High frequency of pathogenic non-founder germline mutations in BRCA1 and BRCA2 in families with breast and ovarian cancer in a founder population

J Maksimenko; A Irmejs; G Trofimovičs; D Bērziņa; E Skuja; G Purkalne; E Miklaševičs; J Gardovskis

doi:10.1186/s13053-018-0094-0

. 2018 Jun 5;16:12. doi: 10.1186/s13053-018-0094-0

High frequency of pathogenic non-founder germline mutations in BRCA1 and BRCA2 in families with breast and ovarian cancer in a founder population

J Maksimenko ^1,^✉, A Irmejs ¹, G Trofimovičs ¹, D Bērziņa ¹, E Skuja ¹, G Purkalne ¹, E Miklaševičs ¹, J Gardovskis ¹

PMCID: PMC5989401 PMID: 29928469

Abstract

Background

Pathogenic BRCA1 founder mutations (c.4035delA, c.5266dupC) contribute to 3.77% of all consecutive primary breast cancers and 9.9% of all consecutive primary ovarian cancers. Identifying germline pathogenic gene variants in patients with primary breast and ovarian cancer could significantly impact the medical management of patients. The aim of the study was to evaluate the rate of pathogenic mutations in the 26 breast and ovarian cancer susceptibility genes in patients who meet the criteria for BRCA1/2 testing and to compare the accuracy of different selection criteria for second-line testing in a founder population.

Methods

Fifteen female probands and 1 male proband that met National Comprehensive Cancer Network (NCCN) criteria for BRCA1/2 testing were included in the study and underwent 26-gene panel testing. Fourteen probands had breast cancer, one proband had ovarian cancer, and one proband had both breast and ovarian cancer. In a 26-gene panel, the following breast and/or ovarian cancer susceptibility genes were included: ATM, BARD1, BLM, BRCA1, BRCA2, BRIP1, CDH1, CHEK2, EPCAM, FAM175A, MEN1, MLH1, MRE11A, MSH2, MSH6, MUTYH, NBN, PALB2, PMS2, PTEN, RAD50, RAD51C, RAD51D, STK11, TP53, and XRCC2. All patients previously tested negative for BRCA1 founder mutations.

Results

In 44% (7 out of 16) of tested probands, pathogenic mutations were identified. Six probands carried pathogenic mutations in BRCA1, and one proband carried pathogenic mutations in BRCA2. In patients, a variant of uncertain significance was found in BRCA2, RAD50, MRE11A and CDH1. The Manchester scoring system showed a high accuracy (87.5%), high sensitivity (85.7%) and high specificity (88.9%) for the prediction of pathogenic non-founder BRCA1/2 mutations.

Conclusion

A relatively high incidence of pathogenic non-founder BRCA1/2 mutations was observed in a founder population. The Manchester scoring system predicted the probability of non-founder pathogenic mutations with high accuracy.

Keywords: Pathogenic non-founder BRCA1/2 mutations, Triple-negative breast cancer, Familial breast cancer

Background

Hereditary breast cancers account for approximately 10% of all breast cancers, and approximately 23% of all ovarian cancers are considered hereditary [1, 2]. According to Plakhins et al., BRCA1 pathogenic founder mutations (c.4035delA, c.5266dupC) contribute to 3.77% of all consecutive primary breast cancers and 9.9% of all consecutive primary ovarian cancers [3]. BRCA1 and BRCA2 pathogenic founder mutation analysis is a relatively straightforward and cost-effective screening strategy to identify mutation carriers [4]. In Latvia, all consecutive breast and ovarian cancer cases are eligible for BRCA1 pathogenic founder mutations (c.181 T > G, c.4035delA, c.5266dupC) screening [5], and the costs of the test are covered by the public health care system. However, according to recent studies, non-founder BRCA1 and BRCA2 pathogenic mutations account for up to 21.6% of all BRCA1 and BRCA2 pathogenic mutations in the Aschkenazi Jewish population [6, 7]. There is little information about pathogenic BRCA1/2 non-founder mutations in Latvia. In a study published by Berzina et al., pathogenic non-founder mutations in BRCA1 and BRCA2 were identified in 4 out of 30 high-risk breast/ovarian cancer families from the Latvian population [8]. In another study published by Tihomirova et al., non-founder pathogenic mutations in BRCA1 and BRCA2 were detected in 9 out of 160 patients with breast and ovarian cancer [5]. These findings suggest that the proportion of pathogenic BRCA1/2 non-founder mutations is small and that family cancer history alone is of limited value to find subgroups of individuals, where expensive complete BRCA1/2 testing is indicated.

The remaining hereditary breast and ovarian cancer cases are associated with mutations in other breast and ovarian cancer susceptibility genes, such as BRCA1/2, TP53, PTEN, CDH1, STK11, MLH1, MSH2, MSH6, PMS2, PALB2, CHEK2, ATM, RAD51C, RAD51D, BRIP1 and other [9]. Patients and their relatives harbouring mutations in hereditary cancer predisposing genes could benefit prevention and screening strategies or novel therapeutic approaches [10, 11]. Advances in next-generation sequencing allowed the implementation of low-cost multi-gene panel testing in clinical practice to detect pathogenic mutations in hereditary cancer predisposing genes [12].

Therefore, knowledge of the frequency and phenotypical features of pathogenic mutations beyond BRCA1 pathogenic founder mutations in breast and ovarian cancer susceptibility genes is essential for determining the role of second-line testing with multi-gene panels in counselling unsolved high-risk breast and ovarian cancer patients.

The aim of the study was to evaluate the rate of pathogenic mutations in the 26 breast and ovarian cancer susceptibility genes in patients who meet the criteria for BRCA1/2 testing and to compare the accuracy of different selection criteria for second-line testing in a founder population.

Methods

Patient group

Sixteen sequential patients with primary breast and/or ovarian cancer who met all inclusion criteria were included in the study between October 2016 and August 2017. The inclusion criteria were as follows: 1) fulfil at least one of the National Comprehensive Cancer network (NCCN) BRCA1/2 testing criteria (Table 1) (www.nccn.org); 2) previously tested negative for BRCA1 pathogenic founder mutations (c.181 T > G, c.4035delA, c.5266dupC); 3) able to cover the cost of the 26 multi-gene tests.

Table 1.

NCCN selection criteria for screening of mutations in BRCA1and BRCA2

At least one of the following criteria has to be met:
1. Personal history of breast cancer diagnosed < age 45 years
2. Personal history of breast cancer diagnosed < age 50 years and at least one case of breast cancer at any age in close blood relative
3. Personal history of triple negative breast cancer diagnosed < age 60 years
4. Personal history of breast cancer diagnosed at any age and at least two cases of breast cancer diagnosed at any age or at least one close blood relative with breast cancer diagnosed ≤50 years or at least one blood relative with ovarian carcinoma or a close male blood relative with breast cancer
5. Personal history of ovarian cancer
6. Personal history of male breast cancer

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The following clinical information was obtained: age at testing, personal cancer history, age at cancer diagnosis, breast and/or ovarian cancer pathology, BRCA1/2 testing history, a family cancer history that covers a 3-generation pedigree according to probands information. The median patient age was 45.6 years (33–63 years). Fifteen out of 16 (93.75%) patients were females, and 1 out of 16 (6.25%) patients was male. Thirteen patients had unilateral breast cancer, 1 patient had bilateral breast cancer, 1 patient had ovarian cancer, and in 1 patient had both breast and ovarian cancer. Four out of 16 (25%) breast cancers were luminal-like HER2 negative, 2 out of 16 (12.5%) breast cancers were luminal B HER2 positive, 8 out of 16 (50%) breast cancers were triple-negative, and 1 out of 16 (6.25%) breast cancers was HER2 positive. The patient characteristics are summarized in Table 2.

Table 2.

The baseline characteristics of patient group

Nr.	Probands age at diagnosis (years)	Primary cancer site	Morphological subtype	Breast cancersubtype	Tumor grade	Family history
1	54	Breast	Ductal	Luminal	missing	Mother and maternal aunt – breast cancer age 60; daughter - polycytemia vera age15, brother – melanoma age 60
2	40	Breast	Ductal	Triple-negative*	G3	Mother - Breast and ovarian cancer age 40
3	33 and 38	Left Breast/ Right Breast	Ductal/ Ductal	Triple-negative/ Luminal	G3/G3	Paternal grandmother - unknown primary gynecological cancer age 50
4	63	Breast and Ovaries	Ductal	Triple-negative	G2	Mother with breast cancer age 55; sister - ovarian cancer age 59
5	37	Ovaries	NA	NA	NA	Mother - breast cancer age 64
6	58	Breast	Lobular	Luminal	G2	Mother and maternal aunt – breast cancer age > 60
7	43	Breast	Ductal	Triple-negative	G3	No
8	42	Breast	Ductal/Medullary	Triple-negative	G2	Mother - breast cancer age 60
9	50	Breast	Ductal	Triple-negative	G3	Mother - breast cancer age 52
10	35	Breast	Ductal	Triple-negative	G3	Mother - breast cancer age 46
11	52	Breast	Ductal	Luminal B HER2 positive	G2	Mother and maternal aunt – breast cancer age > 50
12	41	Breast	Ductal	HER2 positive	G3	No
13	53	Breast	Ductal	Triple-negative	missing	No
14	36	Breast	Ductal	Luminal	missing	No
15	53	Breast	Ductal	Luminal	missing	Mother and maternal grandmother – breast cancer age > 60 years
16	40	Breast	Ductal	Luminal B HER2 positive	missing	No

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DNA testing

Informed consent for genetic testing was obtained for all patients. All patients underwent DNA testing with a 26-gene panel (myBRCA HiRisk Hereditary Breast and Ovarian Cancer screening Test, VeritasGenetics, USA) that is a targeted next-generation sequencing assay for the detection of mutations in 26 breast and ovarian cancer susceptibility genes. The genes included high-penetrance breast-ovarian genes (BRCA1, BRCA2, PTEN, TP53, CDH1, STK11, PALB2), moderate-penetrance breast and/or ovarian genes (CHEK2, BRIP1, ATM), and additional genes (BARD1, BLM, EPCAM, RAD50, RAD51C, RAD51D, MEN1, MRE11A, MUTYH MSH2, MLH1, NBN, MSH6, PMS2, FAM175A, XRCC2). In all patients, the test was performed using saliva. The specificity and sensitivity of the assay are 99.9% for point mutations and small insertions/deletions in the 24 sequenced genes and 99.9% for structural variations in BRCA1 and BRCA2.

Statistical analysis

The specificity, sensitivity and accuracy of the NCCN criteria, Manchester scoring system and Swedish Breast cancer group criteria for the prediction of pathogenic non-founder mutations were evaluated. The Manchester score of 15 points threshold was used to assess the likelihood of BRCA1/2 pathogenic mutation [13]. The specificity, sensitivity and accuracy of different selection criteria for BRCA1/2 testing in our cohort were calculated using MedCalc Statistical Software version 17.9.

Results

In seven out of sixteen (44%) patients included, pathogenic non-founder BRCA1/2 mutations were identified. Six patients carried pathogenic variants of BRCA1 and one of BRCA2. In four patients, variants of uncertain significance of BRCA2, RAD50, MRE11A and CDH1 were found. Detailed results are shown in Table 3. The NCCN criteria showed a high sensitivity (100%) with low specificity (50%) for the prediction of non-founder pathogenic BRCA1/2 mutations. The Swedish Breast cancer group criteria showed a low sensitivity (57.1%) with three false negative results. The Manchester scoring system showed a high accuracy (87.5%) for the prediction of pathogenic non-founder BRCA1/2 mutations with high sensitivity (85.7%) and specificity (88.9%). The sensitivity, specificity and accuracy of different criteria/scoring systems for the detection of probability of BRCA1/2 pathogenic mutations in our cohort are compared in Table 4.

Table 3.

Results

Nr.	Mutation	Clinical significance of mutation	NCCN inclusion criteria	Manchester score [13]	Swedish Breast cancer group criteria for screening of mutation in BRCA1 and BRCA2
1	RAD50c.980G > A	VUS	NCCN4	17	One case of male breast cancer
2	BRCA1c.5075-?_5152 +?del	PAT	NCCN2	29	One case of triple-negative breast cancer ≤age 40
3	BRCA1c.1-?_c.134 +?del	PAT	NCCN3	20	One case of breast cancer ≤age 35
4	BRCA2c.6998dupT	PAT	NCCN4	19	Breast cancer and ovarian cancer in one individual.
5	BRCA1c.5117G > A	PAT	NCCN5	15	Do not match
6	RAD50c.251 T > A	VUS	NCCN4
6	MRE11Ac.1715G > A	VUS		6	NA
7	BRCA1c.1961delA	PAT	NCCN3	14	Do not match
8	BRCA2c.280C > T	VUS	NCCN4	14	Do not match
9	BRCA1c.5117G > A	PAT	NCCN4	16	Do not match
10	BRCA1c.4996_4997dupTA	PAT	NCCN4	20	One case of triple-negative breast cancer ≤age 40
11	Negative	Negative	NCCN4	2	Do not match
12	Negative	Negative	NCCN1	2	Do not match
13	Negative	Negative	NCCN3	8	Do not match
14	Negative	Negative	NCCN1	8	Do not match
15	CDH1 c.808 T > G	VUS	NCCN4	8	Do not match
16	Negative	Negative	NCCN1	0	Do not match

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PAT, pathological; VUS, variant of uncertain significance; *Triple-negative breast cancer was defined as ER-0%; PR-0%; HER2- negative;

Table 4.

Comparison of different selection criteria for BRCA1/2 testing in our cohort

Criteria	Sensitivity	Specificity	Accuracy
NCCN	100%	50%	64%
Manchester scoring system	85.7%	88.9%	87.5%
Swedish Breast cancer group	57.1%	88.9%	75%

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Discussion

Our study is the first report on the use of a 26 gene panel in to examine breast and ovarian cancer susceptibility genes in patients in Latvia. We demonstrated a high frequency of pathogenic non-founder germline mutations in BRCA1 and BRCA2 genes. In seven out of sixteen (44%) primary breast and ovarian cancer patients matching the criteria for BRCA1/2 testing pathogenic non-founder BRCA1/2 mutations were identified. All 7 pathogenic mutations, including 2 large deletions, are novel in populations of Latvia [5, 8]. These results may suggest that the present practice of testing only the 3 most frequent BRCA1 pathogenic founder mutations is insufficient and fails to detect a considerable number of pathogenic mutations in BRCA1/2. However, our study comprises a relatively small cohort of selected patients. In a study published by Frank et al., 21.6% of patients with Ashkenazi ancestry pathogenic non-founder BRCA1 and BRCA2 mutations were identified [6]. In contrast, in the Finnish population of high-risk individuals tested negative for 28 BRCA1/2 pathogenic founder mutations, additional pathogenic mutations in BRCA1 and BRCA2 accounted for just 1.2% [12]. Much larger numbers are necessary to assess the real proportion of pathogenic non-founder mutations in the population of Latvia.

Despite the drawbacks of such a small study group, the initial results raised some observations.

Interestingly, probands that carried a pathogenic non-founder mutation had some common features. All six breast cancer patients in our study with proven pathogenic non-founder BRCA1/2 mutations had a triple-negative phenotype. It is well established that approximately 80% of all BRCA1/2– related tumours have a triple-negative phenotype [14–18]. The prevalence of pathogenic germline BRCA1/2 mutations in the selected triple-negative breast cancer patients ranged from 9.2 to 34.4% [19–22]. Additional analyses of cDNA microarray data from van’t Veer showed that BRCA1-related tumours have a sporadic basal-like breast cancer gene expression profile [23]. Additionally, according to Richardson et al., loss of BRCA1 function could play a role in the development of basal-like breast cancers [24]. Couch et al. identified BRCA1/2 pathogenic mutations in 11.2% of triple-negative breast cancer patients and other breast-ovarian cancer predisposing gene mutations in 3.7% of triple-negative breast cancer patients [25].

In our study we used the NCCN criteria for screening pathogenic mutations in BRCA1 and BRCA2, where triple-negative breast cancer is used as a criterion together with an age limit < 60. Only one out of six breast cancer patients in our study who carried a pathogenic BRCA1/2 non-founder mutation was older than 60 years of age, but in this case, family cancer history was positive in the study published by Couch et al., 3.1% of triple-negative breast cancer patients older than 60 years and only 1.4% with no family history of breast or ovarian cancer were diagnosed with BRCA1/2 pathogenic mutation [25]. Therefore, our study results support the current NCCN guidelines for screening all triple-negative breast cancer patients younger than 60 years of age.

In contrast, the application of the upper age limit for triple-negative breast cancer patients of 40 years (Swedish Breast cancer group criteria for screening for mutations in BRCA1 and BRCA2) would miss several BRCA-positive cases in our cohort [26].

Our small study showed the high accuracy of the Manchester scoring system for the prediction of pathogenic non-founder BRCA1/2 mutations in founder mutation-negative patients. Our finding is supported by several other studies performed on the validation of the Manchester scoring system in populations of UK, Germany and South East Asia [13, 27, 28]. However, larger numbers of cases are needed for comprehensive validation of these criteria in the population of Latvia.

Additionally, three out of eight patients tested negative for 26 breast and ovarian cancer susceptibility genes were HER2 positive. According to a recently published study, only 9% of BRCA1-related breast tumours and 13% of BRCA2-related breast tumours were HER2 positive [29]. HER2 positivity is also included in the Manchester scoring system as a BRCA1/2 probability decreasing factor [13].

Ovarian cancer in a personal or family history was documented in three out of seven patients who carried a pathogenic BRCA1/2 non-founder mutation. Additionally, in one case, unknown gynaecological cancer was reported in a paternal aunt. According to recent studies, the presence of ovarian cancer in personal or family history of pathogenic BRCA1 founder-negative breast cancer patients increases the possibility of carrying previously undetected pathogenic BRCA1/2 non-founder mutations [30, 31]. Recently, in a study published by Couch et al., ovarian cancer in family history was documented only in 1 of 54 pathogenic non-BRCA1/2 mutation carriers with triple-negative breast cancer [25].

In our study, no pathogenic mutations were detected in another 24 genes included in the panel. Some previously published studies demonstrated that the rate of pathogenic mutations in non-BRCA1/2 genes ranged from 2.9 to 9.3% [32–35].

Four of the 16 (25%) patients were identified to have a variant of unknown significance (VUS) in BRCA2, RAD50, CDH1 and MRE11. Unfortunately, due to an insufficient sample size in our study, we cannot elaborate upon those results.

Conclusion

A relatively high incidence of pathogenic non-founder BRCA1/2 mutations was observed among patients with triple-negative familial breast cancer in a founder population. The Manchester scoring system predicted the probability of non-founder pathogenic mutations with high accuracy.

Acknowledgments

Funding

This work was supported by State Research Program “Biomedicine for the public health (BIOMEDICINE)” project 5 “Personalised cancer diagnostics and treatment effectiveness evaluation”.

Availability of data and materials

The datasets generated during and/or analyzed during the current study are available from the corresponding author on reasonable request.

Abbreviations

ATM: Ataxia-telangiectasia mutated
BARD1: BRCA1 (Breast Cancer 1) Associated RING Domain 1 gene
BLM: Bloom’s syndrome gene
BRCA1: Breast cancer susceptibility gene 1
BRCA2: Breast cancer susceptibility gene 2
BRIP1: BRCA1-interacting protein 1 gene
CDH: Cadherin-1 gene
cDNA: Complementary Deoxyribonucleic Acid
CHEK2: Checkpoint kinase 2 gene
DNA: Deoxyribonucleic Acid
EPCAM: epithelial cell adhesion molecule gene
ER: Estrogen receptor
FAM175A: Family with sequence similarity 175A gene
G2: Moderately differentiated
G3: Well differentiated
HER2: Human epidermal growth factor receptor 2
MEN1: multiple endocrine neoplasia type 1
MLH: MutL homolog 1 gene
MRE11A: MRE11 meiotic recombination 11 homolog A gene
MSH6: MutL homolog 6 gene
MUTYH: MutY DNA glycosylase
NA: Not applicable
NBN: Nibrin gene
NCCN: National Comprehensive Cancer Network
PALB2: Partner and localizer of BRCA2 gene
PAT: Pathological
PMS2: postmeiotic segregation increased 2
PR: Progesterone receptor
PTEN: Phosphatase and tensin homolog gene
RAD50: Human homolog of S. cerevisiae RAD50 gene
RAD51: RAD51 paralog D
RAD51C: RAD51 homolog C
STK11: serine/threonine kinase 11 gene
TP53: tumor protein p53 gene
USA: United States of America
VUS: Variant of uncertain significance
XRCC2: X-ray repair cross-complementing protein 2

Authors’ contributions

JM, AI and GT analyzed and interpreted the patient data regarding the disease. ES and GP analyzed and interpreted patient data regarding chemotherapy. EM and DB analyzed and interpreted genetic screening results. JM, AI, EM and JG were major contributors in writing the manuscript. All authors read and approved the final manuscript.

Ethics approval and consent to participate

The study was approved by a Central Medical Ethics Committee of Latvia. Written consent was obtained.

Competing interests

The authors declare that they have no competing interests.

Publisher’s Note

Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.

Contributor Information

J. Maksimenko, Email: Jelena.Maksimenko@rsu.lv

A. Irmejs, Email: Arvids.Irmejs@rsu.lv

G. Trofimovičs, Email: Genadijs.Trofimovics@rsu.lv

D. Bērziņa, Email: Dace.Berzina@rsu.lv

E. Skuja, Email: Elina.Skuja@stradini.lv

G. Purkalne, Email: Gunta.Purkalne@rsu.lv

E. Miklaševičs, Email: Edvins.Miklasevics@rsu.lv

J. Gardovskis, Email: Janis.Gardovskis@rsu.lv

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Associated Data

This section collects any data citations, data availability statements, or supplementary materials included in this article.

Data Availability Statement

The datasets generated during and/or analyzed during the current study are available from the corresponding author on reasonable request.

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[CR23] 23.Sorlie T, Tibshirani R, Parker J, Hastie T, Marron JS, Nobel A, Deng S, Johnsen H, Pesich R, Geisler S, Demeter J, Perou CM, Lønning PE, Brown PO, Børresen-Dale AL, Botstein D. Repeated observation of breast tumor subtypes in independent gene expression data sets. Proc Natl Acad Sci U S A. 2003;100(14):8418. doi: 10.1073/pnas.0932692100. [DOI] [PMC free article] [PubMed] [Google Scholar]

[CR24] 24.Richardson AL, Wang ZC, De Nicolo A, Lu X, Brown M, Miron A, Liao X, Iglehart JD, Livingston DM, Ganesan S. X chromosomal abnormalities in basal-like human breast cancer. Cancer Cell. 2006;9(2):121. doi: 10.1016/j.ccr.2006.01.013. [DOI] [PubMed] [Google Scholar]

[CR25] 25.Couch FJ, Hart SN, Sharma P, Toland AE, Wang X, Miron P, Olson JE, Godwin AK, Pankratz VS, Olswold C, Slettedahl S, Hallberg E, Guidugli L, Davila JI, Beckmann MW, Janni W, Rack B, Ekici AB, Slamon DJ, Konstantopoulou I, Fostira F, Vratimos A, Fountzilas G, Pelttari LM, Tapper WJ, Durcan L, Cross SS, Pilarski R, Shapiro CL, Klemp J, Yao S, Garber J, Cox A, Brauch H, Ambrosone C, Nevanlinna H, Yannoukakos D, Slager SL, Vachon CM, Eccles DM, Fasching PA. Inherited mutations in 17 breast cancer susceptibility genes among a large triple-negative breast cancer cohort unselected for family history of breast cancer. J Clin Oncol. 2015;33(4):304. doi: 10.1200/JCO.2014.57.1414. [DOI] [PMC free article] [PubMed] [Google Scholar]

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[CR27] 27.Kast K, Schmutzler RK, Rhiem K, Kiechle M, Fischer C, Niederacher D, Arnold N, Grimm T, Speiser D, Schlegelberger B, Varga D, Horvath J, Beer M, Briest S, Meindl A, Engel C. Validation of the Manchester scoring system for predicting BRCA1/2 mutations in 9,390 families suspected of having hereditary breast and ovarian cancer. Int J Cancer. 2014;135(10):2352–2361. doi: 10.1002/ijc.28875. [DOI] [PubMed] [Google Scholar]

[CR28] 28.Chew W, Moorakonda RB, Courtney E, Soh H, Li ST, Chen Y, Shaw T, Allen JC, Evans DGR, Ngeow J. Evaluation of the relative effectiveness of the 2017 updated Manchester scoring system for predicting BRCA1/2 mutations in a southeast Asian country. J Med Genet. 2017;55:344–350. doi: 10.1136/jmedgenet-2017-105073. [DOI] [PubMed] [Google Scholar]

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[CR31] 31.Lee JS, John EM. McGuire Breast and Ovarian cancer in relatives of cancer patients, with and without BRCA mutations. Cancer Epidemiol Biomarkers Prev. 2006;15:359. doi: 10.1158/1055-9965.EPI-05-0687. [DOI] [PubMed] [Google Scholar]

[CR32] 32.Susswein LR, Marshall ML, Nusbaum R, Postula KJV, Weissman SM, Yackowski L, Vaccari EM, Bissonnette J, Booker JK, Laura Cremona M, Gibellini F, Murphy PD, Pineda-Alvarez DE, Pollevick GD, Zhixiong X, Richard G, Bale S, Klein RT, Hruska KS, Chung WK. Pathogenic and likely pathogenic variant prevalence among the first 10,000 patients referred for next-generation cancer panel testing. Genet Med. 2016;18(8):823. doi: 10.1038/gim.2015.166. [DOI] [PMC free article] [PubMed] [Google Scholar]

[CR33] 33.Desmond A, Kurian AW, Gabree M, Mills MA, Anderson MJ, Kobayashi Y, Horick N, Yang S, Shannon KM, Tung N, Ford JM, Lincoln SE, Ellisen LW. Clinical Actionability of multigene panel testing for hereditary breast and ovarian Cancer risk assessment. JAMA Oncol. 2015;1(7):943. doi: 10.1001/jamaoncol.2015.2690. [DOI] [PubMed] [Google Scholar]

[CR34] 34.Thompson ER, Rowley SM, Li N, McInerny S, Devereux L, Wong-Brown MW, Trainer AH, Mitchell G, Scott RJ, James PA, Campbell IG. Panel testing for familial breast Cancer: calibrating the tension between research and clinical care. J Clin Oncol. 2016;34(13):1455. doi: 10.1200/JCO.2015.63.7454. [DOI] [PubMed] [Google Scholar]

[CR35] 35.Schroeder C, Faust U, Sturm M, Hackmann K, Grundmann K, Harmuth F, Bosse K, Kehrer M, Benkert T, Klink B, Mackenroth L, Betcheva-Krajcir E, Wimberger P, Kast K, Heilig M, Nguyen HP, Riess O, Schröck E, Bauer P, Rump A. HBOC multi-gene panel testing: comparison of two sequencing centers. Breast Cancer Res Treat. 2015;152(1):129. doi: 10.1007/s10549-015-3429-9. [DOI] [PubMed] [Google Scholar]

PERMALINK

High frequency of pathogenic non-founder germline mutations in BRCA1 and BRCA2 in families with breast and ovarian cancer in a founder population

J Maksimenko

A Irmejs

G Trofimovičs

D Bērziņa

E Skuja

G Purkalne

E Miklaševičs

J Gardovskis

Abstract

Background

Methods

Results

Conclusion

Background

Methods

Patient group

Table 1.

Table 2.

DNA testing

Statistical analysis

Results

Table 3.

Table 4.

Discussion

Conclusion

Acknowledgments

Funding

Availability of data and materials

Abbreviations

Authors’ contributions

Ethics approval and consent to participate

Competing interests

Publisher’s Note

Contributor Information

References

Associated Data

Data Availability Statement

ACTIONS

PERMALINK

RESOURCES

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