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. 2015 Aug 28;10(8):e0136362. doi: 10.1371/journal.pone.0136362

Fig 3. Western blotting confirms that TAPI-identified proteins are trapped in large, detergent-resistant Htt-polyQ aggregates.

Fig 3

(A) Immunoblotting reveals that Htt-Q103-GFP, but not Htt-Q25-GFP, forms large detergent-resistant aggregates that fractionate in the pellet (partial TAPI purification; see methods) and remain at the top of an acrylamide gel under SDS-PAGE conditions. (B) Immunoblotting confirms that HA-tagged Bmh1p, Def1p, Ent2p, and Sgt2p (proteins identified by mass spec) get trapped in the detergent-resistant aggregates that can be seen stuck at the top of the gels in the pellet fractions. As a negative control, HA-tagged His3p (not identified by mass spec) shows no susceptibility to co-aggregation with Htt-Q103-GFP. Note that Def1p was not easily visualized in the supernatant fraction because it is prone to degradation (data not shown). Samples were spun at 45,000 rpm, except Ent2p (10,000 rpm). S = supernatant; P = pellet fraction.