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Identification of the BRCA1 and BRCA2 genes was a major advance in the understanding of the familial forms of breast cancer, as alterations of these genes result in a high predisposition to breast cancer.1,2 To date, analysis of BRCA1 and BRCA2 coding sequences by mutation screening methods based on PCR sequencing protocols has allowed the identification of at least 900 different point or small disease causing germline alterations (Breast Cancer Information Core, BIC database). Furthermore, several large BRCA1 rearrangements have been reported, detected by Southern blotting, lymphocyte transcript analysis, or long range PCR.3–14 The majority of characterised rearrangements result from unequal recombination events between Alu sequences. We have estimated that the contribution of large rearrangements to the spectrum of BRCA1 mutations is close to 10% in French breast-ovarian cancer families.15 Only two rearrangements of the BRCA2 gene have been detected to date: a 5 kb deletion skipping exon 3 and a 6.2 kb deletion removing exons 12-13.16,17 However, few groups have systematically looked for BRCA2 rearrangements in defined series of breast cancer cases.17–19
In order to detect such rearrangements, we have developed a bar code on combed DNA for the BRCA2 gene, which leads to a panoramic view of this gene and its flanking regions, as previously described for BRCA1.20,21 We have concurrently used BRCA1 and BRCA2 bar codes to analyse a series of 26 highly selected French patients with a family history of breast cancer only, who were previously found to be negative for point or small mutations in both BRCA1 and BRCA2 genes.
From January 1991 to December 1999, women with breast cancer (index cases), ascertained in the Institut Curie cancer genetic clinic were referred to our laboratory for BRCA1/2 analysis. Familial criteria for genetic testing were: at least three cases of breast cancer at any age in the same lineage. Each of the index cases was an affected family member. The probability of being a carrier of a breast cancer predisposing allele (whatever the gene involved) was obtained by using the MLINK program of the LINKAGE package with the parameters of the Claus segregation model modified by Easton, as previously described.22,23 After informing index cases of the aims and limits of genetic testing, blood samples were collected with their written consent for DNA extraction and lymphoblastoid cell line establishment required for DNA combing and RNA studies. DNA was tested for point mutations in both BRCA1 and BRCA2 genes using a combination of DGGE-DHPLC and FAMA-PTT-DHPLC techniques, respectively.23–25
DNA was extracted from lymphoblastoid cell lines using agarose blocks, as previously described.20,26 Combing relies on homogeneous stretching of DNA molecules at a constant rate of 2 kb/μm.26,27 It was performed using the Molecular Combing ApparatusTM (Institut Pasteur, Paris). Hybridisation and probe detection were performed as previously described.20,26 Full signals, corresponding to the BRCA1 or BRCA2 genes, were observed under an epifluorescence Leica DMRB microscope and captured with IPLab Spectrum-SU2 software (Vysis, Downers Grove, IL) using a NU 200 CCD camera (Photometrics, Tucson, AZ). The first view of full signal images is considered to constitute qualitative analysis. Full signals were captured during screening of the slide. To facilitate viewing and analyses, they were then aligned. Measurement of probes on each full signal was performed with CartographiX software using the 2 kb/μm factor, as previously described, and was considered to constitute quantitative analysis.20,26
In order to estimate the number of large rearrangements in the BRCA1 and BRCA2 genes, a series of 26 highly selected French patients with a family history of breast cancer only was analysed using BRCA1 and BRCA2 bar codes on combed DNA.
One BRCA1 deletion was detected, whereas no BRCA2 rearrangement was identified.
This study confirms the low frequency of BRCA2 rearrangements in breast cancer families.
Twenty-six unrelated French cases with a personal and family history of breast cancer (three to eight cases per family), and with at least a 90% predisposition probability (90-98%) were selected for BRCA1 and BRCA2 bar code analyses as (1) they were previously negatively tested for BRCA1/2 point or small mutations and (2) a lymphoblastoid cell line was available (table 1).
The BRCA1 bar code used has been previously described.20,26 In this series of breast cancer cases, microscopic analysis of IC1421 DNA showed BRCA1 signals without LR9-12 and with half of the LR13-15 probes (fig 1). This deletion resembled the previously reported 23.8 kb deletion of exons 8-13 of family IC568.5,20 The use of primers specifically designed for genetic testing of IC568 family members detected an identical 923 bp PCR product in patient IC1421, suggesting that these two deletions resulted from a common mutation event in these two unrelated families. This was confirmed by the characterisation of a common haplotype associated with the carrier status in the two families, namely tel - D17S1327, 131 bp - D17S1323, deleted - D17S1322, 121 bp - D17S855, 141 bp - D17S1185, 216 bp - cen (data not shown). In order to examine the frequency of this large deletion among breast cancer only families, we screened for the presence of the specific 923 bp PCR product a series of 245 women with breast cancer, ascertained at the Institut Curie cancer genetic clinic according to previously reported family criteria23 and negatively tested for BRCA1 and BRCA2 point mutations. No 923 bp fragment was observed, suggesting that this large deletion is not frequent in the study population (data not shown). No other rearrangement of the BRCA1 gene was detected by either qualitative or quantitative analysis.
The BRCA2 gene sequence is present in PACs 214K23 and 92M18 corresponding to exons 1-24 and exons 25-27 respectively (Genbank accession numbers Z74739 and Z73359). In the “Human BAC End” database (The Sanger Centre), BAC 486O17 was found to comprise both 5‘ and 3‘ ends of the BRCA2 gene, spreading over 84 kb. Intron sizes were precisely determined based on available data on sequences of both BRCA2 exons28 and PACs. Long range (LR) PCR primers were designed to obtain probes for the BRCA2 bar code (available on the Institut Curie web site), varying from 3.2 to 9 kb and spreading over several exons. This bar code is slightly different from the BRCA1 bar code, since all but two of the exons (exons 10 and 11, owing to their large sizes) are included in LR probes, and large introns are covered by the green BAC 486O17 (fig 2). A total of eight probes designed the bar code, splitting the BRCA2 gene into 13 fragments. The series of 26 breast cancer cases was analysed with the BRCA2 bar code. No rearrangement of the BRCA2 gene, on either qualitative or quantitative analysis, was detected.
The aim of the present study was to estimate the number of rearrangements in the BRCA1 and BRCA2 genes in a series of highly selected French breast cancer families. A set of 26 cases defined by an at least 90% predisposition probability (that is, an average of 4.5 breast tumours per family), absence of a point mutation in BRCA1/2, and availability of a lymphoblastoid cell line, was analysed by BRCA1 and BRCA2 bar codes on combed DNA. The previously reported 23.8 kb BRCA1 deletion of exons 8-135 was detected in one family, whereas no BRCA2 rearrangement was identified in this set of families.
Several studies have examined the BRCA1 gene for rearrangements over the past five years, but few have analysed the BRCA2 gene. Only two BRCA2 deletions have been reported to date, with one detected by RT-PCR as a case report16 and the second by Southern blotting.17 Three series looked for BRCA2 rearrangements17–19: a total of 187 families with breast only or breast-ovarian cancer history were analysed and only one deletion was detected (0.53%).17 We have developed another approach, a BRCA2 bar code, in order to look for deletion, duplication, or inversion in the BRCA2 gene. As no BRCA2 rearrangement was observed in our family series, assuming the detection of a rearrangement at least 2 kb long, this study confirms the low frequency of BRCA2 rearrangements in breast cancer families.
The frequency of large gene rearrangements in human diseases varies from 5 to 50%.29–31 The contribution of rearrangements to the BRCA1 mutation spectrum ranges from 10 to 15%.5,15 In the Dutch population, an even higher value is observed, owing to founder effects, since two deletions account for 36% of the alterations.3 The lower contribution of rearrangements to the BRCA2 mutation spectrum as compared to BRCA1 may be explained by two hypotheses: (1) the longer coding sequence (10 257 v 5592 bp) split into about 20 exons (26 v 22) and encompassing similar genomic sequence sizes (84 v 81 kb)28,32 and (2) the lower intronic density of Alu sequences (20 v 41.5%) which are the most frequently repetitive elements involved in the appearance of large gene rearrangements.29,32,33
Despite complete screening for point mutations and large rearrangements in both BRCA1 and BRCA2, only one family among the 26 highly selected families of this series was explained by the identification of a BRCA1 alteration. Therefore, 25 families including three with male breast cancer still remained unexplained. This is striking as the contribution of BRCA1/2 mutations, estimated from linkage analyses, is 65% and 96% in breast only cancer families and in families with at least one male breast cancer, respectively.34 The failure to detect mutations may be the result of mutations not detected by the methods used, especially mutations located in introns and far from splice sites. Index cases may also be sporadic cases occurring in families with a segregating predisposing mutation. Finally, such large families with a high predisposition probability may be the result of a single gene with a recessive transmission mode or more likely additional gene variations with multiplicative effects.35 Considerable work remains to be done to explain breast cancer families with no BRCA1/2 mutation.
The search for BRCA1 rearrangements may now be systematically included in genetic testing.15 However, because of the lack of evidence for a significant contribution of BRCA2 rearrangements, it does not seem justified to include the search for them in routine genetic testing at the present time. Additional studies are needed to define clearly their role in breast cancer genetic testing.
We are indebted to the families for participating in this study. We gratefully acknowledge Isabelle Eugene and Sandrine Miglierina for their daily and efficient support in the organization of the genetic clinic. We also wish to thank Isabelle Lambert and Isabelle Bezier for establishing the lymphoblastoid cell lines (Généthon, Evry). This work was supported by the Institut Curie “Programme Incitatif et Coopératif: Génétique et Biologie des Cancers du Sein”. SG and IC are supported by a fellowship from the Association pour la Recherche contre le Cancer (ARC). AA thanks the Ligue Nationale Contre le Cancer.
Database information: Breast Cancer Information Core (BIC): http://www.nhgri.nih.gov/Intramural_research/Lab_transfer/Bic/ The Institut Curie web site: www.curie.net/genetique The Sanger Centre: www.sanger.ac.uk/HGP
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