Genetic predisposition to neural crest-derived tumors: revisiting the role of KIF1B

in Endocrine Connections
Authors:
Catherine Cardot Bauters CHU Lille, Service d’Endocrinologie, Diabétologie, Métabolisme-Nutrition, Hôpital Claude Huriez, Lille, France

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Emmanuelle Leteurtre Univ. Lille, Inserm, CHU Lille, UMR-S 1277-CANTHER, Cancer Heterogeneity, Plasticity & Resistance to Therapies, Lille, France

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Bruno Carnaille CHU Lille, Service de Chirurgie Endocrine, Hôpital Claude Huriez, Lille, France

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Christine Do Cao CHU Lille, Service d’Endocrinologie, Diabétologie, Métabolisme-Nutrition, Hôpital Claude Huriez, Lille, France

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Stéphanie Espiard CHU Lille, Service d’Endocrinologie, Diabétologie, Métabolisme-Nutrition, Hôpital Claude Huriez, Lille, France

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Malo Penven CHU Lille, Service de Biochimie Hormonologie, Métabolisme, Nutrition-Oncologie, Centre de Biologie Pathologie Génétique, Lille, France

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Evelyne Destailleur CHU Lille, Service de Biochimie Hormonologie, Métabolisme, Nutrition-Oncologie, Centre de Biologie Pathologie Génétique, Lille, France

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Isabelle Szuster CHU Lille, Service de Biochimie Hormonologie, Métabolisme, Nutrition-Oncologie, Centre de Biologie Pathologie Génétique, Lille, France

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Tonio Lovecchio CHU Lille, Service de Biochimie Hormonologie, Métabolisme, Nutrition-Oncologie, Centre de Biologie Pathologie Génétique, Lille, France

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Julie Leclerc Univ. Lille, Inserm, CHU Lille, UMR-S 1277-CANTHER, Cancer Heterogeneity, Plasticity & Resistance to Therapies, Lille, France
CHU Lille, Service de Biochimie Hormonologie, Métabolisme, Nutrition-Oncologie, Centre de Biologie Pathologie Génétique, Lille, France

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Fredéric Frénois Univ. Lille, CHU Lille, EA-7364 RADEME, Faculté de Médecine, Lille, France

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Emmanuel Esquivel Dept Medicine, Mays Cancer Center, University of Texas Health Science Center at San Antonio, San Antonio, Texas, USA

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Patricia L M Dahia Dept Medicine, Mays Cancer Center, University of Texas Health Science Center at San Antonio, San Antonio, Texas, USA

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Emilie Ait-Yahya CHU Lille, Institut de Biochimie & Biologie Moléculaire, Centre de Biologie Pathologie Génétique, Lille, France

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Michel Crépin CHU Lille, Service de Biochimie Hormonologie, Métabolisme, Nutrition-Oncologie, Centre de Biologie Pathologie Génétique, Lille, France

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Pascal Pigny CHU Lille, Service de Biochimie Hormonologie, Métabolisme, Nutrition-Oncologie, Centre de Biologie Pathologie Génétique, Lille, France

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Correspondence should be addressed to P Pigny: pascal.pigny@chru-lille.fr
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Objective

We previously described a family in which predisposition to pheochromocytoma (PCC) segregates with a germline heterozygous KIF1B nucleotide variant (c.4442G>A, p.Ser1481Asn) in three generations. During the clinical follow-up, one proband’s brother, negative for the KIF1B nucleotide variant, developed a bilateral PCC at 31 years. This prompted us to reconsider the genetic analysis.

Design and methods

Germline DNA was analyzed by next-generation sequencing (NGS) using a multi-gene panel plus MLPA or by whole exome sequencing (WES). Tumor-derived DNA was analyzed by SnapShot, Sanger sequencing or NGS to identify loss-of-heterozygosity (LOH) or additional somatic mutations.

Results

A germline heterozygous variant of unknown significance in MAX (c.145T>C, p.Ser49Pro) was identified in the proband’s brother. Loss of the wild-type MAX allele occurred in his PCCs thus demonstrating that this variant was responsible for the bilateral PCC in this patient. The proband and her affected grandfather also carried the MAX variant but no second hit could be found at the somatic level. No other pathogenic mutations were detected in 36 genes predisposing to familial PCC/PGL or familial cancers by WES of the proband germline. Germline variants detected in other genes, TFAP2E and TMEM214, may contribute to the multiple tumors of the proband.

Conclusion

In this family, the heritability of PCC is linked to the MAX germline variant and not to the KIF1B germline variant which, however, may have contributed to the occurrence of neuroblastoma (NB) in the proband.

Abstract

Objective

We previously described a family in which predisposition to pheochromocytoma (PCC) segregates with a germline heterozygous KIF1B nucleotide variant (c.4442G>A, p.Ser1481Asn) in three generations. During the clinical follow-up, one proband’s brother, negative for the KIF1B nucleotide variant, developed a bilateral PCC at 31 years. This prompted us to reconsider the genetic analysis.

Design and methods

Germline DNA was analyzed by next-generation sequencing (NGS) using a multi-gene panel plus MLPA or by whole exome sequencing (WES). Tumor-derived DNA was analyzed by SnapShot, Sanger sequencing or NGS to identify loss-of-heterozygosity (LOH) or additional somatic mutations.

Results

A germline heterozygous variant of unknown significance in MAX (c.145T>C, p.Ser49Pro) was identified in the proband’s brother. Loss of the wild-type MAX allele occurred in his PCCs thus demonstrating that this variant was responsible for the bilateral PCC in this patient. The proband and her affected grandfather also carried the MAX variant but no second hit could be found at the somatic level. No other pathogenic mutations were detected in 36 genes predisposing to familial PCC/PGL or familial cancers by WES of the proband germline. Germline variants detected in other genes, TFAP2E and TMEM214, may contribute to the multiple tumors of the proband.

Conclusion

In this family, the heritability of PCC is linked to the MAX germline variant and not to the KIF1B germline variant which, however, may have contributed to the occurrence of neuroblastoma (NB) in the proband.

Introduction

We previously described a family in which predisposition to pheochromocytoma (PCC), segregates into three generations with a germline heterozygous nucleotide variant of KIF1B (c.4442G>A, p.Ser1481Asn) which encodes the kinesin-like protein KIF1B (1). KIF1B isoform β (KIF1Bβ) is a molecular motor protein that participates in the transport of synaptic vesicle precursors and is essential for neuronal survival and differentiation (2). In vitro, the p.Ser1481Asn variant decreases the ability of KIF1Bβ to promote the apoptosis of primary rat sympathetic neurons (3) and thus may facilitate tumorigenesis later on. Conversely enforced expression of KIF1B resulted in an induction of apoptosis of neuroblastoma (NB) cells (4). Thus, the KIF1Bβ neuronal pro-apoptotic effect combined with the mapping of KIF1B on chromosome 1p36, a region frequently deleted in PCC and NB (5), suggested that KIF1B might function as a tumor suppressor gene (TSG) in these diseases (3). However, in our kindred, we did not identify a loss of the wild type (WT) allele of KIF1B at the somatic level in the PCC or NB of the proband, deviating from the Knudson two hits theory (1). At that time, we thus hypothesized that the p.S1481N variant of KIF1Bβ functions in haploinsufficiency in these tumors (1) but its exact mechanisms of action remain unclear (6).

Since our initial report, the large size KIF1B gene has been rarely incorporated in the PCC/PGL gene panels which are analyzed in patients with PCC or PGL by next-generation sequencing to identify familial tumors. Welander et al. (7) described one PCC patient with a germline variant of KIF1B classified as disease-causing in their cohort thus representing a prevalence of 1.1%. The PCC had a sporadic presentation in this woman who later presented with endometrial carcinoma. Curras-Freixes et al. (8) reported three germline variants of unknown significance (VUS) of KIF1B in their cohort of PCC patients, representing a prevalence of 0.66% (3/453) in line with our own estimation of the prevalence of KIF1B VUS at 1.3% (1/74 patients with PCC/PGL analyzed by NGS between 2017 and 2019, unpublished data).

In conclusion, only 1–2% of the patients with PCC or PGL had a germline pathogenic variant of KIF1B thus leading to frequent questioning on its involvement in the heritability of PCC/PGL (9, 10).

At the time of our report in 2008, the proband’s two brothers, who did not carry the KIF1B germline variant, were clinically asymptomatic (1). However, during the clinical follow-up, one of proband’s brother developed a bilateral PCC at 31 years. This prompts us to extend the genetic analysis in this family and to reconsider the molecular pathogenesis of the PCC.

Materials and methods

Clinical data

The pedigree of the family has been updated in Fig. 1. In brief, the proband III-1 developed NB of the broad ligament at 17 months which was treated by surgery, radiation therapy and chemotherapy. At age 22 years, she developed a right PCC plus a ganglioneuroma at the site of the original NB and also an ileal schwannoma. At that time, she had hypertension and high normetanephrines levels (exact data not available). Six years later, the patient underwent adrenal surgery for a left PCC associated with a mature ganglioneuroma. At the same time, a well-differentiated leiomyosarcoma arising from the mesosigmoid was detected and surgically removed. At 39 years, several cutaneous metastases of the leiomyosarcoma were surgically removed. At 42 years, a 9-cm moderately differentiated hepatic carcinoma was diagnosed and surgically removed. Finally, at 43 years a uterine leiomyoma, and two metastases (parietal and peritoneal) from the leiomyosarcoma were removed. Her paternal grandfather (I-1) had bilateral PCC at 70 years and her father (II-2) had a lung adenocarcinoma at 47 years and prostatic cancer at 54 years. The proband’s youngest brother (III-3) presented at 31 years with a cardiomyopathy complicated by a Takotsubo’s syndrome which led to the diagnosis of bilateral PCC. The proband’s paternal uncle (II-3) was diagnosed at 56 years with an oligo-symptomatic adrenal nodule exhibiting a high [18F]-DOPA uptake at PET.

Figure 1
Figure 1

Phenotype and genotype of the family. The proband is patient III.1.

Citation: Endocrine Connections 9, 10; 10.1530/EC-20-0460

Custom endocrine tumors NGS panel

In compliance with the French regulation, each patient gave his/her written informed consent before performing genetic testing which is an integral part of the patient’s care. Moreover, this protocol was reviewed and validated by the Ethical Committee (Comité de Protection des Personnes Nord Ouest IV) under the number HP 20/04. A custom panel based on the hybridization and capture technology (Haloplex, Agilent Technologies) was designed to be compatible with the Illumina MiSeq platform. Probes covered the coding regions and intronic flanking sites of 21 susceptibility genes for endocrine tumors, either PCC/PGL (VHL, RET, SDHA, SDHAF2, SDHB, SDHC, SDHD, TMEM127, KIF1B, MAX, PHD2) or pituitary tumors/hyperparathyroidism (MEN1, HRPT2, AIP, CASR, CYP24A1, GCM2, PTH, GNA11, AP2S1, CDKN1B). Genomic DNA extracted from blood cells was fragmented with restriction enzymes; then digested DNA was hybridized to Haloplex probes which resulted in circularization of DNA fragments and sample indexing. Target DNA was captured with streptavidin-coated magnetic beads, ligated and eluted before bridge PCR amplification of the libraries. After quantification of enriched target DNA, samples were pooled for multiplexed sequencing. NGS sequencing data were aligned to hg19 human reference and annotated using two independent bioinformatic pipelines (alignment using bwa v0.7.15-r1140 followed by best practices for germline variant detection using GATK v3.7 (11) and SeqNext V4.4 (JSI) (12)). Data were filtered using an in-house database (DVD) to remove recurrent sequencing errors. Regions with coverage <30X were reanalyzed using Sanger sequencing.

Somatic cancer panel analysis

DNA extracted from three separate regions of the frozen left PCC from proband (III-1) was analyzed for somatic nucleotide variants in hot spot regions of 48 commonly mutated cancer genes using the Illumina TruSeq Amplicon Cancer Panel (ABL1, AKT1, ALK, APC, ATM, BRAF, CDH1, CDKN2A, CSF1R, CTNNB1, EGFR, ERBB2, ERBB4, FBXW7, FGFR1, FGFR2, FGFR3, FLT3, GNA11, GNAQ, GNAS, HNF1A, HRAS, IDH1, JAK2, JAK3, KDR, KIT, KRAS, MET, MLH1, MPL, NOTCH1, NPM1, NRAS, PDGFRA, PIK3CA, PTEN, PTPN11, RB1, RET, SMAD4, SMARCB1, SMO, SRC, STK11, TP53, VHL), run on Illumina MiSeq following standard protocols, and analyzed using the filter settings described previously.

WES (whole exome sequencing) analysis

Genomic DNA extracted from fresh blood cells from the proband and her father with QiAmp DNA mini kit (Qiagen) was captured using Agilent in-solution enrichment methodology with their biotinylated oligonucleotides probes library (SureSelect Clinical Research Exome V2, Agilent Technologies), followed by paired-end 75 bases massively parallel sequencing on Illumina HiSeq4000 (IntegraGen SA, Evry, France), as reported (13). Sequence capture, enrichment and elution were performed according to manufacturer’s instruction and protocols (SureSelect, Agilent) without modification, except for library preparation performed with NEBNext® Ultra kit (New England Biolabs). For library preparation, 600 ng of each genomic DNA were fragmented by sonication and purified to yield fragments of 150–200 bp. Paired-end adaptor oligonucleotides were ligated on repaired fragments then purified and enriched by 8 PCR cycles. A total of 1200ng of the purified Libraries were then hybridized to the SureSelect oligo probe capture library for 72 h. After hybridization and washing, the eluted fraction was PCR-amplified, purified and quantified by qPCR. Each eluted-enriched DNA library was then sequenced on an Illumina HiSeq4000 as paired-end 75 bp reads. Image analysis and base calling were performed using Illumina Real Time Analysis (2.7.7) with default parameters.

Bioinformatic analysis

After demultiplexing and FASTQ generation, the paired-end reads were trimmed using TrimGalore v0.4.4. The paired-end reads were then aligned to hg19 human reference genome with BWA v0.7.15-r1140 (11). We applied the GATK v3.7 pipeline (12) for indel realignment, duplicate removal, and performed SNP and INDEL discovery as well as share genotype across both the proband and her father’s samples simultaneously according to GATK Best Practices recommendations (14, 15). Variants were annotated and filtered with Agilent Technologies Bench Lab NGS v5.0.2. To select putative pathogenic variants, filters were applied as follows (Supplementary Fig. 1, see section on supplementary materials given at the end of this article): (i) variants common to proband and her father were filtered out; (ii) low quality reads were filtered out; (iii) only heterozygous variants were retained; (iv) variants predicted as pathogenic (Supplementary Fig. 1) were retained; (v) variants in exonic regions or near splicing sites were retained; (vi) variants with a frequency ≥0.01 in the general population (using Exac database, release 0.3, 1000 Genomes Phase1 release v3.20101123, ESP6500SI-V2, 1000 Genomes Phase 3 release v5.20130502) were filtered out. Relevant nucleotide variants were validated by Sanger sequencing on Applied Biosystems 3730 platform.

Search for large rearrangements

The analysis of large rearrangements was performed with the Multiplex Ligation-dependent Probe Amplification (MLPA) technology for FH and SDHx genes and by multiplex PCR (QMPSF) for VHL. MLPA probes (ref. SALSA MLPA Probemix P198, P226 and P429) and reagents were manufactured and supplied by MRC-Holland (Amsterdam, The Netherlands). The MLPA procedure was conducted according to manufacturer’s specifications. The amplified probes were analyzed on a 3130XL DNA Analyzer (Life Tech, ThermoFisher). Regarding FH analysis, the proband DNA sample was tested twice in the same run along with 10 negative samples and one positive control with total deletion of the FH gene. Data were interpreted with Coffalyser software (MRC Holland).

LOH analysis

DNA from formalin-fixed paraffin-embedded (FFPE) tumor samples was extracted using the QIAAmp DNA FFPE kit (Qiagen). Tissue samples of the proband available for LOH analysis are detailed in Supplementary Table 1. LOH of selected nucleotide variant was searched by SNaPshot analysis as previously described (16). PCR and extension primers details are available upon request. Extension products were analyzed on Applied Biosystems 3730 along with GeneScan 120LIZ molecular marker using the Genemapper software. In addition, visualization of the variant peaks on Sanger sequence traces was done using the Mutation Quantifier tool (Surveyor program, Softgenetics).

Immunohistochemical analysis

Fumarate Hydratase expression was assessed on paraffin-embedded tumors using an anti-FH antibody 1:1000 dilution as previously described (17).

In silico analysis

Prediction of the missense variant of MAX protein was carried out with the Phyre2 server (Protein Homology/analogY Recognition Engine V2.0). We compared the deduced human amino‐acid 3D structure with the 3D resolved structure of the Homo sapiens MAX protein (99% sequence identity) using The PyMOL Molecular Graphics System (v2.0, Schrödinger, LLC). The SuperPose server v.1.0 (18) was used to estimate the structural homology, measuring the average distance between the backbones of superimposed proteins.

Results

During the clinical follow-up of the family, patient III-3, who did not harbor the KIF1B c.4442G>A nucleotide variant in his germline DNA, developed bilateral PCC at 31 years. His germline DNA was analyzed by NGS using a custom endocrine tumor panel which includes 11 major susceptibility genes for familial PCC/PGL (PHD2, KIF1Bβ, SDHA, SDHB, SDHC, SDHD, SDHAF2, VHL, MAX, TMEM127 and RET). The only heterozygous variant identified was in MAX (NM_002382.5): c.145T>C, p.Ser49Pro. A large rearrangement of SDHA, SDHB, SDHC, SDHD, SDHAF2, FH and VHL was excluded by MLPA or QMPSF analysis, respectively. Using the ACMG guidelines and Varsome tool (19), the MAX nucleotide variant was classified as a VUS. The secretory profile of his tumors consisted of increased urinary normetanephrines at 1979 nmol/mmol of creatinine (8x the upper limit range) with normal total metanephrines at 182 nmol/mmol of creatinine (<190), reminiscent of the pattern observed in patients with a MAX pathogenic variant (20). The p.Ser49Pro MAX variant is predicted to show the Proline 49 with an opened cycle which is impossible, leading probably to the precipitation of the protein (Fig. 2). Proline is a constrained amino acid due to its pyroxylin cycle hindering the rotation of the ϕ angle with the previous amino acid and thus altering the amino acid connection. Therefore, this variant is likely deleterious.

Figure 2
Figure 2

(A) 3D structure of the human native MAX protein (pdb code: 1AN2) (amino acids 22–104); (B) 3D structural prediction of the human Ser49Pro mutated MAX protein (amino acids 22–104).

Citation: Endocrine Connections 9, 10; 10.1530/EC-20-0460

We thus reanalyzed the germline DNAs of the proband (III-1), her father (II-1) and grandfather (I-1), who had been previously found to be carriers of the KIF1B c.4442G>A nucleotide variant (1), using the NGS panel. All also carried the MAX c.145T>C variant at the heterozygous level. No other pathogenic variant in the nine other susceptibility genes for PCC/PGL was identified (Fig. 1). We also excluded a large rearrangement of SDHA, SDHB, SDHC, SDHD, SDHAF2, FH and VHL in the proband by MLPA or QMPSF analysis, respectively. The MAX c.145T>C variant was also detected by Sanger sequencing at the heterozygous level in the germline DNA of the proband’s paternal uncle (II-3), who was KIF1B negative (Fig. 1). Interestingly, II-3 recently developed, at age 56, a 11-mm hypervascular nodule in his right adrenal which remains clinically silent but strongly uptakes [18F]-DOPA during PET, suggestive of PCC or adrenomedullary nodule. Plasma free normetanephrines were at the upper limit of the normal values. Pre-operatively, patient I-1 had high urinary normetanephrines (5x the upper limit range) and chromogranin-A levels (x3 the upper limit range). By contrast, patient II-2, who had a regular follow-up by PET imaging due to his lung and prostatic cancers, never demonstrated an adrenal uptake of [18F]-deoxy-glucose. Moreover, his levels of metanepherines/normetanephrines were in the normal range at each follow-up, both elements being in disfavor of a PCC.

Since MAX behaves as a TSG (20), we analyzed the tumor DNAs of patient III-3 and identified loss of the MAX WT allele in both tumors (Fig. 3) suggesting that this variant is indeed responsible for the bilateral PCC in this patient. In contrast, no LOH of the WT allele of MAX was found in the 2 PCCs of the proband (III-1), using DNA obtained from three independent samples, FFPE samples from left and right PCCs (Fig. 3), and one fresh frozen sample from the left PCC (Supplementary Fig. 2). The oldest of the samples (the right PCC) in fact showed complete absence of the variant allele (Fig. 3), which could be due to allelic dropout in the PCR, a well-recognized cause of errors in DNA from suboptimal samples (21). Although the estimated proportion of tumor cells of the left PCC FFPE sample was high (Fig. 3), this estimate was not available from the bulk frozen specimen from this tumor nor the right PCC, so it is unclear to what extent normal cell admixture may have contributed to the allelic count. We also excluded, by Sanger sequencing, the presence of an additional somatic MAX mutation, which might have functioned as the second hit in the absence of LOH in the DNA extracted from the left PCC of the proband. We further examined the DNA from the three separate fragments from the left PCC to search for additional somatic mutations in 48 cancer genes using NGS. The three fragments displayed similar variant allele frequencies across these genes, suggesting that the left PCC was homogeneous with respect to both genetic and cell composition. Moreover, these fragments lacked areas of allelic imbalance, in favor of a high level of normal cells in these fragments. Only a few VUS were detected (Supplementary Table 2); however, no variant frequency suggestive of LOH was observed in these three samples. Finally, FH expression evaluated by immunohistochemistry was conserved on the uterine leiomyoma and pelvic leiomyosarcoma of the proband (Supplementary Fig. 3), which strongly suggests the absence of somatic pathogenic variants of FH responsible for these 2 tumors in the proband.

Figure 3
Figure 3

Search for a LOH of MAX and KLHL7 in the DNA extracted from the pheochromocytomas of patients III.1 and III.3 by SnapShot analysis.

Citation: Endocrine Connections 9, 10; 10.1530/EC-20-0460

Since the proband (III-1) and her father (II-2) shared the same genotype for MAX and KIF1B despite very different phenotypes (Fig. 1), we considered that the proband may carry additional variants in known/new susceptibility genes that modified cancer predisposition, which might have been inherited from her mother or have occurred de novo. WES was performed on the germline DNA of III-1 and II-2. First, the proband had no pathogenic variant in NF1, IDH1, IDH2, FH, MDH2 or SLC25A11 which predispose to familial PCC/PGL nor in a group of 30 cancer-predisposing genes (22), that is, APC, ATM, BAP1, BARD1, BMPR1A, BRCA1, BRCA2, BRIP1, CDH1, CDKN2A, CDK4, CHEK2, EPCAM, GREM1, MITF, MLH1, MSH2, MSH6, MUTYH, NBN, PALB2, PMS2, POLD1, POLE, PTEN, RAD51C, RAD51B, SMAD4, STK11 and TP53. Thus, we decided to focus on the nucleotide variants which were present in the germline of III-1 but absent in II-2 in agreement with our working hypothesis. One hundred twenty-five nucleotide variants were identified as unique to III-1 (Supplementary Fig. 1). Class 1 and 2 variants (benign or probaby benign) were filtered out using Varsome, leading to a list of 24 variants all classified as VUS (Class 3) (Table 1). After the interrogation of several resources such as PUBMED (for a link between the gene of interest and cancer), UniProt (for information on encoded protein function), HGMD (for information on germline mutations currently identified), TCGA (for somatic mutations catalogue), Protein Atlas and CTEX databases (for detailed information on tissue expression), the list was narrowed down to five variants occurring in five genes (Table 1). KLH7 and PKM were good candidate genes for hereditary PCC since they encode proteins expressed in adrenals (23) and are mutated (though rarely) at the somatic level in PCC (TCGA PCPG). RIPK3, TFAP2E and TMEM214 were good candidates for the non-neural crest tumors since they are mutated in sarcomas (TCGA SARC), myomatous neoplasms and in hepatocarcinomas (TCGA LIHC) at the somatic level. No protein expression data were available for TMEM214, TFAP2E and RIPK3 in the Protein Atlas (23). Sanger sequencing confirmed the presence of the five nucleotide variants in the germline of the proband and her mother but absence in her father as expected (Table 2), none were de novo. Patient III-3 was heterozygous only for the KLHL7 variant.

Table 1

List of the 24 nucleotide variants identified by WES in patient III.1 germline DNA and classified as VUS.

Chromosome dbSNP Zygosity Gene Protein HGVS cDNA level nomenclature Read depth (infoDP) Allele 1 reads Allele 2 reads VARSOME analysis Classification GnomAD exomes non-cancer allele frequency GnomAD exomes non-cancer allele frequency PopMax lien varsome
1 rs145119239 Heterozygous wt/var TFAP2E p.R363C NM_178548.3:c.1087C>T  94  41 53 PP3 VUS 3.01883e−03 4.94826e−03 varso.me/L4rN
1 rs41264582 Heterozygous wt/var EDEM3 p.P192L NM_001319960.1:c.575C>T  38  19 19 PP3 VUS 9.47575e−03 1.46391e−02 varso.me/L4rg
1 rs776729303 Heterozygous wt/var TMCC2 p.A344V NM_014858.3:c.1031C>T 149  92 57 PM2 + PP3 VUS 8.44509e−06 1.94791e−05 varso.me/L4tC
2 rs199779856 Heterozygous wt/var TMEM214 p.G263S NM_017727.4:c.787G>A 123  78 45 PP3 VUS 9.53110e−04 2.01455e−03 varso.me/L4t6
2 rs148295709 Heterozygous wt/var ABHD1 p.Y372C NM_032604.3:c.1115A>G 165  98 67 PP3 VUS 1.89069e−03 3.54258e−03 varso.me/L4th
3 rs759213356 Heterozygous wt/var BSN p.M3497T NM_003458.3:c.10490T>C 144  71 73 BP4 VUS 2.54304e−05 5.87982e−05 varso.me/L4um
4 rs150771247 Heterozygous wt/var WFS1 p.R228H NM_006005.3:c.683G>A  93  40 53 PP2 + PP3 VUS 7.30517e−04 1.51794e−03 varso.me/ILKo
5 rs200904107 Heterozygous wt/var TMCO6 p.Y153* NM_001300980.1:c.459C>A  75  34 41 PP3 VUS 2.57003e−05 7.08015e−05 varso.me/L4uu
7 Heterozygous wt/var KLHL7 p.G440D NM_018846.4:c.1319G>A  67  35 32 PM2 + PP2 + PP3 VUS NA NA varso.me/Knaj
7 rs75395437 Heterozygous wt/var PSPH p.G90S NM_004577.3:c.268G>A 110  93 17 PP3 + BP1 VUS 1.98379e−04 1.20700e−03 varso.me/DDqg
7 rs144546424 Heterozygous wt/var CPA1 p.G166D NM_001868.3:c.497G>A 179  80 99 PP3 VUS 1.64439e−03 3.09990e−03 varso.me/KgMU
10 rs750208278 Heterozygous wt/var SEC24C p.R1033Q NM_004922.3:c.3098G>A  34  20 14 PM2 + PP3 VUS 1.68808e−05 3.89287e−05 varso.me/L5Ea
11 rs143772626 Heterozygous wt/var RSF1 p.V1120I NM_016578.3:c.3358G>A  50  32 18 PP3 VUS 3.40055e−05 4.89438e−05 varso.me/L5Eg
12 rs61741949 Heterozygous wt/var FOXN4 p.R316H NM_213596.2:c.947G>A  44  19 25 PP3 + BS1 VUS 7.42860e−03 1.02144e−02 varso.me/L5Ej
14 rs146886719 Heterozygous wt/var RIPK3 p.R422* NM_006871.3:c.1264C>T 205 117 88 PP3 VUS 1.57979e−03 3.59334e−03 varso.me/L4lf
14 rs752702606 Heterozygous wt/var FOXA1 p.A232T NM_004496.3:c.694G>A 100  48 52 PP3 VUS 4.70142e−05 1.08505e−04 varso.me/L5Eq
14 rs201974904 Heterozygous wt/var TMEM251 p.Met114Thr NM_001098621.3:c.341T>C  89  49 40 PM2 + PP3 VUS NA NA varso.me/L5FI
15 rs367984298 Heterozygous wt/var TRPM1 p.P798S NM_001252020.1:c.2392C>T  38  20 18 PM2 + PP3 VUS NA NA varso.me/L4lv
15 rs201044858 Heterozygous wt/var C2CD4B p.P27R NM_001007595.2:c.80C>G  70  40 30 PP3 + BS1 VUS 5.00137e−03 4.33071e−03 varso.me/L5F2
15 rs180716407 Heterozygous wt/var PKM p.S5* NM_001316318.1:c.14C>G  92  55 37 PVS1 + BP4 VUS 7.04204e−03 1.22892e−02 varso.me/L5F5
16 rs151150316 Heterozygous wt/var ABCC12 p.Q831* NM_033226.2:c.2491C>T  44  22 22 PP3 VUS 2.41188e−03 4.65328e−03 varso.me/KvbT
19 rs772237909 Heterozygous wt/var PNKP p.N461S NM_007254.3:c.1382A>G  67  36 31 PM2 + PP3 + BP1 VUS 0.00000e+00 NA varso.me/L5Fp
22 rs201399007 Heterozygous wt/var SBF1 p.R1308W NM_002972.3:c.3922C>T  92  45 47 PP3 VUS 6.46441e−04 1.91916e−03 varso.me/FsDo
X rs140505250 Heterozygous wt/var ARR3 p.P351R NM_004312.2:c.1052C>G 102  50 52 PP3 VUS 1.59134e−03 2.69648e−03 varso.me/L5Fw
Table 2

Distribution of the five VUS in the germline DNA of the different family members.

Gene TMEM214 KLHL7 PKM RIPK3 TFAP2E
Nucleotide variant c.787G>A c.1319G>A c.14C>G c.1264C>T c.1087C>T
Protein change p.G263S p.G440D p.S5* p.R422* p.R363C
Patients
 III.1 + + + + +
 III.2 + Wild type + + Wild type
 III.3 Wild type + Wild type Wild type Wild type
 II.1 + + + + +
 II.2 Wild type Wild type Wild type Wild type Wild type
 II.3 Wild type Wild type Wild type Wild type Wild type
 I.1 Wild type Wild type Wild type Wild type Wild type

Tumor DNA from eight different FFPE tumors from the proband (Supplementary Table 1) were analyzed by SnapShot to screen for LOH of the candidate genes. No LOH of KLH7 WT allele was found in the PCC of the proband nor in those of her brother III.3 (Fig. 3). Unfortunately, the data were not informative for PKM (not shown). Regarding TFAP2E, LOH of the WT allele was found in the DNA from the uterine leiomyoma whereas no LOH occurred in the parietal and peritoneal metastasis of the leiomyosarcoma (Fig. 4). By contrast, a LOH of the WT allele of TMEM214 was found in the parietal and peritoneal metastasis of the leiomyosarcoma (Fig. 4) whereas the data were not informative in the hepatocarcinoma (not shown).

Figure 4
Figure 4

Search for a LOH of TFAP2E and TMEM214 in the DNA extracted from the different tumors from patient III.1 by SnapShot analysis.

Citation: Endocrine Connections 9, 10; 10.1530/EC-20-0460

Discussion

The occurrence of a bilateral PCC at a young age in a relative (patient III.3) who did not carry the germline KIF1B c.4442G>A variant suggested that other susceptibility gene(s) might be implicated in the PCC/PGL predisposition of this family. Indeed, analysis of a panel of 11 classic susceptibility genes for PCC/PGL (17,18) by NGS led to the identification of a heterozygous variant of MAX: c.145T>C, p.Ser49Pro. This variant was also found in the germline of the two other individuals with PCC in this family, III-1 and I-1. This variant has not been previously found in the germline of patients with PCC/PGL or at the somatic level based on the LOVD Leiden and TCGA database, respectively. Using the pathogenicity criteria proposed by the ACMG, this variant was classified as a VUS rendering the interpretation more complex. However, several elements are in favor of its pathogenic role. First, the secretory pattern of the tumors of patient III-3 and I-1 is compatible with those classically observed in patients with MAX pathogenic variants (20). Secondly, the loss of the WT allele of MAX in both PCCs of III-3 suggests the role of MAX gene and causality of the p.Ser49Pro variant in the pathogenesis of the PCCs. Thirdly, the introduction of a proline at position 49 seems incompatible with a native 3D conformation for the MAX protein. In addition, although histology of the adrenal nodule identified in patient II-3 is presently not available, its imaging pattern is compatible with a PCC. If confirmed in the follow-up, this diagnosis provides support to the pathogenic role of the MAX variant since II-3 is WT for KIF1B.

The interpretation of the pathogenesis of the PCCs occurring in the proband and her grandfather is more intricate. They both have the MAX p.Ser49Pro plus the KIF1B p.Ser1481Asn germline variants. We were unable to identify LOH of KIF1B (1) or MAX WT alleles in the proband’s PCC despite the analyses of multiple separate fragments from the most recently removed PCC which was not fixed in Bouin’s reagent known to be deleterious for DNA (21). However, as discussed previously, our additional data on this tumor does not allow us to rule out the contribution of high levels of nontumoral tissue to the lack of detectable LOH. Although we cannot exclude that both KIF1B and MAX may contribute to the PCC phenotype or to the clinical variability in this family, KIF1B pathogenic variants have rarely been described in patients with PCC/PGL since our initial report in 2008 (1, 7, 8). Only one, a p.Tyr835Cys variant, was reported by Welander et al. in a 54-year-1old woman with a unilateral PCC and an endometrial carcinoma (7). This patient had no germline variants in any of the 11 other major susceptibility genes for PCC/PGL but no somatic LOH of the wild-type allele was found, so preventing any definitive conclusion on the pathogenic relevance of this novel variant.

Given the phenotypic variability of this family, with multiple non-PCC/PGL cancers in patient III.1, and to evaluate the possibility that other susceptibility events were at play, we performed WES on the germline DNAs from patient III.1 and II.2. Our working model was that patient III.1 had de novo or maternally-inherited mutations in new/known susceptibility genes for hereditary cancers or, alternatively, in ‘modifier genes’ which could have an impact on cancer-promoting pathways (24). These additional nucleotide variants, combined with the KIF1B and MAX germline variants, might explain the very severe phenotype of this patient. WES excluded a pathogenic mutation in other genes predisposing to familial PCC/PGL and also in 30 other hereditary cancer susceptibility genes (22). Among the 125 variants which were private to the proband most were classified as benign or probably benign and were filtered out; the 24 remaining variants were all classified as VUS. Based on bibliographic data, tissue pattern of expression, biological function of the encoded protein, and a catalog of somatic mutations, we narrowed down the list to five variants in five different genes which may be implicated either in the pathogenesis of PCC (KLHL7 and PKM) or sarcomas (RIPK3, TMEM214 and TFAP2E). We did not detect a LOH of the WT allele of KLHL7 or PKM in the proband’s PCC. Thus, we cannot assign any causality in the pathogenesis of the proband’s PCCs to one of these variants.

We propose that in this family the genetic susceptibility to PCC/PGL is linked to the MAX nucleotide variant which is however associated with an incomplete penetrance since patient II-2 did not develop any symptomatic adrenal lesion. The KIF1B isoform β p.Ser1481Asn variant, which is partly defective in the apoptotic culling of neural crest progenitors, may also contribute to the occurrence of NB in the childhood of patient III-1, similar to other rare observations in NB (3). Finally, the leiomyosarcoma and hepatic carcinoma of the proband, and her father’s lung adenocarcinoma may be MAX and KIF1B independent. The involvement of TFAP2E and TMEM214 variants is an attractive hypothesis but the pathways acting in disease development remain to be determined.

Supplementary materials

This is linked to the online version of the paper at https://doi.org/10.1530/EC-20-0460.

Declaration of interest

The authors declare that there is no conflict of interest that could be perceived as prejudicing the impartiality of the research reported.

Funding

This work was supported in part by the Association de Recherche en Endocrinologie et Métabolismes (grant to P P).

Acknowledgements

This work is dedicated to the memory of Pr Charles Proye who was the first to take care of this family and to highlight the hereditary nature of the PCC. We thank Mrs Shahida Flores for her help with data analysis, Dr N Burnichon and B Bressac de Paillerets for their help with FH analysis.

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    Muller M, Guillaud-Bataille M, Salleron J, Genestie C, Deveaux S, Slama A, Bressac de Paillerets B, Richard S, Benusiglio PR & Ferlicot S Pattern multiplicity and FH/2-succino-cysteine staining but not eosinophilic nuclei with perinucleolar halos differentiate hereditary leiomyomatosis and RCC-associated RCC from kidney tumors without FH gene alteration. Modern Pathology 2018 31 9749 83. (https://doi.org/10.1038/s41379-018-0017-7)

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    • Search Google Scholar
    • Export Citation
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    Greer CE, Peterson SL, Kiviat NB & Manos MM PCR amplification from paraffin-embedded tissues. Effects of fixative and fixation time. American Journal of Clinical Pathology 1991 95 117124. (https://doi.org/10.1093/ajcp/95.2.117)

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  • Collapse
  • Expand
  • Figure 1

    Phenotype and genotype of the family. The proband is patient III.1.

  • Figure 2

    (A) 3D structure of the human native MAX protein (pdb code: 1AN2) (amino acids 22–104); (B) 3D structural prediction of the human Ser49Pro mutated MAX protein (amino acids 22–104).

  • Figure 3

    Search for a LOH of MAX and KLHL7 in the DNA extracted from the pheochromocytomas of patients III.1 and III.3 by SnapShot analysis.

  • Figure 4

    Search for a LOH of TFAP2E and TMEM214 in the DNA extracted from the different tumors from patient III.1 by SnapShot analysis.

  • 1

    Yeh IT, Lenci RE, Qin Y, Buddavarapu K, Ligon AH, Leteurtre E, Do Cao C, Cardot-Bauters C, Pigny P & Dahia PLM A germline mutation of the KIF1Bβ gene on 1p36 in a family with neural and nonneural tumors. Human Genetics 2008 124 2792 85. (https://doi.org/10.1007/s00439-008-0553-1)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 2

    Zhao C, Takita J, Tanaka Y, Setou M, Nakagawa T, Takeda S, Yang HW, Terada S, Nakata T & Takei Y et al. Charcot-Marie-Tooth disease type 2A caused by mutation in a microtubule motor KIF1Bβ. Cell 2001 105 5875 97. (https://doi.org/10.1016/s0092-8674(0100363-4)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 3

    Schlisio S, Kenchappa RS, Vredeveld LCW, George RE, Stewart R, Greulich H, Shahriari K, Nguyen NV, Pigny P & Dahia PL et al. The kinesin KIF1Bβ acts downstream from EgIN3 to induce apoptosis and is a potential 1p36 tumor suppressor. Genes and Development 2008 22 884893. (https://doi.org/10.1101/gad.1648608)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 4

    Munirajan AK, Ando K, Mukai A, Takahashi M, Suenaga Y, Ohira M, Koda T, Hirota T, Ozaki T & Nakagawara A KIF1Bb functions as a haploinsufficient tumor suppressor gene mapped to chromosome 1p36.2 by inducing apoptotic death. Journal of Biological Chemistry 2008 283 24426244 34. (https://doi.org/10.1074/jbc.M802316200)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 5

    Aarts M, Dannenberg H, de Leeuw RJ, van Nederveen FH, Verhofstad AA, Lenders JW, Dinjens WNM, Speel EJM, Lam WL & de Krijger RR Microarray-based CGH of sporadic and syndrome-related pheochromocytomas using a 0.1–0.2Mb BAC array spanning chromosome arm 1p. Genes, Chromosomes and Cancer 2006 45 8393. (https://doi.org/10.1002/gcc.20268)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 6

    Chen ZX, Wallis K, Fell SM, Sobrado VR, Hemmer MC, Ramskold D, Hellman U, Sansberg R, Kenchappa RS & Martinson T et al. RNA helicase A is a downstream mediator of KIF1Bb tumor-suppressor function in neuroblastoma. Cancer Discovery 2014 4 4344 51. (https://doi.org/10.1158/2159-8290.CD-13-0362)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 7

    Welander J, Andreasson A, Christofer Juhlin CC, Wiseman RW, Backdahl M, Hoog A, Larsson C, Gimm O & Soderkvisst P Rare germline mutations identified by targeted next-generation sequencing of susceptibility genes in pheochromocytoma and paraganglioma. Journal of Clinical Endocrinology and Metabolism 2014 99 E1352E 1360. (https://doi.org/10.1210/jc.2013-4375)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 8

    Curras-Freixes M, Pineiro-Yanez E, Montero-Conde C, Apellaniz-Ruiz M, Calsina B, Mancikova V, Remacha L, Richter S, Ercolino T & Rogowski-Lehmann N et al. PheoSeq : a targeted next-generation sequencing assay for pheochromocytoma and paraganglioma diagnostics. Journal of Molecular Diagnostics 2017 19 5755 88. (https://doi.org/10.1016/j.jmoldx.2017.04.009)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 9

    Neumann HPH, Young WF & Eng C Pheochromocytoma and paraganglioma. New England Journal of Medicine 2019 381 5525 65. (https://doi.org/10.1056/NEJMra1806651)

  • 10

    Toledo RA, Burnichon N, Cascon A, Benn DE, Bayley JP, Welander J, Tops CM, Firth H, Dwight T & Ercolino T et al. NGSnPPGL study group. Nature Reviews Endocrinology 2017 13 233247. (https://doi.org/10.1038/nrendo.2016.185)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 11

    Li H & Durbin R Fast and accurate long-read alignment with Burrows Wheeler transform. Bioinformatics 2010 26 5895 95. (https://doi.org/10.1093/bioinformatics/btp698)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 12

    McKenna A, Hanna M, Banks E, Sivachenko A, Cibulskis K, Kernytsky A, Garimella K, Alsthuler D, Gabriel S & Daly M et al. The Gonome Analysis ToolKit: a MapReduce Framework for analyzing next-generation DNA sequencing data. Genome Research 2010 20 12971 303. (https://doi.org/10.1101/gr.107524.110)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 13

    Gnirke A, Melnikov A, Maguire J, Rogov P, LeProust EM, Brockman W, Fennell T, Giannoukos G, Fisher S & Russ C et al. Solution hybrid selection with ultra-long oligonucleotides for massively parallel targeted sequencing. Nature Biotechnology 2009 27 18218 9. (https://doi.org/10.1038/nbt.1523)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 14

    DePristo MA, Banks E, Poplin R, Garimella KV, Maguire JR, Hartl C, Philippakis AA, del Angel G, Rivas MA & Hanna M et al. A framework for variation discovery and genotyping using next generation sequencing data. Nature Genetics 2011 43 49149 8. (https://doi.org/10.1038/ng.806)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 15

    Van der Auwera GA, Carneiro MO, Hartl C, Poplin R, Del Angel G, Levy-Moonshine, Jordan A, Shakir T, Roazen KD & Thibault J et al. From FastQ data to high confidence variants calls: the Genome Analysis Tool Kit best practices pipeline. Current Protocols in Bioinformatics 2013 43 1 1.1 0.111.10.33. (https://doi.org/10.1002/0471250953.bi1110s43)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 16

    Kern B, Coppin L, Romanet P, Crépin M, Szuster I, Renaud F, Leteurtre E, Frénois F, Wemeau JL & Carnaille B et al. Multiple HABP2 variants in familial papillary thyroid carcinoma: contribution of a group of ‘thyroid checked’ controls. European Journal of Medical Genetics 2017 60 178184. (https://doi.org/10.1016/j.ejmg.2017.01.001)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 17

    Muller M, Guillaud-Bataille M, Salleron J, Genestie C, Deveaux S, Slama A, Bressac de Paillerets B, Richard S, Benusiglio PR & Ferlicot S Pattern multiplicity and FH/2-succino-cysteine staining but not eosinophilic nuclei with perinucleolar halos differentiate hereditary leiomyomatosis and RCC-associated RCC from kidney tumors without FH gene alteration. Modern Pathology 2018 31 9749 83. (https://doi.org/10.1038/s41379-018-0017-7)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 18

    Maiti R, van Domselaar GH, Zhang H & Wishart DS SuperPose: a simple server for sophisticated structural superposition. Nucleic Acids Research 2004 32 W590W59 4. (https://doi.org/10.1093/nar/gkh477)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 19

    Kopanos C, Tsiolkas V, Kouris A, Chapple CE, Albarca Aguilera M, Meyer R & Massouras A VarSome: the human genomic variant search engine. Bioinformatics 2019 35 197819 80. (https://doi.org/10.1093/bioinformatics/bty897)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 20

    Burnichon N, Cascón A, Schiavi F, Morales NP, Comino-Méndez I, Abermil N, Inglada-Pérez L, de Cubas AA, Amar L & Barontini M et al. MAX mutations cause hereditary and sporadic pheochromocytoma and paraganglioma. Clinical Cancer Research 2012 18 282828 37. (https://doi.org/10.1158/1078-0432.CCR-12-0160)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 21

    Greer CE, Peterson SL, Kiviat NB & Manos MM PCR amplification from paraffin-embedded tissues. Effects of fixative and fixation time. American Journal of Clinical Pathology 1991 95 117124. (https://doi.org/10.1093/ajcp/95.2.117)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 22

    Neben CL, Zimmer AD, Stedden W, van der Akker J, O’Connor R, Chan RC, Chen E, Tan Z, Leon A & Ji J et al. Multi-gene panel testing of 23,179 individuals for hereditary cancer risk identifies pathogenic variant carriers missed by current genetic testing guidelines. Journal of Molecular Diagnostics 2019 21 646657. (https://doi.org/10.1016/j.jmoldx.2019.03.001)

    • PubMed
    • Search Google Scholar
    • Export Citation
  • 23

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