2A), cotransplantation with which also effectively protected islet allografts from rejection (Supporting Fig. 2B). Induction of H-MC by HSC was not a strain-specific phenomenon, because similar results were seen in other strains, BALB/c and C3H (data not shown). To determine whether the induction
of H-MC was mediated by cell-cell direct contact or by soluble factor(s), Venetoclax ic50 BM cells and HSC were cultured in transwell plates which blocked cell-cell direct contact but allowed free communication of soluble factors. Generation of CD11b+CD11c− cells in transwell plates was similar to culture in conventional plates, suggesting that soluble factor(s) secreted by HSC plays a pivotal role in induction of H-MC (Fig. 5E). This was confirmed by addition of HSC culture supernatant into the BM cell culture. The generation of CD11b+CD11c− cells correlated selleck inhibitor with the dose of the added supernatant (Fig. 5E). The responsible soluble factor(s) were likely proteins or peptides because their biological activity was largely impaired following heating at 56°C for 30 minutes (Fig. 5E, right panel). Upon activation, HSC produce multiple
factors, including vascular endothelial growth factor (VEGF), GM-CSF, G-CSF,11 which have been shown to promote expansion of MDSC.16 We tested the role of these factors using the HSC isolated from G-CSF or GM-CSF knockout mice. Because knockout of VEGF causes embryonic lethality, and neutralizing antimouse Ab is not available, VEGF in HSC was silenced by treatment with specific small interfering RNA (siRNA). The results show that none MCE of these factors appeared to be responsible for induction of H-MC (Supporting Fig. 3A). To identify the responsible
soluble factor(s), the interference of bovine serum proteins was avoided by using serum-free medium, which induced similar levels of H-MC to medium-containing serum. The HSC culture was fractioned according to molecular size using the centrifugal filters (Millipore). The 100-250KD portion was most bioactive in inducing H-MC. Electrophoresis analysis (sodium dodecyl sulfate-polyacrylamide gel electrophoresis [SDS-PAGE]) revealed a few bands from 75 to 250 kD in HSC supernatant that was absent in control (Supporting Fig. 3B). These bands were analyzed for peptide sequences by capillary liquid chromatography (LC) tandem mass spectrometry (MS) and the CID spectra. The sequences were searched against the mouse RefSeq Database (NCBI), as well as against the Bovine Protein Database (to rule out possible bovine protein interferences). Two groups of molecules were detected (Supporting Table 1): (1) extracellular matrices, which were expected; (2) complement, including complement component 3 (C3) and complement factor H (FH), which was beyond expectation, because C3 and FH are mainly produced by hepatocytes.