Brief Genetics Report

Polymorphisms in Both Promoters of Hepatocyte
Nuclear Factor 4-� Are Associated With Type 2
Diabetes in the Amish
Coleen M. Damcott,

1
Nicole Hoppman,

1
Sandra H. Ott,

1
Laurie J. Reinhart,

1
Jian Wang,

1

Toni I. Pollin,
1

Jeffrey R. O’Connell,
1

Braxton D. Mitchell,
1

and Alan R. Shuldiner
1,2

Hepatocyte nuclear factor 4-� (HNF4A) is a transcrip-
tion factor located on chromosome 20q13 that regulates

expression of genes involved in glucose metabolism and

homeostasis. Recently, two groups independently iden-

tified single nucleotide polymorphism (SNPs) in an

alternate upstream promoter (P2) of HNF4A that were

associated with type 2 diabetes in Ashkenazi Jews and

Finns. We genotyped haplotype-tagging SNPs (htSNPs)

across the two promoter regions and the coding region

of HNF4A in individuals with type 2 diabetes (n � 137),
impaired glucose tolerance (IGT) (n � 139), and normal
glucose tolerance (n � 342) from the Amish Family
Diabetes Study (AFDS) to test for association with type

2 diabetes. In the P1 promoter region, we observed a

significant association between the A allele of

rs2425640 and type 2 diabetes (odds ratio [OR] 1.60,

P � 0.03). Furthermore, the mean age of type 2 diabetes
onset was, on average, 5.1 years earlier in those with the

AA or GA genotype at SNP rs2425640 than in those with

the GG genotype (57.8 vs. 62.9 years, P � 0.011). In the
P2 promoter, the htSNP rs1884614 showed borderline

association with both type 2 diabetes (OR 1.40, P �
0.09) and the combined type 2 diabetes/IGT trait (1.35,

P � 0.07). In an expanded set of 698 nondiabetic AFDS
subjects, we found association between rs1884614 and

glucose area under the curve during an oral glucose

tolerance test (additive model, P � 0.022; dominant
model, P � 0.010). The results of this study provide
evidence that variants in both the P1 and P2 promoters

of HNF4A increase risk for typical type 2 diabetes.

Diabetes 53:3337–3341, 2004

H
epatocyte nuclear factor 4-� (HNF4A) is a
transcription factor that is expressed in several
tissues, including liver and pancreas, where it
regulates expression of genes involved in glu-

coneogenesis and glucose-stimulated insulin secretion,
respectively (1– 4). Relatively rare mutations in HNF4A
have been identified that cause maturity-onset diabetes of
the young type 1 (rev. in 5), a dominantly inherited,
early-onset form of type 2 diabetes characterized by im-
paired glucose-induced insulin secretion due to pancreatic
�-cell dysfunction (6 –9). HNF4A expression patterns are
complex as a result of alternative splicing and transcrip-
tion from two different promoters, the proximal P1 pro-
moter and the P2 promoter, which lies �45 kb upstream of
the P1 promoter (10 –13).

The 12 coding exons of HNF4A span �29 kb on chro-
mosome 20q13, a region of overlapping linkage to type 2
diabetes in several Caucasian (14 –19) and Asian (20,21)
populations. Recently, through fine-mapping efforts in this
region of chromosome 20q, two groups concurrently iden-
tified single nucleotide polymorphisms (SNPs) in the P2
and P1 promoter regions and coding exons of HNF4A that
are associated with type 2 diabetes in the Ashkenazi Jews
(22) and Finns (FUSION 1 [Finland-United States Investi-
gation of NIDDM Genetics 1]) (23). Silander et al. (23)
identified 10 SNPs across a 64-kb region spanning the P2
and P1 promoter regions and exons 1–3 of HNF4A that
were associated with type 2 diabetes in the FUSION 1
population. In the Ashkenazi Jewish cohort, the SNPs
closer to the P1 promoter and coding exons were not
associated with type 2 diabetes (22); however, four SNPs
spanning a �10-kb region encompassing the P2 promoter
were associated with type 2 diabetes (rs4810424,
rs1884613, rs1884614, and rs2144908). These four SNPs are
located in a 177-kb region of strong linkage disequilibrium
(LD), including �140 kb upstream of the P2 promoter (23).
A second haplotype block was observed within the
HNF4A coding region, while LD tended to decay across
the �45-kb gap separating HNF4A from P2 (22,23). In
addition to the observed association with type 2 diabetes,
these P2 SNPs appeared to explain a significant portion of
the linkage to chromosome 20q12-q13 observed in both the
Ashkenazi Jews and Finns. The replicating evidence pre-

From the 1Division of Endocrinology, Diabetes and Nutrition, University of
Maryland School of Medicine, Baltimore, Maryland; and the 2Geriatric Re-
search and Education Clinical Center, Veterans Administration Medical Cen-
ter, Baltimore, Maryland.

Address correspondence and reprint requests to Alan R. Shuldiner, MD,
Division of Endocrinology, Diabetes and Nutrition, University of Maryland
School of Medicine, 660 West Redwood St., Room 494, Baltimore, MD 21201.
E-mail: ashuldin@medicine.umaryland.edu.

Received for publication 16 June 2004 and accepted in revised form 27
August 2004.

AFDS, Amish Family Diabetes Study; HNF, hepatocyte nuclear factor;
htSNP, haplotype-tagging single nucleotide polymorphism; IGT, impaired
glucose tolerance; LD, linkage disequilibrium; NGT, normal glucose tolerance;
OGTT, oral glucose tolerance test; SNP, single nucleotide polymorphism.

© 2004 by the American Diabetes Association.

DIABETES, VOL. 53, DECEMBER 2004 3337



sented by these studies suggests that SNPs near the P2
promoter of HNF4A increase susceptibility to type 2
diabetes.

Although no evidence for linkage to type 2 diabetes was
detected on chromosome 20q12-q13 in our genome-wide
scan (average marker density � 9.7 cM) in the Old Order
Amish (logarithm of odds � 0.00 between markers
D20S107 and D20S119, which are �6 cM apart) (24), we
tested whether SNPs in HNF4A and its promoters were
associated with type 2 diabetes in the Amish. We selected
six haplotype-tagging SNPs (htSNPs) spanning the P2 and
P1 promoters and the HNF4A coding region from the LD
blocks defined in the Ashkenazi Jews (22) and Finns (23).
Given that the Amish are a young founder population, we
hypothesized that haplotype blocks would be as large as or
larger than those in the other populations, thus allowing us
to capture most or all of the variation across the gene with
these SNPs. These SNPs were genotyped in 618 individuals
enrolled in the Amish Family Diabetes Study (AFDS),
which included 137 subjects with type 2 diabetes, 139
individuals with impaired glucose tolerance (IGT), and 342
control subjects with normal glucose tolerance (NGT).
The NGT control subjects selected were �38 years of age
in order to increase the probability of their capacity for
diabetes resistance. Table 1 summarizes the allele frequen-
cies in individuals with type 2 diabetes, IGT, and NGT and
the results of genotypic association analysis for each SNP.
All SNPs conformed to Hardy-Weinberg expectations. For
rs2425640, one of the SNPs located in the P1 promoter
region, the frequency of the A allele was significantly
higher in the type 2 diabetic group than in the control
group in the Amish (genotypic odds ratio [OR] 1.60, P �
0.030). Furthermore, the mean age of diabetes onset was

58.0 years in subjects with the AA genotype for SNP
rs2425640, 57.8 years in those with the GA genotype, and
62.9 years in those with the GG genotype. The mean age of
type 2 diabetes onset was, on average, 5.1 years earlier in
those with the AA or GA genotype at SNP rs2425640 than
in those with the GG genotype (57.8 vs. 62.9 years, P �
0.011).

We genotyped one (rs1884614) of the four P2 promoter
SNPs reported to be associated with type 2 diabetes and in
near-perfect LD with each other in both the Ashkenazi
Jewish and Finnish populations. In the Amish, the frequency
of the A allele at the rs1884614 SNP was lower in control
subjects with NGT than in both the the type 2 diabetic group
(genotypic OR 1.40, P � 0.09) and the combined type 2
diabetic/IGT group (genotypic OR 1.35, P � 0.07), although
these differences did not achieve statistical significance, as
observed in the Ashkenazi Jews and Finns. None of the other
SNPs in the P1 promoter region or the coding region were
associated with type 2 diabetes in the Amish, including the
other SNPs observed to be associated with type 2 diabetes in
the Finns (rs2425637 and rs3212183) and Ashkenazi
Jews (rs3818247). Haplotype analysis revealed that only
those haplotypes containing the rs2425640 A allele and
rs1884614 A allele were associated with increased type 2
diabetes prevalence (results not shown).

Table 2 shows the pairwise LD (�D�� and r2) among the
genotyped SNPs in the Amish. The haplotype block struc-
ture in the Amish appears very similar to that reported in
Finns and Ashkenazi Jews, suggesting that the SNP den-
sity we chose is adequate for the detection of most of the
common variation in HNF4A. As shown in the Ashkenazi
Jews and the Finns, the SNP representing the P2 haplotype
block that was genotyped in the Amish (rs1884614) was

TABLE 1
Allele frequencies and results of association analysis in subjects with type 2 diabetes, IGT, and NGT for SNPs in the HNF4A region

Minor allele frequency
Diabetes
vs. NGT*

Diabetes �
IGT

vs. NGT*
SNP location
(kb)†

SNP
name

Major/minor
allele

Type 2 diabetes
(n � 137)

IGT
(n � 139)

NGT
(n � 342) OR P OR P

	3.926 rs1884614 G/A 0.208 0.180 0.139 1.40 0.09 1.35 0.07
39.604 rs2425637 G/T 0.380 0.368 0.372 1.00 0.99 1.04 0.82
43.592 rs2425640 G/A 0.414 0.363 0.363 1.60 0.03 1.26 0.16
50.693 rs3212183 T/C 0.377 0.374 0.368 0.97 0.88 0.98 0.89
66.316 rs1028583 G/T 0.411 0.358 0.382 0.83 0.35 0.94 0.67
73.035 rs3818247 G/T 0.255 0.281 0.265 0.93 0.82 0.87 0.53

*P values are based on genotype frequencies, and ORs reflect the odds of disease associated with having two copies of the minor allele versus
the odds of disease associated with having two copies of the major allele and were adjusted for age, sex, and pedigree structure. Reported
P values are not adjusted for multiple comparisons. P values 
0.05 are shown in bold.

TABLE 2
Pairwise LD among HNF4A SNPs in the Amish*

rs1884614 rs2425637 rs2425640 rs3212183 rs1028583 rs3818247

rs1884614 — 0.40 0.12 0.13 0.38 0.52
rs2425637 0.05 — 0.81 0.83 0.06 0.11
rs2425640 0 0.28 — 0.65 0.33 0.35
rs3212183 0.01 0.65 0.17 — 0.12 0.21
rs1028583 0.04 0 0.09 0.01 — 0.63
rs3818247 0.13 0.01 0.07 0.01 0.27 —

*Values in the upper right represent �D�� , while values in the bottom left represent r2. Shown in bold are the two SNPs, rs1884614 and
rs2425640, in the P2 and P1 promoters, respectively, that were associated with type 2 diabetes and glucose traits.

HNF4A AND TYPE 2 DIABETES IN THE AMISH

3338 DIABETES, VOL. 53, DECEMBER 2004



clearly not in LD with rs2425640 in the P1 promoter or
with the other HNF4A SNPs.

In addition to the case/control analysis, we genotyped
rs1884614 and rs2425640 in an additional 217 nondiabetic
Amish subjects to create an expanded set of 698 nondia-
betic individuals (NGT [n � 568] and IGT [n � 130]) and
performed an association analysis with diabetes-related
quantitative traits. Figure 1 shows the mean plasma glu-
cose levels at 30-min intervals during a 3-h oral glucose
tolerance test (OGTT) according to genotype at the
rs1884614 SNP. Carriers of the A “risk” allele for the
rs1884614 SNP exhibited significantly higher total glucose
area under the curve during the OGTT (additive model,
P � 0.022; dominant model, P � 0.010). Higher glucose
levels in nondiabetic A carriers provides additional evi-
dence that the A allele of rs1884614 (or a haplotype
marked by this allele) influences glucose homeostasis and
type 2 diabetes risk. However, presence of the A allele was
not associated with either fasting insulin or total insulin
area under the OGTT curve (Fig. 1). Although we do not
have direct measures of insulin secretion, the finding of
increased OGTT glucose levels without differences in
OGTT insulin levels in carriers of the A “risk” allele
suggests a relative deficiency in insulin secretion in these

individuals. This interpretation is consistent with the hy-
pothesis that the A allele, present in the islet-specific P2
promoter, may decrease expression of HNF4A in insulin-
secreting �-cells, thus affecting �-cell function. The quan-
titative trait analysis for rs2425640 in the P1 promoter
showed no association with glucose- or insulin-related
traits.

In conclusion, we found that htSNPs in the P1 and P2
regions of HNF4A are associated with type 2 diabetes and
diabetes-related traits in the Amish. Rs2425640 in the P1
region was also associated with type 2 diabetes in the
Finns; however, contrary to our findings in the Amish, in
which the A allele was the at-risk allele for both type 2
diabetes risk and an earlier onset of diabetes, the fre-
quency of the G allele was significantly higher in Finnish
subjects with type 2 diabetes. This discrepancy between
the two populations may indicate that this SNP is not the
functional SNP but is marking an at-risk haplotype that
differs between the Amish and Finns. Of note, this SNP
was not associated with type 2 diabetes in the Ashkenazi
Jews, but others in the region were associated with type 2
diabetes, suggesting again that the SNPs thus far examined
may be marking at-risk haplotypes in the different popu-
lations. Alternatively these discrepancies between popula-

FIG. 1. Mean plasma glucose (A) and insulin (B) levels at 30-min intervals during a 3-h 75-g OGTT according to SNP rs1884614 genotype groups.
Carriers of the A “risk” allele exhibited higher total glucose area under the curve during the OGTT (additive model, P � 0.022; dominant model,
P � 0.010). There was no association with total insulin area under the curve during the OGTT (additive model, P � 0.919; dominant model, P �
0.919).

C.M. DAMCOTT AND ASSOCIATES

DIABETES, VOL. 53, DECEMBER 2004 3339



tions could represent false-positive or false-negative
results. Rs1884614, an htSNP in the P2 region of HNF4A
was associated with glucose levels during an OGTT in the
Amish and was also associated with type 2 diabetes in
both the Ashkenazi Jews and the Finns. In all populations
studied to date, the P1 and P2 SNPs reside in different
haplotype blocks, suggesting the presence of two indepen-
dent variants influencing type 2 diabetes risk. This repli-
cation across several studies lends further support to the
possibility that variation in the P1 and P2 regions of
HNF4A, or SNPs in strong LD with these regions, contrib-
utes to the pathogenesis of type 2 diabetes. Of note, our
genome scan did not provide any evidence for linkage to
type 2 diabetes or related traits to this region of chromo-
some 20 in the Amish (24). This observation is likely due to
the relative insensitivity of linkage analysis compared with
association analysis and suggests that this allele may also
influence type 2 diabetes risk more broadly in other
populations. Although HNF4A is the strongest candidate
gene for type 2 diabetes in this region, the P2 SNPs reside
in a large haplotype block that contains several other
known and predicted genes and expressed sequence tags;
therefore, the possibility must be considered that the
pathogenic SNP(s) may reside in another gene. Further
studies in other populations, as well as functional analysis,
will be required to further define the role of variation in
HNF4A in type 2 diabetes pathogenesis.

RESEARCH DESIGN AND METHODS

The AFDS was initiated in 1995 with the goal of identifying susceptibility
genes for type 2 diabetes and related traits in a cohort of individuals from the
Old Order Amish population in Lancaster County, Pennsylvania. Details of the
AFDS design, recruitment, phenotyping, and pedigree structure have been
described previously (25). Briefly, probands with previously diagnosed type 2
diabetes (onset between 35 and 65 years of age) and all first- and second-
degree relatives of probands and spouses over the age of 18 were recruited.
Phenotypic characterization of study participants included medical and family
history, anthropometry, and a 3-h 75-g OGTT with insulin levels. The diagnosis
of type 2 diabetes was defined on the basis of the OGTT using criteria of the
American Diabetes Association (2-h glucose �11.1 mmol/l or fasting glucose
�7 mmol/l), by current treatment with diabetes medications, or by a previous
physician-documented diagnosis of diabetes. IGT was defined by a 2-h OGTT
glucose between 7.8 and 11.1 mmol/l. NGT was defined by a fasting glucose

6.1 mmol/l and a 2-h OGTT glucose 
7.8 mmol/l. The total glucose and
insulin areas under the curve during the 3-h OGTT were calculated using the
trapezoid method. BMI was calculated as weight (in kilograms) divided by
height (in meters) squared. The mean age of diagnosis of diabetes in the AFDS
cohort was 57.8 � 5.7 years, and the mean BMI was 27.2 � 5.0 kg/m2 (range
22.4 –38.3). Informed consent was obtained from all study subjects, and the
Institutional Review Board at the University of Maryland School of Medicine
approved the study protocol.
Genotyping. Genotyping was completed using the Orchid/Beckman
SNPstream Ultra High Throughput genotyping platform. This genotyping
method is described in detail elsewhere (26). Briefly, the protocol involved
PCR amplification of target sequences surrounding the SNPs to be assayed in
panels of 12-plex reactions. Following enzymatic purification, the PCR prod-
ucts were subjected to single-base primer extension with fluorescent-labeled
dye terminators. Each extension primer contained a unique 20-nucleotide tail
at its 5� end whose sequence was designed to hybridize to its complementary
probe immobilized in a mini-array within each well of a 384-well SNP-IT plate
(Beckman Coulter, Fullerton, CA). The microarray plate was imaged by the
SNPscope reader (Beckman Coulter). The two-color system allowed the
detection of the SNP by comparing signals from the two fluorescent dyes. The
image signals were then transferred to genotyping software that translated the
images of the arrays into genotype calls. The error rate based upon blind
replicates for the SNPs examined in the present study was 0 –1.2%.
Statistical analysis. Before analysis, genotypes were checked for Mendelian
consistency using the pedigree information and inconsistencies (
.5% of
genotypes) were resolved or removed before analysis. Allele frequencies were
calculated for each SNP by gene counting, and observed genotypes were

tested for fit to the expectations of Hardy-Weinberg using the �2 test. Pairwise
LD was computed between the SNPs using the two most commonly used
statistics �D�� and r2, and haplotypes were inferred for each individual using
an expectation maximization algorithm implemented in the ZAPLO software
program (27).

We evaluated the association between SNP genotype and disease status
(type 2 diabetes versus NGT and type 2 diabetes/IGT versus NGT) using a
variance component approach, in which we modeled the probability that the
subject was a case or control subject, as a function of the individual’s age, sex,
and genotype, conditional on the correlations in phenotype among relative
pairs. For the primary analysis, we considered an additive genetic model in
which the genotype was coded as 0, 1, or 2, depending on whether the subject
was homozygous for the minor allele (genotype � 2), heterozygous (geno-
type � 1), or homozygous for the major allele (genotype � 0). Statistical
testing was accomplished using the likelihood ratio test, in which we
compared the likelihood of the data under a model in which the genotype
effect was estimated against the likelihood of a nested model in which the
genotype effect was constrained to be zero. Secondary analyses were carried
out under the dominant and recessive genetic models by imposing appropriate
constraints on the genotypic effects. Parameter estimates (i.e., � coefficients)
were obtained by maximum likelihood and ORs by taking the inverse log of
the � coefficient. The OR for the additive model was scaled to reflect the odds
that a case was homozygous for the minor allele versus the odds that the case
was homozygous for the major allele. The variance components analysis was
carried out using the SOLAR software program (28).

Finally, mean levels of glucose (fasting and glucose area under the curve
during a 3-h OGTT) and insulin (fasting and insulin area under the curve
during a 3-h OGTT) were estimated according to HNF4A genotypes in an
expanded set of nondiabetic AFDS subjects (n � 698). To account for the
relatedness among family members, the measured genotype approach was
used (29), in which we estimated the likelihood of specific genetic models
given the pedigree structure. Parameter estimates were obtained by maximum
likelihood methods, and the significance of association was tested by likeli-
hood ratio tests. Within each model, we simultaneously estimated the effects
of age and sex. Insulin values were transformed by their natural logarithms
(ln) to reduce skewness. Quantitative trait analyses were conducted using the
SOLAR program (28).

ACKNOWLEDGMENTS

This work was supported by research grants R01-
DK54261, K24-DK02673, U01-DK58026, and K07-CA67960;
the University of Maryland General Clinical Research
Center Grant M01 RR 16500; the General Clinical Research
Centers Program; the National Center for Research Re-
sources (NCRR); the National Institutes of Health; and the
Baltimore Veterans Administration Geriatric Research and
Education Clinical Center.

We gratefully acknowledge our Amish liaisons and field
workers and the extraordinary cooperation and support of
the Amish community, without whom these studies would
not be possible.

REFERENCES

1. Stoffel M, Duncan SA: The maturity-onset diabetes of the young (MODY1)
transcription factor HNF4alpha regulates expression of genes required for
glucose transport and metabolism. Proc Natl Acad Sci U S A 94:13209 –
13214, 1997

2. Wang H, Maechler P, Antinozzi PA, Hagenfeldt KA, Wollheim CB: Hepato-
cyte nuclear factor 4alpha regulates the expression of pancreatic beta-cell
genes implicated in glucose metabolism and nutrient-induced insulin
secretion. J Biol Chem 275:35953–35959, 2000

3. Bartoov-Shifman R, Hertz R, Wang H, Wollheim CB, Bar-Tana J, Walker
MD: Activation of the insulin gene promoter through a direct effect of
hepatocyte nuclear factor 4 alpha. J Biol Chem 277:25914 –25919, 2002

4. Rhee J, Inoue Y, Yoon JC, Puigserver P, Fan M, Gonzalez FJ, Spiegelman
BM: Regulation of hepatic fasting response by PPARgamma coactivator-
1alpha (PGC-1): requirement for hepatocyte nuclear factor 4alpha in
gluconeogenesis. Proc Natl Acad Sci U S A 100:4012– 4017, 2003

5. Ryffel GU: Mutations in the human genes encoding the transcription
factors of the hepatocyte nuclear factor (HNF)1 and HNF4 families:
functional and pathological consequences. J Mol Endocrinol 27:11–29,
2001

HNF4A AND TYPE 2 DIABETES IN THE AMISH

3340 DIABETES, VOL. 53, DECEMBER 2004



6. Hattersley AT: Maturity-onset diabetes of the young: clinical heterogeneity
explained by genetic heterogeneity. Diabet Med 15:15–24, 1998

7. Fajans SS, Bell GI, Polonsky KS: Molecular mechanisms and clinical
pathophysiology of maturity-onset diabetes of the young. N Engl J Med
345:971–980, 2001

8. Stride A, Hattersley AT: Different genes, different diabetes: lessons from
maturity-onset diabetes of the young. Ann Med 34:207–216, 2002

9. Winter WE: Newly defined genetic diabetes syndromes: maturity onset
diabetes of the young. Rev Endocr Metab Disord 4:43–51, 2003

10. Nakhei H, Lingott A, Lemm I, Ryffel GU: An alternative splice variant of the
tissue specific transcription factor HNF4alpha predominates in undiffer-
entiated murine cell types. Nucleic Acids Res 26:497–504, 1998

11. Thomas H, Jaschkowitz K, Bulman M, Frayling TM, Mitchell SM, Roosen S,
Lingott-Frieg A, Tack CJ, Ellard S, Ryffel GU, Hattersley AT: A distant
upstream promoter of the HNF-4alpha gene connects the transcription
factors involved in maturity-onset diabetes of the young. Hum Mol Genet
10:2089 –2097, 2001

12. Boj SF, Parrizas M, Maestro MA, Ferrer J: A transcription factor regulatory
circuit in differentiated pancreatic cells. Proc Natl Acad Sci U S A
98:14481–14486, 2001

13. Eeckhoute J, Moerman E, Bouckenooghe T, Lukoviak B, Pattou F,
Formstecher P, Kerr-Conte J, Vandewalle B, Laine B: Hepatocyte nuclear
factor 4 alpha isoforms originated from the P1 promoter are expressed in
human pancreatic beta-cells and exhibit stronger transcriptional potentials
than P2 promoter-driven isoforms. Endocrinology 144:1686 –1694, 2003

14. Bowden DW, Sale M, Howard TD, Qadri A, Spray BJ, Rothschild CB, Akots
G, Rich SS, Freedman BI: Linkage of genetic markers on human chromo-
somes 20 and 12 to NIDDM in Caucasian sib pairs with a history of diabetic
nephropathy. Diabetes 46:882– 886, 1997

15. Ji L, Malecki M, Warram JH, Yang Y, Rich SS, Krolewski AS: New
susceptibility locus for NIDDM is localized to human chromosome 20q.
Diabetes 46:876 – 881, 1997

16. Zouali H, Hani EH, Philippi A, Vionnet N, Beckmann JS, Demenais F,
Froguel P: A susceptibility locus for early-onset non-insulin dependent
(type 2) diabetes mellitus maps to chromosome 20q, proximal to the
phosphoenolpyruvate carboxykinase gene. Hum Mol Genet 6:1401–1408,
1997

17. Ghosh S, Watanabe RM, Hauser ER, Valle T, Magnuson VL, Erdos MR,
Langefeld CD, Balow J Jr, Ally DS, Kohtamaki K, Chines P, Birznieks G,
Kaleta HS, Musick A, Te C, Tannenbaum J, Eldridge W, Shapiro S, Martin
C, Witt A, So A, Chang J, Shurtleff B, Porter R, Boehnke M: Type 2 diabetes:
evidence for linkage on chromosome 20 in 716 Finnish affected sib pairs.
Proc Natl Acad Sci U S A 96:2198 –2203, 1999

18. Ghosh S, Watanabe RM, Valle TT, Hauser ER, Magnuson VL, Langefeld CD,
Ally DS, Mohlke KL, Silander K, Kohtamaki K, Chines P, Balow JJ,
Birznieks G, Chang J, Eldridge W, Erdos MR, Karanjawala ZE, Knapp JI,
Kudelko K, Martin C, Morales-Mena A, Musick A, Musick T, Pfahl C, Porter
R, Rayman JB: The Finland-United States investigation of non-insulin-
dependent diabetes mellitus genetics (FUSION) study. I. An autosomal

genome scan for genes that predispose to type 2 diabetes. Am J Hum
Genet 67:1174 –1185, 2000

19. Permutt MA, Wasson JC, Suarez BK, Lin J, Thomas J, Meyer J, Lewitzky S,
Rennich JS, Parker A, DuPrat L, Maruti S, Chayen S, Glaser B: A genome
scan for type 2 diabetes susceptibility loci in a genetically isolated
population. Diabetes 50:681– 685, 2001

20. Luo TH, Zhao Y, Li G, Yuan WT, Zhao JJ, Chen JL, Huang W, Luo M: A
genome-wide search for type II diabetes susceptibility genes in Chinese
Hans. Diabetologia 44:501–506, 2001

21. Mori Y, Otabe S, Dina C, Yasuda K, Populaire C, Lecoeur C, Vatin V, Durand
E, Hara K, Okada T, Tobe K, Boutin P, Kadowaki T, Froguel P: Genome-
wide search for type 2 diabetes in Japanese affected sib-pairs confirms
susceptibility genes on 3q, 15q, and 20q and identifies two new candidate
Loci on 7p and 11p. Diabetes 51:1247–1255, 2002

22. Love-Gregory LD, Wasson J, Ma J, Jin CH, Glaser B, Suarez BK, Permutt
MA: A common polymorphism in the upstream promoter region of the
hepatocyte nuclear factor-4 � gene on chromosome 20q is associated with
type 2 diabetes and appears to contribute to the evidence for linkage in an
ashkenazi jewish population. Diabetes 53:1134 –1140, 2004

23. Silander K, Mohlke KL, Scott LJ, Peck EC, Hollstein P, Skol AD, Jackson
AU, Deloukas P, Hunt S, Stavrides G, Chines PS, Erdos MR, Narisu N,
Conneely KN, Li C, Fingerlin TE, Dhanjal SK, Valle TT, Bergman RN,
Tuomilehto J, Watanabe RM, Boehnke M, Collins FS: Genetic variation
near the hepatocyte nuclear factor-4 � gene predicts susceptibility to type
2 diabetes. Diabetes 53:1141–1149, 2004

24. Hsueh WC, St Jean PL, Mitchell BD, Pollin TI, Knowler WC, Ehm MG, Bell
CJ, Sakul H, Wagner MJ, Burns DK, Shuldiner AR: Genome-wide and
fine-mapping linkage studies of type 2 diabetes and glucose traits in the
Old Order Amish: evidence for a new diabetes locus on chromosome 14q11
and confirmation of a locus on chromosome 1q21– q24. Diabetes 52:550 –
557, 2003

25. Hsueh WC, Mitchell BD, Aburomia R, Pollin T, Sakul H, Gelder EM,
Michelsen BK, Wagner MJ, St Jean PL, Knowler WC, Burns DK, Bell CJ,
Shuldiner AR: Diabetes in the Old Order Amish: characterization and
heritability analysis of the Amish Family Diabetes Study. Diabetes Care
23:595– 601, 2000

26. Bell PA, Chaturvedi S, Gelfand CA, Huang CY, Kochersperger M, Kopla R,
Modica F, Pohl M, Varde S, Zhao R, Zhao X, Boyce-Jacino MT, Yassen A:
SNPstream UHT: ultra-high throughput SNP genotyping for pharmacog-
enomics and drug discovery. Biotechniques (Suppl.):70 –72, 74, 76 –77,
2002 [erratum in Biotechniques 34:496, 2003]

27. O’Connell JR: Zero-recombinant haplotyping: applications to fine mapping
using SNPs. Genet Epidemiol 19 (Suppl. 1):S64 –S70, 2000

28. Almasy L, Blangero J: Multipoint quantitative-trait linkage analysis in
general pedigrees. Am J Hum Genet 62:1198 –1211, 1998

29. Boerwinkle E, Chakraborty R, Sing CF: The use of measured genotype
information in the analysis of quantitative phenotypes in man. I. Models
and analytical methods. Ann Intern Med 50:181–194, 1986

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