Detailed descriptions of all individuals are shown in Table 1. Collection and storage of serum samples. Blood samples were collected before any treatment initiation. The whole blood samples were collected in 4 ml BD Vacutainers without anticoagulation and clotted at room temperature for up to 1 h, and then samples were centrifuged at 4 °C for 5 min at 9000 g. Immediately, collected, aliquoted and stored these fresh sera at −80 °C to avoid variations
in the procedure. No sample underwent more than one freeze-thaw cycle before analysis. Serum pretreatments and MALDI-TOF MS detection. Serum samples were pretreated with WCX magnetic beads of protein fingerprinting detection kit (SED™) (Beijing SED Science and Technology, Inc., Beijing, China). Briefly, 5 μl of each serum sample was mixed with 10 μl of U9 solution in a 0.5 μl centrifuge Roxadustat ic50 tube for denaturation. After incubating for 30 min at room temperature, denatured serum sample was diluted with 185 μl washing buffer. Meanwhile, 50 μl of magnetic beads was added to a PCR tube, and the tube was placed in a magnet separator for 1 min followed by carefully removing the supernatant. The magnetic beads were then washed twice with 100 μl washing buffer. Hundred microlitre of diluted serum sample was added to the activated
magnetic beads, mixed carefully and thoroughly. The mixture was incubated for 1 h at room temperature and then washed twice with 100 μl washing buffer. The bound proteins were eluted from the magnetic beads
using 10 μl Hydroxychloroquine cost elution buffer. Then, 4 μl of the eluted sample was diluted in the ratio of 1:2 with 4 μl of SPA (saturated solution of sinapinic acid in 50% acetonitrile with 0.5% trifluoroacetic acid). Two microlitre of Immune system the resulting mixture was aspirated and spotted onto an 8-spot Au-chip (Ciphergen Biosystems Inc., Fremont, CA, USA). After air-drying for about 5 min at room temperature, protein crystals on the chip were detected by MALDI-TOF MS (Ciphergen, PBS IIc). The instrument was calibrated weekly using the Ciphergen all-in-one peptide reference standard, which contained vasopressin (1084 Da), somatostatin (1637 Da), bovine insulin β chain (3495 Da), human insulin recombinant (5807 Da), hirudin (7033 Da). And mass calibration helps guarantee that mass error was <3 Da. The detective parameters of MALDI-TOF MS were as follows: optimized mass range (2000–20,000 Da), laser intensity (149), laser sensitivity (7). It started with two warming shots at intensity of 154, then 110 shots at laser intensity of 149. Eighty-eight shots of the latter set were randomly kept, and results were generated from their average level. All the information including mass and intensity of peaks over the range mass/charge ratio (m/z) 0–50,000 Da was collected by ProteinChip@ Software Version 3.21 (PCS; Ciphergen). Data processing. Spectra from all samples were initially processed with baseline subtraction and normalization using PCS.