The frozen cryovials were transferred from APEC to Exsera BioLabs, a College of American Pathologists (CAP)/Clinical Laboratory Improvement Amendments (CLIA)-certified laboratory, for analysis. Complement factors C1q, C4, C2, MBL, C4b, C3, factor B, factor D, Properdin, C3a, C3b, Ba, factor H, factor I, C5, and C5a were measured, as well as albumin for normalization. Measurement of complement components and activation fragments was performed by two methods. The Ba and C3a levels were measured by ELISA (Quidel Corp, San Diego, CA, USA). The remaining measurements were performed by multiplex Luminex immunoassays (MilliporeSigma, Burlington, MA, USA). For both methods, Exsera had previously optimized the methods to measure the low-concentration vitreous. For both plasma and vitreous humor, the methods were optimized and validated to the level required for regulated laboratory analysis. All analyses were performed in duplicate with the resulting mean values used for analyses. For the multiplex Luminex data, the mean fluorescent intensity was the raw value, and for the ELISA analysis, the raw value was optical density. Six nonpoint, standard curves were fit with a four-parameter parametric curve fit to calculate the absolute quality in pg/mL, ng/mL, or µg/mL, as appropriate. Three quality controls (QCs) were included in each run, including at least one laboratory-developed and characterized QC. The QCs were monitored for performance. For all testing in the study, the values returned were within the required parameter of assay performance.