β2-adrenergic receptor and UCP3 variants modulate the relationship between age and type 2 diabetes mellitus

We studied 342 type 2 diabetic patients, aged 35–70 years, seen at the outpatient diabetic clinic of a health district in the province of Naples over a six-month period. A cohort of 305 unrelated non-diabetic glucose-tolerant control subjects [25] were randomly selected among telephone company employees taking part in a company sponsored health screening. All study participants were Caucasians of Italian origin, unrelated and residents of the same geographical area. The local ethics committee approved the study and informed consent was obtained from all study participants.

Weight, height and waist circumference were measured according to a standard protocol, with participants wearing light clothing and no shoes, BMI was calculated as body weight (in kilograms) divided by squared height (in metres). A blood sample was taken in the fasting state for biochemical measurements. Glucose, triglycerides, total, LDL and HDL cholesterol were measured by standard laboratory methods on fresh plasma. Sitting blood pressure was measured on the right arm after five minutes rest, three readings were taken two minutes apart and the average value was used in the analysis. Use of medication was recorded. Hypertension was defined as blood pressure ≥ 140/90 mmHg or use of antihypertensive medication. For analytical purposes study participants were stratified according to BMI ≥ 30 kg/m² (obese) or BMI < 30 kg/m² (non-obese).

Genomic DNAs were extracted from 300μl of peripheral blood by using Biorobot EZ1 Qiagen according to manufacturer's protocols. Genotyping was performed using Allele Specific Amplification (ASA) on the Real-Time PCR ABI PRISM 7000 (PE Applied Biosystem, Foster City, CA USA). The following SNPs were tested: Gly389Arg of ADRB1 (dbSNP rs1801253), Arg16Gly of ADRB2 (dbSNP rs1042713), Gln27Glu of ADRB2 (dbSNP rs1042714), G(-866)A of UCP2 (dbSNP rs659399) and C(-55)T of UCP3 (dbSNP rs1800849). All the oligoprimers were tested by PCR to optimize the melting temperature. Sequence information for all oligonucleotide primers is available as supplementary information [see Additional file 1].

To test for association between genes polymorphisms and the disease, we adopted a multistep strategy. We first performed a parametric monofactorial analysis (mainly performing χ² tests and computing the Odds Ratios), and then we used the Multifactor Dimensionality Reduction (MDR), a non-parametric multifactorial analysis, to test the combined effect of several genetic and environmental factors. Broadly, MDR outputs the number and the list of factors that could be involved in the disease without giving any additional information on the details of the interaction. To try to explain such interaction we performed a series of monofactorial analyses on the combination of the factors output by MDR analysis. In the latter step, we used a priori and genetic knowledge to reduce the number of analyses. For the monofactorial statistical analyses we considered as significant a p value < 0.05 and to keep a significant result we adopted the Bonferroni multiple testing correction method [26]. Having 3 samples and 5 SNPs we consider 15 monofactorial tests and we obtained a modified p threshold of 0.003. It should be underlined that, in these conditions, this correction method could be considered "highly conservative and may miss real differences" [26]. We estimated the power for our genetic association study using CATS software [27]. To further explore the association between single genetic factors and disease prevalence we calculated the Odds Ratio with 95% Confidence Intervals for the SNP having the greatest χ² value.

The multifactorial analysis was performed using MDR. MDR is implemented in software (ver. 1.4.1) designed by the Computational Genetics Laboratory (CGL) at Dartmouth Medical School in Lebanon, NH, USA. [24].

For each MDR analysis, the user has to input the population characteristics (disease status, genotypes, and other risk factor data) and the number, n, of factors involved in the interaction simultaneously. MDR tries to define the rules involving n factors that best predict the disease status. The output of the analysis is the combination of n factors and two values that describe the strength of the association: Prediction Error (PE) and Cross Validation (CV). PE is the percent of subjects whose disease-status is wrongly classified according to the rules, suggesting which portion of the disease risk can be predicted by the output factors. CV represents the self-consistency score of the analysis, computed by performing the same analysis in different subsets of the original data. The latter value measures the likelihood that the result is not incorrect due only to a portion of the dataset [28]. To calculate the p value of the MDR analyses we performed a permutation test. We permutated all the values for each sample and subsample in the disease status column, breaking association between the status, genetic and clinical data. We reiteratively performed this procedure 1000 times and, at the end of each permutation, we performed, again, the MDR analyses for each of the n value considered. We collected all PE and CV values for the factors combinations identified. Then we compared the PE and CV values of the real dataset versus the 1000 by n values of the permutated dataset. Sorting the permutated dataset for ascending PE and descending CV, we ranked the real result and obtained a value that divided by 1000 by n gave us the p value. We performed MDR analyses on three datasets (the whole sample and the two, obese and non-obese, subsample) and therefore we corrected the p value threshold to 0.016 according to the Bonferroni method [26].

The MDR analyses were performed on the whole sample and on the obese and non-obese subsamples. The data entered in the analyses were five SNPs [Gly389Arg of ADRB1 (dbSNP rs1801253), Arg16Gly of ADRB2 (dbSNP rs1042713), Gln27Glu of ADRB2 (dbSNP rs1042714), G(-866)A of UCP2 (dbSNP rs659399) and C(-55)T of UCP3 (dbSNP rs1800849)] and two non-genetic factors (gender and age) that we considered as environmental factors. It is of relevance that MDR accepts as input discrete variables only. While the first (gender) is by its nature dichotomous, age had to be classified into three main age ranges: 34–53; 54–63 and 64–79. The number, n, of interactions tested was 2 and 3.

In addition, to clarify the MDR results we computed the χ² and the OR (with 95% CI) considering the set of factors selected by MDR. To lessen the number of possible combinations we only analysed dominant models. Again, we corrected the p value by the Bonferroni method.

Finally to confirm the interaction we looked for possible transcript co-regulations among the genes studied. We screened WebQTL [29] a repository of gene expression data of several mouse strains [30].