Vitamin e-loaded membrane dialyzers reduce hemodialysis inflammaging

This study was a randomized controlled observational crossover trial. Eighteen patients randomly sampled from our hemodialysis unit, have been included in the study. Exclusion criteria included recent illness (within the previous 2 months), significant anemia (Hb < 10 g/dl), autoimmune disease, current/previous (6 months) immunosuppressive treatment, but also systemic diseases such as diabetes, vasculitis, amyloidosis, rheumatic disease; HBV, HCV, HIV positivity, other active viral and/or bacterial infection, active cancer or after remission and previous transplantation.

All 18 chronic hemodialysis patients have been on a thrice−weekly hemodialysis regimen for at least 6 months, treated with standard low−flux polysulfone dialysis. In random sequence hemodialysis patients underwent a 4−hour thrice−weekly, 3−month period of a) standard low–flux bicarbonate hemodialysis with polysulfone membrane dialyzers, (BHD; FX10 Low−Flux, Helixone® membrane, ^©Fresenius Medical Care AG & Co. KGaA, Bad Hamburg, Germany), b) HDF (pre−dilution 70 ± 12 ml/min) with polysulfone membrane dialyzers (FX100 High−Flux, Helixone® membrane, ^©Fresenius Medical Care AG & Co. KGaA, Bad Hamburg, Germany) and c) standard low–flux VIT−E BHD (VitabranE® membrane E18, Asahi Kasei Kuraray Medical Co., Japan). Blood samples were taken at the end of the long interdialytic interval, at the beginning and at the end of each 3–month period of the study respectively. In order to evaluate the interference of the vitamin E–loaded membrane dialyzers on NO serum levels, blood samples were also taken simultaneously from arterial and venous lines at the beginning and 60 minutes after starting the same hemodialysis session and at the end of the last long interdialytic interval of each 3–month period of the study. Current therapy remained unchanged for the duration of the study. European Renal Best Practice (ERBP) guidelines for anaemia in chronic kidney disease (CKD) were applied [31]. In detail, intravenous iron supplements were administrated as sodium ferric gluconate complex, or ferric caboxymaltose were administrated at the end of a hemodialysis session according to prescription, in order to maintain ferritin blood levels ≤ 800 ng/ml and transferrin saturation > 20%. Correction of hyperparathyroidism and hypertension treatment remained unchanged throughout the study. A control group of 14 hospital staff individuals, healthy for at least 6 months, were also recruited. Participant characteristics are summarized on Table 1.

Serum (1 ml) was deproteinized by 100 μl 30% trichloroacetic acid (Sigma−Aldrich, Italy). An amount (250 μl) of supernatant was added to 50 μl of aqueous solution 49.4 μmol/l of theophilline as per Internal Standard (IS, Sigma−Aldrich, Italy). For delayed analysis, deproteinised samples were stored at -80 °C for at least one month. Standard stock aqueous solutions (2.47 mmol/l for Kyn and 4.41 mmol/l for Trp, both from Sigma−Aldrich, Italy) were prepared and kept frozen at -80 °C. Working standard solutions were made by appropriate dilution of a standard mixture.

HPLC method issued from separation conditions for Kyn and L−Trp was developed by Zhen et al [32]. In the present method, separation was achieved on HP1100 LC system (Agilent Tecnologies S.p.A., Italy) using a column Supelco C18 LC18DB (Sigma−Aldrich, Italy) (150 mm x 4.6 mm, particles size 5 μ) by isocratic elution (30 °C, 30 minutes). Mobile phase consisted of 50 mmol/l acetic-acetate buffer pH 4,6 (Sigma−Aldrich, Italy) and Methanol HPLC grade (VWR International PBI s.r.l, Italy) (95:5 v/v) at a flow rate of 0.8 ml/min. Eluates were monitored by DAD set at λ 360 nm for Kyn and λ 275 nm for L−Trp and IS. Absorbancy at λ 220 nm and λ 302 nm were also obtained, absorbance ratios were used for identification and purity assessment of each peak. Sample injection was 50 μl.

IDO1 activity was assessed in sera as change of L−Trp and its catabolic product Kyn (Kyn/Trp ratio), simultaneously measured using an isocratic RP HPLC method with UV detection.

We investigated the effects of dialysis treatment on NO serum levels in peripheral blood. Blood samples were obtained at the end of the long interdialytic interval of the last 3−month hemodialysis treatment periods. Moreover, during the last 3−month session of each hemodialysis treatment period, at the end of the long interdialytic interval, blood specimens were also taken 60 minutes after the beginning of the same hemodialysis session, simultaneously from the arterial and venous dialysis lines. We measured NO by photometric analysis with a nitrate/nitrite colorimetric assay kit (R&D Systems, Minneapolis, MN, USA). NO production was determined as NO₂⁺ NO₃^- with the Griess reagent after reduction of nitrate, to nitrite with nitrate reductase. Although several authors showed inflammation marker and oxidative stress peaks after already 15–30 minutes from the beginning of a hemodialysis session [33, 34], we designed this study consistently with a previous paper [26] where we found a significant variation of NO serum levels for 60 minutes. Readings were at 540 nm, and baseline correction was carried out at 620 nm. The sensitivity limit of the assay was 1.35 μmol/l.

The CRP (n.v. ≤ 6 mg/dl) was measured by the local hospital laboratory using the Latex C-Reactive Protein immunoturbidimetric assay (Alpha Laboratories Eastleigh Hampshire, UK).

Data are presented as count or M ± SD and were analyzed by SPSS version 19.0 (Chicago, IL, USA). ANOVA with Bonferroni analysis was performed on all dependent variables. Percentage data were compared by X² test to assess p-value significance. Two-tailed tests were conducted on all comparisons, and P < 0.05 was considered significant.

Table 2 summarized the data of IDO1 activity, as Kyn, Trp blood levels and Kyn/Trp ratio in controls and all hemodialysis patients at the beginning and at the end of the study respectively. Regardless to hemodialysis procedure, the Kyn/Trp ratio was significantly higher when compared to controls (P < 0.01) showing an increased IDO1 blood activity in hemodialysis patients. A significantly increased IDO1 blood activity was also observed regardless of hemodialysis procedure or hemofilter membrane utilized when compared to controls.

L−Trp levels in hemodialysis patients were significantly lower when compared to controls (P < 0.05), whereas Kyn increased significantly in hemodialysis patients vs controls (P < 0.05).

However, different hemodialysis treatments influenced IDO1 blood activity (Table 3). Treatment with VIT−E reduced significantly IDO1 activity when compared to treatment without vitamin E−loaded polysulfone membranes, regardless of BHD (P < 0.05) or HDF treatments (P < 0.05). Kyn in VIT−E hemodialysis patients was significantly lower when compared to both BHD (P < 0.05) and HDF (P < 0.05).

Figure 1 shows percent variation of IDO1 blood activity in different hemodialysis treatments compared to controls.

Data have been shown in Table 4. NO blood levels were significantly lower in controls when compared to patients under any hemodialysis procedures. NO levels were significantly higher in blood samples taken before hemodialysis treatment, in BHD and HDF when compared to VIT−E hemodialysis patients (P < 0.05). Surprisingly, NO serum levels of blood sampled from the venous line of VIT−E hemodialysis patients were significantly lower when compared to the arterial blood sampled from the same hemodialysis line. They were measured simultaneously, throughout the same treatment, at the end of the long interdialytic interval during the last VIT−E period hemodialysis session, after 1−hour VIT−E hemodialysis (Fig. 2). Percent reduction of venous vs arterial line was -22.6%. On the other hand, both BHD and HDF NO concentrations in venous hemodialysis line increased compared to arterial hemodialysis line.

Figure 1 shows comparison among percent variations of NO formation in all hemodialysis treatments and controls.