1b) In previous Phos-tag assays

(Sogame et al, 2011b),

1b). In previous Phos-tag assays

(Sogame et al., 2011b), protein phosphorylation was detected in a broader molecular weight range (20–80 kDa). However, in the present study (Figs 1, 3c and 4), the phosphorylation signal was difficult to detect in a molecular weight range higher than 50 kDa. This may reflect an age-related difference between cultures used. In the previous study, cells were cultured for 0.5–1.0 days, whereas in the present study, cells were cultured for 1.0–2.0 days, before encystment induction. ABT-737 purchase As shown in Fig. 2a, immunoblotting analysis using antiphosphoserine antibody showed that the antibody cross-reacted with all of the phosphoproteins detected by Phos-tag/ECL, although some Dabrafenib signals from the antibody did not coincide in intensity with those obtained with the Phos-tag/ECL system, most probably reflecting the epitope specificity of the antibody. These results indicate that encystment-dependent phosphorylated proteins have serine residues. Therefore, the localization of the phosphorylated proteins was visualized

by immunofluorescence microscopy (Fig. 2b) using antiphosphoserine antibody. In Fig. 2b, each pair (b-1/b-2, b-3/b-4, and b-5/b-6) of the photomicrographs represents Nomarski (left) and immunofluorescence (right) images of identical cells labeled with antiphosphoserine antibody. The macronucleus (ma) and C1GALT1 other compartments were immunostained in encystment-induced cells (Fig. 2b-4), but no fluorescence was detected

in cells in which encystment was not induced (Fig. 2b-2) or encystment-induced cells treated with only secondary antibody (Fig. 2b-6). To determine which phosphorylated proteins are localized in the macronucleus, isolated macronuclei (Fig. 3a and b; left, Nomarski images; right, DAPI-fluorescence images) were analyzed by CBB staining and biotinylated Phos-tag/ECL detection assays (Fig. 3c). The isolated macronuclei aggregated through sticky mucus-like materials (Fig. 3a-1 and 2). Such clumps of macronuclei were dispersed by treatment with lysozyme (Fig. 3b-1 and 2), suggesting that the sticky materials may have been mucopolysaccharide. Judging from the photomicrographs of isolated macronuclei (Fig. 3a and b), the samples seem to have contained mainly macronuclei. Among the proteins (Fig. 3c, P-tag ‘Cells’) phosphorylated by encystment induction, an intense signal of p33 was detected in the isolated macronuclei sample (without treatment of lysozyme) (Fig. 3c, ‘P-tag, Macronuclei’), although weak signals of several proteins (p27, p31, and p37) were detected. A major protein contained in the band corresponding to 33 kDa obtained from isolated macronuclei sample (Fig.

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