Genetic variants affecting bone mineral density and bone mineral content at multiple skeletal sites in Hispanic children

Genetic variants affecting bone mineral density and bone mineral content at multiple skeletal sites in Hispanic children

Journal Pre-proof Genetic variants affecting bone mineral density and bone mineral content at multiple skeletal sites in Hispanic children Ruixue Hou...
Download PDF
3MB Sizes 0 Downloads 48 Views
Report

Journal Pre-proof Genetic variants affecting bone mineral density and bone mineral content at multiple skeletal sites in Hispanic children

Ruixue Hou, Shelley A. Cole, Mariaelisa Graff, Karin Haack, Sandra Laston, Anthony G. Comuzzie, Nitesh R. Mehta, Kathleen Ryan, Diana L. Cousminer, Babette S. Zemel, Struan F.A. Grant, Braxton D. Mitchell, Roman J. Shypailo, Margaret L. Gourlay, Kari E. North, Nancy F. Butte, V. Saroja Voruganti PII:

S8756-3282(19)30469-7

DOI:

https://doi.org/10.1016/j.bone.2019.115175

Reference:

BON 115175

To appear in:

Bone

Received date:

27 June 2019

Revised date:

22 November 2019

Accepted date:

22 November 2019

Please cite this article as: R. Hou, S.A. Cole, M. Graff, et al., Genetic variants affecting bone mineral density and bone mineral content at multiple skeletal sites in Hispanic children, Bone(2019), https://doi.org/10.1016/j.bone.2019.115175

This is a PDF file of an article that has undergone enhancements after acceptance, such as the addition of a cover page and metadata, and formatting for readability, but it is not yet the definitive version of record. This version will undergo additional copyediting, typesetting and review before it is published in its final form, but we are providing this version to give early visibility of the article. Please note that, during the production process, errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.

© 2019 Published by Elsevier.

Journal Pre-proof

Genetic variants affecting bone mineral density and bone mineral content at multiple skeletal sites in Hispanic children Ruixue Hou1, PhD, Shelley A. Cole2, PhD, Mariaelisa Graff3, PhD, Karin Haack2, PhD, Sandra Laston4, RN, PhD, Anthony G. Comuzzie5, PhD, Nitesh R. Mehta6, MS, Kathleen Ryan, MPH, MS7, Diana L. Cousminer, PhD8, Babette S. Zemel9, PhD, Struan FA. Grant8, 10, PhD, Braxton D. Mitchell, PhD7, Roman J. Shypailo6, Margaret L. Gourlay11, PhD, Kari E. North3, PhD, Nancy F.

ro

of

Butte6, PhD, V. Saroja Voruganti1*, PhD

-p

1. Department of Nutrition and Nutrition Research Institute, University of North Carolina at Chapel Hill, Kannapolis, NC, USA

re

2. Population Health Program, Texas Biomedical Research Institute, San Antonio, TX, USA 3. Department of Epidemiology, University of North Carolina at Chapel Hill, Chapel Hill, NC,

lP

USA

4. South Texas Diabetes and Obesity Institute and Department of Human Genetics, University of

na

Texas of the Rio Grande Valley, Brownsville, TX, USA 5. The Obesity Society, Silver Spring, MD, USA

ur

6. Department of Pediatrics and USDA/ARS Children Nutrition Research Center, Baylor College

Jo

of Medicine, Houston, TX, USA

7. Division of Endocrinology, Diabetes and Nutrition, Department of Medicine, University of Maryland School of Medicine, Baltimore, MD. Geriatrics Research and Education Clinical Center, Baltimore Veterans Administration Medical Center, Baltimore, MD 8. Division of Human Genetics, Children’s Hospital of Philadelphia, Philadelphia; Department of Genetics, University of Pennsylvania, Philadelphia; Center for Spatial and Functional Genomics, Children’s Hospital of Philadelphia, Philadelphia 9. Division of GI, Hepatology and Nutrition, The Children’s Hospital of Philadelphia. Philadelphia, PA, USA 10. Department of Pediatrics, University of Pennsylvania, Philadelphia; Institute for Diabetes, Obesity and Metabolism, Perelman School of Medicine, University of Pennsylvania, 1

Journal Pre-proof Philadelphia, PA; Division of Endocrinology and Diabetes, Children’s Hospital of Philadelphia, Philadelphia, PA 11. Department of Family Medicine, University of North Carolina at Chapel Hill, Chapel Hill, NC, USA

*Corresponding Author: V. Saroja Voruganti, PhD

of

Address: Department of Nutrition and UNC Nutrition Research Institute, University of North

ro

Carolina at Chapel Hill, 500 Laureate Way, Kannapolis, NC 28081.

-p

Telephone Number: 704-250-5009

Jo

ur

na

lP

re

Email Address: [email protected]

2

Journal Pre-proof Abstract Context: Osteoporosis is a major public health burden with significant economic costs. However, the correlates of bone health in Hispanic children are understudied. Objective: We aimed to identify genetic variants associated with bone mineral density (BMD) and bone mineral content (BMC) at multiple skeletal sites in Hispanic children. Methods: We conducted a cross-sectional genome-wide linkage analysis, genome-wide and

of

exome-wide association analysis of BMD and BMC. The Viva La Familia Study is a family-

ro

based cohort with a total of 1,030 Hispanic children (4-19 years old at baseline) conducted in

-p

Houston, TX. BMD and BMC were measured by Dual-energy X-ray absorptiometry. Results: Significant heritability were observed for BMC and BMD at multiple skeletal sites

re

ranging between 44 and 68% (P<2.8×10-9). Significant evidence for linkage was found for BMD

lP

of pelvis and left leg on chromosome 7p14, lumbar spine on 20q13 and left rib on 6p21, and

na

BMC of pelvis on chromosome 20q12 and total body on 14q22-23 (logarithm of odds score > 3). We found genome-wide significant association between BMC of right arm and rs762920 at

ur

PVALB (P = 4.6×10-8), and between pelvis BMD and rs7000615 at PTK2B (P = 7.4 ×10-8).

Jo

Exome-wide association analysis revealed novel association of variants at MEGF10 and ABRAXAS2 with left arm and lumber spine BMC, respectively (P<9×10-7). Conclusions: We identified novel loci associated with BMC and BMD in Hispanic children, with strongest evidence for PTK2B. The findings provide better understanding of bone genetics and shed light on biological mechanisms underlying BMD and BMC variation.

Key words: Bone; Genetic variants; Hispanic; Children; Osteoporosis

3

Journal Pre-proof Introduction Osteoporosis and low bone mass are currently estimated to be a major public health threat for almost 54 million people aged 50 and older in the U.S [1]. Mexican Americans have a higher overall age-adjusted prevalence of osteoporosis and the most rapid projected increase in osteoporosis burden, compared to other ethnicities [1,2]. However, the correlates of bone health in Hispanic individuals, especially Hispanic children, are understudied.

of

Genetic factors account for up to 80% of the variance in bone mass [3]. Multiple family-

ro

based linkage studies have identified chromosomal regions linked to bone mineral density (BMD)

-p

and bone mineral content (BMC) [3,4]. Common variants identified through genome-wide

re

association studies (GWAS) explain only about 5% of the genetic variance in BMC and BMD, and the missing heritability may be explained by low-frequency and rare variants, whose

lP

contribution to BMC and BMD are still largely unknown [3,5]. Most genetic studies have been

na

conducted in adults, while only a few studies have investigated the genetic effects on bone in children and adolescents [6–9]. Although genetic variants affecting metabolic diseases have

ur

been discovered in both adults and children, some novel variants have been found only in

Jo

children [9–11]. Compared to adults, bone mass in children is largely affected by bone acquisition and less affected by environmental factors [11]. Pediatric genetic studies provide opportunities to identify novel loci affecting bone health. As genetic studies related to bone health have been conducted in European or Asian populations and mainly in older adults, it is not certain whether those variants are also associated with bone health in Hispanic children. Therefore, we elected to identify genetic variants associated with gold standard Dual-Energy XRay Absorptiometry (DXA)-derived BMD and BMC at multiple skeletal sites in a family-based study, Viva La Familia Study (VFS) which includes children and their siblings of ages 4 -19

4

Journal Pre-proof years [12,13]. By studying a mixed-age pediatric population, the results might be more generalizable to the broad pediatric population, instead of a smaller age range or puberty stage. Materials and Methods Study Population The Viva La Familia Study (VFS). The VFS is a family study designed to examine the genetic and environmental factors influencing obesity and its comorbidities in 1030 Hispanic

of

children (4-19y) from 319 families, enrolled in Houston, TX between November 2000 and

ro

August 2004, with details described previously [14]. Pedigrees were validated using genomic

-p

data. Phenotypic assessments were conducted over the course of 3 study visits. During the first

re

visit, interviews were conducted to obtain family pedigree, sociodemographic, lifestyle information, medical histories, and puberty stages. Anthropometric traits were assessed in both

lP

children and their parents.

na

BMC and BMD of skeletal sites were determined by DXA with a Delphi-A whole-body scanner (Hologic Inc., Waltham, MA, USA). We examined total body and lumbar spine bone

ur

sites as primary outcomes because these measures are the most reproducible skeletal sites for

Jo

BMC and BMD in children [15] . As hip BMD is recommended to measure to diagnose osteoporosis in adults [15], we also considered pelvis BMC and BMD in our children cohort as primary outcomes. Other skeletal sites (e.g. leg, arm) were examined as secondary outcomes. Left and right bone sites were considered separately due to limb bone bilateral asymmetry [16]. Written informed consent or assent was given by all enrolled children and their parents. The protocol was approved by the Institutional Review Boards for Human Subject Research at Baylor College of Medicine and Affiliated Hospitals, Texas Biomedical Research Institute and the analysis was approved by University of North Carolina at Chapel Hill.

5

Journal Pre-proof Genotyping Genotyping of Microsatellites for Genome-wide Linkage Analysis. Genotyping of microsatellites has been described in detail previously [17]. In short, DNA was prepared from whole blood with the Wizard Genomic DNA Purification Kit (Promega, Madison, WI, USA). Short tandem repeats (STR) that were spaced at an average interval of 10cM (range, 2.4-24.1), were genotyped for all participants. The autosomal markers used were from the ABI PRISM

of

Linkage Mapping Set-MD10 Version 2.5 (Applied Biosystems, Foster City, CA, USA).

ro

Polymerase chains reaction (PCR) was used to amplify each marker and the PCR products were

-p

pooled with others with a Robbins Hydra-384 microdispenser. The STRs were quantified using

re

fluorescent emissions by comparing with a standard, and the genotype scoring was performed using the genotype software package (Applied Biosystems). Pedigree errors were detected by

lP

PREST and Mendelian errors were detected by SIMWALK2 [18] . LOKI was used to compute

na

the identify-by-descent matrix for linkage analysis [19]. The chromosomal map was developed based on marker locations reported by deCODE Genetics [20].

ur

Genotyping of Common Variants. Genotyping for 1.1 million SNPs was conducted

Jo

using marker assays included on the Illumina HumanOmni1-Quad v1.0 BeadChip [21]. Genotype calls were obtained after scanning on the Illumina BeadStation 500GX and were analyzed using the GenomeStudio software. The genotyping error rate (based on duplicates) was 2 per 100,000 genotypes. The average call rate per individual sample was 97%. Specific markers were removed from analysis if they had call rates < 95% (~4000 SNPs) or deviated from HardyWeinberg equilibrium at a 5% false discovery rate (12 SNPs). Single nucleotide polymorphisms (SNP) genotypes were checked for Mendelian consistency using the program SimWalk2 [18].

6

Journal Pre-proof The estimates of allele frequencies and their standard errors were obtained using the software program Sequential Oligogenic Linkage Analysis Routines (SOLAR version 7.6.2) [22]. Whole Exome Sequencing and Genome Variant Identification. The custom NimbleGen VCRome 2.1 capture reagent was used to capture the entire exome for each DNA sample [23]. The reagent targets coding exons from the consensus coding sequence, Vega human genome annotations, and NCBI RNA reference sequences. Sequencing on the Illumina platform

of

using standard protocols followed capture enrichment and Illumina sequence analysis was

ro

conducted based on the Human Genome Sequencing Center’s integrated Mercury pipeline

-p

[24,25]. Burrows-Wheeler Aligner was used to map the sequencing reads to the GRCh37 human

re

reference sequence and the Atlas suite was used to call single-nucleotide variants. Variant annotation was accomplished using the Cassandra annotation suite. Quality control was

lP

performed using a custom pipeline, which followed the guidelines for the CHARGE-S project

Covariates Measurements

na

[26].

ur

Body weight was measured with a digital balance to the nearest 0.1 kg, and height was

Jo

measured to the nearest 1 mm with a stadiometer. BMI was calculated as kg/m2. BMI Z-score, a relative weight measure adjusted for age and sex, was determined using reference data from the Centers for Disease Control and Prevention (CDC) [27].Tanner stages of sexual maturation were self-reported based on pubic hair and breast and penis development illustrated with drawings. Puberty stages were categorized based on Tanner stages. Children in Tanner stage 1 were considered as “pre-pubertal” and children in other Tanner stages were considered as “pubertal”. Statistical analysis

7

Journal Pre-proof Linkage analysis. The variance components decomposition method was used to estimate heritability and identify the chromosomal location(s) affecting variation in bone outcomes. To estimate the genetic component in the variation of bone outcomes, heritability was estimated first. A multipoint linkage analysis was conducted to find a putative quantitative trait locus (QTL) or loci (QTLs) that affect bone outcomes [22]. The method has been described in detail elsewhere [22]. In brief, this is an extension of the variance components method where a QTL component is

of

added to the basic model. The correlations of phenotype within families were modeled as the

ro

cumulative effects of identity by descent (IBD) for the family at a specific QTL associated with a

-p

marker, with residual genetic and environmental effects. The model was adjusted for age, sex,

re

age2, age × sex, age2 × sex and BMI Z- score and binary puberty stages for the genome-wide linkage analysis. A logarithm of odds score (LOD) >3 was considered as significant and a LOD

lP

between 2 and 3 was considered as suggestive evidence for linkage. Further association analysis

na

was conducted with SNPs in the one-LOD support interval and relevant bone phenotypes.

association.

ur

Bonferroni correction was used for each one-LOD support interval to identify significance for

Jo

Genome-Wide Association Study (GWAS). A measured genotype analysis (MGA) approach was used to identify genetic loci associated with bone phenotypes. This approach accounts for both the random effects of kinship and the main effects of SNP genotypes [28]. Inverse normalization was used for all bone outcomes to ensure normality assumptions. Because BMI and puberty stages could affect bone density and bone content among children, the covariates age, sex, age*sex, age2, age2*sex, BMI Z-score, and binary puberty stage were included in the model [29]. In SOLAR, each SNP genotype was converted to 0, 1, or 2 based on the number of minor alleles. These were included in variance-components mixed models for

8

Journal Pre-proof MGA compared to null models which included the random effects of kinship and fixed effects of age and sex. The thresholds for genome-wide significant and suggestively significant association were based on the distribution of P values obtained from 10,000 simulation GWASs [21]. Each SNP was tested independently as a 1 degree of freedom likelihood ratio test with a P value threshold for significant evidence of association set at 1.01×10-7 and suggestive evidence at 1.0 ×10-6 [21]. The genome-wide P value threshold was computed accounting for kinships. A

of

quantitative transmission disequilibrium test was used to test for population stratification [30].

ro

Conditional analysis was then performed using an additive model for the remaining SNPs,

-p

conditioned on the previously identified genome-wide significant SNPs in the GWAS analysis.

re

The software SOLAR (version 7.6.2) was used for the statistical analysis [22]. Exome-Sequencing Association analysis. Single-variant association analysis was

lP

conducted using RVtest software [31]. All analyses used additive genetic models, and the

na

empirical pedigree information was transformed into a kinship matrix and included in the association analysis. Covariates used in this analysis were the same as those included in the

ur

GWAS. Principal component analysis (PCA) was conducted by the PC-AiR method in the

Jo

GENESIS package [32]. Population structure was accounted for by adding the top 10 PCs in the model. Single variant association score summary statistics and variant-specific parameters were generated. Single-variant analysis included variants with minor allele frequency (MAF) greater than or equal to 0.01. The significance level was calculated for each phenotype using a Bonferroni correction. SNP Lookups for Novel Loci Identified in VFS. To investigate if SNPs identified in our cohort associated with bone outcomes in multiple skeletal sites in childhood cohorts of other ethnicities and Hispanic adults, we performed a look-up of published pediatric cohort results

9

Journal Pre-proof from the Bone Mineral Density in Childhood Study (BMDCS) [8], and Hispanic adults cohort of the San Antonio Family Osteoporosis Study(SAFOS) [33]. Potential Functional Roles for Identified Loci. To examine the potential functional roles of identified loci, we looked up the SNPs in GTEx (https://gtexportal.org/home/) and eQTL Catalog (https://eqtl.onderzoek.io/) [34,35]. Results

of

A total of 1,030 children participated in the study (boys = 510, girls = 520). The mean

ro

age and BMI were 11.0 ± 4.1 y and 25.1 ± 7.6 kg/m2, respectively. The phenotype and genotype

-p

data were available for about 750 children. The heritabilities of BMC and BMD were significant

re

for all skeletal sites ranging from 0.44 to 0.68 (Table 1).

Linkage analyses are used to identify broad genomic regions that contain the putative

lP

disease loci. The genome-wide linkage analysis results are shown in Table 2 and Figure 1. The

na

most significant result was the linkage of pelvis BMD (LOD = 4.8) with genetic loci within the chromosomal region of 7p14 between markers D7S484 and D7S510, which was also linked with

ur

left leg BMD (LOD = 3.4). Other regions that were significantly linked with BMD were 20q13

Jo

for lumbar spine (LOD = 3.2) and 6p21 for left rib BMD (LOD = 3.0). For BMC, the best LOD score was obtained for pelvis BMC (LOD = 3.4) on chromosomal region of 20q12 followed by total body BMC (LOD = 3.0) on chromosomal region of 14q22. We also identified 10 loci with suggestive evidence of linkage at various chromosomal regions (2 < LOD ≤ 3) for different sites, with details shown in Table 2. To narrow down to smaller regions, association analyses were conducted in the identified statistically significant linkage regions (LOD > 3) for BMC or BMD. The rs6018245 at EYA Transcriptional Coactivator and Phosphatase 2 (EYA2) (β (SE) = -1.41 (0.32), P = 1×10-5) on 20q13.12 was found to be statistically significantly associated with pelvis

10

Journal Pre-proof BMC based on the extent of multiple testing correction applied. After accounting for rs6018245 on pelvis BMC in conditional linkage, the LOD score on pelvis BMC decreased from 3.4 to 2.4 on chromosome 20, indicating this SNP could explain about 29% of the variation of pelvis BMC. To complement linkage analysis with broad region identification, we also performed genome-wide association study (GWAS) to identify common variants, usually with smaller effects than linkage [36]. In GWAS, two significant loci (rs7000615 and rs762920) were

of

identified, with results for primary and secondary skeletal sites shown in Table 3 and

ro

Supplemental Table 1, respectively. The Manhattan plots and regional association plots for the

-p

two signals are shown in Figures 2 and 3 respectively. The SNP rs7000615 near the gene encoding protein tyrosine kinase 2 beta (PTK2B) was statistically significantly associated with

re

pelvis BMD (P = 7.4×10-8). In addition, multiple other SNPs at PTK2B also nominally

lP

associated with both pelvis BMC and BMD (Table 3). The SNP rs762920 was found to be

na

genome-wide statistically significantly associated with right arm BMC (P = 4.6×10-8) and it was also nominally significantly associated with left arm BMC (P = 1.8×10-7) and right leg BMC (P

ur

= 4.1×10-7) (Supplemental Table 1). In further conditional analysis to identify secondary signals,

Jo

no statistically significant or suggestive associations were observed. As GWASs are usually used to identify common variants, exome-wide association analysis was also used to examine exonic variants, which include low-frequency variants. After Bonferroni correction, the P value significance level was 9.2 × 10-7. The exome-wide association results for primary and secondary skeletal sites are shown in Table 4 and Supplemental Table 2, respectively. We observed three novel statistically significant associations including one synonymous variant rs2303611 in the gene encoding abraxas 2 BRISC complex subunit (ABRAXAS2) with lumbar spine BMC (Table 4) and two missense variants rs17164935 (P =

11

Journal Pre-proof 5.8×10-7) and rs3812054 (P = 8.9×10-7) near gene encoding ‘multiple EGF like domains 10’ (MEGF10) associated with left arm BMC (Supplemental Table 2). To investigate whether SNPs identified in VFS were associated with any skeletal sites BMD or BMC in other studies, we performed SNP look-ups in one pediatric cohort BMDCS and a Hispanic adults cohort SAFOS (Table 5). Two SNPs (rs17164935 and rs3812054) were not available in BMDCS and rs762920 was not available in SAFOS. Results of SNPs that were

of

available in both cohorts (rs7000615 and rs2303611) are shown in Table 7. In SAFOS,

ro

rs7000615 was nominally associated with Ward’s triangle BMD (P = 0.049) and Ward’s triangle

-p

BMC (P = 0.045) and the directions were consistent with the initial observations. No evidence of

re

suggestive or significant evidence of association was found in BMDCS. With further investigations in the GTEx and eQTL catalog, SNP rs7000615 at PTK2B

lP

was found to be cis-regulated in testis tissue in GTEx and eQTL Catalog, while no eQTL

na

information was available for rs762920 at PVALB. In GTEx, SNP rs2303611 at ABRAXAS2, rs17164935 and rs3812054 was found to be cis-regulated in multiple tissues including muscle-

Discussion

Jo

SNPs in eQTL Catalog.

ur

skeletal tissue, but no significant evidence was found for cis or trans-regulation for these three

Our genome-wide linkage and association studies identified several novel loci for BMD and BMC, with stronger evidence on rs7000615 at PTK2B. Our findings support the site-specific genetic effects on BMD and BMC. Significant linkages for BMD and BMC were found at 7p, 20q, 6p and 14q for different skeletal sites. Further examination of SNP association under the linkage peak yielded a significant variant, rs6018245 at EYA2, after Bonferroni correction. In genome-wide and exome-wide association analysis, we found five novel loci: rs762920 (PVALB)

12

Journal Pre-proof with right arm BMC and rs7000615 (PTK2B) with pelvis BMD, rs17164935 (MEGF10) and rs3812054 (MEGF10) with left arm BMC, and rs2303611 (ABRAXAS2) with lumbar spine BMC. Moreover, rs7000615 (PTK2B) was found to be suggestively associated with BMD in SAFOS with directional consistency, and to be cis-regulated in both GTEx and eQTL Catalog, indicating the potential functional roles of this locus. The exonic SNPs rs17164935, rs3812054 and rs2303611 were also cis-regulated in multiple tissues based on GTEx.

of

The significant linkage regions identified in our study were previously reported in

ro

literature, which increases confidence in our findings. The highest linkage peak observed on

-p

7p14.2-7p14.1 has been previously linked to lumbar spine and femoral neck BMD in Caucasians

re

[37,38], and total hip BMD in Chinese populations [39]. The chromosome 20q12-q13 region was also linked to BMD and bone geometry in Europeans [38,40,41]. The chromosome 14q22-q23

lP

and 6p21-6p12, were linked to femoral neck BMD in younger Amish populations [42,43] and

na

lumbar spine BMD in Caucasians [10,44]. The linkage regions were identified in various populations, suggesting these broad regions harbor important genes related to bone health across

ur

races. However, as many bone-related genes could be located in the same linkage region, the

Jo

specific genes or genetic variants on identified linkage regions could still be race-specific, which could be identified in smaller regions by association analysis. In further association analysis under the linkage peaks, SNP rs6018245 at the EYA2 locus on chromosome 20 was significantly associated with pelvic BMC and the linkage signal was not significant after adjusting for rs6018245 in conditional linkage, suggesting EYA2 is the functional gene. The EYA2 locus was associated with heel BMD in Europeans of UK Biobank but the reported SNPs were not available in our data [45,46]. It is possible that there is a different tag or locus heterogeneity as we investigated in Hispanic population, rather than Europeans.

13

Journal Pre-proof In genome-wide and exome-wide association analysis, four novel genes, PTK2B, PVALB, MEGF10 and ABRAXAS2, were identified in association with BMD or BMC. The SNP rs7000615 (PTK2B) was genome-wide significantly associated with pelvis BMD in Hispanic children of VFS and suggestively associated with BMC and BMD in Hispanic adults of SAFOS, but not in Caucasian/African Americans of BMDCS. It is possible that this SNP is ethnicspecific since VFS and SAFOS are both primarily Hispanic/Mexican American population but

of

more studies are needed to confirm this possibility. There was also evidence in GTEx and eQTL

ro

catalog shown that rs7000615 was cis-regulated, suggesting the functional role of this locus.

-p

Biologically, PTK2B has been found to have a role in osteoclast maturation and bone resorption

re

in vitro, and PTK2B/PYK2 inhibitors might be used to treat osteoporosis based on findings from mice studies [47]. PVALB and MEFG10 are also biologically relevant to bone metabolism.

lP

PVALB is a high affinity calcium ion-binding protein and one study in Pvalb knockout mice

na

found that the lack of parvalbumin is associated with stronger bones and abnormal calcium handling [48] and MEGF10 is a Runx2-responsive genes that is related to osteoblast proliferation

ur

[49]. ABRAXAS2 is involved in processes related to protein metabolism, deubiquitination

Jo

pathways, and myocardial infarction [50], but the mechanism underlying its relationship with bone health is still unknown. The identified genes in GWAS and exome-wide association analysis were not overlapped mainly due to the fact of variants sequenced are different. The majority of GWAS identified SNPs are intronic, while exome-wide analysis could complement GWAS results with exonic variants [51]. Our study has a few limitations. First, the sample size is small and may suffer from insufficient power and a high false discovery rate, which are potential problems for genome-wide scans [52]. We also had limited ability to detect rare variants (MAF < 0.01) due to small sample

14

Journal Pre-proof size. Second, the identified SNPs may not be causal and could be in LD with the underlying causal variants and we also do not provide definitive biological mechanisms of the association found in our study. Future studies on potential functional SNPs with gene expression and translational studies are needed to elucidate the findings. Third, DXA-derived measurement may poorly capture the effects of genetic variants on bone structure and geometry, which are also important aspects for bone health [53]. Moreover, there could be residual confounding that is not

of

accounted for, therefore future studies on mechanisms and function are needed to confirm the

ro

findings. Finally, obesity can impact BMD and BMC, especially as our cohort was made up of

-p

about two-thirds of children who were overweight/obese, which may limit our generalizability

re

[54]. However, about one-third of children were normal-weight and the analysis was adjusted for BMI Z-score to account for the effects of obesity on bone outcomes.

lP

Our study also has several strengths. This study examining genetic variation underlying

na

BMD and BMC is novel and fills the knowledge gaps in three prospective. First, the study was conducted in Hispanic population, which is understudied compared to Europeans and provides

ur

opportunity to identify novel variants as well as support for early identified variants[55]. Second,

Jo

the study was conducted in children with bone accrual playing a main role and less environmental influence accumulated compared to adults, and a few novel loci related to BMD were only identified in pediatric GWAS studies. The discovery of variants associated with peak bone mass might be used to predict osteoporosis risk as adult. Third, as site specificity of genetics on BMD were found [56–58], multiple skeletal sites were examined to identify novel loci and better understand the genetic heterogeneity of different effects on BMD or BMC. Besides novelty, another strength is that we used a combination of genome-wide linkage and association (genome-wide and exome-wide) analyses approaches. Linkage studies with family

15

Journal Pre-proof data can find larger genomic regions while association analysis could narrow down to smaller regions. Also, linkage in families may be able to detect rare variants, while genome-wide and exome-wide association could identify common and low frequency variants. Finally, we use both BMD and BMC to assess pediatric bone health, where areal BMD values may better reflect bone matrix mineralization and BMC may better capture volumetric bone mass [59]. In summary, our study is the first genome-wide linkage scan, with GWAS and exome-

of

wide analysis to examine underlying genetic loci associated with BMD and BMC in Hispanic

ro

children. Our findings provide insights into the biological mechanism underlying BMD and

-p

BMC in Hispanic children. The genetic loci identified may be used to predict osteoporosis risk in

re

adults and contribute to identification of new drug targets for osteoporosis prevention and treatment. Further functional studies and replication studies are warranted to elucidate the precise

Ethical standards

na

lP

biological mechanisms and to validate our findings.

ur

Written informed consent or assent was given by all enrolled children and their parents from the

Jo

Viva La Familia Study. The protocol was approved by the Institutional Review Boards for Human Subject Research at Baylor College of Medicine and Affiliated Hospitals, Texas Biomedical Research Institute and the analysis was approved by University of North Carolina at Chapel Hill.

Funding The Viva La Familia Study was supported by NIH DK080457 and USDA/Agricultural Research Service (Corporative agreement 625-51000-053). The development of SOLAR was supported by

16

Journal Pre-proof NIH grant MH59490. This work was supported by the National Institutes of Health R01 DK092238 to VSV, R01 HD58886 to BZ and SG; American Diabetes Association Grant 1-17PDF-077 (to DC); and the Institute for Translational Medicine and Therapeutics (ITMAT) Transdisciplinary Program in Translational Medicine and Therapeutics (to DC and SG). Dr. Grant is funded by the Daniel B. Burke Endowed Chair for Diabetes Research. We thank the participants of the Viva la Familia Study for their extraordinary cooperation and involvement in

of

this project.

Jo

ur

na

lP

re

-p

All authors state that they have no conflicts of interest

ro

Conflict of interest

17

Journal Pre-proof References [1]

N.C. Wright, A.C. Looker, K.G. Saag, R. Jeffrey, J.R. Curtis, E.S. Delzell, S. Randall, B. Dawson-Hughes, The recent prevalence of osteoporosis and low bone mass in the United States based on bone mineral density at the femoral neck or lumbar spine, J. Bone Miner. Res. 29 (2014) 2520–2526.

[2]

R. Burge, B. Dawson-Hughes, D.H. Solomon, J.B. Wong, A. King, A. Tosteson,

J.B. Richards, H.-F. Zheng, T.D. Spector, Genetics of osteoporosis from genome-wide

-p

[3]

ro

2005-2025, J. Bone Miner. Res. 22 (2007) 465–475.

of

Incidence and Economic Burden of Osteoporosis-Related Fractures in the United States,

re

association studies: advances and challenges, Nat. Rev. Genet. 13 (2012) 576–588. http://www.nature.com/doifinder/10.1038/nrg3228. J.M. Kaufman, A. Ostertag, A. Saint-Pierre, M. Cohen-Solal, A. Boland, I. Van

lP

[4]

na

Pottelbergh, K. Toye, M.C. De Vernejoul, M. Martinez, Genome-wide linkage screen of bone mineral density (BMD) in European pedigrees ascertained through a male relative

ur

with low BMD values: Evidence for quantitative trait loci on 17q21-23, 11q12-13, 13q12-

[5]

Jo

14, and 22q11, J. Clin. Endocrinol. Metab. 93 (2008) 3755–3762. J.A. Morris, J.P. Kemp, S.E. Youlten, L. Laurent, J.G. Logan, R.C. Chai, N.A. Vulpescu, V. Forgetta, A. Kleinman, S.T. Mohanty, An atlas of genetic influences on osteoporosis in humans and mice, Nat. Genet. 51 (2019) 258. [6]

S.E. McCormack, D.L. Cousminer, A. Chesi, J.A. Mitchell, S.M. Roy, H.J. Kalkwarf, J.M. Lappe, V. Gilsanz, S.E. Oberfield, J.A. Shepherd, K.K. Winer, A. Kelly, S.F.A. Grant, B.S. Zemel, Association between linear growth and bone accrual in a diverse cohort of children and adolescents, JAMA Pediatr. 171 (2017) 1–9.

18

Journal Pre-proof [7]

C. Medina-Gomez, J.P. Kemp, K. Trajanoska, J. Luan, A. Chesi, T.S. Ahluwalia, D.O. Mook-Kanamori, A. Ham, F.P. Hartwig, D.S. Evans, R. Joro, I. Nedeljkovic, H.F. Zheng, K. Zhu, M. Atalay, C.T. Liu, M. Nethander, L. Broer, G. Porleifsson, B.H. Mullin, S.K. Handelman, M.A. Nalls, L.E. Jessen, D.H.M. Heppe, J.B. Richards, C. Wang, B. Chawes, K.E. Schraut, N. Amin, N. Wareham, D. Karasik, N. Van der Velde, M.A. Ikram, B.S. Zemel, Y. Zhou, C.J. Carlsson, Y. Liu, F.E. McGuigan, C.G. Boer, K. Bønnelykke, S.H.

of

Ralston, J.A. Robbins, J.P. Walsh, M.C. Zillikens, C. Langenberg, R. Li-Gao, F.M.K.

ro

Williams, T.B. Harris, K. Akesson, R.D. Jackson, G. Sigurdsson, M. den Heijer, B.C.J.

-p

van der Eerden, J. van de Peppel, T.D. Spector, C. Pennell, B.L. Horta, J.F. Felix, J.H.

re

Zhao, S.G. Wilson, R. de Mutsert, H. Bisgaard, U. Styrkársdóttir, V.W. Jaddoe, E. Orwoll, T.A. Lakka, R. Scott, S.F.A. Grant, M. Lorentzon, C.M. van Duijn, J.F. Wilson, K.

lP

Stefansson, B.M. Psaty, D.P. Kiel, C. Ohlsson, E. Ntzani, A.J. van Wijnen, V. Forgetta, M.

na

Ghanbari, J.G. Logan, G.R. Williams, J.H.D. Bassett, P.I. Croucher, E. Evangelou, A.G. Uitterlinden, C.L. Ackert-Bicknell, J.H. Tobias, D.M. Evans, F. Rivadeneira, Life-Course

ur

Genome-wide Association Study Meta-analysis of Total Body BMD and Assessment of

[8]

Jo

Age-Specific Effects, Am. J. Hum. Genet. 102 (2018) 88–102. A. Chesi, J.A. Mitchell, H.J. Kalkwarf, J.P. Bradfield, J.M. Lappe, D.L. Cousminer, S.M. Roy, S.E. McCormack, V. Gilsanz, S.E. Oberfield, H. Hakonarson, J.A. Shepherd, A. Kelly, B.S. Zemel, S.F.A. Grant, A Genomewide Association Study Identifies Two SexSpecific Loci, at SPTB and IZUMO3, Influencing Pediatric Bone Mineral Density at Multiple Skeletal Sites, J. Bone Miner. Res. 32 (2017) 1274–1281. [9]

J.A. Mitchell, D.L. Cousminer, B.S. Zemel, S.F.A. Grant, A. Chesi, Genetics of pediatric bone strength, Bonekey Rep. 5 (2016) 1–6.

19

Journal Pre-proof [10] C. Medina-Gomez, J.P. Kemp, K. Estrada, J. Eriksson, J. Liu, S. Reppe, D.M. Evans, D.H.M.M. Heppe, L. Vandenput, L. Herrera, S.M. Ring, C.J. Kruithof, N.J. Timpson, M.C. Zillikens, O.K. Olstad, H.F. Zheng, J.B. Richards, B. St. Pourcain, A. Hofman, V.W.V. V Jaddoe, G.D. Smith, M. Lorentzon, K.M. Gautvik, A.G. Uitterlinden, R. Brommage, C. Ohlsson, J.H. Tobias, F. Rivadeneira, Meta-analysis of genome-wide scans for total body BMD in children and adults reveals allelic heterogeneity and age-specific

of

effects at the WNT16 locus, PLoS Genet. 8 (2012) e1002718.

ro

[11] N.J. Timpson, J.H. Tobias, J.B. Richards, N. Soranzo, E.L. Duncan, A.M. Sims, P.

-p

Whittaker, V. Kumanduri, G. Zhai, B. Glaser, J. Eisman, G. Jones, G. Nicholson, R.

re

Prince, E. Seeman, T.D. Spector, M.A. Brown, L. Peltonen, G.D. Smith, P. Deloukas, D.M. Evans, Common variants in the region around Osterix are associated with bone

lP

mineral density and growth in childhood, Hum. Mol. Genet. 18 (2009) 1510–1517.

na

[12] S.S. Wildman, M.J. Henwood-finley, Pediatric DXA: A Review of Proper Technique and Correct Interpretation, J. Am. Coll. Radiol. 1 (2012) 17–26.

ur

[13] A. G. Comuzzie, S. A. Cole, S.L. Laston, V.S. Voruganti, K. Haack, R.A. Gibbs,

Jo

N.F.Butte. Novel genetic loci identified for the pathophysiology of childhood obesity in the Hispanic population, PLoS One. 7 (2012) e51954 [14] N.F. Butte, G.W. Cai, S.A. Cole, A.G. Comuzzie, Viva la Familia Study: genetic and environmental contributions to childhood obesity and its comorbidities in the Hispanic population, Am. J. Clin. Nutr. 84 (2006) 646–654. [15] E.M. Lewiecki, C.M. Gordon, S. Baim, N. Binkley, J.P. Bilezikian, D.L. Kendler, D.B. Hans, S. Silverman, N.J. Bishop, M.B. Leonard, M.L. Bianchi, H.J. Kalkwarf, C.B. Langman, H. Plotkin, F. Rauch, B.S. Zemel, Special report on the 2007 adult and pediatric

20

Journal Pre-proof Position Development Conferences of the International Society for Clinical Densitometry, Osteoporos. Int. 19 (2008) 1369–1378. [16] B.M. Auerbach, C.B. Ruff, Limb bone bilateral asymmetry: Variability and commonality among modern humans, J. Hum. Evol. 50 (2006) 203–218. [17] V.S. Voruganti, H.H.H. Göring, V.P. Diego, G. Cai, N.R. Mehta, K. Haack, S.A. Cole, N.F. Butte, A.G. Comuzzie, Genome-wide scan for serum ghrelin detects linkage on

of

chromosome 1p36 in Hispanic children: Results from the Viva La Familia study, Pediatr.

ro

Res. 62 (2007) 445–450.

-p

[18] E. Sobel, K. Lange, Descent graphs in pedigree analysis: applications to haplotyping,

re

location scores, and marker-sharing statistics., Am. J. Hum. Genet. 58 (1996) 1323. [19] S.C. Heath, Markov chain Monte Carlo segregation and linkage analysis for oligogenic

lP

models., Am. J. Hum. Genet. 61 (1997) 748.

na

[20] A. Kong, D.F. Gudbjartsson, J. Sainz, G.M. Jonsdottir, S.A. Gudjonsson, B. Richardsson, S. Sigurdardottir, J. Barnard, B. Hallbeck, G. Masson, A high-resolution recombination

ur

map of the human genome, Nat. Genet. 31 (2002) 241.

Jo

[21] V.S. Voruganti, S. Laston, K. Haack, N.R. Mehta, S.A. Cole, N.F. Butte, A.G. Comuzzie, Serum uric acid concentrations and SLC2A9 genetic variation in Hispanic children: the Viva La Familia Study, Am. J. Clin. Nutr. April. 101 (2015) 725–732. [22] L. Almasy, J. Blangero, Multipoint quantitative-trait linkage analysis in general pedigrees, Am. J. Hum. Genet. 62 (1998) 1198–1211. [23] A. Sabo, P. Mishra, S. Dugan-Perez, V.S. Voruganti, J.W. Kent, D. Kalra, S.A. Cole, A.G. Comuzzie, D.M. Muzny, R.A. Gibbs, N.F. Butte, Exome sequencing reveals novel genetic loci influencing obesity-related traits in Hispanic children, Obesity. 25 (2017) 1270–1276.

21

Journal Pre-proof [24] J.G. Reid, A. Carroll, N. Veeraraghavan, M. Dahdouli, A. Sundquist, A. English, M. Bainbridge, S. White, W. Salerno, C. Buhay, Launching genomics into the cloud: deployment of Mercury, a next generation sequence analysis pipeline, BMC Bioinformatics. 15 (2014) 30. [25] M.N. Bainbridge, M. Wang, Y. Wu, I. Newsham, D.M. Muzny, J.L. Jefferies, T.J. Albert, D.L. Burgess, R.A. Gibbs, Targeted enrichment beyond the consensus coding DNA

of

sequence exome reveals exons with higher variant densities, Genome Biol. 12 (2011) R68.

ro

[26] B. Yu, S.L. Pulit, S.-J. Hwang, J.A. Brody, N. Amin, P.L. Auer, J.C. Bis, E. Boerwinkle,

-p

G.L. Burke, A. Chakravarti, Rare exome sequence variants in CLCN6 reduce blood

re

pressure levels and hypertension risk, Circ. Genomic Precis. Med. (2015) CIRCGENETICS-115.

lP

[27] R.J. Kuczmarski, C.L. Ogden, L.M. Grummer-Strawn, K.M. Flegal, S.S. Guo, R. Wei, Z.

Data. (2000) 1–27.

na

Mei, L.R. Curtin, A.F. Roche, C.L. Johnson, CDC growth charts: United States., Adv.

ur

[28] E. Boerwinkle, R. Chakraborty, C.F. Sing, The use of measured genotype information in

Jo

the analysis of quantitative phenotypes in man, Ann. Hum. Genet. 50 (1986) 181–194. [29] H. Aschard, B.J. Vilhjálmsson, A.D. Joshi, A.L. Price, P. Kraft, Adjusting for heritable covariates can bias effect estimates in genome-wide association studies, Am. J. Hum. Genet. 96 (2015) 329–339. doi:10.1016/j.ajhg.2014.12.021. [30] L.M. Havill, T.D. Dyer, D.K. Richardson, M.C. Mahaney, J. Blangero, The quantitative trait linkage disequilibrium test: a more powerful alternative to the quantitative transmission disequilibrium test for use in the absence of population stratification, BMC Genet. 6 (2005) S91.

22

Journal Pre-proof [31] X. Zhan, Y. Hu, B. Li, G.R. Abecasis, D.J. Liu, RVTESTS: An efficient and comprehensive tool for rare variant association analysis using sequence data, Bioinformatics. 32 (2016) 1423–1426. [32] M.P. Conomos, M.B. Miller, T.A. Thornton, Robust inference of population structure for ancestry prediction and correction of stratification in the presence of relatedness, Genet. Epidemiol. 39 (2015) 276–293.

of

[33] R.L. Mitchell, B.D., Kammerer, C.M., Schneider, J.L., Perez, R. and Bauer, B.D. Mitchell,

ro

C.M. Kammerer, J.L. Schneider, R. Perez, R.L. Bauer, Genetic and environmental

-p

determinants of bone mineral density in Mexican Americans: Results from the San

re

Antonio Family Osteoporosis Study, Bone. 33 (2003) 839–846. [34] R. Jansen, J.-J. Hottenga, M.G. Nivard, A. Abdellaoui, B. Laport, E.J. de Geus, F.A.

lP

Wright, B.W.J.H. Penninx, D.I. Boomsma, Conditional eQTL analysis reveals allelic

na

heterogeneity of gene expression, Hum. Mol. Genet. 26 (2017) 1444–1451. [35] J. Lonsdale, J. Thomas, M. Salvatore, R. Phillips, E. Lo, S. Shad, R. Hasz, G. Walters, F.

Jo

580.

ur

Garcia, N. Young, The genotype-tissue expression (GTEx) project, Nat. Genet. 45 (2013)

[36] N.M. Laird, C. Lange, Family‐ based methods for linkage and association analysis, Adv. Genet. 60 (2008) 219–252. [37] H. Shen, Y.Y. Zhang, J.R. Long, F.H. Xu, Y.Z. Liu, P. Xiao, L.J. Zhao, D.H. Xiong, Y.J. Liu, V. Dvornyk, S. Rocha-Sanchez, P.Y. Liu, J.L. Li, T. Conway, K.M. Davies, R.R. Recker, H.W. Deng, A genome-wide linkage scan for bone mineral density in an extended sample: Evidence for linkage on 11q23 and Xq27, J. Med. Genet. 41 (2004) 743–751. [38] S.H. Ralston, N. Galwey, I. Mackay, O.M.E. Albagha, L. Cardon, J.E. Compston, C.

23

Journal Pre-proof Cooper, E. Duncan, R. Keen, B. Langdahl, A. McLellan, J. O’Riordan, H.A. Pols, D.M. Reid, A.G. Uitterlinden, J. Wass, S.T. Bennett, Loci for regulation of bone mineral density in men and women identified by genome wide linkage scan: The FAMOS study, Hum. Mol. Genet. 14 (2005) 943–951. [39] H.Y.G. Li, W.C.A. Kung, Q.Y. Huang, Bone mineral density is linked to 1p36 and 7p1513 in a southern Chinese population, J. Bone Miner. Metab. 29 (2011) 80–87.

of

[40] Y.H. Lee, Y.H. Rho, S.J. Choi, J.D. Ji, G.G. Song, Meta-analysis of genome-wide linkage

ro

studies for bone mineral density, J. Hum. Genet. 51 (2006) 480–486.

-p

[41] D.H. Xiong, H. Shen, P. Xiao, Y.F. Guo, J.R. Long, L.J. Zhao, Y.Z. Liu, H.Y. Deng, J.L.

re

Li, R.R. Recker, H.W. Deng, Genome-wide scan identified QTLs underlying femoral neck

Res. 21 (2006) 424–437.

lP

cross-sectional geometry that are novel studied risk factors of osteoporosis, J. Bone Miner.

na

[42] J.P. Ioannidis, M.Y. Ng, P.C. Sham, E. Zintzaras, C.M. Lewis, H.-W. Deng, M.J. Econs, D. Karasik, M. Devoto, C.M. Kammerer, T. Spector, T. Andrew, L.A. Cupples, E.L.

ur

Duncan, T. Foroud, D.P. Kiel, D. Koller, B. Langdahl, B.D. Mitchell, M. Peacock, R.

Jo

Recker, H. Shen, K. Sol-Church, L.D. Spotila, A.G. Uitterlinden, S.G. Wilson, A.W. Kung, S.H. Ralston, Meta-Analysis of Genome-Wide Scans Provides Evidence for Sexand Site-Specific Regulation of Bone Mass, J. Bone Miner. Res. 22 (2006) 173–183. http://doi.wiley.com/10.1359/jbmr.060806. [43] E.A. Streeten, D.J. McBride, T.I. Pollin, K. Ryan, J. Shapiro, S. Ott, B.D. Mitchell, A.R. Shuldiner, J.R. O’Connell, Quantitative trait loci for BMD identified by autosome-wide linkage scan to chromosomes 7q and 21q in men from the Amish Family Osteoporosis Study, J. Bone Miner. Res. 21 (2006) 1433–1442.

24

Journal Pre-proof [44] D.L. Koller, G. Liu, M.J. Econs, P.A. Morin, J.C. Christian, S.L. Hui, L.A. Rodriguez, P.M. Conneally, G. Joslyn, C.C. Johnston, T. Foroud, M. Peacock, Genome screen for QTLs contributing to normal variation in femoral structure and risk for osteoporotic fracture., J. Bone Miner. Res. 15 (2000) S162–S162. [45] S.K. Kim, Identification of 613 new loci associated with heel bone mineral density and a polygenic risk score for bone mineral density, osteoporosis and fracture, PLoS One. 13

of

(2018) 1–20.

ro

[46] J.P. Kemp, J.A. Morris, C. Medina-Gomez, V. Forgetta, N.M. Warrington, S.E. Youlten, J.

-p

Zheng, C.L. Gregson, E. Grundberg, K. Trajanoska, J.G. Logan, A.S. Pollard, P.C.

re

Sparkes, E.J. Ghirardello, R. Allen, V.D. Leitch, N.C. Butterfield, D. Komla-Ebri, A.T. Adoum, K.F. Curry, J.K. White, F. Kussy, K.M. Greenlaw, C. Xu, N.C. Harvey, C.

lP

Cooper, D.J. Adams, C.M.T. Greenwood, M.T. Maurano, S. Kaptoge, F. Rivadeneira, J.H.

na

Tobias, P.I. Croucher, C.L. Ackert-Bicknell, J.H.D. Bassett, G.R. Williams, J.B. Richards, D.M. Evans, Identification of 153 new loci associated with heel bone mineral density and

ur

functional involvement of GPC6 in osteoporosis, Nat. Genet. 49 (2017) 1468–1475.

Jo

[47] L. Buckbinder, D.T. Crawford, H. Qi, H.Z. Ke, L.M. Olson, K.R. Long, P.C. Bonnette, A.P. Baumann, J.E. Hambor, W.A. Grasser, Proline-rich tyrosine kinase 2 regulates osteoprogenitor cells and bone formation, and offers an anabolic treatment approach for osteoporosis, Proc. Natl. Acad. Sci. 104 (2007) 10619–10624. [48] E. Riveira-Munoz, O. Devuyst, H. Belge, N. Jeck, L. Strompf, R. Vargas-Poussou, X. Jeunemaître, A. Blanchard, N. V Knoers, M. Konrad, Evaluating PVALB as a candidate gene for SLC12A3-negative cases of Gitelman’s syndrome, Nephrol. Dial. Transplant. 23 (2008) 3120–3125.

25

Journal Pre-proof [49] S.K. Baniwal, P.K. Shah, Y. Shi, J.H. Haduong, Y.A. DeClerck, Y. Gabet, B. Frenkel, Runx2 promotes both osteoblastogenesis and novel osteoclastogenic signals in ST2 mesenchymal progenitor cells, Osteoporos. Int. 23 (2012) 1399–1413. [50] L. Cilenti, M.P. Balakrishnan, X.-L. Wang, C. Ambivero, M. Sterlicchi, F. del Monte, X.L. Ma, A.S. Zervos, Regulation of Abro1/KIAA0157 during myocardial infarction and cell death reveals a novel cardioprotective mechanism for Lys63-specific deubiquitination, J.

of

Mol. Cell. Cardiol. 50 (2011) 652–661.

ro

[51] K.N. Lazaridis, A.C. Cheung, Whole exome sequencing leading to novel therapeutic

-p

discovery, Gastroenterology. 155 (2018) 1264–1265.

re

[52] J. Altmüller, L.J. Palmer, G. Fischer, H. Scherb, M. Wjst, Genomewide Scans of Complex Human Diseases: True Linkage Is Hard to Find, Am. J. Hum. Genet. 69 (2002) 936–950.

lP

[53] R.M. Daly, M.A. Petit, Optimizing bone mass and strength: the role of physical activity

na

and nutrition during growth, 2007.

[54] B.A. Gower, K. Casazza, Divergent Effects of Obesity on Bone Health, J. Clin. Densitom.

ur

16 (2013) 450–454.

Jo

[55] M.I. McCarthy, G.R. Abecasis, L.R. Cardon, D.B. Goldstein, J. Little, J.P.A. Ioannidis, J.N. Hirschhorn, Genome-wide association studies for complex traits: consensus, uncertainty and challenges, Nat. Rev. Genet. 9 (2008) 356–369. [56] K. Estrada, U. Styrkarsdottir, E. Evangelou, Y.-H. Hsu, E.L. Duncan, E.E. Ntzani, L. Oei, O.M.E. Albagha, N. Amin, J.P. Kemp, D.L. Koller, G. Li, C.-T. Liu, R.L. Minster, A. Moayyeri, L. Vandenput, D. Willner, S.-M. Xiao, L.M. Yerges-Armstrong, H.-F. Zheng, N. Alonso, J. Eriksson, C.M. Kammerer, S.K. Kaptoge, P.J. Leo, G. Thorleifsson, S.G. Wilson, J.F. Wilson, V. Aalto, M. Alen, A.K. Aragaki, T. Aspelund, J.R. Center, Z.

26

Journal Pre-proof Dailiana, D.J. Duggan, M. Garcia, N. Garcia-Giralt, S. Giroux, G. Hallmans, L.J. Hocking, L.B. Husted, K.A. Jameson, R. Khusainova, G.S. Kim, C. Kooperberg, T. Koromila, M. Kruk, M. Laaksonen, A.Z. Lacroix, S.H. Lee, P.C. Leung, J.R. Lewis, L. Masi, S. MencejBedrac, T. V Nguyen, X. Nogues, M.S. Patel, J. Prezelj, L.M. Rose, S. Scollen, K. Siggeirsdottir, A. V Smith, O. Svensson, S. Trompet, O. Trummer, N.M. van Schoor, J. Woo, K. Zhu, S. Balcells, M.L. Brandi, B.M. Buckley, S. Cheng, C. Christiansen, C.

of

Cooper, G. Dedoussis, I. Ford, M. Frost, D. Goltzman, J. González-Macías, M. Kähönen,

ro

M. Karlsson, E. Khusnutdinova, J.-M. Koh, P. Kollia, B.L. Langdahl, W.D. Leslie, P. Lips,

-p

Ö. Ljunggren, R.S. Lorenc, J. Marc, D. Mellström, B. Obermayer-Pietsch, J.M. Olmos, U.

re

Pettersson-Kymmer, D.M. Reid, J.A. Riancho, P.M. Ridker, F. Rousseau, P.E.S. Lagboom, N.L.S. Tang, R. Urreizti, W. Van Hul, J. Viikari, M.T. Zarrabeitia, Y.S. Aulchenko, M.

lP

Castano-Betancourt, E. Grundberg, L. Herrera, T. Ingvarsson, H. Johannsdottir, T. Kwan,

na

R. Li, R. Luben, C. Medina-Gómez, S. Th Palsson, S. Reppe, J.I. Rotter, G. Sigurdsson, J.B.J. van Meurs, D. Verlaan, F.M.K. Williams, A.R. Wood, Y. Zhou, K.M. Gautvik, T.

ur

Pastinen, S. Raychaudhuri, J.A. Cauley, D.I. Chasman, G.R. Clark, S.R. Cummings, P.

Jo

Danoy, E.M. Dennison, R. Eastell, J.A. Eisman, V. Gudnason, A. Hofman, R.D. Jackson, G. Jones, J.W. Jukema, K.-T. Khaw, T. Lehtimäki, Y. Liu, M. Lorentzon, E. McCloskey, B.D. Mitchell, K. Nandakumar, G.C. Nicholson, B.A. Oostra, M. Peacock, H.A.P. Pols, R.L. Prince, O. Raitakari, I.R. Reid, J. Robbins, P.N. Sambrook, P.C. Sham, A.R. Shuldiner, F.A. Tylavsky, C.M. van Duijn, N.J. Wareham, L.A. Cupples, M.J. Econs, D.M. Evans, T.B. Harris, A.W.C. Kung, B.M. Psaty, J. Reeve, T.D. Spector, E.A. Streeten, M.C. Zillikens, U. Thorsteinsdottir, C. Ohlsson, D. Karasik, J.B. Richards, M.A. Brown, K. Stefansson, A.G. Uitterlinden, S.H. Ralston, J.P.A. Ioannidis, D.P. Kiel, F. Rivadeneira,

27

Journal Pre-proof Genome-wide meta-analysis identifies 56 bone mineral density loci and reveals 14 loci associated with risk of fracture, Nat. Genet. 44 (2012) 491–501. [57] J.P. Kemp, C. Medina-Gomez, K. Estrada, B. St Pourcain, D.H.M. Heppe, N.M. Warrington, L. Oei, S.M. Ring, C.J. Kruithof, N.J. Timpson, L.E. Wolber, S. Reppe, K. Gautvik, E. Grundberg, B. Ge, B. van der Eerden, J. van de Peppel, M.A. Hibbs, C.L. Ackert-Bicknell, K. Choi, D.L. Koller, M.J. Econs, F.M.K. Williams, T. Foroud, M.

of

Carola Zillikens, C. Ohlsson, A. Hofman, A.G. Uitterlinden, G. Davey Smith, V.W.V.

ro

Jaddoe, J.H. Tobias, F. Rivadeneira, D.M. Evans, Phenotypic Dissection of Bone Mineral

-p

Density Reveals Skeletal Site Specificity and Facilitates the Identification of Novel Loci

re

in the Genetic Regulation of Bone Mass Attainment, PLoS Genet. 10 (2014). [58] J.A. Mitchell, A. Chesi, D.L. Cousminer, S.E. Mccormack, H.J. Kalkwarf, J.M. Lappe, V.

lP

Gilsanz, S.E. Oberfield, J.A. Shepherd, A. Kelly, B.S. Zemel, S.F. Grant,

na

Multidimensional Bone Density Phenotyping Reveals New Insights Into Genetic Regulation of the Pediatric Skeleton, J. Bone Miner. Res. 33 (2018) 812–821.

ur

[59] L.A. Binkovitz, M.J. Henwood, Pediatric DXA: Technique and interpretation, Pediatr.

Jo

Radiol. 37 (2007) 21–31.

28

Journal Pre-proof Figure Legends Figure 1. Multipoint LOD scores for linkage of BMC and BMD at different skeletal sites (only significant results are shown). BMDLRI, left rib BMD; BMCLRI, left rib BMC; BMDLLE, left leg BMD; BMDPEL, pelvis BMD; BMDRLE, right leg BMD; DXBMD, total body BMD; DXBMC, total body BMC; BMCLLE, left leg BMC; BMCPEL, pelvis BMC; BMDLSP, lumbar spine BMD.

of

Figure 2. Genome-wide association of BMC and BMD on multiple skeletal sites (only

ro

significant results are shown). A. Manhattan Plot of the genome wide association analysis of

-p

right arm BMC and B. Manhattan Plot of the genome wide association analysis of pelvis BMD.

re

The analyses were adjusted for age, sex, age*sex, age2*sex, kinship, puberty stage and BMI Zscore.

lP

Figure 3. Association Plots. A. SNP association plot for right arm BMC-associated region at

na

chromosome 22q12.3. B. SNP association plot for pelvis BMD-associated region at chromosome

Jo

Table Legends

ur

8p21.2. Genetic coordinates are according to hg19/1000 Nov 2014 Genomes AMR.

Table 1. Heritability for BMC and BMD. The models were adjusted for age, age2, sex, age*sex, age2*sex, kinship, puberty stage and BMI Z- score. Table 2. Genome-wide Linkage Results on BMC and BMD. The models were adjusted for age, age2, sex, age*sex, age2*sex, and kinship. Statistically significant results (Logarithm of Odds score (LOD) >3) are depicted in bold) and suggestive results (LOD>2) are shown. Table 3. Genome-wide association results for BMD and BMC. SNP with statistically significant (p<1×10-7) or suggestive results (p<1×10-6) at any of the three primary sites are shown. The models were adjusted for age, age2, sex, age*sex, age2*sex, kinship, BMI Z-score and puberty 29

Journal Pre-proof stages, with statistically significant results depicted in bold. Abbreviations: PTK2B, protein tyrosine kinase 2 beta; STMN4, stathmin 4; LRIF1, Ligand Dependent Nuclear Receptor Interacting Factor 1; MEGF10, multiple EGF-like-domains 10; ABRAXAS2, abraxas 2, BRISC complex subunit. Table 4. Exome sequencing association results for BMD and BMC. SNP with statistically significant (p<9.2×10-7) or suggestive results (p<9.2×10-6) on any of the three primary sites were

of

shown. The models were adjusted for age, age2, sex, age*sex, age2*sex, kinship, BMI Z-score

ro

and puberty stages, with statistically significant results depicted in bold. Abbreviations: MAP4K3,

-p

Mitogen-Activated Protein Kinase Kinase Kinase Kinase 3; FOXN1, Forkhead Box N1; CXCR6,

re

C-X-C Motif Chemokine Receptor 6; MEGF10, multiple EGF-like-domains 10; ABRAXAS2, abraxas 2, BRISC complex subunit; HERC2, HECT and RLD Domain Containing E3 Ubiquitin

lP

Protein Ligase 2.

na

Table 5. BMDCS and SAFOS lookups for novel loci identified in VFS. BMDCS, Bone Mineral Density in Childhood Study; SAFOS, San Antonio Family Osteoporosis Study; VFS, the Viva

ur

La Familia Study; BMC, Bone mineral content; BMD, Bone mineral density; PTK2B, protein

Jo

tyrosine kinase 2 beta; ABRAXAS2, abraxas 2 BRISC complex subunit.

30

Journal Pre-proof Table 1. Heritability for BMC and BMD Mean SD h2 SE p value Bone Mineral Content (g) Left arm 94.3 49.2 0.61 0.083 8.5×10-17 Left leg 291.5 140.4 0.59 0.082 2.3×10-16 Left rib 68.3 28.3 0.44 0.083 2.8×10-9 Lumbar spine 29.6 15.7 0.58 0.081 7.2×10-16 Pelvis 158.1 92.9 0.56 0.085 1.6×10-13 Right arm 100.7 52.6 0.59 0.081 2.4×10-16 Right leg 292.4 139.9 0.57 0.082 1.7×10-15 Right rib 65.1 27.6 0.48 0.083 8.5×10-11 Thoracic spine 68.3 33.6 0.44 0.081 1.1×10-9 Total body 1510.5 635.3 0.6 0.082 8.9×10-17 2 Bone Mineral Density (g/cm ) Left arm 0.62 0.10 0.68 0.08 3.4×10-20 Left leg 0.97 0.19 0.51 0.081 1.3×10-12 Left rib 0.57 0.09 0.56 0.081 5.8×10-15 Lumbar spine 0.80 0.18 0.58 0.083 3.7×10-15 Pelvis 1.00 0.24 0.51 0.083 3.4×10-12 Right arm 0.62 0.10 0.66 0.081 5.3×10-20 Right leg 0.97 0.19 0.44 0.079 3.1×10-10 Right rib 0.56 0.09 0.67 0.082 7.2×10-20 Thoracic spine 0.66 0.15 0.44 0.081 4.8×10-10 Total body 0.92 0.14 0.6 0.082 8.8×10-17 The models were adjusted for adjusted for age, age2, sex, age*sex, age2*sex, kinship, puberty stage and BMI Z- score.

f o

l a

o r p

r P

e

n r u

Jo

31

Journal Pre-proof Table 2. Genome-wide Linkage Results on BMC and BMD Trait Chr cM Location Nearby Markers LOD Bone Mineral Content Left arm 19 65 19q12, 19q13.13 D19S414, D19S220 2.0 Left leg 20 31 20p12.3, 20p12.2 D20S115, D20S186 2.5 Left rib 7 61 7p14.2, 7p14.1 D7S484, D7S510 2.2 Pelvis 20 75 20q12, 20q13.12 D20S107, D20S119 3.4 Right arm 9 35 9p24.1, 9p22.3 D9S286, D9S285 2.4 Right leg 19 65 19q12, 19q13.13 D19S414, D19S220 2.8 Thoracic spine 9 41 9p22.2, 9p21.3 D9S157, D9S171 2.6 Total body 14 65 14q22.3, 14q23.2 D14S276, D14S63 3.0 Bone Mineral Density Left arm 3 123 3p12.3, 3q12.2 D3S3681, D3S1271 2.6 Left leg 7 61 7p14.2, 7p14.1 D7S484, D7S510 3.4 Left rib 6 64 6p21.2, 6p12.1 D6S1610, D6S257 3.0 Lumbar spine 20 79 20q13.12, 20q13.13 D20S119, D20S178 3.2 Pelvis 7 62 7p14.2, 7p14.1 D7S484, D7S510 4.8 Right leg 7 61 7p14.2, 7p14.1 D7S484, D7S510 2.6 Thoracic spine 1 275 1q42.2, 1q43 D1S2800, D1S2785 2.1 Total body 7 59 7p15.1, 7p14.2 D7S516, D7S484 2.9 2 2 The models were adjusted for age, age , sex, age*sex, age *sex, and kinship. Statistically significant results (Logarithm of Odds score (LOD) >3) are depicted in bold) and suggestive results (LOD>2) are shown.

f o

l a

o r p

r P

e

n r u

Jo

32

Journal Pre-proof Table 3. Genome-wide association results on primary skeletal sites for BMD and BMC SNP

Effect Allele (Freq) Bone Mineral Density rs7000615 C(0.36)

Chr

8

rs11775958 C(0.35) rs891391

Position

Nearest Gene

Total body Beta(SE)

P value

Lumbar Spine Beta(SE) P value

Pelvis Beta(SE)

P value

27405916

PTK2B

-0.22(0.06)

2.1×10-4

-0.24(0.06)

7.3×10-5

-0.28(0.05) -0.27(0.05)

7.4×10-8 2.5×10-7

8

27412367

PTK2B

-0.17(0.06)

2.7×10-3

-0.23(0.06)

A(0.34)

8

27417992

PTK2B

-0.17(0.06)

3.2×10-3

-0.25(0.06)

2.5×10-5

-0.27(0.05)

2.9×10-7

rs1541845

A(0.36)

8

27421883

PTK2B

-0.18(0.06)

2.5×10-3

-0.25(0.06)

-0.28(0.05)

1.8×10-7

1.6×10-3

-0.25(0.06)

1.8×10-5

-0.28(0.05)

1.6×10-7

1.3×10-3

ro

1.4×10-5

rs2241652

G(0.36)

8

27422188

PTK2B

-0.19(0.06)

rs3739214

A(0.34)

8

27243762

STMN4

-0.19(0.06)

-0.29(0.06)

2.4×10-7

-0.22(0.05)

2.5×10-5

Bone Mineral Content rs12567355 A(0.03)

1

110921002

LRIF1

-0.65(0.15)

1.3×10-5

-0.87(0.17)

2.2×10-7

-0.68(0.16)

3.4×10-5

rs1712674

C(0.03)

1

110923431

LRIF1

-0.61(0.14)

1.8×10-5

-0.81(0.17)

3.9×10-7

-0.63(0.15)

5.5×10-5

rs1780569

C(0.03)

1

110927141

LRIF1

-0.61(0.14)

1.8×10-5

-0.81(0.16)

3.9×10-7

-0.63(0.15)

5.5×10-5

rs3739214

A(0.34)

8

27243762

STMN4

-0.22(0.05)

3.1×10-5

-0.27(0.06)

6.1×10-6

-0.28(0.06)

7.1×10-7

rs3735759

G(0.34)

8

27345522

PTK2B

-0.20(0.05)

1.8×10-4

-0.20(0.06)

5.8×10-4

-0.29(0.06)

4.8×10-7

rs7834529

C(0.35)

8

27353816

PTK2B

-0.20(0.05)

5.7×10-5

-0.18(0.06)

1.4×10-3

-0.28(0.05)

2.4×10-7

rs7000336

A(0.33)

8

27388820

-0.20(0.05)

1.6×10-4

-0.20(0.06)

6.5×10-4

-0.30(0.06)

2.6×10-7

8

27390918

PTK2B

-0.19(0.05)

3.5×10-4

-0.19(0.06)

1.1×10-3

-0.28(0.06)

8.4×10-7

A(0.34)

8

J

PTK2B

rs11987089 A(0.33) rs2059970

27401909

PTK2B

-0.19(0.05)

3.1×10-4

-0.20(0.06)

5.3×10-4

-0.29(0.06)

4.3×10-7

rs7000615

C(0.36)

8

27405916

PTK2B

-0.24(0.05)

5.0×10-6

-0.24(0.06)

4.3×10-5

-0.30(0.06)

1.7×10-7

rs11775958 C(0.35)

8

27412367

PTK2B

-0.22(0.05)

4.5×10-5

-0.24(0.06)

7.4×10-5

-0.29(0.06)

7.4×10-7

rs891391

A(0.34)

8

27417992

PTK2B

-0.22(0.05)

2.5×10-5

-0.25(0.06)

3.1×10-5

-0.29(0.06)

4.0×10-7

rs1541845

A(0.36)

8

27421883

PTK2B

-0.23(0.05)

1.9×10-5

-0.25(0.06)

2.3×10-5

-0.30(0.06)

3.2×10-7

rs2241652

G(0.36)

8

27422188

PTK2B

-0.23(0.05)

1.7×10-5

-0.25(0.06)

3.6×10-5

-0.29(0.06)

4.4×10-7

rs1055256

A(0.39)

10

124758023

METTL10

0.18(0.05)

5.1×10-4

0.28(0.06)

6.5×10-7

0.20(0.06)

3.8×10-4

rn

l a

u o

p e

r P

2.2×10-5

f o

33

Journal Pre-proof rs10901818 G(0.39)

10

124760859

rs11245366 G(0.38)

10

124794280

rs10901823 G(0.38)

10

124800091

rs2303611

G(0.38)

10

124829420

rs17112849 A(0.01)

14

106513959

0.18(0.05)

5.1×10-4

0.28(0.06)

6.1×10-7

0.20(0.06)

3.7×10-4

0.20(0.05)

1.6×10-4

0.29(0.06)

3.4×10-7

0.22(0.06)

5.8×10-5

ABRAXAS2

0.18(0.05)

3.2×10-4

0.28(0.06)

9.2×10-7

0.22(0.06)

7.2×10-5

ABRAXAS2

0.18(0.05)

3.2×10-4

0.28(0.06)

9.2×10-7

0.22(0.06)

7.2×10-5

-1.33(0.30)

7.8×10-6

-1.73(0.33)

2.1×10-7

-1.60(0.32)

6.3×10-7

METTL10

SNPs with statistically significant (p<1×10-7) or suggestive results (p<1×10-6) for any of the three primary sites are shown. The models were adjusted for age, age2, sex, age*sex, age2*sex, kinship, BMI Z-score and puberty stages, with statistically significant results depicted in bold. Abbreviations: PTK2B, protein tyrosine kinase 2 beta; STMN4, stathmin 4; LRIF1, Ligand Dependent Nuclear Receptor Interacting Factor 1; MEGF10, multiple EGF-like-domains 10; ABRAXAS2, abraxas 2, BRISC complex subunit.

f o

l a

o r p

r P

e

n r u

Jo

34

Journal Pre-proof Table 4. Exome sequencing association results on primary skeletal sites for BMD and BMC SNP

Effect Allele (Freq)

Chr

Position

Gene

SNP type

Bone Mineral Density rs370055571 A(0.01)

2

39485723

MAP4K3

missense

rs532648

C(0.35)

17

26864302

FOXN1

missense

Bone Mineral Content rs56287545 A(0.02)

3

Total body Beta P value (SE) 5.3×10-6

-1.19 (0.26) -0.22 (0.05)

3‘ UTR

Lumbar Spine Beta P value (SE)

Pelvis Beta (SE)

4.8×10-2

-0.89 (0.24) -0.24 (0.05)

-7.29 (0.26) -0.18 (0.05)

f o

8.0×10-5

7.5×10-4

P value

1.7×10-4 9.7×10-7

o r p

0.45 2.0×10-3 0.78 4.5×10-6 0.51 1.4×10-3 (0.15) (0.17) (0.16) -3 -6 rs41289620 T(0.02) 3 46003735 FYCO1 missense 0.46 2.2×10 0.80 4.4×10 0.52 1.6×10-3 (0.15) (0.18) (0.17) rs3812054 A(0.06) 5 126732427 MEGF10 missense 0.46 4.2×10-6 0.32 4.8×10-3 0.44 6.4×10-5 (0.10) (0.11) (0.11) rs17164935 A(0.07) 5 126791282 MEGF10 missense 0.43 2.1×10-6 0.32 2.6×10-3 0.43 1.6×10-5 (0.09) (0.10) (0.10) -4 -7 rs2303611 G(0.38) 10 126517989 ABRAXAS2 synonymous -0.17 6.9×10 -0.23 2.5×10-5 0.28 7.7×10 (0.05) (0.05) (0.06) rs151179905 T(0.01) 15 28517394 HERC2 synonymous 0.90 7.3×10-6 0.66 4.6×10-3 0.79 3.2×10-4 (0.20) (0.23) (0.22) SNP with statistically significant (p<9.2×10-7) or suggestive results (p<9.2×10-6) on any of the three primary sites were shown. The model adjusted for age, age2, sex, age*sex, age2*sex, kinship, BMI Z-score and puberty stages, with statistically significant results depicted in bold. Abbreviations: MAP4K3, Mitogen-Activated Protein Kinase Kinase Kinase Kinase 3; FOXN1, Forkhead Box N1; CXCR6, C-X-C Motif Chemokine Receptor 6; MEGF10, multiple EGF-like-domains 10; ABRAXAS2, abraxas 2, BRISC complex subunit; HERC2, HECT and RLD Domain Containing E3 Ubiquitin Protein Ligase 2. 45989461

CXCR6

l a

r P

e

n r u

Jo

35

Journal Pre-proof Table 5. BMDCS and SAFOS lookups for novel loci identified in VFS Chr SNP

Position

Nearest Trait SAFOS BMDCS Gene MAF Beta(SE) P value MAF Beta(SE) P value 8 rs7000615 27405916 PTK2B Total Hip BMC 0.33 0.31 -0.45(0.45) 8 rs7000615 27405916 PTK2B Total Hip BMD 0.33 0.18 0.16 0.33 -0.01(0.01) 0.05(0.05) 8 rs7000615 27405916 PTK2B Interchrochanter BMC 0.33 0.57 -0.19(0.33) 8 rs7000615 27405916 PTK2B Interchrochanter BMD 0.33 0.11 -0.02(0.01) 8 rs7000615 27405916 PTK2B Femoral Neck BMC 0.33 0.46 -0.03(0.05) 8 rs7000615 27405916 PTK2B Femoral Neck BMD 0.33 0.31 0.16 0.11 -0.01(0.01) 0.08(0.05) 8 rs7000615 27405916 PTK2B Spine BMC 0.33 0.69 -0.31(0.79) 8 rs7000615 27405916 PTK2B Spine BMD 0.33 0.26 0.16 0.60 -0.01(0.01) 0.02(0.05) 8 rs7000615 27405916 PTK2B Trochanter BMC 0.33 0.05 -0.2(0.1) 8 rs7000615 27405916 PTK2B Trochanter BMD 0.33 0.22 -0.01(0.01) 8 rs7000615 27405916 PTK2B Ward's Triangle BMC 0.33 0.045 -0.02(0.01) 8 rs7000615 27405916 PTK2B Ward's Triangle BMD 0.33 0.049 -0.02(0.01) 8 rs7000615 27405916 PTK2B Radius BMD 0.16 0.19 0.06(0.05) 8 rs7000615 27405916 PTK2B Total body less head BMC 0.16 0.15 0.05(0.04) 10 rs2303611 126517989 ABRAXAS2 Total Hip BMC 0.44 0.25 -0.5(0.44) 10 rs2303611 126517989 ABRAXAS2 Total Hip BMD 0.44 0.33 0.43 0.22 -0.01(0.01) 0.05(0.04) 10 rs2303611 126517989 ABRAXAS2 Interchrochanter BMC 0.44 0.21 -0.41(0.32) 10 rs2303611 126517989 ABRAXAS2 Interchrochanter BMD 0.44 0.42 -0.01(0.01) 10 rs2303611 126517989 ABRAXAS2 Femoral Neck BMC 0.44 0.43 -0.04(0.05) 10 rs2303611 126517989 ABRAXAS2 Femoral Neck BMD 0.44 0.31 0.43 0.29 -0.01(0.01) 0.04(0.04) 10 rs2303611 126517989 ABRAXAS2 Spine BMC 0.44 0.38 -0.68(0.77) 10 rs2303611 126517989 ABRAXAS2 Spine BMD 0.44 0.74 0.43 0.45 -0.003(0.01) 0.03(0.04) 10 rs2303611 126517989 ABRAXAS2 Trochanter BMC 0.44 0.53 -0.06(0.1) 10 rs2303611 126517989 ABRAXAS2 Trochanter BMD 0.44 0.37 -0.01(0.01) 10 rs2303611 126517989 ABRAXAS2 Ward's Triangle BMC 0.44 -0.001(0.01) 0.92 10 rs2303611 126517989 ABRAXAS2 Ward's Triangle BMD 0.44 0.94 -0.001(0.01) 10 rs2303611 126517989 ABRAXAS2 Radius BMD 0.43 -0.03(0.04) 0.47 10 rs2303611 126517989 ABRAXAS2 Total body less head BMC 0.43 0.062 0.05(0.03) BMDCS, Bone Mineral Density in Childhood Study; SAFOS, San Antonio Family Osteoporosis Study; VFS, the Viva La Familia Study; BMC, Bone mineral content; BMD, Bone mineral density; PTK2B, protein tyrosine kinase 2 beta; ABRAXAS2, abraxas 2 BRISC complex subunit

f o

l a

o r p

r P

e

n r u

Jo

36

Journal Pre-proof HIGHLIGHTS 1. Osteoporosis and low bone mass are a major public health threat for US 2. The correlates of bone health in children are understudied. 3. We aimed to identify genetic variants associated with bone health in Hispanic children utilizing genome-wide linkage,

f o

genome-wide association and exome-based analysis approaches.

o r p

4. We identified novel loci associated with BMC and BMD in Hispanic children, with strongest evidence for PTK2B

l a

r P

e

n r u

Jo

37

Figure 1

Figure 2

Figure 3