Brief Report

Meta-Analysis of Genome-Wide Linkage Studies of
Quantitative Lipid Traits in Families Ascertained for
Type 2 Diabetes
Alka Malhotra,

1
Steven C. Elbein,

2
Maggie C.Y. Ng,

3
Ravindranath Duggirala,

4
Rector Arya,

5

Giuseppina Imperatore,
6

Adebowale Adeyemo,
7

Toni I. Pollin,
8

Wen-Chi Hsueh,
9

Juliana C.N. Chan,
3

Charles Rotimi,
7

Robert L. Hanson,
10

Sandra J. Hasstedt,
11

Johanna K. Wolford,
1

and the American

Diabetes Association GENNID Study Group*

Dyslipidemia is a major risk factor for coronary heart
disease, which is the predominant cause of mortality in
individuals with type 2 diabetes. To date, nine linkage
studies for quantitative lipid traits have been performed in
families ascertained for type 2 diabetes, individually yield-
ing linkage results that were largely nonoverlapping. Dis-
crepancies in linkage findings are not uncommon and are
typically due to limited sample size and heterogeneity. To
address these issues and increase the power to detect
linkage, we performed a meta-analysis of all published
genome scans for quantitative lipid traits conducted in
families ascertained for type 2 diabetes. Statistically sig-
nificant evidence (i.e., P < 0.00043) for linkage was ob-
served for total cholesterol on 7q32.3-q36.3 (152.43–182 cM;
P � 0.00004), 19p13.3-p12 (6.57–38.05 cM; P � 0.00026),
19p12-q13.13 (38.05– 69.53 cM; P � 0.00001), and 19q13.13-
q13.43 (69.53–101.1 cM; P � 0.00033), as well as LDL on
19p13.3-p12 (P � 0.00041). Suggestive evidence (i.e., P <
0.00860) for linkage was also observed for LDL on 19p12-
q13.13, triglycerides on 7p11-q21.11 (63.72–93.29 cM), tri-
glyceride/HDL on 7p11-q21.11 and 19p12-q13.13, and LDL/
HDL on 16q11.2-q24.3 (65.2–130.4 cM) and 19p12-q13.13.

Linkage for lipid traits has been previously observed on
both chromosomes 7 and 19 in several unrelated studies
and, together with the results of this meta-analysis, pro-
vide compelling evidence that these regions harbor impor-
tant determinants of lipid levels in individuals with type 2
diabetes. Diabetes 56:890 – 896, 2007

C
oronary heart disease (CHD) is the leading
cause of death in individuals with type 2 diabe-
tes (1). The high prevalence of CHD among
these individuals is largely due to dyslipidemia,

which is influenced by both environmental and genetic
factors (2). Over 90 genome scans have been performed to
identify loci for lipid levels, including nine linkage studies
of quantitative lipid traits performed in ethnically diverse
populations of families ascertained for type 2 diabetes
(3–10). Common chromosomal regions have been identi-
fied in some of these studies; for example, linkage on
chromosome 19 was observed for triglyceride levels in
families with Northern-European ancestry (6) and total
cholesterol levels in Pima Indians from Arizona and Afri-
can Americans from the Genetics of NIDDM (GENNID)
Study (3,5). Similarly, linkage on chromosome 3 was
observed for LDL cholesterol levels in an Old Order Amish
population (10) and for triglyceride/HDL levels in Cauca-
sian families from the GENNID Study (3). However, most
of the regions observed in these genome scans have not
been overlapping, including linkage on 15q and 9p for
plasma triglycerides and HDL cholesterol, respectively, in
Mexican-American families (7,8); chromosome 7 for HDL
cholesterol in Africans (9); chromosome 6 for triglycerides
in a Chinese population from Hong Kong (4); and chromo-
some 11 for triglyceride/HDL cholesterol in Hispanics
from the GENNID Study (3). While some of these analyses
yielded logarithm of odds (LOD) �3.0, the majority of LOD
scores reported in these studies were well below the
threshold normally considered statistically significant.

While disparities in linkage findings for lipid traits in
families ascertained for type 2 diabetes and lack of statis-
tically significant evidence for linkage can result from both
locus heterogeneity and utilization of different study de-
signs, in most cases, they are most commonly attributable
to inadequately sized study samples. In the nine genome
scans for lipid traits conducted in families with type 2
diabetes, sample sizes ranged from 240 to 998 individuals,
and most of these studies had low power to detect statisti-

From the 1Diabetes and Obesity Research Unit, Translational Genomics
Research Institute, Phoenix, Arizona; the 2Endocrinology Section, University
of Arkansas, Little Rock, Arkansas; the 3Department of Medicine and Thera-
peutics, Chinese University of Hong Kong, Shatin, Hong Kong; the 4Depart-
ment of Genetics, Southwest Foundation for Biomedical Research, San
Antonio, Texas; the 5Division of Clinical Epidemiology, University of Texas
Health Sciences Center, San Antonio, Texas; the 6Division of Diabetes
Translation, Centers for Disease Control and Prevention, Atlanta, Georgia; the
7National Human Genome Center, Howard University, Washington, DC; the
8Division of Endocrinology, Diabetes, and Nutrition, University of Maryland,
Baltimore, Maryland; the 9Department of Medicine, University of California
San Francisco, San Francisco, California; the 10Diabetes and Arthritis Epide-
miology Section, National Institute of Diabetes and Digestive and Kidney
Diseases, Phoenix, Arizona; and the 11Human Genetics Department, Univer-
sity of Utah, Salt Lake City, Utah.

Address correspondence and reprint requests to Alka Malhotra, Diabetes
and Obesity Research Unit, Genetic Basis of Human Disease, Translational
Genomics Research Institute, 445 N. 5th St., Phoenix, AZ 85004. E-mail:
amalhotra@tgen.org.

Received for publication 28 July 2006 and accepted in revised form 12
December 2006.

*A complete list of the American Diabetes Association GENNID Study
Group members can be found in the ACKNOWLEDGMENTS.

AADM, Africa-America Diabetes Mellitus; AFDS, Amish Family Diabetes
Study; CHD, coronary heart disease; GENNID, Genetics of NIDDM; GSMA,
Genome Scan Meta-Analysis; HKFDS, Hong Kong Family Diabetes Study;
LOD, logarithm of odds; SAFADS, San Antonio Family Diabetes Study.

DOI: 10.2337/db06-1057
© 2007 by the American Diabetes Association.
The costs of publication of this article were defrayed in part by the payment of page

charges. This article must therefore be hereby marked “advertisement” in accordance

with 18 U.S.C. Section 1734 solely to indicate this fact.

890 DIABETES, VOL. 56, MARCH 2007



cally significant evidence for linkage. The goal of this
study, therefore, was to overcome many of the limitations
associated with detecting statistically significant evidence
of linkage for a complex trait and augment the power to
detect statistically significant evidence of linkage for lipid
traits in families with type 2 diabetes. To this end, we
combined LOD scores from each of the nine genome scans
using a meta-analysis approach. This study is the first
meta-analysis of linkage results for quantitative lipid traits
measured in families ascertained for type 2 diabetes and
represents the largest genetic linkage study of lipid traits
conducted to date in a population with diabetes.

RESEARCH DESIGN AND METHODS

Characteristics of participants from the nine populations used in the present
study are shown in Table 1. Linkage results for quantitative lipid traits
(triglycerides, total cholesterol, LDL, HDL, triglyceride/HDL, and LDL/HDL)
were used from the following populations with families ascertained for type 2
diabetes: 59 African-American families, 153 Caucasian families, and 115
Hispanic families from the GENNID Study (3); 179 Chinese nuclear families
from the Hong Kong Family Diabetes Study (HKFDS) (4); 292 (998 siblings),
201 (590 siblings), and 188 (548 siblings) Pima Indian families for total
cholesterol, HDL cholesterol, and triglycerides, respectively, from the Gila
River Indian Community in Arizona (5); 415 individuals from 27 families as
part of the San Antonio Family Diabetes Study (SAFADS) (7,8); 19 families
(379 individuals) with Northern-European ancestry (6); 295 sibling pairs from
the Africa-America Diabetes Mellitus (AADM) Study (9); and 28 Old Order
Amish pedigrees collected as part of the Amish Family Diabetes Study (AFDS)
(10). Extensive details of the study populations and methods used in each
study have been previously described (3–10).
Statistical analysis. The Genome Scan Meta-Analysis (GSMA) program
(11,12) was used to assess evidence for linkage utilizing results from analyses
of triglycerides, LDL, total cholesterol, HDL, LDL/HDL, and triglyceride/HDL.
Bins were created using Marshfield map distances. Of the nine genome scans,
only two used marker maps with Marshfield map distances; for the remaining
studies, distances were converted to Marshfield map distances by inserting the
marker names in the Marshfield database (http://research.marshfieldclinic.
org/genetics/). In total, 116 bins of �30 cM (range 26.2–32.9) spanning the
genome were created. Following this, the maximum LOD score for a bin in
each study was identified and were used to assign ranks to each bin in each
separate study. Ranks were then summed across studies and used to estimate
the probability of observing a bins summed rank by chance, i.e., the propor-
tion of replicates with summed rank equal to or greater than that observed
when combining the results of all studies (11). We have described this method
in detail elsewhere (13).

Because sample sizes varied considerably among the studies evaluated
here, both unweighted and weighted GSMA analyses were performed. The
data were weighted according to the number of individuals genotyped in the
respective study populations, such that weight � [�N(genotyped individu-
als)]/[mean of �N(genotyped individuals) over all studies] where n � 612,
415, 572, 897, 819, 582, 240, 379, and 998 (or 548 or 590 depending on the trait
being analyzed) for the AFDS, SAFADS, AADM, HKFDS, GENNID (Cauca-
sians), GENNID (Hispanics), GENNID (African Americans), Caucasians with
Northern-European ancestry, and Pima Indian studies, respectively (3–10).

Statistically significant evidence for linkage, equivalent to Lander and
Kruglyak’s (14) definition of one false positive per 20 meta-analyses, was
assessed using a Bonferroni correction (0.05/116), giving P � 0.00043, whereas
suggestive evidence for linkage, defined as one false positive per meta-
analysis, corresponded to P � 0.00860. We, however, did not correct for the
six lipid traits because they were correlated.

RESULTS

Nine genome scans for lipid traits have been performed in
families ascertained for type 2 diabetes. Characteristics of
the participants from each study are shown in Table 1.
These populations were drawn from diverse ethnic back-
grounds including American-Indian, Old Order Amish,
African, African-American, and Chinese study samples, as
well as two groups of unrelated Caucasian and Hispanic
individuals. We performed a meta-analysis for the follow-
ing quantitative lipid traits: LDL (seven studies), HDL (nine
studies), triglycerides (nine studies), total cholesterol

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A. MALHOTRA AND ASSOCIATES

DIABETES, VOL. 56, MARCH 2007 891



(eight studies), triglyceride/HDL (five studies), and LDL/
HDL (five studies). The number of studies included in the
meta-analyses varied according to the availability of trait
data from the original genome scans for a given population
(Table 1).

We observed statistically significant evidence (i.e., P �
0.00043) for linkage in four bins for total cholesterol on
7q32.3-q36.3 (152.43–182 cM), 19p13.3-p12 (6.57–38.05 cM),
19p12-q13.13 (38.05– 69.53 cM), and 19q13.13-q13.43
(69.53–101.1 cM), as well as one bin for LDL on 19p13.3-
p12 (Table 2). To evaluate the distribution of P values
across the genome, summed ranks were plotted against
the bin number for total cholesterol and LDL, which were
the only traits showing statistically significant evidence for
linkage (Figs. 1 and 2, respectively). In addition, eight
regions also showed suggestive evidence (i.e., P �
0.00860) of linkage for different traits: 19p12-q13.13 and
19q13.13-q13.43 for LDL, 7p11-q21.11 (63.72–93.29 cM) and
19p12-q13.13 for triglyceride/HDL, 7p11-q21.11 for triglyc-
erides, and 16q11.2–16q21 (65.2–97.8), 16q21-q24.3 (97.8 –
130.4 cM), and 19p12-q13.13 for LDL/HDL. However, in the
analysis of HDL, no bins met the criteria for statistically
significant or suggestive evidence for linkage, as described
in RESEARCH DESIGN AND METHODS.

DISCUSSION

In this study, we report the results from the first meta-
analysis of linkage data undertaken to date to identify loci
underlying quantitative lipid traits in families ascertained
for type 2 diabetes. We have found statistically significant
evidence of linkage for total cholesterol on 7q32.3-q36.3
and chromosome 19 and for LDL on 19p13.3-p12. Sugges-
tive evidence for linkage was also observed on 19p12-
q13.13 and 19q13.13-q13.43 for LDL, 7p11-q21.11 for
triglycerides, 7p11-q21.11 and 19p12-q13.13 for triglycer-
ide/HDL, and 16q11.2–16q21, 16q21-q24.3, and 19p12-
q13.13 for LDL/HDL. These results demonstrate that
combining data from unrelated studies conducted in fam-
ilies ascertained for type 2 diabetes can successfully
address important limitations commonly associated with
linkage analysis, such as relatively modest sample size,
and increase the power to detect statistically significant
evidence for linkage.

The strongest evidence of linkage for lipid traits identi-
fied in this study was found on chromosomes 7 and 19.
Linkage for lipid traits has been previously observed in
both of these regions in several studies. For example,
linkage on chromosome 7 for triglyceride/HDL (15) was
found in randomly ascertained families and for triglyceride
levels in two unrelated studies of families ascertained for
obesity and one study of families ascertained for type 2
diabetes (7,16,17). A statistically significant P value iden-
tified in this meta-analysis, combined with multiple obser-
vations of linkage in unrelated studies, supports the
presence of a gene(s) in this region with important effects
on triglyceride levels. It is worth noting that only nominal
evidence for linkage was observed for this locus in the
individual studies, indicating that meta-analysis may be a
powerful tool for identifying susceptibility loci for com-
plex traits such as lipid levels.

While the 7q32.3-q36.3 locus is a strong candidate for
genetic control of triglyceride levels, the most consistent
and compelling evidence of linkage for lipid traits was
observed on chromosome 19. Linkage for various lipid
traits to chromosome 19 has been observed in severalT

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META-ANALYSIS OF LIPID LEVEL GENOME SCANS

892 DIABETES, VOL. 56, MARCH 2007



studies including total cholesterol in Pima Indians (5) and
African Americans (3), triglycerides in non-Hispanic Cau-
casians (6), and LDL in Old Order Amish (10) and Africans
(9); notably, these five studies involved families ascer-
tained for type 2 diabetes. In addition, linkage to chromo-

some 19 was also observed for LDL cholesterol in
randomly ascertained American Indians (18) and Cauca-
sians (19) and a combination of randomly and obesity-
ascertained families (20), as well as for LDL particle size,
in randomly ascertained Mexican-American families (21)

FIG. 1. Summed ranks in relation to bin number in the analysis of lipid traits. Summed ranks are plotted against the GSMA bin number. There
are a total of 116 bins. Vertical lines divide the bins according to chromosome. A: Total cholesterol levels: three bins on chromosome 19 and one
bin on chromosome 7 showed significant evidence as indicated. B: LDL levels: one bin on chromosome 19 showing significant evidence for linkage.

A. MALHOTRA AND ASSOCIATES

DIABETES, VOL. 56, MARCH 2007 893



and African Americans ascertained for hypertension (22).
Together, these findings are consistent with chromosome
19 being an important locus for regulation of lipid levels
among individuals from diverse ethnic backgrounds. Fur-
ther, the identification of this locus in five of the nine
published genome scans conducted in families ascertained
for type 2 diabetes supports the idea that studies of such
populations, in whom effects of genetic variants affecting

lipid levels may occur earlier or more severely, may
facilitate the discovery of genes with critical roles in lipid
metabolism in individuals with diabetes and in the general
population.

The identification of chromosome 19 both in a single bin
identified for multiple traits (total cholesterol, LDL, triglyc-
eride/HDL, and LDL/HDL) and across multiple bins (total
cholesterol) suggests possible pleiotropic effects of a gene

FIG. 2. LOD score plots for chromosome 7 (A) and chromosome 19 (B). Horizontal lines indicate the LOD score of the meta-analysis for a given
bin that extends 29.57 cM for chromosome 7 and 31.48 cM for chromosome 19, with cM interval for each bin given above the line.

META-ANALYSIS OF LIPID LEVEL GENOME SCANS

894 DIABETES, VOL. 56, MARCH 2007



in this region and/or multiple genes affecting a single trait.
This effect is not unique to our study, as multiple peaks
have also been observed in other studies. Heijmans et al.
(23) identified peaks on each arm of chromosome 19, and
a broad linkage peak extending from the p to the q arm
was observed in an African-American population (3).
There are many genes located in this region that encode
proteins with direct effects on lipid metabolism, including
hormone-sensitive lipase (LIPE at 19q13.1-q13.2), apoli-
poprotein E (APOE at 19q13.2), and LDL receptor (LDLR
at 19p13.2). It is therefore possible that variants in multiple
genes within this region interact with one another to exert
effects of varying magnitude on lipid levels. In addition, the
low proportion of variance of cholesterol levels explained
by these genes, e.g., the APOE locus contributed as low as
10% of the variance in one study (13), might suggest the
role of genes on other chromosomes, including cholesteryl
ester transfer protein (CETP) and apolipoprotein B
(APOB).

While we have found statistically significant evidence
for linkage for different quantitative lipid traits using
meta-analysis, we recognize that utilization of ethnically
diverse populations may yield results that are difficult to
interpret, in light of potential effects of locus heterogene-
ity. However, low heterogeneity was observed for total
cholesterol in bins corresponding to 7q32.3-q36.3, 19p13.3-
p12, 19p12-q13.13, and 19q13.13-q13.43 (results not shown).
The fact that common regions of linkage were identified in
this analysis, despite differences in ethnicity in the study
samples, is consistent with common genetic influences
across the different populations.

In summary, we observed statistically significant evi-
dence for linkage for total and LDL cholesterol on chro-
mosome 19 and for total cholesterol on chromosome 7 in
a meta-analysis of genome scan results from families
ascertained for type 2 diabetes. These findings, combined
with previous reports of linkage on chromosomes 7 and
19, provide compelling evidence that these regions harbor
genes with important effects on lipid levels.

ACKNOWLEDGMENTS

The GENNID Study was supported by the American Dia-
betes Association (ADA). We thank the investigators and
staff who contributed to the GENNID repository, as well as
the individuals who participated in the GENNID Study.
Genetic material collected by, and families characterized
by, the ADA GENNID Study Group, which includes Eric
Boerwinkle, PhD, University of Texas Health Science
Center; John Buse, MD, PhD, University of North Carolina;
Ralph DeFronzo, MD, University of Texas Health Science
Center; David Ehrmann, MD, University of Chicago;
Steven C. Elbein, MD, University of Utah/University of
Arkansas; Wilfred Fujimoto, MD, and Steven E. Kahn, MB,
ChB, University of Washington; Craig L. Hanis, PhD,
University of Texas Health Science Center; Richard A.
Mulivor, PhD, and Jeanne C. Beck, PhD, Coriell Cell
Repositories; Jill Norris, PhD, University of Colorado
School of Medicine; M. Alan Permutt, MD, and Philip
Behn, MD, WA University School of Medicine; Leslie
Raffel, MD, Cedars-Sinai Medical Center; and David C.
Robbins, MD, Medlantic Research Institute.

The SAFADS project was supported by grants from the
National Institute of Diabetes and Digestive and Kidney
Diseases (NIDDK): DK53889, DK42273, and DK47482. We
warmly thank the SAFADS families for their enthusiasm

and cooperation. The study performed in families from
Northern-European ancestry was supported by National
Institutes of Health (NIH) Grant DK39311 and the Re-
search Service of the Department of Veterans Affairs. The
HKFDS study was supported by the Hong Kong Research
Grants Committee (CUHK 4292/99M; 1/04C), the Chinese
University of Hong Kong Strategic Grant Program
(SRP9902), and the Hong Kong Innovation and Technology
Support Fund (ITS/33/00). Support for the AADM study
was provided by NIH grant 3T37TW00041-03S2 from the
Office of Research on Minority Health. AADM was also
supported in part by the National Center for Research
Resources, the National Human Genome Research Insti-
tute, and by the NIDDK grant DK-54001. Genotyping
services were provided by the Center for Inherited Disease
Research (CIDR) (http://www.cidr.jhmi.edu). CIDR is fully
funded through a federal contract from the NIH to Johns
Hopkins University, contract number N01-HG-65403. This
research was supported in part by the intramural research
program of the NIDDK.

We also thank investigators and staff of the AFDS based
at the University of Maryland, including Alan R. Shuldiner,
MD, Braxton D. Mitchell, and associated faculty, including
technical and clinical staff, and especially the outstanding
cooperation of the Amish Community, without which the
AFDS would not have been possible. We thank the AADM
investigators and are deeply grateful to AADM partici-
pants, their families, and physicians.

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896 DIABETES, VOL. 56, MARCH 2007