Characterization of the c.793-1G > A splicing variant in CHEK2 gene as pathogenic: a case report

Characterization of the c.793-1G > A splicing variant in CHEK2 gene as pathogenic: a case report

Abstract Background CHEK2 is involved in the DNA damage repair response Fanconi anemia (FA)-BRCA pathway. An increased risk for breast and other cancers has been documented in individuals who carry a single pathogenic CHEK2 variant. As for other genes involved in cancer predisposition, different typ...

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Main Authors: Konstantinos Agiannitopoulos, Eirini Papadopoulou, Georgios N. Tsaousis, Georgia Pepe, Stavroula Kampouri, Mehmet Ali Kocdor, George Nasioulas
Format: Article
Language:English
Published: BMC 2019-07-01
Series:BMC Medical Genetics
Subjects:
CHEK2
Splicing variant
Next generation sequencing
RNA analysis
Online Access:http://link.springer.com/article/10.1186/s12881-019-0862-3
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spelling doaj-9cd9b6a0109248969a8e2a424e37fa8e2021-04-02T15:54:02ZengBMCBMC Medical Genetics1471-23502019-07-012011410.1186/s12881-019-0862-3Characterization of the c.793-1G > A splicing variant in CHEK2 gene as pathogenic: a case reportKonstantinos Agiannitopoulos0Eirini Papadopoulou1Georgios N. Tsaousis2Georgia Pepe3Stavroula Kampouri4Mehmet Ali Kocdor5George Nasioulas6Genekor Medical S.AGenekor Medical S.AGenekor Medical S.AGenekor Medical S.AGenekor Medical S.AEylul Universitesi HastanesiGenekor Medical S.AAbstract Background CHEK2 is involved in the DNA damage repair response Fanconi anemia (FA)-BRCA pathway. An increased risk for breast and other cancers has been documented in individuals who carry a single pathogenic CHEK2 variant. As for other genes involved in cancer predisposition, different types of pathogenic variants have been observed, including single nucleotide variations, short insertions/deletions, large genomic rearrangements and splicing variants. Splicing variants occurring in the splicing acceptor or donor site result in alternative mature mRNA produced and can cause intron retention, exon skipping, or creation of alternative 3′ and 5′ splice site. Thus, the pathogenicity of this type of alterations should always be explored experimentally and their effect in the mRNA and consequently the protein produced, should be defined. The aim of this study was the delineation of the effect of a splicing variant in the CHEK2 gene. Case presentation A healthy 28-year-old woman with a family history of breast and ovarian cancer was referred for genetic testing. The variant c.793-1G > A (rs730881687) was identified by Next Generation Sequencing (NGS) using a solution-based capture method, targeting 33 cancer predisposition genes (SeqCap EZ Probe library, Roche NimbleGen). Experimental analysis in patient-derived leukocytes using RT-PCR of mRNA followed by cDNA sequencing revealed the deletion of one base from the alternative transcript created (r.793del). This resulted in a frameshift leading to premature termination codon within exon 7 (p.(Asp265Thrfs*10)). Conclusions This finding suggests that the CHEK2 splicing variant c.793-1G > A is a deleterious variant. Our case shows that RNA analysis is a valuable tool for uncharacterized splice site variants in individuals referred for testing and facilitates their personalized management.http://link.springer.com/article/10.1186/s12881-019-0862-3CHEK2Splicing variantNext generation sequencingRNA analysis
collection DOAJ
language English
format Article
sources DOAJ
author Konstantinos Agiannitopoulos
Eirini Papadopoulou
Georgios N. Tsaousis
Georgia Pepe
Stavroula Kampouri
Mehmet Ali Kocdor
George Nasioulas
spellingShingle Konstantinos Agiannitopoulos
Eirini Papadopoulou
Georgios N. Tsaousis
Georgia Pepe
Stavroula Kampouri
Mehmet Ali Kocdor
George Nasioulas
Characterization of the c.793-1G > A splicing variant in CHEK2 gene as pathogenic: a case report
BMC Medical Genetics
CHEK2
Splicing variant
Next generation sequencing
RNA analysis
author_facet Konstantinos Agiannitopoulos
Eirini Papadopoulou
Georgios N. Tsaousis
Georgia Pepe
Stavroula Kampouri
Mehmet Ali Kocdor
George Nasioulas
author_sort Konstantinos Agiannitopoulos
title Characterization of the c.793-1G > A splicing variant in CHEK2 gene as pathogenic: a case report
title_short Characterization of the c.793-1G > A splicing variant in CHEK2 gene as pathogenic: a case report
title_full Characterization of the c.793-1G > A splicing variant in CHEK2 gene as pathogenic: a case report
title_fullStr Characterization of the c.793-1G > A splicing variant in CHEK2 gene as pathogenic: a case report
title_full_unstemmed Characterization of the c.793-1G > A splicing variant in CHEK2 gene as pathogenic: a case report
title_sort characterization of the c.793-1g > a splicing variant in chek2 gene as pathogenic: a case report
publisher BMC
series BMC Medical Genetics
issn 1471-2350
publishDate 2019-07-01
description Abstract Background CHEK2 is involved in the DNA damage repair response Fanconi anemia (FA)-BRCA pathway. An increased risk for breast and other cancers has been documented in individuals who carry a single pathogenic CHEK2 variant. As for other genes involved in cancer predisposition, different types of pathogenic variants have been observed, including single nucleotide variations, short insertions/deletions, large genomic rearrangements and splicing variants. Splicing variants occurring in the splicing acceptor or donor site result in alternative mature mRNA produced and can cause intron retention, exon skipping, or creation of alternative 3′ and 5′ splice site. Thus, the pathogenicity of this type of alterations should always be explored experimentally and their effect in the mRNA and consequently the protein produced, should be defined. The aim of this study was the delineation of the effect of a splicing variant in the CHEK2 gene. Case presentation A healthy 28-year-old woman with a family history of breast and ovarian cancer was referred for genetic testing. The variant c.793-1G > A (rs730881687) was identified by Next Generation Sequencing (NGS) using a solution-based capture method, targeting 33 cancer predisposition genes (SeqCap EZ Probe library, Roche NimbleGen). Experimental analysis in patient-derived leukocytes using RT-PCR of mRNA followed by cDNA sequencing revealed the deletion of one base from the alternative transcript created (r.793del). This resulted in a frameshift leading to premature termination codon within exon 7 (p.(Asp265Thrfs*10)). Conclusions This finding suggests that the CHEK2 splicing variant c.793-1G > A is a deleterious variant. Our case shows that RNA analysis is a valuable tool for uncharacterized splice site variants in individuals referred for testing and facilitates their personalized management.
topic CHEK2
Splicing variant
Next generation sequencing
RNA analysis
url http://link.springer.com/article/10.1186/s12881-019-0862-3
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