Evidence for a protective role for the rs805305 single nucleotide polymorphism of dimethylarginine dimethylaminohydrolase 2 (DDAH2) in septic shock through the regulation of DDAH activity

Of the 408 patients included in the VANISH trial modified intention-to-treat analysis, 209 had buffy-coat samples and 75 had whole blood stored that was suitable for DNA extraction and genotype analysis. In 249 of those patients, at least one plasma sample was available for analysis of methylarginine and L-arginine concentrations. Peak methylarginine concentrations were defined as the highest value measured from available samples for each patient. In patients who did not survive for the full sample collection period, the peak value from the available timepoints was selected. Patients in this subgroup had similar baseline characteristics to those of the VANISH population as a whole and as there was no difference in the primary outcome of renal-failure-free days or mortality between the treatment groups in the VANISH trial, all patients were analysed together in this study (Additional file 1) [34]. In the population that underwent genotyping analysis, median (IQR) duration of shock was 47.5 (26.1–87.5) h.

Plasma L-arginine and methylarginine concentrations were measured at each available time point and temporal patterns analysed (Table 1). Median L-arginine concentration was at its lowest on study inclusion then rose over subsequent study days (Fig. 2a). ADMA concentrations were elevated over normal plasma values [39] and median plasma ADMA concentration increased over the course of the study period (p < 0.001) and was significantly higher on days 5 and 7 than at study inclusion (all p < 0.05, (Fig. 2b). No significant changes in plasma SDMA concentration were observed during the study period, p = 0.478 (Additional file 1: Figure S1A).

The impact of treatment group allocation on L-arginine and methylarginine concentrations was determined in order to rule out any treatment group effect. No differences were detected in plasma L-arginine or methylarginine concentrations across treatment allocations (Additional file 1: Table S1).

Median (IQR) L-arginine concentrations were similar in both survivors and non-survivors at recruitment and on day 3. A pattern of higher L-arginine concentration was, however, associated with non-survivors on days 5 and 7 (Additional file 1: Table S2, Figure S1B).

Plasma concentrations of ADMA and SDMA were elevated at each time point in patients who died compared to survivors (Additional file 1: Table S3 and S4, Figure S1C and S1D, respectively). Peak ADMA and SDMA levels were also elevated in non-survivors (2.73 (2.14–3.52) μM vs 1.98 (1.45–2.64) μM, p < 0.001 and 2.727 (2.14–3.52) μM vs 1.98 (1.45–2.64) μM), p < 0.001), respectively. The area under the receiver operating characteristic curve (SE) for peak ADMA concentration over the study period was 0.705 (0.63–0.78) ) (p < 0.001) and for SDMA it was 0.641 (0.56–0.73) (p < 0.001). The survival analysis showed that mortality rates increased with increasing concentrations of ADMA and SDMA (Fig. 2c and d, both p < 0.001). ADMA concentration in the upper 50% of values was independently associated with mortality in multivariate analysis including SDMA, age, sex, L-arginine and serum creatinine concentration as covariates (hazard ratio 1.82 (1.05–3.14), p = 0.033) (Table 2). The ADMA:arginine ratio displayed a similar pattern in the time course studied, with an increased ratio seen on day 3 (p = 0.004) and a similar trend on day 7 (p = 0.20). (Additional file 1: Figure S1E).

The plasma ADMA concentration was corrected for SDMA concentration as a marker of global DDAH activity. Lower DDAH activity was associated with improved survival on log rank analysis (p = 0.033) (Fig. 3a).

The rs805305 SNP of the DDAH2 promoter region was genotyped. The C:C genotype was seen in 128 (44.7%); the C:G heterozygote in 112 (39.1%) and the homozygote G:G haplotype in 40 (13.9%) The G minor allele of the rs805305 SNP was associated with significantly lower 28-day mortality (31% in the common wild-type C:C genotype, 22% in the C:G heterozygotes and 15% in the less common G:G group, p = 0.02) (Fig. 3b). Mean Sequential Organ Failure Assessment (SOFA) score during the study period was significantly reduced in patients with the G:G genotype (median (IQR) 4.1 (3.25–5.8)) compared to the heterogozygotes (5.0 (3.4–7.2)) and the common C:C genotype (5.2 (3.8–7.7), p = 0.04) (Fig. 3c). ANOVA revealed that duration of shock was also reduced in the G:G genotype (37 (23–79) h) compared to 46 (23–76) h in C:G heterozygotes and 53 (32–109) h in C:C genotype patients (p = 0.02) (Fig. 3d). Hospital length of stay displayed a similar pattern, with length of stay of 15.0 (11.0–47.0), 17 (8.25–35.0) and 19 (8.75–40.5) days in the G:G, C:G and C:C groups respectively, although this trend was not statistically significant (Additional file 1: Figure S2). The plasma ADMA:SDMA ratio was also examined in patients with each of the three genotypes of the rs805305 SNP. In the less common G:G homozygotes the median (IQR) ADMA:SDMA ratio was 1.0 (0.69–1.96), in the C:G heterozygotes it was 0.68 (0.51–0.95) and in the common C:C genotype it was 0.64 (0.40–0.91) (p = 0.004) (Additional file 1: Figure S3). Homozygotes for the less common DDAH1 SNPs genotyped were found in approximately 1% of the study population. No association with outcome was observed when the risk of death for those expressing the common homozygote genotype was compared to a combined group of heterozygotes and rare homozygotes of each SNP (Additional file 1: Table S5).