1 Department of Medicine, University Health Network, University of Toronto, Toronto, Canada
2 Program in Genetics and Genomic Biology, Hospital for Sick Children, Toronto, Canada
3 Department of Public Health Sciences, University of Toronto, Toronto, Canada
4 Samuel Lunenfeld Research Institute of Mount Sinai Hospital, Prosserman Center for Health Research, University of Toronto, Toronto, Canada
5 Leadership Sinai Centre for Diabetes, Department of Medicine, Mount Sinai Hospital, Toronto, Canada
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ABSTRACT |
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Microvascular and neurologic complications of type 1 diabetes result in significant morbidity and mortality. The Diabetes Control and Complications Trial (DCCT) demonstrated that intensive therapy aimed at reducing glycemic exposure reduced the development and progression of long-term complications by as much as 76% compared with conventional therapy (1). In addition to the importance of intensive diabetes management, it is clear that there are other factors, including genetic ones, that contribute to the development of these complications. Epidemiologic studies (2,3) conducted before the use of intensive therapy suggested that 30% of patients with type 1 diabetes developed diabetic nephropathy after 20 years of diabetes; however, modern diabetes care has markedly reduced the incidence of diabetic nephropathy to 1316% (46) after 20 years diabetes duration. A number of studies have documented familial clustering of diabetic nephropathy (79). In the DCCT, there was an increased risk of microalbuminuria (albumin excretion rate [AER] >28 µg/min) in diabetic relatives of microalbuminuria-positive versus -negative DCCT subjects in the secondary intervention cohort (odds ratio 5.4 [95% CI 2.213.7], P < 0.001) after adjustment for covariates (10). Given the evidence for familial clustering of diabetic nephropathy, we have begun a systematic study of candidate genes associated with the development of nephropathy in the DCCT subjects.
ACE plays an important role in the renin-angiotensin-aldosterone pathway and has been studied extensively as a putative mediator of diabetic nephropathy. This enzyme cleaves the COOH-terminal dipeptide of angiotensin I to produce angiotensin II and inactivates bradykinin by removal of COOH-terminal peptides. Increased ACE activity increases intraglomerular pressure (11) and can lead to glomerulosclerosis (12). Plasma ACE activity, a highly heritable trait, is encoded by one of the three known isozymes transcribed from the ACE gene, which is composed of 26 exons located on chromosome 17q23 (13). There are many biallelic single nucleotide polymorphisms (SNPs) within and flanking this gene (14) that are associated with ACE activity; however, the exact etiologic variant(s) is/are as yet undetermined, as these polymorphisms are in strong linkage disequilibrium with each other (15). The most extensively studied polymorphism is the insertion/deletion of a 287-bp Alu repeat in intron 16 (16).
Since the initial report of the protective effect of the I/I insertion/deletion genotype in the development of diabetic nephropathy in type 1 diabetes (17), there have been many other studies of the association of this polymorphism with elevated urinary excretion of albumin and/or nephropathy in patients with type 1 and type 2 diabetes. Meta-analyses (1820) have suggested that discrepant results among studies may be partially attributed to differences in study design, diabetes phenotype (type 1 diabetes versus type 2 diabetes), ethnic composition, methods of quantitation, and estimation of AER (e.g., single measures of AER versus sustained elevations in AER) and definitions of diabetic nephropathy (microalbuminuria versus macroalbuminuria).
The DCCT and its long-term follow-up, the Epidemiology of Diabetes Interventions and Complications (EDIC) study, have measured renal function, albuminuria, and the development of nephropathy for up to 17 years using standardized methods. We have analyzed the association of the insertion/deletion polymorphism of the ACE gene with the time to development of persistent elevation of microalbuminuria and severe nephropathy in 1,365 Caucasian subjects in the DCCT/EDIC study. To capture the genetic variation in the most common Caucasian haplotypes at the ACE locus occurring at frequencies >5% (15), we also genotyped two SNPs (http://www.ncbi.nlm.nih.gov/SNP/), rs1800764 and rs9896208, flanking the insertion/deletion polymorphism in the 5' and 3' untranslated region and analyzed the association of variation at these three loci with nephropathy outcomes using Cox proportional hazards models of complication-free survival. To reduce population heterogeneity, we restrict the analysis to self-identified "white" subjects only, which represent 96% of the original cohort.
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RESEARCH DESIGN AND METHODS |
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Phenotypic characterization of nephropathy.
Two nephropathy outcomes, persistent microalbuminuria and severe nephropathy, were defined using repeated 4-h AER measurements obtained yearly during the DCCT and every 2nd year during EDIC. Persistent microalbuminuria was defined as an AER 20.8 µg/min on two consecutive assessments. The definition of severe nephropathy is also based on repeated measures of AER and represents the progression from persistent microalbuminuria to an AER
208 µg/min or renal replacement therapy (dialysis or transplant). Time to outcome development or censoring was determined as number of visit years from DCCT baseline up to and including the 8th year of EDIC follow-up (2001); mean (±SD) follow-up from DCCT entry was 13.5 ± 2.6 years. Subjects meeting the criteria for persistent microalbuminuria at DCCT baseline and DCCT year 1 (n = 66) were excluded from subsequent analyses of that outcome. Due to the DCCT exclusion criteria, no subjects had severe nephropathy at baseline.
Determination of ACE genotypes.
Genetic variation at the ACE gene has been extensively studied, and haplotypes have been determined (15,22). Fifteen haplotypes were identified by measured haplotype analysis in families, but because of extensive linkage disequilibrium between markers, only four common haplotypes had frequencies >5% (15). In addition to the insertion/deletion polymorphism, we genotyped two SNPs that allowed us to capture the four most common haplotypes occurring with frequency >5% in Caucasian populations. The intermarker distance between the 5' SNP, rs1800764 (T7715C) (15), and the insertion/deletion is 15.4 kb and between the insertion/deletion and the 3' SNP, rs9896208 (T33569C) (15), is 10.4 kb (see online appendix for genotyping protocol).
Statistical analysis.
The primary analysis was to evaluate the association between each of the ACE markers and the risk of complications, taking into account the DCCT/EDIC study design and potential confounding factors, including all physiological traits known to be associated with variation in risk of renal complications. The relative risks associated with different marker genotypes were estimated by the hazard ratio (HR) in the Cox proportional hazards model, with and without including explanatory covariates in the model (see online appendix for further description of analysis).
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RESULTS |
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The quality characteristics of the genotype data were assessed by replicate Centre dEtude du Polymorphisme Humain (CEPH) control samples, and of 498 replicate genotypes at the three markers, only two genotyping errors occurred corresponding to an observed genotyping error rate of 0.4%. The minor allele frequencies for rs1800764, insertion/deletion, and rs9896208 were 0.45, 0.47, and 0.37, respectively. No significant deviations from Hardy-Weinberg equilibrium were observed.
Proportional hazards analysis of the ACE polymorphisms adjusted for DCCT year of entry, cohort, and treatment strata indicate that genotype variation at each of the markers was significantly associated with the risk of developing persistent microalbuminuria (Table 2). Specifically, as depicted in Fig. 1, individuals with either the T/T, I/I, or C/C genotypes at rs1800764, insertion/deletion, and rs9896208, respectively, had a lower risk of progression to persistent microalbuminuria during a maximum of 17 years of follow-up from DCCT baseline. Individuals with the C/C genotype at rs9896208 had a significantly lower risk of development of persistent microalbuminuria (HR 0.70 [95% CI 0.530.93], P = 0.015) (Fig. 1 and Table 2) and severe nephropathy (0.60 [0.390.92], P = 0.020) (online appendix Fig. A1 and Table A2). Genotypes at rs1800764 and insertion/deletion, however, were not significantly (P > 0.05) associated with severe nephropathy in analyses that did not take any of the DCCT baseline physiological trait variables into account (Table 2).
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When we adjusted for the additional covariates (Table 3 legend), the association of each of the three ACE variants with the development of persistent microalbuminuria remained significant (Table 3). Values of R2 indicating the proportion of explained variability in survival times to persistent microalbuminuria were calculated as 0.8, 0.6, and 0.8% for rs1800764, insertion/deletion, and rs9896208 markers, respectively. For severe nephropathy, adjustment for covariates in the multivariate model strengthened the genotype associations (Table 3). At rs1800764, individuals with the T/T genotype had a lower risk than C/T heterozygotes. Individuals with the I/I genotype at the insertion/deletion also had lower risk for severe nephropathy than the D/I heterozygotes, and similarly at rs9896208, individuals with the C/C genotype had a lower risk than those with the C/T genotype. As measured by the R2 statistic, genotypes at rs1800764, insertion/deletion, and rs9896208 accounted for 0.4, 0.4, and 0.6%, respectively, of explained variability in risk for severe nephropathy.
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DISCUSSION |
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When the ACE polymorphisms were examined against our nephropathy outcomes during a period of up to 17 years of observation, we determined that subjects with certain ACE genotypes had a significantly lower risk in progression to persistent microalbuminuria as well as severe nephropathy, which included subjects with AER >208 µg/min, dialysis, or transplant. The effect of the ACE genotypes persisted even when controlling in multivariate models for known covariates that are associated with microalbumin excretion in the DCCT/EDIC cohort, which specifically included sex, age at diagnosis, diabetes duration, DCCT baseline BMI, mean blood pressure, triglycerides, total cholesterol, HDL cholesterol, time-dependent updated HbA1c weighted mean, cohort, and treatment.
A major quantitative trait loci for circulating ACE activity lies within a 16-kb region between intron 5 and downstream of exon 26 of the ACE gene (15). We speculate that genetic variation at the markers that we have analyzed, or at other loci in strong linkage disequilibrium with these markers, affects ACE enzyme activity, which in turn contributes to the development of diabetic nephropathy. Supporting this hypothesis are data from studies of transgenic diabetic mice engineered to have three copies of the Ace gene with resultant ACE enzyme activity 153% relative to two copy diabetic mice (23). The three copy mice had increased blood pressure and overt proteinuria compared with the two copy mice after 12 weeks of streptozotocin-induced diabetes, supporting the hypothesis that a genetic increase in ACE activity was sufficient to accelerate diabetic nephropathy in animal models (23).
The current study provides more definitive support for the role of ACE polymorphisms in diabetic nephropathy than the many previous cross-sectional studies (18,20). Based on our multivariate models adjusted for covariate effects, the three-marker ACE haplotypes explain 0.8% of variability in persistent microalbuminuria and 0.5% of variability in severe nephropathy. The previous studies may therefore lack statistical power to detect small effects of the ACE insertion/deletion polymorphism on renal outcomes. The pooled odds ratios for elevated urinary albumin excretion for I/I versus I/D and D/D genotypes in a meta-analysis (including different ethnic groups) in type 1 diabetes was 0.72 (95% CI 0.511.01) with a borderline significant P value of 0.06 (20). Three type 1 diabetes studies (17,24,25) in that meta-analysis reported odds ratios with 95% CIs excluding unity that indicated a protective effect of the I/I genotype on nephropathy.
The DCCT clinical trial was not initially designed as a genetic study, and to guard against population stratification, a potential source of bias, analyses were limited to subjects self-reported as "white." In addition, the modest number of severe renal end points limits our power to detect small genetic effects. Despite this, there are many strengths of this study. The DCCT/EDIC cohort represents one of the largest collections of genetic and clinical information on subjects with type 1 diabetes. Biochemical measures were performed in one central laboratory, and the cohort is phenotypically well characterized, with longitudinal prospective clinical data on complication status for up to 17 years. The attrition from the EDIC study has been very low, and clinical data continues to be acquired on >90% of those DCCT participants who took part in EDIC. Finally, our genotyping strategy is superior to the many previous cross-sectional studies that only genotyped one polymorphic variant (i.e., insertion/deletion) and subsequently were unable to capture the common variation spanning the entire ACE gene.
Our findings in the DCCT/EDIC cohort therefore offer definitive evidence that in Caucasians, genetic variation at the ACE gene is associated not only with the onset of microalbuminuria but also with severe diabetic nephropathy in subjects with type 1 diabetes.
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ACKNOWLEDGMENTS |
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FOOTNOTES |
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Additional information for this article can be found in an online appendix at http://diabetes.diabetesjournals.org.
Address correspondence and reprint requests to Andrew P. Boright, MD, PhD, Department of Medicine, Division of Endocrinology, University Health Network, 200 Elizabeth St., Toronto, Ontario, Canada M5G 2C4. E-mail: andy{at}genet.sickkids.on.ca
Received for publication October 6, 2004 and accepted in revised form December 23, 2004
AER, albumin excretion rate; DCCT, Diabetes Control and Complications Trial; EDIC, Epidemiology of Diabetes Interventions and Complications; SNP, single nucleotide polymorphism
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REFERENCES |
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