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. 2018 Dec 15;294(7):2470–2485. doi: 10.1074/jbc.RA118.004836

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© 2019 Tan et al.

Published under exclusive license by The American Society for Biochemistry and Molecular Biology, Inc.

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Figure 3. — Serine 198 in the first predicted TM domain of MARCH9 is absolutely required for substrate down-regulation. A, sequences of mutants analyzed in this figure. Red bold font indicates substituted amino acids. Vertical box highlights the position of Ser-198. B–E, 293T cells stably expressing human CD4 were transduced with the indicated lentiviral constructs, and surface levels of HLA-A2 (B and D) and CD4 (C and E) were measured after 48 h of culture with or without dox as in Fig. 1. Serine-to-alanine substitutions were examined in blocks of three or four (3S-A and 4S-A mutants; B and C) and separately for the single-serine mutants as indicated (D and E). Dashed lines indicate mean substrate level remaining on dox-treated cells expressing control WT (lower) and RING mutant W143A (upper) MARCH9. Unpaired t test: ns, not significant. F, Western blot analysis of MARCH9 WT and inactive mutant expression, performed as in Fig. 2E. + marks the position of a cellular product detected by SA-HRP; arrow marks the position of MARCH9 protein. Table shows expression normalized to GAPDH loading control and relative to MARCH9-WT, quantitated by densitometry.