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. 2015 Oct 8;15(1):49–55. doi: 10.1111/acel.12407

Copy number variation associates with mortality in long‐lived individuals: a genome‐wide assessment

Marianne Nygaard 1,2,, Birgit Debrabant 1, Qihua Tan 1,2, Joris Deelen 3, Karen Andersen‐Ranberg 1, Anton JM de Craen 4, Marian Beekman 3, Bernard Jeune 1, Pieternella E Slagboom 3, Kaare Christensen 1,2,5, Lene Christiansen 1
PMCID: PMC4717275  PMID: 26446717

Summary

Copy number variants (CNVs) represent a significant source of genetic variation in the human genome and have been implicated in numerous diseases and complex traits. To date, only a few studies have investigated the role of CNVs in human lifespan. To investigate the impact of CNVs on prospective mortality at the extreme end of life, where the genetic component of lifespan appears most profound, we analyzed genomewide CNV data in 603 Danish nonagenarians and centenarians (mean age 96.9 years, range 90.0–102.5 years). Replication was performed in 500 long‐lived individuals from the Leiden Longevity Study (mean age 93.2 years, range 88.9–103.4 years). First, we assessed the association between the CNV burden of each individual (the number of CNVs, the average CNV length, and the total CNV length) and mortality and found a significant increase in mortality per 10 kb increase in the average CNV length, both for all CNVs (hazard ratio (HR) = 1.024, P = 0.002) and for duplications (HR = 1.011, P = 0.005), as well as per 100 kb increase in the total length of deletions (HR = 1.009, P = 0.0005). Next, we assessed the relation between specific deletions and duplications and mortality. Although no genome–wide significant associations were discovered, we identified six deletions and one duplication that showed consistent association with mortality in both or either of the sexes across both study populations. These results indicate that the genome–wide CNV burden, specifically the average CNV length and the total CNV length, associates with higher mortality in long‐lived individuals.

Keywords: aging, copy number variation, deletions, genetics, long‐lived individuals, mortality

Introduction

Human lifespan is a complex trait with a moderate heritability of around 25% (Herskind et al., 1996). So far, only a limited number of loci have been consistently associated with length of life (Murabito et al., 2012; Deelen et al., 2014), and hence much of the heritability is still unaccounted for. This missing heritability might in part be explained by copy number variants (CNVs) (Manolio et al., 2009).

Copy number variants are defined as DNA segments larger than 1 kb in size that vary in copy number between individuals due to insertion, deletion, or duplication (Feuk et al., 2006a). The mechanisms by which CNVs can affect gene expression and phenotypic traits include alteration of gene dosage and disruption of coding sequences or regulatory elements (Feuk et al., 2006b). CNVs have been implicated in numerous diseases and complex traits, like schizophrenia (International Schizophrenia C, 2008), autism (Marshall et al., 2008), and obesity (Wheeler et al., 2013), but only a few studies have addressed the role of CNVs in survival and longevity.

The first study of CNVs related to human lifespan was performed by Kuningas et al. (2011), who prospectively studied 11 442 individuals with an intake age of 34.0–75.3 years and found that carriers of a higher burden of common deletions larger than 500 kb had a marginally increased risk of mortality [hazard ratio (HR) = 1.04] compared to noncarriers. They also identified two common CNV regions (CNVRs) on chromosome 11p15.5 and 14q21.3 that associated with higher mortality at old age. Next, Glessner and colleagues compared CNV frequencies between 7313 pediatric (aged 0–18 years) and 2701 geriatric individuals (aged > 67 years, mean age 76 years) with replication in 2079 children (mean age 8.6 years) and 4692 elderly adults (mean age 60 years). In total, they identified three deletions and four duplications that were significantly enriched in the pediatric individuals and that primarily encompassed genes involved in RNA splicing, suggesting an impact of this biological mechanism on lifespan (Glessner et al., 2013). Recently, an analysis of the association between 20 common CNVs not typically covered by commercial arrays and longevity in 222 senior American Caucasians with replication in 1283 community‐dwelling senior European Caucasians resulted in the identification of a deletion in the neurexin superfamily member CNTNAP4 on chromosome 16q23.1 that was inversely associated with survival to 80 years in women (Iakoubov et al., 2013). Further investigation of CNVs in other gene members of the neurexin superfamily by the same group additionally led to the detection of a CNV in the CNTNAP2 gene on chromosome 7q35‐36.1 that negatively associated with healthy aging in octogenarian men (Iakoubov et al., 2015).

None of the studies performed so far have focused on the impact of CNVs on mortality at the extreme end of life. Here, we explored this by analyzing the association between the CNV burden of each individual and prospective mortality, as well as between specific deletions and duplications and prospective mortality in long‐lived individuals of Danish descent (DKLS, mean age 96.9 years, range 90.0–102.5 years). The long‐lived individuals are all older than 90 years, and they thus represent the age group where the influence of genetic factors on survival is likely to be most profound (Hjelmborg et al., 2006). Suggestive findings were replicated in a second population of long‐lived individuals from the Leiden Longevity Study (LLS, mean age 93.2 years, range 88.9–103.4 years), and, in addition, a joint analysis of these findings was performed.

Results

The characteristics of the discovery study (DKLS) and the replication study (LLS) populations are summarized in Table 1.

Table 1.

Study population characteristics

Discovery study (DKLS) Replication study (LLS)
N, total 603 500
N, women (%) 453 (75.1%) 302 (60.4%)
Mean age at baseline (range) 96.9 (90.0–102.5) 93.2 (88.9–103.4)
Mean follow‐up time (range) 2.9 (0.01–12.9) 4.1 (0.02–11.5)
N, deaths (%) 521 (86.4%) 457 (91.4%)
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Applying a Bonferroni‐corrected significance level of 0.006, the analysis of the CNV burden of each individual revealed a significant association between a longer average CNV length and increased mortality. In the joint analysis including both the DKLS and the LLS, this was evident for the combined group of CNVs where we detected an increase in HR of 2.4% per 10 kb increase in the average CNV length (HR = 1.024, P = 0.002) as well as for duplications only (HR = 1.011, P = 0.005) (see Table 2). In addition, we observed a significant increase in mortality as a result of a greater part of the genome being occupied by deletions with the HR increasing 0.9% per 100 kb increase in the total length of deletions (HR = 1.009, P = 0.0005).

Table 2.

Association between the copy number variant (CNV) burden of each individual and mortality

All CNVs Deletions Duplications
HR (95% CI) P HR (95% CI) P HR (95% CI) P
Number of CNVsa Discovery study (DKLS) 0.991 (0.919–1.068) 0.811 1.049 (0.957–1.150) 0.307 0.917 (0.814–1.034) 0.158
Replication study (LLS) 1.001 (0.928–1.080) 0.997 1.163 (0.959–1.409) 0.124 0.985 (0.912–1.063) 0.697
Joint analysis 0.996 (0.944–1.050) 0.879 1.069 (0.984–1.162) 0.113 0.965 (0.905–1.029) 0.275
Average CNV lengthb Discovery study (DKLS) 1.025 (1.009–1.041) 0.002 1.015 (1.002–1.027) 0.023 1.011 (1.003–1.020) 0.008
Replication study (LLS) 1.012 (0.963–1.062) 0.644 1.007 (0.980–1.035) 0.598 1.009 (0.977–1.042) 0.597
Joint analysis 1.024 (1.009–1.039) 0.002 1.014 (1.003–1.025) 0.013 1.011 (1.003–1.019) 0.005
Total CNV lengthc Discovery study (DKLS) 1.006 (0.998–1.015) 0.146 1.011 (1.000–1.023) 0.050 1.001 (0.989–1.014) 0.814
Replication study (LLS) 1.004 (0.993–1.015) 0.523 1.009 (1.004–1.014) 0.001 0.999 (0.985–1.014) 0.911
Joint analysis 1.005 (0.999–1.012) 0.107 1.009 (1.004–1.015) 0.0005 1.000 (0.991–1.009) 0.973
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HR, hazard ratio; 95% CI, 95% confidence interval; P, P‐value obtained from a Cox proportional hazard regression adjusted for study relevant covariates or from the joint analysis.

The P‐value is not adjusted for multiple testing. Joint analysis P‐values ≤ 0.006 are shown in bold.

a

Results are per additional 10 CNVs.

b

Results are per additional 10 kb.

c

Results are per additional 100 kb.

Altogether, a total of 272 unique deletions and 131 unique duplications were identified in the DKLS. This distribution of deletions and duplications is unlikely to reflect the actual distribution of CNVs in the human genome and rather represents a detection bias associated with the sensitivity of the CNV detection algorithm used (Zheng et al., 2012). In the association analysis, none of the CNVs reached statistical significance after correcting for multiple testing. However, when using a nominal significance level of P ≤ 0.05, 20 CNVs were found to associate with mortality (see Table 3), and they were thus selected for replication in the LLS. In the joint analysis including both study populations, the association with mortality was consistent for three deletions located on chromosome 6q14.1 (HR 1.35, 95% CI 1.04–1.74, P = 0.023), 10p13 (HR 1.67, 95% CI 1.05–2.66, P = 0.031), and 13q13.2 (HR 1.43, 95% CI 1.07–1.91, P = 0.015) and one duplication located on chromosome 9q21.12 (HR 1.55, 95% CI 1.07–2.25, P = 0.021). All of these CNVs were found to contribute to a higher mortality in carriers compared to noncarriers. Furthermore, sex‐specific analyses (see Table S1 and S2, Supporting Information) revealed three additional deletions on chromosome 1p22.3, 5q31.3, and 8p22 that resulted in higher mortality among carriers in one of the sexes.

Table 3.

Association between specific deletions and duplications and mortality

Discovery study (DKLS) Replication study (LLS) Joint analysis
Copy number varianta Locus Type Size (kb) Freq. (%) HR (95% CI) P Freq. (%) HR (95% CI) P HR (95% CI) P
Chr2:18327703‐18351537 2p24.2 DUP 23.8 1.3 3.48 (1.62–7.45) 0.001 1.2 0.85 (0.52–1.38) 0.512 1.28 (0.85–1.94) 0.239
Chr9:9516348‐9526811 9p23 DUP 10.5 1.0 3.30 (1.45–7.53) 0.005 NA NA NA NA NA
Chr13:32896846‐32922331 13q13.1 DEL 25.5 1.3 2.80 (1.30–6.03) 0.009 NA NA NA NA NA
Chr1:80982632‐81056073 1p31.1 DUP 73.4 1.0 2.97 (1.29–6.80) 0.010 NA NA NA NA NA
Chr6:55828727‐55846527 6p12.1 DEL 17.8 3.3 1.83 (1.14–2.95) 0.012 NA NA NA NA NA
Chr10:13055619‐13058458 10p13 DEL 2.8 2.0 2.08 (1.17–3.72) 0.013 1.2 1.15 (0.53–2.47) 0.729 1.67 (1.05–2.66) 0.031
Chr6:29855945‐29909559 6p22.1 DEL 53.6 11.8 1.38 (1.06–1.79) 0.015 5.0 0.87 (0.55–1.39) 0.565 1.24 (0.99–1.56) 0.057
Chr9:73902148‐73909871 9q21.12 DUP 7.7 1.8 2.05 (1.12–3.75) 0.020 4.0 1.31 (0.81–2.10) 0.272 1.55 (1.07–2.25) 0.021
Chr8:8583109‐8589783 8p23.1 DEL 6.7 1.5 2.18 (1.12–4.26) 0.022 1.0 0.93 (0.23–3.75) 0.918 1.87 (1.02–3.43) 0.042
Chr8:30990110‐31000860 8p12 DEL 10.8 1.0 2.60 (1.14–5.94) 0.023 NA NA NA NA NA
Chr13:34115595‐34143545 13q13.2 DEL 28.0 7.8 1.45 (1.05–2.00) 0.023 2.6 1.32 (0.64–2.70) 0.453 1.43 (1.07–1.91) 0.015
Chr15:102028468‐102305129 15q26.3 DUP 276.7 1.0 2.52 (1.12–5.69) 0.026 NA NA NA NA NA
Chr20:36051525‐42681088 20q11.23, 20q12, 20q13.11, 20q13.12 DEL 6629.6 1.8 0.45 (0.22–0.91) 0.026 1.0 0.89 (0.47–1.70) 0.729 0.65 (0.40–1.05) 0.079
Chr7:118006251‐118070496 7q31.31 DEL 64.2 1.0 2.69 (1.11–6.56) 0.029 NA NA NA NA NA
Chr6:31275246‐31285292 6p21.33 DEL 10.0 2.8 1.76 (1.05–2.96) 0.032 2.4 1.02 (0.67–1.56) 0.923 1.27 (0.92–1.74) 0.150
Chr13:88960710‐89033066 13q31.2 DEL 72.4 1.0 2.38 (1.06–5.37) 0.036 NA NA NA NA NA
Chr22:18844632‐19016663 22q11.21 DUP 172.0 1.3 2.11 (1.04–4.28) 0.039 NA NA NA NA NA
Chr1:161490896‐161617516 1q23.3 DUP 126.6 1.8 0.48 (0.23–0.98) 0.043 1.4 2.60 (1.35–5.04) 0.004 1.17 (0.72–1.90) 0.520
Chr6:77439969‐77448731 6q14.1 DEL 8.8 6.5 1.42 (1.01–2.00) 0.046 4.4 1.27 (0.88–1.84) 0.194 1.35 (1.04–1.74) 0.023
Chr13:82081150‐82087510 13q31.1 DEL 6.4 1.0 2.28 (1.01–5.14) 0.048 NA NA NA NA NA
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a

Copy number variant (CNV), The discovery study CNV position with information about chromosome and start and stop base pair positions based on the GRCh37/hg19 genome build; Freq., frequency; HR, hazard ratio; 95% CI, 95% confidence interval; P, P‐value obtained from a Cox proportional hazard regression adjusted for study relevant covariates or from the joint analysis.

The P‐value is not adjusted for multiple testing. Joint analysis P‐values ≤ 0.05 for variants showing the same direction of effect in the discovery and replication studies are shown in bold. NA, not applicable due to a frequency lower than 1% in the replication study.

The seven nominally significant CNVs have all, at least partially, been reported by the Database of Genomic Variants (DGV, http://dgv.tcag.ca/dgv/app/home; Macdonald et al., 2014), supporting that they represent true findings. They encompass or are positioned nearby a number of genes: COL24A1, PCDHA1PCDHA10, IMPG1, IRAK1BP1, PSD3, TRPM3, TMEM2, CCDC3, and STARD13 (see Table S3). These genes are significantly enriched for several Gene Ontology (GO) terms related to cell adhesion (hemophilic cell adhesion via plasma membrane adhesion molecules, cell–cell adhesion via plasma membrane adhesion molecules, cell–cell adhesion, cell adhesion, and biological adhesion) as well as for the GO term nervous system development. However, when limiting the contribution of the 10 PCDHA genes by including only one of them in the enrichment analysis, no GO terms are significantly over‐ or underrepresented. In addition to genes, the 5q31.3, 8p22, and 13q13.2 deletions all include CpG islands and regions with indications of active regulatory elements. The 5q31.3 deletion also contains a number of eQTLs consisting of single nucleotide polymorphisms (SNPs) that show association with the expression of the WDR55 and ARL4A genes, primarily in brain tissue.

Discussion

In this study, we explored the impact of copy number variation on mortality at the extreme end of life by performing a genome‐wide investigation of the association between CNVs and prospective mortality in nonagenarians and centenarians.

As our main result, we found that an increase in the average CNV length significantly associated with a higher mortality, as did an increase in the total part of the genome occupied by deletions (see Table 2). These findings are consistent with the results of a previous study in which the burden of large deletions was found to be associated with higher mortality (Kuningas et al., 2011), suggesting that longer CNVs, especially deletions, are more disadvantageous. The identified association between a higher CNV burden and increased mortality is generally in line with the proposed role of genome instability, that is, a decrease in genome maintenance and hence an accumulation of genomic changes, in lifespan (Vijg & Suh, 2013) and suggests that even among the very old, the load of genomic alterations is linked to differences in mortality.

Among the specific deletions and duplications, three deletions on chromosome 6q14.1, 10p13, and 13q13.2 and one duplication on chromosome 9q21.12 were consistently associated with higher mortality across the DKLS and LLS populations (see Table 3), as were a deletion on chromosome 5q31.3 in women (see Table S1) and two deletions on chromosome 1p22.3 and 8p22 in men (see Table S2). These seven nominally significant CNVs are surrounded by numerous genes (see Table S3), of which two, TRPM3 and STARD13, have previously been implicated in the regulation of human lifespan (Lunetta et al., 2007; Yashin et al., 2010). The STARD13 gene has moreover been associated (P ≤ 1 × 10−5) with plasma levels of amyloid beta peptides that, among other things, play a role in Alzheimer's disease and hypertension (Chouraki et al., 2014). In addition, also the CCDC3 and IRAK1BP1 genes could be speculated to play a role in human lifespan, as they have been reported to inhibit inflammation (Conner et al., 2008, 2010; Azad et al., 2014), and as revealed by the GO enrichment analysis, the majority of the other genes are involved in cell adhesion, which has previously been linked to longevity and age‐related diseases (Wolfson et al., 2009; Tian et al., 2013).

In addition to their more direct effect on genes, for example, alteration of gene dosage and gene disruption, CNVs may also affect regulatory regions or other functional regions that influence gene expression, and CNVs have indeed been reported to exert their effect over distances of more than 6 Mb (Stranger et al., 2007). Only a few of the seven CNVs found to potentially associate with mortality in long‐lived individuals in this study contain known regulatory elements. The CNVs harboring these elements additionally overlap or include genes, and especially the 5q31.3 region, which includes the genes PCDHA1‐PCDHA10, contains a substantial number of CpG islands. The eQTL analysis revealed that this region also affects the expression of the WRD55 and ARL4A genes, primarily in brain tissue. Epigenetic changes in ARL4A have previously been found to associate with maternal longevity in an epigenome‐wide association study of age and age‐related phenotypes (Bell et al., 2012), indicating a possible link between the 5q31.3 deletion and longevity.

A number of genes known to be of interest for longevity are included in the CNVs associated with mortality in the DKLS. For instance, a deletion in WRN is found to be associated with higher mortality. The WRN gene encodes a RecQ DNA helicase involved in DNA replication and repair, transcription, and telomere maintenance (Rossi et al., 2010). Deleterious mutations in this gene give rise to the premature aging syndrome Werner, and genetic variation in WRN has previously been associated with longevity (Soerensen et al., 2012). Also worth highlighting are the genes SGK2, which is part of the insulin/insulin‐like growth factor 1 (IGF‐1) pathway and has been implicated in human longevity (Deelen et al., 2013), and BRCA2 that is involved in DNA double‐strand break repair (Jensen, 2013) and has been found to play a role in the lifespan of mice (Donoho et al., 2003). These CNVs were, however, not attempted replicated, due to a very low frequency (below 1%) in the LLS sample.

Two studies have recently investigated the potential impact of CNVs on survival and longevity in a genome‐wide manner (Kuningas et al., 2011; Glessner et al., 2013). We did not find any overlap in results between our study and the study by Glessner and co‐workers. However, as this study is a case–control study comparing elderly individuals, primarily in their sixties and seventies, with young individuals under the age of 19, and as the significantly associated CNVs identified were enriched only in the pediatric individuals, a lack of overlap could be expected. In contrast, we saw a minor overlap, although only in sex‐specific analyses, of two CNVs with the study by Kuningas and colleagues, which is the only other longitudinal study on CNVs and mortality published so far. The overlapping CNVs are a duplication on chromosome 14q32.33 and a deletion on chromosome 14q21.2. Due to the use of a different genome build, the 14q21.2 region is reported as 14q21.3 by Kuningas and co‐workers. In both instances, the direction of effect is the same, that is, for the 14q21.2 deletion HR > 1 and for the 14q32.33 duplication HR < 1, which further supports a role for these genetic variations in mortality during old age.

There are a number of possible explanations for the modest agreement between our study and the study by Kuningas and co‐workers. For one, the intake age range of the populations included in the two studies is different (88.9–103.4 years vs. 34.0–75.3 years, respectively). This means that while Kuningas and colleagues focus on mortality from middle age to old age, our study investigates mortality at very advanced ages. Thus, we explore the possible significance of CNVs in individuals belonging to the age group where the genetic component of longevity has been suggested to be most profound and hence more profound that at younger ages (Hjelmborg et al., 2006). In agreement with this, it has previously been shown that the association between the APOE ε4 risk allele and mortality increases with higher ages, even after the age of 100 (Jacobsen et al., 2010). Additionally, the advanced age of our study population means that a larger part of the individuals included in our study died during follow‐up, which results in a relatively high number of events and limits the potential bias associated with censoring. Other parameters affecting the ability to replicate initial findings could be related to differences in sample size and genetic background, the use of different platforms and CNV detection algorithms as well as potential technical and random errors. Compared to the study by Kuningas and colleagues, our sample size is smaller, and our power to detect CNVs with lower effect sizes is therefore reduced. However, despite our smaller sample size, we still detect a higher number of CNVRs (403 vs. 312). Although these numbers are not entirely comparable due to the use of different methods for defining the CNVRs, this difference is likely to partly reflect their use of an array containing a lower number of SNPs, and hence with a lower resolution, than ours.

In conclusion, we found that the genomewide CNV burden, specifically the average CNV length and the total CNV length, associates with higher mortality in long‐lived individuals. Our results indicate that CNVs might be important contributors to the genetic component of human longevity and prompt further investigation.

Experimental procedures

Study populations

Discovery study

The discovery study population, also referred to as the Danish Longevity Study (DKLS), consisted of participants drawn from the Longitudinal Study of Danish Centenarians (LSDC), the 1905 Birth Cohort Study, the 1911–12 Birth Cohort Study, the Study of Danish Old Sibs (DOS), and the Longitudinal Study of Ageing Danish Twins (LSADT). Briefly, the LSDC and the Danish 1905 Birth Cohort Study are prospective follow‐up studies initiated when participants were 100 and 92 years of age, respectively (Andersen‐Ranberg et al., 2001; Nybo et al., 2001), the Danish 1911–12 Birth Cohort Study (Robine et al., 2010; Vestergaard et al. 2015) consists of individuals attaining the age of 100 in the period from May 5th, 2011 to July 5th, 2012, DOS was initiated in 2004 and includes families in which at least two siblings were ≥ 90 years of age at intake, and LSADT was initiated in 1995 and includes Danish twins ≥ 70 years of age (Skytthe et al., 2002).

From DOS and LSADT, one individual from each sib‐ship or twin pair was selected among participants that had reached an age of at least 91 years for DOS and 90 years for LSADT. From the 1905 Birth Cohort Study, participants were selected among individuals reaching an age of minimum 96 years. To avoid immortal follow‐up time, individuals from DOS, LSADT, and the 1905 Birth Cohort Study were followed from age 91, 90, and 96 onwards.

Replication study

The replication study population consisted of nonagenarian individuals from the LLS. In the LLS, long‐lived siblings of European descent were recruited together with their offspring and the spouses of the offspring. Families were included if at least two long‐lived siblings were alive and fulfilled the age criterion of 89 years or older for men and 91 years or older for women, representing < 0.5% of the Dutch population in 2001 (Schoenmaker et al., 2006). In total, 944 long‐lived proband siblings (mean age 94 years, range 89–104 years), 1671 offspring (mean age 61 years, range 39–81 years), and 744 offspring partners (mean age 60 years, range 36–79 years) were included. Here, only long‐lived probands (N = 500), who were previously genotyped using Illumina HumanOmniExpress BeadChips (Illumina Inc., San Diego, CA, USA), were included.

Vital status was followed until death, January 1st, 2014 (in the DKLS), or February 1st, 2014 (in the LLS), whichever came first. Information on survival status was retrieved from the Danish (Pedersen et al., 2006) and Dutch Central Population Registers.

In the DKLS, permissions to collect blood samples and the use of register‐based data were granted by the Danish National Committee on Biomedical Research Ethics. The LLS was approved by the Medical Ethical Committee of the Leiden University Medical Center, and all participants gave written informed consent.

Genotyping and quality control

In the DKLS, DNA was isolated from whole blood using standard methods (Miller et al., 1988) and genotyping was carried out according to the manufacturer's protocol using the Illumina HumanOmniExpress BeadChips (Illumina Inc.) (Deelen et al., 2014), which contains 730 525 SNP markers with a median spacing of 2.1 kb and a mean spacing of 4.0 kb.

Quality control (QC) was performed in Plink (http://pngu.mgh.harvard.edu/~purcell/plink/; Purcell et al., 2007) and samples were evaluated and excluded based on call rate (call rate < 98.5%), inconsistencies between genotypic and phenotypic sex, and family relationships (proportional IBD > 0.1875). Of the 673 originally included samples, 662 samples remained after the genotype‐based QC.

CNV detection and QC

Copy number variants were detected on autosomes only using the PennCNV software (Wang et al., 2007). The hidden Markov model implemented in PennCNV incorporates multiple sources of information, including the total signal intensity [log R ratio (LRR)] and the allelic intensity ratio [B allele frequency (BAF)] of each SNP marker, the distance between the SNPs, and the population frequency of the B allele (PFB) of SNPs. LRR and BAF values were exported from GenomeStudio (Illumina Inc.) and the PFB file was compiled from the DKLS samples based on the BAF of each marker.

After CNV detection, samples with a LRR standard deviation > 0.30 were excluded, as were samples with more than 100 CNVs called and samples with a GC wave factor above 0.05 or below −0.05. Altogether, 59 samples were excluded, resulting in the inclusion of 603 DKLS samples in the final analysis.

Copy number variants were excluded if they were < 1 kb in size or contained < 3 consecutive SNPs indicating a deletion or a duplication.

Generation of CNV datasets

Data on CNV burden, that is, the number of CNVs, the average CNV length, and the total CNV length, were retrieved for each individual using Plink (http://pngu.mgh.harvard.edu/~purcell/plink/; Purcell et al., 2007).

The data on specific deletions and duplications were constructed by merging CNVs of the same state [either deletion (state 0 or 1) or duplication (state 3 or 4)] if they overlapped by at least 50% of the length of the shorter CNV. The outermost boundaries of the merged regions were used to define the CNVs.

Copy number variants overlapping centromeres or telomeres (as defined by UCSC (http://genome.ucsc.edu/) using the Table Browser Software (Karolchik et al., 2004) and the GRCh37/hg19 genome build) were excluded, as were CNVs with a frequency < 1%.

Replication of CNV associations

Copy number variants of the same state overlapping nominally significant findings from the discovery study were evaluated for association with mortality in the LLS individuals (N = 500), who were previously genotyped using the same SNP array as in the DKLS (Illumina HumanOmniExpress BeadChips; Illumina Inc.).

DNA from the LLS was isolated from white blood cells using conventional methods (Beekman et al., 2006). To ensure a high comparability between the DKLS and the LLS, genotyping and CNV detection in the LLS were carried out as described for the DKLS with only minor differences. In the genotype‐based QC, samples were excluded based on a call rate < 95% and no evaluation of family relationships was performed. For the CNV detection, a standard PFB file (OmniExpress_hg19.pfb.new), available on the PennCNV website (http://www.openbioinformatics.org/penncnv/), was used. In addition, a modified GC‐model file based on hg19 was included.

Statistical analysis

All survival analyses were carried out using the statistical software Stata (Stata version 13.1; Stata Corporation, College Station, TX, USA) by applying a left‐truncated Cox proportional hazard regression model adjusted for sex, age at baseline, birth cohort (in the DKLS only), and familial relations (in the LLS only). The adjustment for birth cohort in the DKLS was included in order to account for any confounding due to differences in survival probability between the birth cohorts, which has been shown to be important in genetic studies (Nygaard et al., 2014). The adjustment was carried out by including a categorical variable based on 10‐year birth year intervals in the model.

The joint analysis was performed in Plink (http://pngu.mgh.harvard.edu/~purcell/plink/; Purcell et al., 2007) as a meta‐analysis using a fixed‐effect approach. The HRs and the corresponding standard errors were calculated within each study and combined to obtain a joint analysis HR and P‐value. The 95% confidence intervals of the joint analysis HRs were calculated using R (http://www.r-project.org/).

In the CNV burden analysis, the association between the number of CNVs, the average CNV length, and the total CNV length of each individual and mortality was analyzed for all CNVs as well as for deletions only and duplications only in the DKLS, in the LLS, and in a joint analysis including the two populations. Given that the total CNV length is more or less the product of the number of CNVs and the average CNV length, that ‘all CNVs’ is made up of deletions and duplications, and that the joint analysis includes the DKLS and the LLS, a Bonferroni‐corrected significance level of P ≤ 0.006 was applied. This corresponds to the correction for eight tests, that is, assessing the association between the number of CNVs and the average CNV length of each individual and mortality for deletions only and duplications only in the DKLS and in the LLS.

In the association analysis of specific deletions and duplications and mortality, a P‐value ≤ 1.2 × 10−4 (0.05/403) was used as the cutoff for statistical significance. CNVs associated with mortality with a P‐value lower or equal to 0.05 were considered suggestive associations and were attempted replicated as well as included in the joint analysis.

Gene ontology enrichment analysis and expression quantitative trait loci (eQTL) analysis

The biological processes associated with the genes encompassed by or surrounding the CNVs found to suggestively associate with mortality in the DKLS and the LLS in both genders combined or in women or men only was assessed using the GO enrichment analysis tool offered by the GO Consortium (http://geneontology.org/page/go-enrichment-analysis).

The potential effects on gene expression of SNPs in the CNVs suggestively associated with mortality were examined using the Genotype‐Tissue Expression (GTEx) eQTL database (http://www.ncbi.nlm.nih.gov/gtex/GTEX2/gtex.cgi), which is based on expression data of brain (cerebellum, frontal cortex, temporal cortex, and pons), liver, and lymphoblastoid cell lines.

Funding

This study was financially supported by the INTERREG 4 A programme Syddanmark‐Schleswig‐K.E.R.N (with EU funds from the European Regional Development Fund), the European Union's Seventh Framework Programme (FP7/2007‐2011) under grant agreement no. 259679, the VELUX Foundation, The National Program for Research Infrastructure 2007 (grant no. 09‐063256) from the Danish Agency for Science Technology and Innovation, the US National Institute of Health (P01AG08761), the Danish Agency for Science, Technology and Innovation/The Danish Council for Independent Research (grant no. 11‐107308), and The Danish Interdisciplinary Research Council. The 5‐COOP project (5‐Country Oldest Old Project) is funded by the CERA Foundation (Lyon) and the AXA Research Fund, Paris, and The Health Foundation (Helsefonden), Copenhagen, Denmark. The LLS was supported by a grant from the Innovation‐Oriented Research Program on Genomics (SenterNovem IGE05007), the Centre for Medical Systems Biology, the Netherlands Consortium for Healthy Ageing (grant 050‐060‐810), and the Biobank‐Based Integrative Omics Studies (BIOS) Consortium funded by BBMRI‐NL, a research infrastructure financed by the Dutch government (NWO 184.021.007), all in the framework of the Netherlands Genomics Initiative, Netherlands Organization for Scientific Research (NWO).

Conflict of interest

The authors declare no conflict of interest.

Author contributions

Marianne Nygaard contributed to generation of study concept, study design, acquisition of data, data analysis, interpretation of data, and drafting the manuscript; Birgit Debrabant, to acquisition of data, data analysis, and interpretation of data; Qihua Tan, to acquisition of data, data analysis, and interpretation of data; Joris Deelen, to acquisition of data, data analysis, and interpretation of data; Karen Andersen‐Ranberg, to acquisition of data; Anton J. M. de Craen, to acquisition of data; Marian Beekman, to acquisition of data; Bernard Jeune, to acquisition of data; P. Eline Slagboom, to acquisition of data; Kaare Christensen, to acquisition of data and interpretation of data; Lene Christiansen, to generation of study concept, study design, acquisition of data, and interpretation of data; and all authors have revised the manuscript and given their final approval.

Supporting information

Table S1 Association between specific deletions and duplications and mortality in women.

Table S2 Association between specific deletions and duplications and mortality in men.

Table S3 Genes included in or surrounding the CNVs nominally associated with mortality (P ≤ 0.05) in the DKLS.

Click here for additional data file. (33.8KB, docx)

Acknowledgments

No acknowledgment information provided.

References

  1. Andersen‐Ranberg K, Schroll M, Jeune B (2001) Healthy centenarians do not exist, but autonomous centenarians do: a population‐based study of morbidity among Danish centenarians. J. Am. Geriatr. Soc. 49, 900–908. [DOI] [PubMed] [Google Scholar]
  2. Azad AK, Chakrabarti S, Xu Z, Davidge ST, Fu Y (2014) Coiled‐coil domain containing 3 (CCDC3) represses tumor necrosis factor‐alpha/nuclear factor kappaB‐induced endothelial inflammation. Cell. Signal. 26, 2793–2800. [DOI] [PubMed] [Google Scholar]
  3. Beekman M, Blauw GJ, Houwing‐Duistermaat JJ, Brandt BW, Westendorp RG, Slagboom PE (2006) Chromosome 4q25, microsomal transfer protein gene, and human longevity: novel data and a meta‐analysis of association studies. J. Gerontol. A Biol. Sci. Med. Sci. 61, 355–362. [DOI] [PubMed] [Google Scholar]
  4. Bell JT, Tsai PC, Yang TP, Pidsley R, Nisbet J, Glass D, Mangino M, Zhai G, Zhang F, Valdes A, Shin SY, Dempster EL, Murray RM, Grundberg E, Hedman AK, Nica A, Small KS, Mu TC, Dermitzakis ET, McCarthy MI, Mill J, Spector TD, Deloukas P (2012) Epigenome‐wide scans identify differentially methylated regions for age and age‐related phenotypes in a healthy ageing population. PLoS Genet. 8, e1002629. [DOI] [PMC free article] [PubMed] [Google Scholar]
  5. Chouraki V, De Bruijn RF, Chapuis J, Bis JC, Reitz C, Schraen S, Ibrahim‐Verbaas CA, Grenier‐Boley B, Delay C, Rogers R, Demiautte F, Mounier A, Fitzpatrick AL, Alzheimer's Disease Neuroimaging I , Berr C, Dartigues JF, Uitterlinden AG, Hofman A, Breteler M, Becker JT, Lathrop M, Schupf N, Alperovitch A, Mayeux R, van Duijn CM, Buee L, Amouyel P, Lopez OL, Ikram MA, Tzourio C, Lambert JC (2014) A genome‐wide association meta‐analysis of plasma Abeta peptides concentrations in the elderly. Mol. Psychiatry 19, 1326–1335. [DOI] [PMC free article] [PubMed] [Google Scholar]
  6. Conner JR, Smirnova II, Poltorak A (2008) Forward genetic analysis of Toll‐like receptor responses in wild‐derived mice reveals a novel antiinflammatory role for IRAK1BP1. J. Exp. Med. 205, 305–314. [DOI] [PMC free article] [PubMed] [Google Scholar]
  7. Conner JR, Smirnova II, Moseman AP, Poltorak A (2010) IRAK1BP1 inhibits inflammation by promoting nuclear translocation of NF‐kappaB p50. Proc. Natl Acad. Sci. USA 107, 11477–11482. [DOI] [PMC free article] [PubMed] [Google Scholar]
  8. Deelen J, Uh HW, Monajemi R, van Heemst D, Thijssen PE, Bohringer S, van den Akker EB, de Craen AJ, Rivadeneira F, Uitterlinden AG, Westendorp RG, Goeman JJ, Slagboom PE, Houwing‐Duistermaat JJ, Beekman M (2013) Gene set analysis of GWAS data for human longevity highlights the relevance of the insulin/IGF‐1 signaling and telomere maintenance pathways. Age (Dordr) 35, 235–249. [DOI] [PMC free article] [PubMed] [Google Scholar]
  9. Deelen J, Beekman M, Uh HW, Broer L, Ayers KL, Tan Q, Kamatani Y, Bennet AM, Tamm R, Trompet S, Guethbjartsson DF, Flachsbart F, Rose G, Viktorin A, Fischer K, Nygaard M, Cordell HJ, Crocco P, van den Akker EB, Bohringer S, Helmer Q, Nelson CP, Saunders GI, Alver M, Andersen‐Ranberg K, Breen ME, van der Breggen R, Caliebe A, Capri M, Cevenini E, Collerton JC, Dato S, Davies K, Ford I, Gampe J, Garagnani P, de Geus EJ, Harrow J, van Heemst D, Heijmans BT, Heinsen FA, Hottenga JJ, Hofman A, Jeune B, Jonsson PV, Lathrop M, Lechner D, Martin‐Ruiz C, McNerlan SE, Mihailov E, Montesanto A, Mooijaart SP, Murphy A, Nohr EA, Paternoster L, Postmus I, Rivadeneira F, Ross OA, Salvioli S, Sattar N, Schreiber S, Stefansson H, Stott DJ, Tiemeier H, Uitterlinden AG, Westendorp RG, Willemsen G, Samani NJ, Galan P, Sorensen TI, Boomsma DI, Jukema JW, Rea IM, Passarino G, de Craen AJ, Christensen K, Nebel A, Stefansson K, Metspalu A, Magnusson P, Blanche H, Christiansen L, Kirkwood TB, van Duijn CM, Franceschi C, Houwing‐Duistermaat JJ, Slagboom PE (2014) Genome‐wide association meta‐analysis of human longevity identifies a novel locus conferring survival beyond 90 years of age. Hum. Mol. Genet. 23, 4420–4432. [DOI] [PMC free article] [PubMed] [Google Scholar]
  10. Donoho G, Brenneman MA, Cui TX, Donoviel D, Vogel H, Goodwin EH, Chen DJ, Hasty P (2003) Deletion of Brca2 exon 27 causes hypersensitivity to DNA crosslinks, chromosomal instability, and reduced life span in mice. Genes Chromosom. Cancer 36, 317–331. [DOI] [PubMed] [Google Scholar]
  11. Feuk L, Carson AR, Scherer SW (2006a) Structural variation in the human genome. Nat. Rev. Genet. 7, 85–97. [DOI] [PubMed] [Google Scholar]
  12. Feuk L, Marshall CR, Wintle RF, Scherer SW (2006b) Structural variants: changing the landscape of chromosomes and design of disease studies. Hum. Mol. Genet. 15(Spec No 1), R57–R66. [DOI] [PubMed] [Google Scholar]
  13. Glessner JT, Smith AV, Panossian S, Kim CE, Takahashi N, Thomas KA, Wang F, Seidler K, Harris TB, Launer LJ, Keating B, Connolly J, Sleiman PM, Buxbaum JD, Grant SF, Gudnason V, Hakonarson H (2013) Copy number variations in alternative splicing gene networks impact lifespan. PLoS One 8, e53846. [DOI] [PMC free article] [PubMed] [Google Scholar]
  14. Herskind AM, McGue M, Holm NV, Sorensen TI, Harvald B, Vaupel JW (1996) The heritability of human longevity: a population‐based study of 2872 Danish twin pairs born 1870‐1900. Hum. Genet. 97, 319–323. [DOI] [PubMed] [Google Scholar]
  15. Hjelmborg JV, Iachine I, Skytthe A, Vaupel JW, Mcgue M, Koskenvuo M, Kaprio J, Pedersen NL, Christensen K (2006) Genetic influence on human lifespan and longevity. Hum. Genet. 119, 312–321. [DOI] [PubMed] [Google Scholar]
  16. Iakoubov L, Mossakowska M, Szwed M, Duan Z, Sesti F, Puzianowska‐Kuznicka M (2013) A common copy number variation (CNV) polymorphism in the CNTNAP4 gene: association with aging in females. PLoS One 8, e79790. [DOI] [PMC free article] [PubMed] [Google Scholar]
  17. Iakoubov L, Mossakowska M, Szwed M, Puzianowska‐Kuznicka M (2015) A common copy number variation polymorphism in the CNTNAP2 gene: sexual dimorphism in association with healthy aging and disease. Gerontology 61, 24–31. [DOI] [PubMed] [Google Scholar]
  18. International Schizophrenia C (2008) Rare chromosomal deletions and duplications increase risk of schizophrenia. Nature 455, 237–241. [DOI] [PMC free article] [PubMed] [Google Scholar]
  19. Jacobsen R, Martinussen T, Christiansen L, Jeune B, Andersen‐Ranberg K, Vaupel JW, Christensen K (2010) Increased effect of the ApoE gene on survival at advanced age in healthy and long‐lived Danes: two nationwide cohort studies. Aging Cell 9, 1004–1009. [DOI] [PMC free article] [PubMed] [Google Scholar]
  20. Jensen RB (2013) BRCA2: one small step for DNA repair, one giant protein purified. Yale J. Biol. Med. 86, 479–489. [PMC free article] [PubMed] [Google Scholar]
  21. Karolchik D, Hinrichs AS, Furey TS, Roskin KM, Sugnet CW, Haussler D, Kent WJ (2004) The UCSC Table Browser data retrieval tool. Nucleic Acids Res. 32, D493–D496. [DOI] [PMC free article] [PubMed] [Google Scholar]
  22. Kuningas M, Estrada K, Hsu YH, Nandakumar K, Uitterlinden AG, Lunetta KL, van Duijn CM, Karasik D, Hofman A, Murabito J, Rivadeneira F, Kiel DP, Tiemeier H (2011) Large common deletions associate with mortality at old age. Hum. Mol. Genet. 20, 4290–4296. [DOI] [PMC free article] [PubMed] [Google Scholar]
  23. Lunetta KL, D'Agostino RB Sr, Karasik D, Benjamin EJ, Guo CY, Govindaraju R, Kiel DP, Kelly‐Hayes M, Massaro JM, Pencina MJ, Seshadri S, Murabito JM (2007) Genetic correlates of longevity and selected age‐related phenotypes: a genome‐wide association study in the Framingham Study. BMC Med. Genet. 8(Suppl 1), S13. [DOI] [PMC free article] [PubMed] [Google Scholar]
  24. Macdonald JR, Ziman R, Yuen RK, Feuk L, Scherer SW (2014) The database of genomic variants: a curated collection of structural variation in the human genome. Nucleic Acids Res. 42, D986–D992. [DOI] [PMC free article] [PubMed] [Google Scholar]
  25. Manolio TA, Collins FS, Cox NJ, Goldstein DB, Hindorff LA, Hunter DJ, McCarthy MI, Ramos EM, Cardon LR, Chakravarti A, Cho JH, Guttmacher AE, Kong A, Kruglyak L, Mardis E, Rotimi CN, Slatkin M, Valle D, Whittemore AS, Boehnke M, Clark AG, Eichler EE, Gibson G, Haines JL, Mackay TF, McCarroll SA, Visscher PM (2009) Finding the missing heritability of complex diseases. Nature 461, 747–753. [DOI] [PMC free article] [PubMed] [Google Scholar]
  26. Marshall CR, Noor A, Vincent JB, Lionel AC, Feuk L, Skaug J, Shago M, Moessner R, Pinto D, Ren Y, Thiruvahindrapduram B, Fiebig A, Schreiber S, Friedman J, Ketelaars CE, Vos YJ, Ficicioglu C, Kirkpatrick S, Nicolson R, Sloman L, Summers A, Gibbons CA, Teebi A, Chitayat D, Weksberg R, Thompson A, Vardy C, Crosbie V, Luscombe S, Baatjes R, Zwaigenbaum L, Roberts W, Fernandez B, Szatmari P, Scherer SW (2008) Structural variation of chromosomes in autism spectrum disorder. Am. J. Hum. Genet. 82, 477–488. [DOI] [PMC free article] [PubMed] [Google Scholar]
  27. Miller SA, Dykes DD, Polesky HF (1988) A simple salting out procedure for extracting DNA from human nucleated cells. Nucleic Acids Res. 16, 1215. [DOI] [PMC free article] [PubMed] [Google Scholar]
  28. Murabito JM, Yuan R, Lunetta KL (2012) The search for longevity and healthy aging genes: insights from epidemiological studies and samples of long‐lived individuals. J. Gerontol. A Biol. Sci. Med. Sci. 67, 470–479. [DOI] [PMC free article] [PubMed] [Google Scholar]
  29. Nybo H, Gaist D, Jeune B, Bathum L, McGue M, Vaupel JW, Christensen K (2001) The Danish 1905 cohort: a genetic‐epidemiological nationwide survey. J. Aging Health 13, 32–46. [DOI] [PubMed] [Google Scholar]
  30. Nygaard M, Lindahl‐Jacobsen R, Soerensen M, Mengel‐From J, Andersen‐Ranberg K, Jeune B, Vaupel JW, Tan Q, Christiansen L, Christensen K (2014) Birth cohort differences in the prevalence of longevity‐associated variants in APOE and FOXO3A in Danish long‐lived individuals. Exp. Gerontol. 57, 41–46. [DOI] [PMC free article] [PubMed] [Google Scholar]
  31. Pedersen CB, Gotzsche H, Moller JO, Mortensen PB (2006) The Danish Civil Registration System. A cohort of eight million persons. Dan. Med. Bull. 53, 441–449. [PubMed] [Google Scholar]
  32. Purcell S, Neale B, Todd‐Brown K, Thomas L, Ferreira MA, Bender D, Maller J, Sklar P, de Bakker PI, Daly MJ, Sham PC (2007) PLINK: a tool set for whole‐genome association and population‐based linkage analyses. Am. J. Hum. Genet. 81, 559–575. [DOI] [PMC free article] [PubMed] [Google Scholar]
  33. Robine JM, Cheung SL, Saito Y, Jeune B, Parker MG, Herrmann FR (2010) Centenarians today: new insights on selection from the 5‐COOP study. Curr. Gerontol. Geriatr. Res. 2010, 120354. [DOI] [PMC free article] [PubMed] [Google Scholar]
  34. Rossi ML, Ghosh AK, Bohr VA (2010) Roles of Werner syndrome protein in protection of genome integrity. DNA Repair 9, 331–344. [DOI] [PMC free article] [PubMed] [Google Scholar]
  35. Schoenmaker M, de Craen AJ, de Meijer PH, Beekman M, Blauw GJ, Slagboom PE, Westendorp RG (2006) Evidence of genetic enrichment for exceptional survival using a family approach: the Leiden Longevity Study. Eur. J. Hum. Genet. 14, 79–84. [DOI] [PubMed] [Google Scholar]
  36. Skytthe A, Kyvik K, Holm NV, Vaupel JW, Christensen K (2002) The Danish Twin Registry: 127 birth cohorts of twins. Twin Res. 5, 352–357. [DOI] [PubMed] [Google Scholar]
  37. Soerensen M, Dato S, Tan Q, Thinggaard M, Kleindorp R, Beekman M, Jacobsen R, Suchiman HE, de Craen AJ, Westendorp RG, Schreiber S, Stevnsner T, Bohr VA, Slagboom PE, Nebel A, Vaupel JW, Christensen K, McGue M, Christiansen L (2012) Human longevity and variation in GH/IGF‐1/insulin signaling, DNA damage signaling and repair and pro/antioxidant pathway genes: cross sectional and longitudinal studies. Exp. Gerontol. 47, 379–387. [DOI] [PMC free article] [PubMed] [Google Scholar]
  38. Stranger BE, Forrest MS, Dunning M, Ingle CE, Beazley C, Thorne N, Redon R, Bird CP, de Grassi A, Lee C, Tyler‐Smith C, Carter N, Scherer SW, Tavare S, Deloukas P, Hurles ME, Dermitzakis ET (2007) Relative impact of nucleotide and copy number variation on gene expression phenotypes. Science 315, 848–853. [DOI] [PMC free article] [PubMed] [Google Scholar]
  39. Tian X, Azpurua J, Hine C, Vaidya A, Myakishev‐Rempel M, Ablaeva J, Mao Z, Nevo E, Gorbunova V, Seluanov A (2013) High‐molecular‐mass hyaluronan mediates the cancer resistance of the naked mole rat. Nature 499, 346–349. [DOI] [PMC free article] [PubMed] [Google Scholar]
  40. Vestergaard S, Andersen‐Ranberg K, Skytthe A, Christensen K, Robine JM, Jeune B (2015) Health and function assessments in two adjacent Danish birth cohorts of centenarians: Impact of design and methodology. Eur. J. Ageing. (in press). [DOI] [PMC free article] [PubMed] [Google Scholar]
  41. Vijg J, Suh Y (2013) Genome instability and aging. Annu. Rev. Physiol. 75, 645–668. [DOI] [PubMed] [Google Scholar]
  42. Wang K, Li M, Hadley D, Liu R, Glessner J, Grant SF, Hakonarson H, Bucan M (2007) PennCNV: an integrated hidden Markov model designed for high‐resolution copy number variation detection in whole‐genome SNP genotyping data. Genome Res. 17, 1665–1674. [DOI] [PMC free article] [PubMed] [Google Scholar]
  43. Wheeler E, Huang N, Bochukova EG, Keogh JM, Lindsay S, Garg S, Henning E, Blackburn H, Loos RJ, Wareham NJ, O'Rahilly S, Hurles ME, Barroso I, Farooqi IS (2013) Genome‐wide SNP and CNV analysis identifies common and low‐frequency variants associated with severe early‐onset obesity. Nat. Genet. 45, 513–517. [DOI] [PMC free article] [PubMed] [Google Scholar]
  44. Wolfson M, Budovsky A, Tacutu R, Fraifeld V (2009) The signaling hubs at the crossroad of longevity and age‐related disease networks. Int. J. Biochem. Cell Biol. 41, 516–520. [DOI] [PubMed] [Google Scholar]
  45. Yashin AI, Wu D, Arbeev KG, Ukraintseva SV (2010) Joint influence of small‐effect genetic variants on human longevity. Aging 2, 612–620. [DOI] [PMC free article] [PubMed] [Google Scholar]
  46. Zheng X, Shaffer JR, McHugh CP, Laurie CC, Feenstra B, Melbye M, Murray JC, Marazita ML, Feingold E (2012) Using family data as a verification standard to evaluate copy number variation calling strategies for genetic association studies. Genet. Epidemiol. 36, 253–262. [DOI] [PMC free article] [PubMed] [Google Scholar]

Associated Data

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

Supplementary Materials

Table S1 Association between specific deletions and duplications and mortality in women.

Table S2 Association between specific deletions and duplications and mortality in men.

Table S3 Genes included in or surrounding the CNVs nominally associated with mortality (P ≤ 0.05) in the DKLS.

Click here for additional data file. (33.8KB, docx)

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