The International HapMap Project, launched in October 2002, led to the generation of a database of the common variations (defined as minor allele frequency of greater than 0.05) and the underlying LD structure in the human genome 4849 that provided the foundation for the genome-wide association studies (GWASs) that use high-throughput genotyping platforms composed of common SNP markers that tag a subset of the known common SNPs in the human genome. For example, the Affymetrix GeneChip 500K platform (Affymetrix, Santa Clara, CA, USA) has 68% coverage of the phase II HapMap SNPs at r2 of at least 0.8 in the subjects of European ancestry (CEU), whereas the Illumina Hap300 platform (Illumina, Inc., San Diego, CA, USA) has 77% coverage 49. Furthermore, coverage is less in non-European populations, up to 1% of the common variations are untaggable by other SNPs using LD, and there likely exist millions of 'rare' SNPs not covered by these platforms. Despite their limitations, GWASs allowed a higher-resolution screen of the human genome for common diseases and traits. In the last two years, 11 GWASs in LOAD have been published. In this section, brief summaries of each of these studies are provided, followed by collective conclusions.
Study-specific characteristics and results of the late-onset Alzheimer disease GWASs
The study designs and results of the 11 LOAD GWASs are depicted in detail in Tables 1 and 2, respectively 505152535455565758596061. The first published LOAD GWAS used a select set of 17,343 SNPs from 11,211 genes that were chosen based on their likelihood of being functional polymorphisms 50. These SNPs were weighted heavily toward missense mutations, although there were also variants in transcription factor-binding sites, introns, intergenic regions as well as other putative functional SNPs. Authors used a multi-stage design, in which the SNPs were genotyped in pooled DNA from 380 LOAD and 396 control subjects in the first stage. One thousand five hundred forty-four SNPs with AD association at P values of less than 0.075 or less than 0.1 and in biological candidate genes were genotyped in a second pool of 376 LOAD and 344 control subjects. Of these SNPs, 119 showed association at a P value of less than 0.15 with the same risk allele associating in the second pool. These 119 SNPs were genotyped individually in a total of four series, including the two initial pooled series. Eighteen of these SNPs that had a P value of less than 0.05 in the two pooled series and meta-analysis P value of less than 0.005 in the four series combined were also genotyped in a fifth series. Altogether, nearly 4,000 subjects were genotyped in this study, although the multi-stage design with two pooled DNA series in the initial stages considerably reduced the cost of this study. Nonetheless, some associations may have been missed due to the reduced sensitivity of the pooling approach and the limited number of SNPs assessed. Despite these shortcomings, APOE-related SNPs (SNPs in APOE or in LD with SNPs in APOE) were identified with study-wide significance in this study. Fifteen additional non-APOE SNPs were identified with nominal significance after meta-analyses of all five series, with modest ORs of 1.07 to 1.2 in all series combined. Of these SNPs, one was a missense mutation (rs3745833) in the galanin-like peptide pre cursor (GALP) gene on chromosome 19 which showed suggestive study-wide significance. The galanin gene has been implicated in neuronal survival, regeneration, and neuroprotection and inhibition of learning and memory through reductions in glutamate release and reduction of long-term potentiation (reviewed in 62). Galanin expression has been shown to be upregulated in AD brains, although it is unclear whether this is a cause or effect. In this study, the authors highlighted additional genes among the final 15 - such as phosphoenolpyruvate carboxykinase 1 (PCK1), trafficking protein, kinesin binding 2 (TRAK2), and tyrosine kinase, non-receptor 1 (TNK1) - with potential biological relevance in AD.
<p>Table 1</p>Late-onset Alzheimer disease genome-wide association study: summary of methodologies.
Discovery series
Replication series
Reference
Ethnicity/Source
Samples
Study design
Genotyping platform
SNPsa
AD patients
Controls
AD patients
Controls
Follow-up criteria
Grupe et al. 50, February 2007
UK/US
Case control
1 discovery (pooled DNA) and 5 replication series (1 pooled)
Gene-based putative functional polymorphisms
17,343 (in 11,211 genes)
380
396
1,428
1,666
P < 0.075 or P < 0.1 and biology (stage 1)
P < 0.15 and same risk allele (stage 2)
P < 0.05 in UK1 and WU and P meta < 0.005 (stage 3)
Coon et al. 51, April 2007
US/The Netherlands
Case control
Single-stage study
Affymetrix 500K
502,627
664
422
-
-
Single-stage
Reiman et al. 52, June 2007b
US/The Netherlands
Case control
1 discovery and 2 replication series
Affymetrix 500K
312,316
446
290
415
260
All SNPs genotyped in both stages.
Li et al. 53, January 2008
Canada/UK
Case control
1 discovery and 1 replication series
Affymetrix 500K
469,438
753
736
418
249
Top 120 SNPs
Abraham et al. 54, September 2008
UK
Case control
Single-stage study (first pooled, hen individual enotyping)
Illumina HumanHap300 and llumina Sentrix umanHap240S
561,494
1,082
1,239
-
1,400
Passed three criteria and could be genotyped (stage 1) ≤ 0.05 (stage 2)
Bertram et al. 55, November 2008
US
Family-based
1 discovery and 3 replication series
Affymetrix 500K
404,604
941
404
1,767
838
Significance after weighted-Bonferroni correction
Beecham et al. 56, January 2009
US
Case control
1 discovery and 1 replication series
Illumina HumanHap550
532,000
492
496
238
220
Significance after FDR-BUM criteria
Feulner et al. 57, January 2009
Germany
Case control
Single-stage study
Illumina HumanHap550
555,000
491
479
-
-
Single-stage
Poduslo et al. 58, January 2009b
US
Family-based and case control
1 discovery and 2 replication series
Affymetrix 500K
469,218
19
(family members)
60
(CEPH)
140
(family members)
199
(unrelated)
85
(unrelated)
Genome-wide significance after Bonferroni correction
Carrasquillo et al. 59, February 2009b
US
Case control
3 discovery and 4 replication series
Illumina HumanHap300
313,504
844
1,255
1,547
1,209
25 top SNPs
Harold et al. 60, September 2009b
US/Europe
Case control
13 discovery and 5 replication series
Illumina 610-quad, Illumina umanHap550, or umanHap300
529,205 (up to)
3,941
7,848
2,023
2,340
Genome-wide significance after Bonferroni correction + 12 other CLU/PICALM SNPs
Lambert et al. 61, September 2009b
Europe
Case control
1 discovery and 4 replication series (15 centers)
Illumina Human 610-Quad BeadChip
537,029
2,032
5,328
3,978
3,297
P < 10-5
The study designs of the 11 independent late-onset Alzheimer disease genome-wide association studies are depicted. The Coon et al. 51 and Reiman et al. 52 studies are overlapping. Abraham et al. 54, Grupe et al. 50, and Harold et al. 60 also have overlapping samples. Carrasquillo et al. 59 contributed data to the Harold et al. 60 study. aNumber of single-nucleotide polymorphisms (SNPs) in the initial genotyping stage. bStudies hat yield non-APOE associations that are significant at the genome-wide level after Bonferroni corrections. AD, Alzheimer disease; CEPH, Centre d'Etude du Polymorphisme Humain; FDR-BUM, false discovery rate-beta uniform mixture.
<p>Table 2</p>Late-onset Alzheimer disease genome-wide association study: summary of results.
Non-ApoE hits
ApoE-related hits
Reference
Gene symbol
P valuea
Odds ratioa
P valuea
Odds ratioa
Grupe et al. 50
GALP, TNK1, chr14q32.13, PCK1, LMNA, PGBD1, LOC651924, chr7p15.2, THEM5, MYH13, CTSS, UBD, BCR, AGC1, TRAK2, EBF3
0.001 to 5.0 × 10-5
1.07 to 1.2
7.6 × 10-5 to 1.0 × 10-8
1.19 to 2.73
Coon et al. 51
1.1 × 10-39
4.01
Reiman et al. 52
GAB2
9.7 × 10-11
4.06
-
-
Li et al. 53
GOLPH2, chr9p24.3, chr15q21.2
9.8 × 10-3 to 4.5 × 10-6, b
0.46 to 3.23b
2.3 × 10-44
-
Abraham et al. 54
LRAT
3.4 × 10-6 to 6.1 × 10-7
1.2 to 1.3
4.8 × 10-6 to 4.0 × 10-14
-
Bertram et al. 55
chr14q31.2, chr19q13.41
6.0 × 10-6 to 2.0 × 10-6
1.1 to 1.4c
5.70 × 10-14
-
Beecham et al. 56
12q13
3.40 × 10-7
-
-
-
Feulner et al. 57
MAPT, SORL1, CHRNB2, CH25H, GAB2, PGBD1, PCK1, LMNA
0.05 to 6.8 × 10-3
-
<1.0 × 10-6 to <1.0 × 10-40
-
Poduslo et al. 58
TRPC4AP
3.85 × 10-10 to 5.63 × 10-11, c
0.03d
1.56d
Carrasquillo et al. 59
PCDH11X
3.8 × 10-8
(0.08 to 5.4 × 10-13)e
1.29
(1.17 to 1.75)e
5.9 × 10-6 to
3.7 × 10-120
0.55 to 3.29
Harold et al. 60
CLU
8.5 × 10-10 (CLU)
0.86 (CLU)
3.4 × 10-8 to 1.8 × 10-157
0.63 to 2.5
PICALM
1.3 × 10-9 (PICALM)
0.86 (PICALM)
Lambert et al. 61
CLU
7.5 × 10-9 (CLU)
0.86 (CLU)
5.06 × 10-7 to <2 × 10-16
-
CR1
3.7 × 10-9 (CR1)
1.21 (CR1)
The results of the 11 independent late-onset Alzheimer disease genome-wide association studies are depicted. The results from the original manuscripts shown in the table are (a) from all groups combined, (b) shown separately in each series, (c) from the discovery series, (d) from the follow-up case control series, and (e) variable based on different analytical models.
The second LOAD GWAS used the Affymetrix 500K platform to genotype more than 500,000 SNPs in a histopathologically confirmed series of 664 LOAD patients and 422 controls and identified the APOE locus as the only region with SNPs that reached genome-wide significance after Bonferroni correction for multiple testing 51. The same group reassessed their data by analyzing APOE ε4-positive and -negative subjects separately and dividing their histopathologic series into discovery and replication series 52. They focused on 312,316 SNPs after quality control exclusions and also included a clinical replication cohort in their genotyping and analysis. They identified 10 SNPs in the GRB-associated binding protein 2 (GAB2) gene on chromosome 11q14.1 with nominally significant associations (P = 4.56 × 10-7 to 8.92 × 10-5) in the APOE ε4 carrier subset of the neuropathological discovery cohort composed of 299 LOAD patients and 61 controls. When these 10 SNPs were assessed in the APOE ε4-positive subset of the neuropathological replication cohort (113 LOAD patients and 27 controls) as well as the clinical replication cohort (115 LOAD patients and 29 controls), 6 of them showed nominally significant associations. Moreover, when all three APOE ε4-positive groups were jointly analyzed, 5 SNPs reached genome-wide significance after Bonferroni corrections, with 1 SNP (rs2373115) achieving P = 9.66 × 10-11 and OR = 4.06. The GAB2 SNPs did not associate significantly in the APOE ε4 non-carriers, thereby leading to reductions in the strength of association when all subjects from all series were analyzed collectively as 861 LOAD patients and 550 controls (rs2373115 SNP association had P = 5.56 × 10-4 and OR = 1.66). GAB2 encodes a scaffolding protein, GRB-associated binding protein 2, which is involved in cell signaling pathways, especially in the immune system 63. Its potential role in AD pathophysiology remains to be elucidated; however, preliminary functional studies accompanying this LOAD GWAS revealed differential expression of GAB2 in AD versus control brains, co-localization of GAB2 with dystrophic neurites, and variation of GAB2 expression influencing tau phosphorylation 52.
The third LOAD GWAS 53 analyzed more than 400,000 SNPs from the Affymetrix 500K platform in 753 AD patients and 736 controls from the discovery series and followed up the 120 top SNPs in the 418 AD patients and 249 controls from the replication series. They identified APOE-related SNPs with genome-wide significance in the combined series. Of the top 120 associations, 3 non-APOE SNPs passed their quality control thresholds and had nominal logistic regression P value of less than 0.05 in their replication series. Two of these SNPs, rs7019241 and rs10868366, reside in the Golgi phosphoprotein 2 gene (GOLPH2) on chromosome 9, which is in a suggestive linkage region 35 and encodes a protein functionally involved in Golgi transmembrane trafficking, a subcellular localization where APP cleavage by the γ-secretase complex occurs 64. The other SNP, rs9886784, resides within a copy number deletion polymorphism on chromosome 9. A fourth SNP, rs10519262, which resides in an intergenic region on chromosome 15, was identified with the nominal P cutoff of less than 0.05 using Cox proportional hazards regression analysis for age-at-onset phenotype.
Using a pooled DNA approach on 1,082 LOAD patients and 1,239 controls, the fourth GWAS tested more than 500,000 SNPs from two Illumina platforms 54. These SNPs were submitted to three different analyses to test for allelic frequency differences in this pooled population followed by individual genotyping in the same series. One hundred fourteen of the 237 chosen SNPs could be genotyped individually. In addition to the five APOE related SNPs with a high level of significance (P = 8.97 × 10-5 to 5.89 × 10-9), 74 SNPs had nominal P values of not more than 0.05 and were genotyped in an additional control group of 1,400 subjects. Although this is not truly an independent test, the authors used this approach to detect five non-APOE SNPs that became even more significant, of which rs727153 had the best P value (P = 3.4 × 10-6). This SNP resides in a haplotype block on chromosome 4, including the lecithin retinol acyltransferase gene (LRAT), which is implicated in the retinoid pathway 65. Components of this pathway have been suggested to play a role in AD pathogenesis and proposed as potential drug targets. Genotyping additional SNPs in this study led to improved association signal (rs201825, P = 6.12 × 10-7, OR = 1.3) in the overall group, although none reached genome-wide significance after Bonferroni correction.
The first LOAD GWAS to use family-based analysis tested more than 400,000 SNPs in 941 AD patients versus 404 controls from 410 families of European descent 55. The follow-up was done in three series composed of 1,767 AD patients versus 838 controls from 875 families, also of European descent. The authors used a family-based association approach that assesses disease status and age of onset jointly. To obtain the corrected levels of significance, they used not the traditional Bonferroni method but a weighted-Bonferroni correction approach 66 that first screens all of the markers and estimates the conditional power of each marker, followed by the family-based association tests that are corrected using the weights determined from the screening analysis. According to this paradigm, they detected four non-APOE SNPs with P values of 2.0 × 10-3 to 4.0 × 10-6, which would not have been significant after the traditional Bonferroni correction. These four markers had nominal significance of P = 0.3 to 2.0 × 10-5 in the replication series. The two SNPs with nominal significance in both stages, rs11159647 and rs3826656, achieved P values of 2.0 × 10-6 and 6.0 × 10-6, respectively, for AD association in the combined series, which fell short of genome-wide significance after Bonferroni correction. rs11159647 appeared to have an effect on age of onset as well. These SNPs had a nominal P value of less than 0.05 in another LOAD GWAS 5253. rs11159647 on 14q31.2 and rs3826656 on chromosome 19q13.33 reside in regions without any mapped RefSeq genes, although the latter is in a predicted gene, which overlaps with the CD33 antigen gene. This group also evaluated the top genes from the AlzGene database at the time and determined some variants at P = 0.03 and 0.002. Notably, GAB2 52 showed one of the strongest nominal association signals.
The sixth LOAD GWAS genotyped more than 500,000 SNPs from the Illumina HumanHap550 platform in 492 LOAD cases and 496 controls in addition to imputing genotypes using a previously published LOAD GWAS 52. The authors used a modified false discovery rate approach (false discovery rate-beta uniform mixture, or FDR-BUM) 67 to declare significance at the genome-wide level. Besides APOE-related SNPs, some of which would be significant after Bonferroni correction, rs11610206 on 12q13, which does not reside in a RefSeq gene, was identified at genome-wide significance using the more relaxed FDR-BUM criteria (nominal P = 1.93 × 10-6). When genotyped in the follow-up series of 238 LOAD and 220 control subjects, this SNP was nominally significant at P = 0.0496 and the significance in the joint series improved to P = 3.452 × 10-7, falling short of significance after Bonferroni correction. Additionally, any SNP that had a P value of 0.0001 or less in this study or another LOAD GWAS 52, was imputed in the study that did not genotype that SNP. They identified eight SNPs with a nominal P value of less than 0.05 in the other study, in which the joint P value reached 1.51 × 10-6 for the most significant SNP in ZNF224 on chromosome 19q13. They also evaluated the AlzGene candidates in these two LOAD GWASs by assessing the genotyped or imputed SNPs in these genes for association with AD. Twenty-five SNPs from nine genes (ADAM12, CSF1, GBP2, KCNMA1, NOS2A, SORCS2, SORCS3, SORL1, and WWC1) had nominal P values of 0.003 to 0.05 in the individual LOAD GWAS with P values of 0.0001 to 0.01 in the joint analysis. In addition to providing suggestive evidence for a number of loci in the genome, this study drew attention to the challenges of comparing multiple GWASs via imputation, in which lack of sufficient marker information could lead to false-negative results. In these two studies, this was the case with the APOE SNPs that were highly significant in each study but could not be imputed in the other study, leading to missing the APOE signal in the joint analyses.
A single-stage LOAD GWAS from Germany analyzed 491 AD patients versus 479 younger controls and focused on the SNPs for the top 10 genes from AlzGene at the time of their study and SORL1. Thus, although 555,000 SNPs were genotyped, this study, due to its analytical approach, should be considered a follow-up to other association studies rather than a hypothesis-generating GWAS. Both single SNP and haplotype analyses were performed. In addition to APOE-related SNPs, some of which achieved genome-wide significance after Bonferroni correction, SNPs in 8 of the 11 genes tested (MAPT, SORL1, CHRNB2, CH25H, GAB2, PGBD1, PCK1, and LMNA) revealed nominal significance of P values of 0.05 to 6.8 × 10-3 in this study. None of the non-APOE SNPs achieved genome-wide significance in their study, but the authors provided follow-up analysis results that can be used in meta-analyses of all available data on these genes.
The second family-based LOAD GWAS assessed the smallest sample size to date, focusing on two extended LOAD families with 9 affected and 10 unaffected family members versus 60 unrelated controls from the CEPH (Centre d'Etude du Polymorphisme Humain) collection. In stage I, they genotyped more than 400,000 SNPs and identified association with 6 SNPs in the TRPC4AP (transient receptor potential cation channel, subfamily C, member 4 associated protein) gene at genome-wide significance (P = 5.63 × 10-11 to 3.85 × 10-10). Because this initial analysis compared ADs from families with unrelated controls outside of the families, it cannot be considered a family-based analysis. The authors subsequently genotyped 10 SNPs in TRPC4AP and identified a common haplotype with increased frequency in the AD patients from the families compared with the control spouses. The same haplotype was also associated with LOAD in an unrelated case control series of 199 LOAD versus 85 control subjects. The authors suggest a functional role for this gene in AD through its interaction with proteins in the inflammatory cascade and its role in calcium homeostasis. Despite the genome-wide significant results in this study, the findings need further replication given the small sample sizes and analytic approach in the first stage, which used unrelated controls versus AD patients from the families. Indeed, this is the only GWAS that failed to identify APOE; this could be due to the fact that these families have risk factors that are distinct from the general population, but this could also suggest lack of sufficient power.
The third largest LOAD GWAS to date assessed 844 LOAD subjects versus 1,255 controls in the first stage, which assessed more than 300,000 SNPs on an Illumina platform. The authors followed the top 25 SNPs from this stage for association in the follow-up series of 1,547 LOAD subjects versus 1,209 controls. APOE-related SNPs were the only ones that were significant at the genome-wide level in the first stage. Upon combined analysis of all samples, rs5984894 in the protocadherin 11X (PCDH11X) gene on chromosome Xq21.31 was the only one that achieved genome-wide significance (P = 3.8 × 10-8, OR = 1.29). Multi-variable logistic regression analysis using male sex as a covariate and comparing male hemizygotes, female heterozygotes, and female homozygotes with the female non-carriers yielded global a P value of 3.9 × 10-12 for the global association. Male hemizygotes showed suggestive association (P = 0.07), whereas female heterozygotes and homozygotes had nominally significant associations (P = 0.01 and 2.0 × 10-7, respectively), with OR estimates of 1.18, 1.26, and 1.75, respectively, for these groups. PCDH11X is the first X-chromosomal candidate AD gene identified in a LOAD GWAS. Protocadherins belong to the superfamily of cadherins that are involved in cell adhesion, cell signaling, and neural development. Protocadherins are expressed predominantly in the brain, suggesting their potential role in brain morphogenesis 68. Although the functional role of this gene in AD needs to be established and the genetic effect confirmed through additional studies, it is an intriguing hypothesis that this X-chromosomal gene could explain the increased risk of AD in women.
The two most recent LOAD GWASs are by far the largest ones published to date in this field 6061. One of the two GWASs in LOAD case control series in which non-APOE SNPs reached genome-wide significance after Bonferroni correction in the first stage was performed in 3,941 LOAD and 7,848 control subjects from 13 different centers in Europe and the US, where up to more than 500,000 SNPs were analyzed. In addition to the APOE-related SNPs that revealed genome-wide significance (P = 4.9 × 10-37 to 1.8 × 10-157), rs11136000 in clusterin (CLU or ApoJ) on chromosome 8 and rs3851179 in the phosphatidylinositol-binding clathrin assembly protein (PICALM) gene on chromosome 11 yielded genome-wide significance with P = 1.4 × 10-9 and 1.9 × 10-8, respectively. When genotyped in the follow-up series of 2,023 LOAD versus 2,340 control subjects from five centers in Europe, these SNPs had nominal significance at a P value of less than 0.05. Significance for rs11136000 in CLU improved to P = 8.5 × 10-10 (OR = 0.86) and that for PICALM improved to P = 1.3 × 10-9 (OR = 0.90) in the combined series. In addition, the authors identified more SNPs than would be expected by chance with P values of less than 1.0 × 10-5, including an SNP in the complement receptor 1 gene (rs1408077) that was identified at genome-wide significance in the other largest LOAD GWAS to date 61 (P = 8.3 × 10-6). The authors tested more than 100 SNPs in their series that were identified in other LOAD GWASs and identified nominal significance at a P value of less than 0.05 for a number of these, including PCDH11X and SORL1.
The other large LOAD GWAS analyzed more than 500,000 SNPs in 2,032 LOAD versus 5,328 control subjects from France 61. Like the other large LOAD GWASs, this study identified rs11136000 in CLU with genome-wide significance in the first stage (P = 9.0 × 10-8) in their analysis, correcting for population stratification in addition to APOE-related markers (P = 5.06 × 10-7 to less than 2 × 10-16). Those SNPs with a P value of less than 1.0 × 10-5 were genotyped or imputed in the follow-up series composed of 3,978 LOAD versus 3,297 controls from 15 centers in four countries. CLU SNP rs11136000 had nominal significance in their second stage and enhanced significance of P = 7.5 × 10-9 (OR = 0.86) in their combined series. Another SNP, rs6656401, in complement component receptor 1 (CR1) also achieved genome-wide significance in the combined series with P = 3.7 × 10-9 (OR = 1.21). The authors also identified nominal significance for SNPs in PICALM (P = 1.0 × 10-2 to 1.0 × 10-3) and PCDH11X (0.01 < P < 0.05) in their series, thereby providing additional evidence for these genes identified in other LOAD GWASs 5960.
CLU encodes clusterin or ApoJ, which along with APOE is one of the most abundant apolipoproteins in the human brain. In vivo studies suggest that clusterin, like APOE, is involved in Aβ clearance from the brain (reviewed in 33). There are also studies that revealed a role for clusterin in Aβ fibrillogenesis and neurotoxicity. These results raise the possibility that, in Aβ pathophysiology, clusterin may have a dual role similar to that of APOE. PICALM encodes a protein involved in clathrin-mediated endocytosis, a suggested pathway for trafficking of APP that could also influence Aβ formation 69. There is also evidence that PICALM influences endocytosis of the synaptic vesicle protein VAMP2 from the plasma membrane 70, suggesting a role in synaptic function. CR1 is a receptor for the complement component C3b, which has been suggested to be involved in the peripheral clearance of Aβ 71. Thus, all three candidate genes that emerged from the two largest LOAD GWASs to date have putative functions in the Aβ cascade and synaptic machinery (for PICALM). Additional non-Aβ-mediated pathophysiologic mechanisms for the proteins encoded by these genes may exist and require further investigation.
It is important to note that a number of the 'hits' identified from the LOAD GWASs reside in prior linkage regions (for example, GALP on chromosome 19, LMNA on chromosome 1, GOLPH2 on chromosome 9, and CLU on chromosome 8) and that others (such as MAPT and SORL1) have previously been implicated in candidate gene association studies. Multiple lines of evidence in support of the same gene provide additional support for their role in the risk of AD; however, in general, these results need to be interpreted with caution and special attention to any sample overlaps, effect size, and direction of effect in the different studies. The AlzGene database facilitates the visualization and cross-checking of findings from different linkage and association studies 29.