Abstract
Purpose
BRCA1/BRCA2 predictive test negatives are proven noncarriers of a BRCA1/BRCA2 mutation that is carried by their relatives. The risk of developing breast cancer (BC) or epithelial ovarian cancer (EOC) in these women is uncertain. The study aimed to estimate risks of invasive BC and EOC in a large cohort of BRCA1/BRCA2 predictive test negatives.
Methods
We used cohort analysis to estimate incidences, cumulative risks, and standardized incidence ratios (SIRs).
Results
A total of 1,895 unaffected women were eligible for inclusion in the BC risk analysis and 1,736 in the EOC risk analysis. There were 23 incident invasive BCs and 2 EOCs. The cumulative risk of invasive BC was 9.4% (95% confidence interval (CI) 5.9–15%) by age 85 years and the corresponding risk of EOC was 0.6% (95% CI 0.2–2.6%). The SIR for invasive BC was 0.93 (95% CI 0.62–1.40) in the overall cohort, 0.85 (95% CI 0.48–1.50) in noncarriers from BRCA1 families, and 1.03 (95% CI 0.57–1.87) in noncarriers from BRCA2 families. The SIR for EOC was 0.79 (95% CI 0.20–3.17) in the overall cohort.
Conclusion
Our results did not provide evidence for elevated risks of invasive BC or EOC in BRCA1/BRCA2 predictive test negatives.
Keywords: BRCA1/BRCA2, breast cancer, ovarian cancer, predictive test negatives, risks
Introduction
Several breast and ovarian cancer susceptibility genes have been identified to date. The most important genes in the context of genetic counseling are BRCA1 and BRCA2, which are associated with high risks of developing breast, ovarian, and other cancers.1,2,3,4,5 Genetic testing for BRCA1 and BRCA2 has become an integral part of genetic counseling; the results are used to inform women’s treatment or clinical management options, which involve a combination of screening, prophylactic surgery, and other risk reduction strategies.6,7,8,9,10,11
BRCA1/BRCA2 predictive test negatives are individuals who have been offered a predictive test for a specific BRCA mutation that has been found in a biological relative, and then found to be a noncarrier. Several studies have estimated the risk of developing breast cancer (BC) and epithelial ovarian cancer (EOC) in these women, but estimates vary widely across studies. Although the risks have generally been found to be lower than those in BRCA1 and BRCA2 mutation carriers, retrospective studies have estimated the risks of BC to be two- to fivefold higher than the risk in the general population.12,13 Estimates based on retrospective studies may be overestimated if ascertainment is not correctly allowed for in the analysis. The findings from the eight prospective studies published to date have been conflicting. In five of them, risk to noncarriers was not raised (0.52–0.95) (refs.14,15,16,17,18) while in three studies the estimated risks were significantly increased (2.0–4.57) (refs.19,20,21). An important limitation in all these studies, however, was small sample size, and as a result the point estimates have wide confidence intervals. Data on EOC risks for BRCA1/BRCA2 predictive test negatives are currently scarce and the only estimates available are from retrospective studies.13,22
Here, we used data from a large prospective cohort of BRCA1/BRCA2 predictive test negatives from the United Kingdom to estimate the risks of developing BC or EOC.
Materials and methods
Subjects
The Epidemiological Study of Familial Breast Cancer (EMBRACE) study is a prospective cohort study in the United Kingdom and Republic of Ireland, aiming to characterize cancer risks in BRCA1/BRCA2 mutation carriers and their relatives. Individuals are eligible for inclusion in EMBRACE if they (i) carry a pathogenic mutation in BRCA1 or BRCA2, (ii) are noncarriers in families with a pathogenic BRCA1 or BRCA2 mutation, or (iii) are potential carriers but opt not to undergo a predictive genetic test. Recruitment is organized through regional cancer genetics centers, generally close to the time of genetic testing. Recruitment commenced in 1997 and includes both women and men. The cohort includes individuals with or without personal history of cancer; all participants complete a baseline questionnaire that includes information on BC and EOC risk factors and medical history. The EMBRACE study was approved by the former Anglia and Oxford Medical Research and Ethics Committee (North West Anglia Health Authority, Peterborough, United Kingdom), now East of England–Cambridge South Research Ethics Committee (Nottingham, United Kingdom).
Only noncarrier women were eligible for inclusion in the present study. Information on date and cause of death, and cancer diagnoses, was obtained through linkage with the Health and Social Care Information Centre for England and Wales, and with the National Health Service Central Register for Scotland. For the purpose of the study, the last record linkage was performed on 15 December 2015. The end of follow-up was set as 15 July 2015 to ensure that any cancer diagnoses by this date were likely to have been reported at the time of the record linkage.
Cancer risks for BRCA1/BRCA2 predictive test negatives were estimated separately for incident invasive BC and incident EOC. Women were eligible for inclusion in the analysis if they had not been diagnosed with cancer, other than nonmelanoma skin cancer, before the date at the baseline questionnaire (study recruitment). For the estimation of BC risk, participants were ineligible if they had already undergone risk-reducing bilateral mastectomy at recruitment. In estimating EOC risk, participants were ineligible if they had undergone risk-reducing salpingo-oophorectomy (RRSO) or bilateral salpingectomy (because noncarriers in EMBRACE do not complete follow-up questionnaires after study recruitment, information on prospective prophylactic surgeries occurring after the baseline questionnaire date was not available). Women were followed from baseline until the first of (i) death, (ii) a diagnosis of a cancer other than nonmelanoma skin cancer, (iii) attained age 85 years, or (iv) 15 July 2015. For the BC risk estimation, only women diagnosed with an incident invasive BC were assumed to be affected (i.e., noninvasive BCs were ignored but censored as unaffected at diagnosis) and for the EOC analysis only women diagnosed with an EOC were assumed to be affected.
Statistical analysis
Annual incidences of invasive BC and EOC per 1,000 person-years were estimated for the age intervals 18–24, 25–34, 35–44, 45–54, 55–64, 65–74, and 75–84 using standard cohort analysis. Kaplan–Meier analysis was used to estimate the cumulative risks. The probability of experiencing the event of interest up to a given time-point was calculated as 1−Kaplan-Meier estimate of the survival probability. Differences in cancer risks between members of BRCA1 families and members of BRCA2 families were assessed using Cox regression. The hazard ratio was defined as the ratio between the hazard function at age t for noncarriers from BRCA2 families and the hazard function at age t for noncarriers from BRCA1 families. To account for possible variation in risk due to year of birth (i.e., cohort effect), the analysis was adjusted for year of birth using a categorical variable based on the observed quartiles (1922 to 1953, 1954 to 1963, 1964 to 1972, 1973 to 1995).
We assessed the difference between the estimated incidence rates of invasive BC and EOC in the sample under study and the corresponding incidence rates in a reference population by estimating the standardized incidence ratio (SIR). A SIR is the ratio between the number of observed incident cases and the number of expected incident cases in the study population over the period of observation. For this purpose, we used the population incidences for England23 and assumed they also apply to women recruited from Scotland and Wales. Expected cases were calculated by applying the calendar period–specific, age-specific, and cancer-specific incidences for England to the eligible sample of noncarriers. These rates were available from 1998 to 2014. Rates for 1998 and 2014 were assumed to apply for the years 1997 and 2015, respectively. To allow for the fact that multiple individuals from the same family may be included in the analyses robust standard errors were calculated by clustering on family.24
Results
The process of generating the eligible sets for inclusion in the BC and EOC analyses are described in the appendix (Supplementary Figures S1 and S2 online). Table 1 summarizes the eligible cohort characteristics.
Table 1.
Eligible set for invasive BC analysis | Eligible set for EOC analysis | |||||
---|---|---|---|---|---|---|
Overall | BRCA1 a | BRCA2 a | Overall | BRCA1 a | BRCA2 a | |
Sample, N (%) | 1,895 | 1,042 (55) | 849 (45) | 1,736 | 939 (54) | 793 (46) |
Mean age at questionnaire (SD) | 45.1 (13.1) | 44.6 (13.1) | 45.6 (13) | 44.2 (13.1) | 43.5 (13) | 45.1 (13.1) |
Mean follow-up in years (SD) | 7.1 (4.5) | 7.4 (6.6) | 6.6 (4.3) | 7.0 (4.5) | 7.3 (4.7) | 6.6 (4.3) |
Failures | 23 | 12 | 11 | 2 | 0 | 2 |
Mean age at failure (SD) | 57.2 (8.8) | 60.5 (9.7) | 53.6 (6.2) | 50.5 (8.0) | — | 50.5 (8.0) |
Ethnicity (%) | ||||||
Unknown | 1 (0) | 0 | 1 (0) | 1 (0) | 0 | 1 (0) |
White | 1,810 (96) | 982 (94) | 824 (97) | 1,658 (95) | 885 (94) | 769 (97) |
Indian | 5 (0.3) | 4 (0.4) | 1 (0.1) | 5 (0.4) | 4 (0.5) | 1 (0.1) |
Black-Caribbean | 3 (0.2) | 3 (0.3) | 0 | 3 (0.2) | 3 (0.3) | 0 |
Ashkenazi Jewish | 47 (2) | 34 (3.4) | 13 (1.8) | 45 (3) | 32 (3.4) | 13 (1.8) |
Bangladeshi | 1 (0) | 1 (0.1) | 0 | 1 (0) | 1 (0.1) | 0 |
Pakistani | 3 (0.2) | 2 (0.2) | 1 (0.1) | 3 (0.2) | 2 (0.2) | 1 (0.1) |
Black other | 5 (0.3) | 5 (0.5) | 0 | 4 (0.3) | 4 (0.5) | 0 |
Chinese | 1 (0) | 0 | 1 (0.1) | 0 | 0 | 0 |
Other | 19 (1) | 11 (1.1) | 8 (0.9) | 16 (0.9) | 8 (1) | 8 (1) |
Number of families (%) | 1,602 | 887 (55) | 711 (45) | 1,488 | 812 (55) | 672 (45) |
Families by number of noncarriers (%) | ||||||
1 | 1,381 (86) | 767 (86) | 610 (86) | 1,300 (87) | 714 (88) | 582 (88) |
2 | 179 (11) | 98 (11) | 81 (11) | 152 (11) | 80 (10) | 72 (11) |
3 | 25 (2) | 14 (2) | 11 (1.6) | 24 (1.5) | 11 (1.3) | 13 (0.3) |
4 | 14 (1) | 6 (0.8) | 8 (1.3) | 9 (0.5) | 5 (0.5) | 4 (0.6) |
5 | 1 (0) | 1 (0.1) | 0 | 1 (0) | 1 (0.1) | 0 |
6 | 0 | 0 | 0 | 0 | 0 | 0 |
7 | 0 | 0 | 0 | 1 (0) | 1 (0.1) | 0 |
8 | 1 (0) | 1 (0.1) | 0 | 0 | 0 | 0 |
9 | 0 | 0 | 0 | 0 | 0 | 0 |
10 | 0 | 0 | 0 | 0 | 0 | 0 |
11 | 0 | 0 | 0 | 0 | 0 | 0 |
12 | 1 (0) | 0 | 1 (0.1) | 1 (0) | 0 | 1 (0.1) |
BC, breast cancer; EOC, epithelial ovarian cancer.
aIn four individuals family identification number and family mutation were missing. In reference to familial clustering, these individuals were assumed to be independent. No assumptions were made on family mutation; therefore, in the stratified analysis by family mutation, these individuals were not considered.
Risk of invasive BC
Among 1,895 BRCA1/BRCA2 predictive test negatives eligible for inclusion in the BC analysis, 23 incident invasive BCs occurred, 12 in women from BRCA1 families and 11 in women from BRCA2 families. The estimated incidences, cumulative risks, and SIRs are shown in Table 2. The crude incidence rate of invasive BC in the overall sample was estimated to be 1.72 per 1,000 person-years (95% confidence interval (CI) 1.16–2.66). The incidence rate increased rapidly at young ages up to age 45 but remained relatively constant after that age, ranging from 2.33 to 3.04 per 1,000 person-years. The estimate was similar when analysis was restricted to individuals of European ancestry (1.74/1,000 person-years, 95% CI 1.17–2.70). The incidence rate in members of BRCA2 families (1.95/1,000 person-years, 95% CI 1.11–3.79) was slightly, but not significantly (p value 0.58), higher than the rate in members of BRCA1 families (1.55/1,000 person-years, 95% CI 0.90–2.92). After adjustment for birth cohort, the hazard ratio estimate for members of BRCA2 families versus members of BRCA1 families was 1.20 (95% CI 0.53–2.70, Wald test p value=0.6). The SIR estimate for invasive BC was 0.93 (95% CI 0.62–1.40). In the age-specific analysis the highest SIR was estimated for age group 45–55 (SIR=1.30, 95% CI 0.72–2.35), but SIRs were estimated to be <1 for all other age groups (range: 0.35–0.89). There was no apparent trend in the SIRs with age. The SIR was estimated to be 0.85 (95% CI 0.48–1.50) for members of a BRCA1 family with the highest SIR estimated for age group 65–75 (SIR=1.56, 95% CI 0.59–4.16) and 1.03 (95% CI 0.57–1.87) for relatives of BRCA2 mutation carriers with the highest SIR occurring for ages 45–55 (SIR=1.85, 95% CI 0.88–3.87) (Table 2). The risk of developing invasive BC in the pooled sample was estimated to be 3% (95% CI 1.7–5.3%) by age 55 years and 9.4% (95% CI 5.9–15%) by age 85 years (Figure 1). When analysis was restricted to members of BRCA1 families, the cumulative risk of invasive BC was estimated to be 1.8% (95% CI 0.7–4.8%) by age 55 and 11% (95% CI 5.6–19%) by age 85. For members of BRCA2 families, the risk of developing invasive BC was 4.5% (95% CI 2.3–8.8%) by age 55 and 7.7% (95% CI 4.2–14%) by age 85 (Supplementary Figure S3 online). Sensitivity analyses, after excluding women with bilateral oophorectomy, excluding the first year of follow-up or by including in situ BCs yielded similar results (sensitivity analyses described in the appendix (Supplementary Table S1 online)).
Table 2.
Overall sample | Relatives ofBRCA1mutation carriers | Relatives ofBRCA2mutation carriers | |||||||||||||
---|---|---|---|---|---|---|---|---|---|---|---|---|---|---|---|
py | Incident invasive BCs | IR per 1,000 py (95 % CI) | SIR (95% CI) | Cumulative risk,% (95% CI) | py | Incident invasive BCs | IR per 1,000 py (95 % CI) | SIR (95% CI) | Cumulative risk,% (95% CI) | py | Incident invasive BCs | IR per 1,000 py (95% CI) | SIR (95% CI) | Cumulative risk,% (95% CI) | |
Overall | 13,398.1 | 23 | 1.72 (1.16–2.66) | 0.93 (0.62–1.40) | NA | 7,738.7 | 12 | 1.55 (0.90–2.92) | 0.85 (0.48–1.50) | NA | 5,632.4 | 11 | 1.95 (1.11–3.79) | 1.03 (0.57–1.87) | NA |
Age group | |||||||||||||||
≥18 to <25 | 187.5 | 0 | 0 | 0 | 0 | 116.1 | 0 | 0 | 0 | 0 | 68.8 | 0 | 0 | 0 | 0 |
≥25 to <35 | 1,556.4 | 0 | 0 | 0 | 0 | 904.8 | 0 | 0 | 0 | 0 | 646.1 | 0 | 0 | 0 | 0 |
≥35 to <45 | 3,426.1 | 1 | 0.29 (-) | 0.35 (0.05–2.45) | 0.3 (0–1.8) | 2,114.1 | 0 | 0 | 0 | 0 | 1,312 | 1 | 0.76 (-) | 0.90 (0.13–6.42) | 0.7 (0.1–4.7) |
≥45 to <55 | 3,908.9 | 11 | 2.81 (1.59–5.47) | 1.30 (0.72–2.35) | 3 (1.7–5.3) | 2,157.6 | 4 | 1.85 (0.70–6.64) | 0.86 (0.32–2.30) | 1.8 (0.7–4.8) | 1,751.2 | 7 | 4.00 (1.95–9.52) | 1.85 (0.88–3.87) | 4.5 (2.3–8.8) |
≥55 to <65 | 2,574.4 | 6 | 2.33 (1.06–6.13) | 0.84 (0.38–1.87) | 5.5 (3.5–8.8) | 1,437.3 | 3 | 2.09 (0.65–10.2) | 0.75 (0.24–2.31) | 3.9 (1.8–8.2) | 1,137.1 | 3 | 2.64 (0.82–12.9) | 0.96 (0.31–2.97) | 7.7 (4.2–14) |
≥65 to <75 | 1,316 | 4 | 3.04 (1.14–10.9) | 0.89 (0.33–2.37) | 8.1 (5.2–12) | 754.7 | 4 | 5.3 (1.99–18.9) | 1.56 (0.59–4.16) | 8.4 (4.5–15) | 555.1 | 0 | 0 | 0 | 7.7 (4.2–14) |
≥75 to <85 | 428.8 | 1 | 2.33 (-) | 0.65 (0.09–4.59) | 9.4 (5.9–15) | 253.9 | 1 | 3.94 (-) | 1.09 (0.15–7.73) | 11 (5.6–19) | 162 | 0 | 0 | 0 | 7.7 (4.2–14) |
European ancestry | 13,184.4 | 23 | 1.74 (1.17–2.70) | 0.94 (0.63–1.42) | NA | 7,587.7 | 12 | 1.58 (0.91–2.98) | 0.87 (0.49–1.53) | NA | 5,569.6 | 11 | 1.97 (1.12–3.83) | 1.04 (0.58–1.88) | NA |
Incidence rates, SIRs, and cumulative risks are reported for the overall sample and by family mutation.
BC, breast cancer; CI, confidence interval; IR, incidence rate; NA, not applicable; py, person-years; SIR, standardized incidence ratio.
Risk of EOC
In the cohort of 1,736 noncarriers eligible for the EOC analysis, two incident EOCs were observed, both in individuals from BRCA2 families, with ages at diagnosis 44.8 and 56.1 years. The crude EOC incidence rate in the overall sample was 0.16 per 1,000 person-years (95% CI 0.03–1.66). The estimated SIR for EOC was 0.79 (95% CI 0.20–3.17) for all age groups. With only two incident EOCs, SIR estimates by age group and by family mutation were either not possible or associated with wide confidence intervals. They are not therefore reported. The estimated absolute risk of EOC in noncarriers was 0.6% (95% CI 0.2–2.6%) by age 85 years. In a sensitivity analysis that included women with a prior BC diagnosis in the eligible cohort, results were unchanged (Supplementary Material online).
Discussion
This is the largest prospective cohort study of BRCA1/BRCA2 predictive test negatives to date. We found no evidence of an increased BC or EOC risk in relatives of BRCA1 or BRCA2 mutation carriers. The BC risk estimates were not influenced by the inclusion of individuals with prior bilateral salpingo-oophorectomy. When the four noninvasive prospective BCs were also considered as events, to rule out the possibility that some cancers were being wrongly excluded, the SIR estimates were similar. Similarly, after censoring individuals at an earlier date (15 June 2014) to allow for possible risk underestimation due to delayed cancer notification, results were unchanged.
Early clinical recommendations on hereditary BC and EOC recommended standard surveillance for BRCA1/BRCA2 predictive test negatives.25 In 2013, the United States Preventive Services Task Force issued a recommendation reiterating that noncarriers were at population risk.26,27 According to the National Institute for Health and Care Excellence guidelines,6 women at population risk should be given standard surveillance and discussion of any further risk-reducing intervention would not be appropriate. If, however, BRCA1/BRCA2 predictive test negatives are at increased risk of developing BC, as recently suggested,19,20,21 the recommendations for women at moderate to high risk of developing BC may apply.
In five of the eight prospective studies published to date, the estimated SIR for BC was in line with our results (range of SIRs = 0.52–0.95) (refs.14,15,16,17,18). In three studies a significant two- to fivefold increased risk of BC was reported compared with population risks, but there were inconsistencies between these studies.19,20,21 Evans et al.19 found a statistically significant increased risk only for relatives of BRCA2 mutation carriers, while Vos et al.21 found a statistically significant increased risk only for relatives of BRCA1 mutation carriers. Both studies only included first-degree relatives of known mutation carriers. The authors argued that common genetic variants, which modify risks in BRCA1/BRCA2 carriers, also may modify risk in noncarriers. These predisposing variants would be more likely to segregate in families with multiple affected individuals, such as those ascertained in genetics clinics. Korde et al.17 and Nielsen et al.,18 however, did not find an increase in the risk of BC for BRCA predictive test negatives who were first-degree relatives of mutation carriers. A limitation of all these studies was the small sample size (none included more than 21 BC cases). In the present study we were not able to restrict analysis to only first-degree relatives of known mutation carriers because the exact familial relationships were not available. Similarly, we were not able to investigate the variation in risk by family history of cancer. Korde et al.17 reported a nonsignificant increase in the risk of BC for noncarriers with an affected first-degree relative. In Harvey et al.16 the estimated SIR of BC in predictive test negatives without affected relatives in the parental lineage not associated with the BRCA mutation was 0.48, albeit statistically not significant.
Only a few published studies provided a SIR for EOC (range of SIRs reported: 0–4.6) (refs.13,22) but all were based on retrospective studies. Three prospective studies15,20,21 aimed to estimate a SIR for EOC. In Domchek et al.15 and Rowan et al.20 no events occurred during the follow-up, while Vos et al.21 reported two EOCs but the corresponding SIR was not provided. This is the first study to estimate a SIR for EOC based on a prospective cohort, but the confidence intervals were wide due to the small number of events.
The sample size of this study is larger than previous studies and the confidence limits are correspondingly narrower. Nonetheless, when considering BC risk estimates by age group and family mutation, caution is needed due to the relatively small number of events in each stratum. Because this is a prospective cohort, estimates are less likely to be prone to ascertainment or reporting biases, usually associated with retrospective or historical cohort studies.
Limitations of this study include the following:
The SIRs were calculated using incidences from England, but EMBRACE noncarriers were also recruited in Scotland and Wales. Age-specific estimates for these countries were not readily available; however, data from previous periods indicate that the incidence rates are similar amongst countries. Moreover, the large majority of study participants (83.3%) were from clinics based in England.
Surgeries unrelated to cancer diagnoses prior to recruitment were not verified through surgical records, but bias due to misreporting or underreporting was probably small given the life-changing sexual and physical impact of risk-reducing surgery.28,29,30
No information on prophylactic surgeries after recruitment was available. Such surgeries are unlikely in women testing negative for mutations; however, if risk-reducing surgeries are more frequent in the noncarriers within families with BRCA1 and BRCA2 mutations compared with the general population this may lead to an underestimation of the SIR. In an approximate calculation, assuming the same proportion (i.e., 0.88%) of bilateral mastectomies in the prospective cohort as in the retrospective data, 17 such procedures would be expected. In the unlikely event that all these individuals would have developed invasive BC if they had not undergone surgery, the observed/expected ratio would have been 1.61 (95% CI 1.18–2.2). In the retrospective data, 5.4% of noncarriers from BRCA1 families had undergone bilateral oophorectomy with or without bilateral salpingectomy, compared with 3.3% of noncarriers from BRCA2 families, possibly reflecting differential counseling toward risk-reducing surgery when a BRCA1 mutation segregates in the family. In the current sample, 98% of noncarriers from BRCA1 families who underwent bilateral oophorectomy (or bilateral salpingectomy) at baseline had the procedure before genetic testing, whereas only 3% underwent RRSO after notification of the negative result. If the uptake of RRSO (after notification of mutation carrier status) was similar in the prospective cohort, this may have led to some underestimation of the EOC SIR for relatives of BRCA1 mutation carriers and in the overall sample. However, the size of these biases is most likely small because risk-reducing bilateral mastectomy and RRSO after the disclosure of a negative result are less likely.
The noncarrier’s degree of relationship with the mutation carrier and cancer family history were not available. Although women were ascertained through clinical genetics centers and most would have come from high-risk families, ascertainment criteria with respect to family history can vary. Therefore, it is not possible to rule out that risk in noncarriers may be increased if multiple family members or first-degree relatives are affected.
No information on the date of the most recent screening mammogram or breast magnetic resonance imaging was available. If BRCA1/BRCA2 predictive test negatives with a normal breast imaging close to the genetic test discontinue surveillance following the notification of noncarrier status, they may be subject to a reverse lead time effect if they are diagnosed with a BC and this may lead to some underestimation of the risk. We investigated this by calculating the BC incidence in 3-year intervals following the genetic test. Although there was a suggestion of a higher BC incidence rate between 3 and 6 years following the genetic test compared with the initial years, the differences were not significant. Larger sample sizes will be required to clarify this potential bias.
Although this is the largest prospective study, the mean follow-up time in the cohort was still relatively short (7.1 years) and longer follow-up will be required to investigate the risks at older ages with more precision.
Based on the confidence interval of the invasive BC SIRs, a 1.5-fold increase in risk in noncarriers from BRCA1 families and a 1.9-fold increase in noncarriers from BRCA2 families cannot be ruled out. Translating these SIRs to lifetime risk yields an upper bound of risk of ~17% to age 80 years for relatives of BRCA1 mutation carriers and ~20% to age 80 years for relatives of BRCA2 mutation carriers, based on UK general population incidences.31 Hence, even at the upper bound of the 95% CI, BRCA1/BRCA2 predictive test negatives would not be classified as being at high risk of developing invasive BC according to the National Institute for Health and Care Excellence guidelines.6
The familial aggregation of BC is known to be determined by other factors, including multiple common genetic variants, in addition to BRCA1 and BRCA2 mutations. Thus, one would predict that BRCA1/BRCA2 predictive test negatives in cohorts such as the present study, who have a family history of BC and are hence more likely to carry other predisposing variants, would still be at increased risk relative to general population. We therefore investigated whether the present estimates are consistent with predictions given by the Breast and Ovarian Analysis of Disease Incidence and Carrier Estimation Algorithm (BOADICEA) model, which models the familial aggregation of BC in terms of BRCA1/2 mutation status and a residual polygenic component. We computed the predicted lifetime risk of BC for a 20-year-old true negative, with two different family histories: (i) a mutation-positive mother diagnosed with BC at age 50 years, and (ii) a mother and maternal grandmother both diagnosed with BC at age 50 and carrying a mutation. The predicted BC risks to age 80 years in these two scenarios were 12 and 13% for a BRCA1 positive family, and 14 and 15% for a BRCA2 positive family. These women would be classified as at near population risk according to BOADICEA. Nevertheless, the predicted risks are somewhat higher than the point estimates in the present study, but within or close to the upper confidence interval bounds of the estimated cumulative risks. These observations suggest that the BOADICEA model may overestimate slightly the risks to individuals with a negative predictive test. However, larger sample sizes will be required to resolve this issue: if the true risks were in line with those predicted by BOADICEA, a prospective study with at least 100 events would be required to provide sufficient statistical power.
Our results suggest that BRCA1/BRCA2 predictive test negatives can be classified as being at near-population risk as defined by the National Institute for Health and Care Excellence guidelines.6 Therefore, it would not be appropriate to offer risk-reducing bilateral mastectomy and RRSO to these individuals. In practice a proportion of women undergo preventative surgery based solely on the family history. Based on these data, predictive genetic testing of female relatives of a known BRCA1/BRCA2 mutation carrier is strongly beneficial in terms of avoiding unnecessary surgical procedures for those found to be BRCA1/BRCA2 negative. Standard surveillance may be offered, unless personal risk factors warrant further consideration such as strong family history of cancer in the parental lineage not associated with the known mutation or history of lobular carcinoma in situ or atypical ductal hyperplasia.32,33
Electronic supplementary material
Acknowledgments
This work was supported by Cancer Research–UK grants C12292/A20861, C1287/A10118, C1287/A11990, C1287/A23382, C1287/A17523, and C1287/A16563.
Disclosure
D.E. has received honoraria from AstraZeneca and has reported consulting or advisory role in AstraZeneca. The other authors declare no conflict of interest.
Electronic supplementary material
Supplementary material is linked to the online version of the paper 10.1038/gim.2018.44
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