultrasonography showed missing nasal bone and increased echogenicity in both renal cortex in 26+4th week.

There are 111 pathogenic variants of the DYNC2H1 gene that have been identified in 73 families (Zhang et al., 2018). Missense variants in the DYNC2H1 gene had the highest frequency (71/111). Characterized phenotypes were polydactyly with a prevalence 30/73 (Zhang et al., 2018) and short limbs with a prevalence of 23/29 (Schmidts et al., 2013), while abnormal retina, kidney, and liver were rare (Schmidts et al., 2013). Prenatal cases in our report were distinguished by profound abnormalities of the skeleton, including markedly short ribs, extremely short limbs, and polydactyly.

In conclusion, this report expands prenatal clinical manifestations of ciliopathies and adds novel variants in CPLANE1, TMEM67, NPHP4, and DYNC2H1 to the literature. Furthermore, detailed prenatal phenotypes of different ciliopathies provide evidence for prenatal WES testing.

Data Availability Statement

The data presented in the study are deposited in the China National GeneBank DataBase (CNGBdb) repository, accession number CNP0002142.

Ethics Statement

The studies involving human participants were reviewed and approved by the Medical Ethics Committee of Huai’an Maternity and Child Health Hospital. Written informed consent to participate in this study was provided by the participants’ legal guardian/next of kin.

Author Contributions

YL, HW, and XJ contributed to the conception. YL collected relevant studies and wrote the manuscript. QS and QP. contributed to the revision, and final approval of the manuscript.

Funding

The present study was supported by grants from by the Maternal and Child Health project of Jiangsu Province (No. F201714, F201707); Open project of Jiangsu Province Key Laboratory (XZSYSKF2020024).

Conflict of Interest

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.

Publisher’s Note

All claims expressed in this article are solely those of the authors and do not necessarily represent those of their affiliated organizations, or those of the publisher, the editors and the reviewers. Any product that may be evaluated in this article, or claim that may be made by its manufacturer, is not guaranteed or endorsed by the publisher.

Supplementary Material

The Supplementary Material for this article can be found online at: https://www.frontiersin.org/articles/10.3389/fgene.2021.705808/full#supplementary-material

References

Baala, L., Romano, S., Khaddour, R., Saunier, S., Smith, U. M., Audollent, S., et al. (2007). The Meckel-Gruber Syndrome Gene, MKS3, Is Mutated in Joubert Syndrome. Am. J. Hum. Genet. 80 (1), 186–194. doi:10.1086/510499

PubMed Abstract | CrossRef Full Text | Google Scholar

Bachmann-Gagescu, R., Dempsey, J. C., Phelps, I. G., O'Roak, B. J., Knutzen, D. M., Rue, T. C., et al. (2015). Joubert Syndrome: a Model for Untangling Recessive Disorders with Extreme Genetic Heterogeneity. J. Med. Genet. 52 (8), 514–522. doi:10.1136/jmedgenet-2015-103087

CrossRef Full Text | Google Scholar

Bonnard, C., Shboul, M., Tonekaboni, S. H., Ng, A. Y. J., Tohari, S., Ghosh, K., et al. (2018). Novel Mutations in the Ciliopathy-Associated Gene CPLANE1 (C5orf42) Cause OFD Syndrome Type VI rather Than Joubert Syndrome. Eur. J. Med. Genet. 61 (10), 585–595. doi:10.1016/j.ejmg.2018.03.012

PubMed Abstract | CrossRef Full Text | Google Scholar

Brancati, F., Iannicelli, M., Travaglini, L., Mazzotta, A., Bertini, E., Boltshauser, E., et al. (2009). MKS3/TMEM67mutations Are a Major Cause of COACH Syndrome, a Joubert Syndrome Related Disorder with Liver Involvement. Hum. Mutat. 30 (2), E432–E442. doi:10.1002/humu.20924

PubMed Abstract | CrossRef Full Text | Google Scholar

Consugar, M. B., Kubly, V. J., Lager, D. J., Hommerding, C. J., Wong, W. C., Bakker, E., et al. (2007). Molecular Diagnostics of Meckel-Gruber Syndrome Highlights Phenotypic Differences between MKS1 and MKS3. Hum. Genet. 121 (5), 591–599. doi:10.1007/s00439-007-0341-3

PubMed Abstract | CrossRef Full Text | Google Scholar

Copeland, J. (2020). Actin-based Regulation of Ciliogenesis - the Long and the Short of it. Semin. Cel Developmental Biol. 102, 132–138. doi:10.1016/j.semcdb.2019.12.005

PubMed Abstract | CrossRef Full Text | Google Scholar

Doherty, D., Glass, I. A., Siebert, J. R., Strouse, P. J., Parisi, M. A., Shaw, D. W. W., et al. (2005). Prenatal Diagnosis in Pregnancies at Risk for Joubert Syndrome by Ultrasound and MRI. Prenat. Diagn. 25 (6), 442–447. doi:10.1002/pd.1145

PubMed Abstract | CrossRef Full Text | Google Scholar

Doherty, D., Parisi, M. A., Finn, L. S., Gunay-Aygun, M., Al-Mateen, M., Bates, D., et al. (2010). Mutations in 3 Genes (MKS3, CC2D2A and RPGRIP1L) Cause COACH Syndrome (Joubert Syndrome with Congenital Hepatic Fibrosis). J. Med. Genet. 47 (1), 8–21. doi:10.1136/jmg.2009.067249

PubMed Abstract | CrossRef Full Text | Google Scholar

El Hokayem, J., Huber, C., Couvé, A., Aziza, J., Baujat, G., Bouvier, R., et al. (2012). NEK1andDYNC2H1are Both Involved in Short Rib Polydactyly Majewski Type but Not in Beemer Langer Cases. J. Med. Genet. 49 (4), 227–233. doi:10.1136/jmedgenet-2011-100717

CrossRef Full Text | Google Scholar

Hirokawa, N., Tanaka, Y., Okada, Y., and Takeda, S. (2006). Nodal Flow and the Generation of Left-Right Asymmetry. Cell 125 (1), 33–45. doi:10.1016/j.cell.2006.03.002

PubMed Abstract | CrossRef Full Text | Google Scholar

Hoefele, J., Sudbrak, R., Reinhardt, R., Lehrack, S., Hennig, S., Imm, A., et al. (2005). Mutational Analysis of theNPHP4 Gene in 250 Patients with Nephronophthisis. Hum. Mutat. 25 (4), 411. doi:10.1002/humu.9326

PubMed Abstract | CrossRef Full Text | Google Scholar

Iannicelli, M., Brancati, F., Mougou-Zerelli, S., Mazzotta, A., Thomas, S., Elkhartoufi, N., et al. (2010). NovelTMEM67mutations and Genotype-Phenotype Correlates in Meckelin-Related Ciliopathies. Hum. Mutat. 31 (5), a–n. doi:10.1002/humu.21239

CrossRef Full Text | Google Scholar

Khaddour, R., Smith, U., Baala, L., Martinovic, J., Clavering, D., Shaffiq, R., et al. (2007). Spectrum ofMKS1andMKS3mutations in Meckel Syndrome: a Genotype-Phenotype Correlation. Hum. Mutat. 28 (5), 523–524. doi:10.1002/humu.9489

PubMed Abstract | CrossRef Full Text | Google Scholar

König, J., Kranz, B., König, S., Schlingmann, K. P., Titieni, A., Tönshoff, B., et al. (2017). Phenotypic Spectrum of Children with Nephronophthisis and Related Ciliopathies. Cjasn 12 (12), 1974–1983. doi:10.2215/CJN.01280217

PubMed Abstract | CrossRef Full Text | Google Scholar

Lopez, E., Thauvin-Robinet, C., Reversade, B., Khartoufi, N. E., Devisme, L., Holder, M., et al. (2014). C5orf42 Is the Major Gene Responsible for OFD Syndrome Type VI. Hum. Genet. 133 (3), 367–377. doi:10.1007/s00439-013-1385-1

PubMed Abstract | CrossRef Full Text | Google Scholar

McConnachie, D. J., Stow, J. L., and Mallett, A. J. (2021). Ciliopathies and the Kidney: A Review. Am. J. Kidney Dis. 77 (3), 410–419. doi:10.1053/j.ajkd.2020.08.012

CrossRef Full Text | Google Scholar

Radhakrishnan, P., Nayak, S. S., Shukla, A., Lindstrand, A., and Girisha, K. M. (2019). Meckel Syndrome: Clinical and Mutation Profile in Six Fetuses. Clin. Genet. 96 (6), 560–565. doi:10.1111/cge.13623

PubMed Abstract | CrossRef Full Text | Google Scholar

Reiter, J. F., and Leroux, M. R. (2017). Genes and Molecular Pathways Underpinning Ciliopathies. Nat. Rev. Mol. Cel Biol 18 (9), 533–547. doi:10.1038/nrm.2017.60

CrossRef Full Text | Google Scholar

Schmidts, M., Arts, H. H., Bongers, E. M. H. F., Yap, Z., Oud, M. M., Antony, D., et al. (2013). Exome Sequencing identifiesDYNC2H1mutations as a Common Cause of Asphyxiating Thoracic Dystrophy (Jeune Syndrome) without Major Polydactyly, Renal or Retinal Involvement. J. Med. Genet. 50 (5), 309–323. doi:10.1136/jmedgenet-2012-101284

CrossRef Full Text | Google Scholar

Smith, U. M., Consugar, M., Tee, L. J., McKee, B. M., Maina, E. N., Whelan, S., et al. (2006). The Transmembrane Protein Meckelin (MKS3) Is Mutated in Meckel-Gruber Syndrome and the Wpk Rat. Nat. Genet. 38 (2), 191–196. doi:10.1038/ng1713

PubMed Abstract | CrossRef Full Text | Google Scholar

Srour, M., Schwartzentruber, J., Hamdan, F. F., Ospina, L. H., Patry, L., Labuda, D., et al. (2012). Mutations in C5ORF42 Cause Joubert Syndrome in the French Canadian Population. Am. J. Hum. Genet. 90 (4), 693–700. doi:10.1016/j.ajhg.2012.02.011

PubMed Abstract | CrossRef Full Text | Google Scholar

Suzuki, T., Miyake, N., Tsurusaki, Y., Okamoto, N., Alkindy, A., Inaba, A., et al. (2016). Molecular Genetic Analysis of 30 Families with Joubert Syndrome. Clin. Genet. 90 (6), 526–535. doi:10.1111/cge.12836

PubMed Abstract | CrossRef Full Text | Google Scholar

Szymanska, K., Berry, I., Logan, C. V., Cousins, S. R., Lindsay, H., Jafri, H., et al. (2012). Founder Mutations and Genotype-Phenotype Correlations in Meckel-Gruber Syndrome and Associated Ciliopathies. Cilia 1 (1), 18. doi:10.1186/2046-2530-1-18

PubMed Abstract | CrossRef Full Text | Google Scholar

Vilboux, T., Doherty, D. A., Glass, I. A., Parisi, M. A., Phelps, I. G., Cullinane, A. R., et al. (2017). Molecular Genetic Findings and Clinical Correlations in 100 Patients with Joubert Syndrome and Related Disorders Prospectively Evaluated at a Single center. Genet. Med. 19 (8), 875–882. doi:10.1038/gim.2016.204

PubMed Abstract | CrossRef Full Text | Google Scholar

Wu, Q., Yang, S., Wang, C., Shi, H., Ren, S., Jiao, Z., et al. (2020). Ultrasonographic Manifestation and Genetic Analysis of a Fetus with Nephronophthisis Type 2. Zhonghua Yi Xue Yi Chuan Xue Za Zhi 37 (5), 559–562. doi:10.3760/cma.j.issn.1003-9406.2020.05.016

PubMed Abstract | CrossRef Full Text | Google Scholar

Zhang, W., Taylor, S. P., Ennis, H. A., Forlenza, K. N., Duran, I., Li, B., et al. (2018). Expanding the Genetic Architecture and Phenotypic Spectrum in the Skeletal Ciliopathies. Hum. Mutat. 39 (1), 152–166. doi:10.1002/humu.23362

PubMed Abstract | CrossRef Full Text | Google Scholar

Zhu, H., Chen, W., Ren, H., Zhang, Y., Niu, Y., Wu, D., et al. (2021). Non-classic Splicing Mutation in the CPLANE1 (C5orf42) Gene Cause Joubert Syndrome in a Fetus with Severe Craniocerebral Dysplasia. Eur. J. Med. Genet. 64 (6), 104212. doi:10.1016/j.ejmg.2021.104212

CrossRef Full Text | Google Scholar

Keywords: ciliopathies, prenatal clinical phenotype, occipital encephalocele, polydactyly, polycystic kidneys, whole-exome sequencing

Citation: Liu Y, Wang H, Jin X, Shao Q and Pan Q (2021) Molecular Diagnosis and Prenatal Phenotype Analysis of Eight Fetuses With Ciliopathies. Front. Genet. 12:705808. doi: 10.3389/fgene.2021.705808

Received: 06 May 2021; Accepted: 30 August 2021;
Published: 05 October 2021.

Edited by:

Kathleen M. Gorman, Temple Street Children’s University Hospital, Ireland

Reviewed by:

Maria Paola Lombardi, University of Amsterdam, Netherlands
Qifei Li, Boston Children’s Hospital and Harvard Medical School, United States

Copyright © 2021 Liu, Wang, Jin, Shao and Pan. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.

*Correspondence: Qixiang Shao, shao_qx@ujs.edu.cn; Qiong Pan, jonespan@163.com

These authors have contributed equally to this work

Disclaimer: All claims expressed in this article are solely those of the authors and do not necessarily represent those of their affiliated organizations, or those of the publisher, the editors and the reviewers. Any product that may be evaluated in this article or claim that may be made by its manufacturer is not guaranteed or endorsed by the publisher.