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. 2024 Jul 18;20(7):e1012411. doi: 10.1371/journal.ppat.1012411

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© 2024 Pasquarelli et al

This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

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Fig 7 — A) Diagram of the fragments of BCC0, IMC32, and IMC43 used for pairwise Y2H assays. Residues included in each fragment are indicated. “Myr.” = predicted myristoylation site. “Palm.” = predicted palmitoylation site. “CC” = coiled-coil domain. “LOC” = IMC43 localization domain. “EID” = IMC43 essential interaction domain. B) Pairwise Y2H assays testing for binding between fragments of BCC0 and IMC32. Pairs of fragments that were unable to be tested due to auto-activation of both fragments in the pB27 vector are indicated. Growth on permissive (-L/W) media indicates the presence of both the pB27 and pP6 bait and prey plasmids. Growth on restrictive (-L/W/H) media indicates binding between the indicated fragments of each protein. C) Pairwise Y2H assays testing for binding between fragments of BCC0 and IMC43.