APC-β exhibits superior inhibition of cerebral injury in murine ischemic stroke. (A) 293T cells transfected with EPCR and PAR1-AP were incubated with mAPC or mAPCN329Q (6.25-50 nM) for 3 hours. AP activity was assessed using QUANTI Blue AP substrate, as before. RAW264.7 macrophages were incubated with mAPC (black bars) or mAPCN329Q (red bars) (12.5-50 nM) for 3 hours before stimulation with LPS (50 ng/mL) for 18 hours. Secretion of (B) TNFα and (C) IL-6 was measured by ELISA. (D) Schematic description of the ischemic stroke model and study protocol. (E) Sodium dodecyl sulfate polyacrylamide gel electrophoresis analysis under reducing conditions of purified recombinant mAPCPS and mAPCPS/N329Q. Proteins were stained with Coomassie Brilliant Blue. The heavy chain of mAPCPS migrates as a diffuse band composed of the APC-α heavy chain and APC-β glycoform heavy chain fractions. The heavy chain of mAPCPS/N329Q is composed solely of the APC-β fraction. (F) Brain infarct volumes post-stroke and t-PA administration were calculated in each mouse by staining 20-μm coronal brain sections with thionine, which is unable to stain lesion areas. For volume analysis, 1 section of every 10 covering the entire lesion was analyzed. Individual values and the median of each group are represented; n = 9-15; *P = .006, **P = .004. (G) Images corresponding to 2 thionine-stained sections of representative mice from each group are shown. Lesion areas are unstained, whereas remaining healthy tissue is stained purple.