The study was conducted between 2008 and 2012. We evaluated a Spanish cohort of 677 consecutive CAD patients with severe (≥70 %) stenosis who had been scheduled to undergo diagnostic coronary angiography at the Centre Cardiovascular Sant Jordi (CCSJ) or the Hospital Universitari Vall d’Hebron (HUVH) in Barcelona, Spain. The protocol was approved by the Bioethics Committee of the two centers (Ethics Committee of Clinical Research of the HUVH and the Bioethics Committee of the CCSJ), and authorized written consent was obtained from all the subjects. The exclusion criteria were: recent (less than 1 month previously) acute myocardial infarction; anemia; recent angioplasty; prior revascularization by percutaneous coronary intervention; coronary artery bypass surgery; and renal infection, inflammation or chronic failure. Epidemiological and clinical data included hypertension, diabetes mellitus (DM), DM type, hyperlipidemia, smoking history, family history of cardiopathies (FHC), history of angina, angina type and acute myocardial infarctions (AMI); with those not referring to type recorded as present or absent.

Selective coronary angiography was performed using multiple orthogonal projections via the Judkins technique. Injection of the contrast in the donor artery was performed at a sustained high pressure with an automated controlled machine (ACIST CVi Contrast Delivery System®). CCC was assessed angiographically using a “modified” Rentrop’s method [6] without occlusion of the recipient artery. The following scale was used to assess the level of filling of the channels: 0 = no visible filling of any collateral channels; 1 = collateral filling of branches of the vessel to be dilated without any dye reaching the epicardial segment of that vessel (that is, right coronary artery injection showing retrograde filling of septal branches to their origin from the left anterior descending artery, without visualization of the latter occluded artery); 2 = partial collateral filling of the epicardial segment of the vessel being dilated; and 3 = complete collateral filling of the vessel being dilated. In patients with more than one collateral vessel, the highest Rentrop score was recorded.

CAD patients were classified according to the degree of CCC as either poor CCC (Rentrop 0–1) (n = 546) or good CCC (Rentrop 2–3) (n = 131). CCC was assessed by three experienced cardiologists who were blinded to the epidemiological, clinical and genetic data. The degree of agreement in the evaluation of CCC was high among the 3 observers, as determined by the kappa coefficient: κ = 0.987; 95 % confidence interval (95 %CI), 0.953-1.000 (P < 0.001) using the first 100 angiograms.

22 SNPs of genes involved in postischemic neovascularization were selected attending the following criteria: a) their suspected or proved functional or/and clinical significance regarding angiogenesis or arteriogenesis when known; b) their location within coding, 5' or 3' untranslated, or intronic sequences with known potential sites for factor binding; and c) a minor allele frequency of more than 5 % in the population studied (NCBI). We searched genes directly or indirectly involved in angiogenesis and/or arteriogenesis containing functional polymorphisms. Particularly, HIF1A [7‐9], VEGFA [10‐12], KDR [13, 14], NOS3 [15, 16], TGFB1 [17‐19] and LGALS2 [20, 21] have been involved in both processes. Furthermore, CCL2 [22] and ICAM1 [23] play an important role in arteriogenesis, while CD53, which controls TNFα levels [24], also plays an important role in this process [25]; and POSTN has been reported to be involved in angiogenesis [26] (Table 1). The SNPs located in or near these genes that were analyzed in this study are listed in Table 1 and details of them are as follows. HIF1A rs11549465 and rs2057482 affect mRNA production and are associated with CAD [27]; the first is also related to collateral circulation [28]. VEGFA rs2010963, rs1570360 and rs699947 influence protein production [29], and along with rs3025039 and rs833061 they have also been related to VEGFA serum levels [30‐32]. Moreover, VEGFA rs2010963 and rs699947 have been associated with collateral circulation [33] and CAD [34]. KDR rs1870377 and rs2305948 affect primary protein structure, whereas rs2071559 is located 5’ upstream, being all related to CAD [35]. CCL2 rs1024611 affects mRNA production [36‐38]; and along with rs1024610, MCP1 plasma levels [39‐41]. CCL2 rs1024611 and rs1024610 have been associated with myocardial infarction [39, 42]. NOS3 rs1799983 has functional consequences for the protein [43, 44] which are associated with coronary arteriogenesis [45, 46] and CAD [47]. ICAM1 rs5498 affects the primary structure of the protein and both it and rs3093030, located near the 3’ end of the gene, are related to sICAM1 plasma levels [48‐51] and to coronary artery calcification [52]. TGFB1 rs1800469 is located towards the 5’ end of the gene and has been associated with coronary heart disease complications [53]. CD53 rs6679497 is an intronic polymorphism associated with TNFα levels [24] which plays a role in modulating arteriogenesis [25]. POSTN rs3829365 and rs1028728 are located in the 5’ UTR of the gene, with the first being associated with heart failure [54]. Finally, LGALS2 rs7291467 is located in intron 3 and has been associated with arteriogenesis [21] and CAD [55‐57].

Blood samples were drawn from patients undergoing coronary artery catheterization. Genomic DNA was isolated using the QIAmp DNA Blood kit following the manufacturer’s protocol (Qiagen©, UK). TaqMan SNP genotyping assays (Applied Biosystems, Foster City, CA, USA) were performed to determine genotypes from the blood samples using a 7900HT Fast Real-Time PCR System (Applied Biosystems, Foster City, CA, USA). Genotype assessments were reproduced in three independent assays.

Data were summarized and presented in the form of mean, standard deviation and percentage as descriptive statistics. Continuous data that were not normal-distributed were analyzed using the Mann–Whitney U test. In this study, age does not show a normal distribution (Shapiro-Wilk p-value <0.001). Associations among categorical data were assessed using Fisher’s exact or chi-square test, and Hardy Weinberg equilibrium was assessed using the chi-square test. Multivariate logistic regression models were adjusted using clinically relevant variables to estimate odds ratios (ORs) and 95 %CIs among genotypes, haplotypes and the risk of poor CCC. Interaction terms between SNPs, haplotypes and significant covariates were also analyzed in the multivariate regression models. Statistical analysis was performed using STATA 11.2 software. The power to detect a genetic association was estimated using the same statistical package. The SNPStats software available at http://​bioinfo.​iconcologia.​net/​en/​SNPStats_​web was used to calculate linkage disequilibrium (measured as Lewontin’s D0-values) between SNPs, to estimate haplotype frequencies, and to evaluate haplotype association with CCC.