Genome-wide association study identifies loci and candidate genes for non-idiopathic pulmonary hypertension in Eastern Chinese Han population

Totally 208 individuals were enrolled in the present study, including 109 non-idiopathic PH patients and 99 healthy controls. Patients were consecutively recruited from the Affiliated Hospital of Jiangsu University between May 2014 and July 2016. Clinical information was obtained from medical records, including gender, age, drink, smoke and coronary artery disease (CAD) history and so on. Baseline profiles of the studied population were summarized in Table 2. None of the patients have connective tissue diseases, HIV infection, portal hypertension, congenital heart diseases or thyroid dysfunction. The control subjects were collected from healthy volunteers who visited the Sir Run Run Hospital Nanjing Medical University for medical examination during the same period. The study was performed with the approval of the ethics committee of the Nanjing Medical University and the informed consent was obtained from each participant.

Genomic DNA was extracted from 200 μl EDTA-anticoagulated peripheral blood using a commercial extraction kit (Tiangen Biotech Corporation, Beijing, China) according to the instruction manual. The 143 tag SNPs in 109 PH patients were firstly genotyped by using Illumina X-10 platform, and the sequencing was done by commercial company (Decode Genomics BioTech Co., Ltd, Nanjing, China). The genotyping results were then compared with healthy individuals from Southern Han Chinese (CHS) population of 1000G database. And 2 SNPs emerged at a significant level (P < 3×10^-4) (Fig. 1). To confirm the finding, we further genotyped 2 SNPs in 99 healthy individuals from Nanjing, Jiangsu by performing fluorescent PCR and Ligase detection reaction (LDR). The primers were designed by using Primer 3 online software version 0.4.0 (http://​frodo.​wi.​mit.​edu/​) and Oligo software version 6.3.1 (Molecular Biology Insights, USA). The SNPs were amplified in a final volume of 20 μl that contained 50 ng of DNA, 2 μl 1×buffer, 0.6 μl 3 mM Mg2+, 2 μl 2 mM dNTP, 0.2 μl Taq DNA polymerase (1 unit/μl) and appropriate concentrations of primers. The PCR reaction was subjected to an initial denaturation at 95 °C for 2 min, followed by 40 cycles of amplification consisting of denaturation at 94 °C for 30 s, annealing at 53 °C for 90 s, extension at 65 °C for 30 s, followed by final extension at 65 °C for 10 mim. The LDR was carried out on the PRISM 3730 DNA analyzer (Thermo Fisher Scientific, USA). The LDR were performed in a total volume of 10 μl that contained 4 μl PCR production, 1 μl 1×buffer, 1 μl probe mix, 0.05 μl Taq DNA polymerase (2 unit/μl). The LDR condition was 95 °C for 2 mim, followed by 40 cycles of 15 s at 94 °C and 25 s at 50 °C. The SNPs were further genotyped by using Genemapper.

All data were analyzed by using SPSS 19 (SPSS Inc., Chicago, IL). Genotype frequencies of SNPs were obtained by directed computing. Genotypic association analyses in a case-control pattern assuming codominant, dominant, recessive and overdominant genetic models were performed using SNPstats [3]. Odds ratio (OR) and respective 95% confidence interval were reported to evaluate the effects of any differences between allele and genotype frequencies.

Totally 143 SNPs were successfully genotyped in 109 PH patients. After comparing the genotyping results with the data generated from 105 individuals from Southern Han Chinese population in 1000G database, the results demonstrated that 2 SNPs were associated with PH with overall susceptibility at p < 3×10^− 4 after Bonferroni adjustment. The related analysis was shown in Fig. 1. The top hit was rs6557421 (p = 4.5×10^− 9), which is located in Nox3 gene on chromosome 6. Another SNP rs3744439 located in Tbx4 gene, also showed evidence of association with PH susceptibility (p = 1.2×10^− 6).

We further genotyped the 2 SNPs in 99 healthy control subjects. The distribution of genotype frequencies of rs6557421 and rs3744439 was illustrated in Fig. 2. Dramatic differences existed between PH patients and controls. As shown in Table 3, individuals with rs6557421 TT genotype had a 10.72-fold/14.20-fold increased risk to develop PH when compared with GG or GG/GT carriers in codominant or recessive model, respectively (TT versus GG: 95%CI = 4.79–24.00; TT versus GG/GT: 95%CI = 6.65–30.33). In dominant model, significantly increased PH susceptibility was associated with GT/TT genotypes compared with GG genotype (OR = 2.48, 95%CI = 1.39–4.41). Furthermore, dramatically decreased PH risk was associated with GT genotype when compared with GG/TT genotypes in an overdominant model.

As shown in Fig. 2b and Table 4, rs3744439 AG genotype only occurred in healthy controls which had not been observed in PH patients.

Stratification analysis was also performed, and PH patients were divided into three groups according to the Nox3 rs6557421 genotypes. The distribution of patients’ left atrial diameter (LA), left ventricular end diastolic diameter (LvIDd), interventricular septal thickness (IVST), left ventricular ejection fraction (LVEF) and systolic pulmonary artery pressure (PAP) were compared between each groups (Fig. 3). No significant differences were observed among different genotyping groups.

We further validated the observation by using 26 different populations from five regions around the globe, including African (AFR), American (AMR), East Asian (EAS), European (EUR), and South Asian (SAS). As illustrated in Fig. 4a and b, the distribution of rs6557421 and rs3744439 genotypes’ frequencies of control group from Chinese Han population was quite similar to which from Asian populations. In consistent to the present case-control study’s results, significantly different genotype frequencies existed between PH Patients and healthy individuals from all over the world (Fig. 4a and b).