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. 2020 Nov 26;23(4):740–750. doi: 10.1038/s41436-020-01027-3

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© The Author(s) 2020, corrected publication 2021

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Fig. 3 — Fibroblasts of control subjects (n = 6) and p.Arg480His/Cys FAR1 patients (P1–P3) were treated for 24 and 48 hours with 10 μM HDG followed by immunoblot analysis for FAR1 and measurement of the plasmalogen levels. Two independent experiments were performed (^a indicating the first experiment, ^b the second), each including three (×2) control cell lines and the three patient cell lines (P1 = square, P2 = circle, P3 = triangle). a Immunoblot analysis of FAR1 in fibroblast homogenates of controls and patients using antibodies against FAR1 (59 kDa) and β-actin as loading control (same blot reprobed). Blots (cropped) of both experiments are shown. b Quantification of the FAR1 protein level as ratio over β-actin in control and patient cells in untreated and HDG-treated cells. Results are shown for each cell line as % of the untreated condition. c C16:0-Plasmalogen levels (expressed as % of total palmitate [C16:0]) in untreated and HDG-treated control and patient cells.