View larger version (16K):
[in a new window]
|
Fig. 1. Co-immunoprecipitation of IP3R and FKBP12 and the presence of mTOR in colonic smooth muscle. IP3R1 (the major isoform present; data not shown) was immunoprecipitated from solubilised colonic smooth muscle. (A,B) Immunoblots were probed with rabbit anti-IP3R1 and rabbit anti-FKBP12 antibodies for the presence of (A) IP3R1 and (B) FKBP12, respectively. Lane 1 in each panel shows the immunoprecipitated protein from colon. Lane 2 shows the relevant positive control (10 µg solubilised supernatant for IP3R or 50 ng recombinant FKBP12). Arrows on the right indicate the position of molecular-mass markers run in parallel to indicate protein migration on the gel. The detection of a band at 12 kDa (B) indicates that FKBP12 is present and associated with IP3R1 in these myocytes. These data are representative of four experiments. (C) FKBP12-IP3R1 association in colon is disrupted by FK506 and rapamycin. IP3R1 was immunoprecipitated from solubilised colon. Immunoprecipitates were probed for the presence of IP3R1 (C) and FKBP12 (D). Lanes 1-4 in each panel are the immunoprecipitated protein from colon, lane 5 is antibody alone (negative control), lane 6 is solubilised colon protein plus IgG sepharose without antibody (negative control) and lane 7 the relevant positive control [solubilised supernatant (C) and recombinant FKBP12 (D)]. The detection of a band in untreated control preparations at 12 kDa (D, lanes 3 and 4) indicates that FKBP12 is present and associated with IP3R1 (n=2). This FKBP12-IP3R1 association was disrupted by the addition of FK506 (D, lane 1, 20 µM) and rapamycin (D, lane 2, 20 µM), each of which reduced the FKBP12 signal. Arrows indicate the position of molecular-mass markers run in parallel to indicate protein migration on the gel. (E) mTOR is present in colonic myocytes. Immunoblots were probed with the anti-mTOR antibody (lane 1). Lane 2 shows the molecular-mass marker to show protein migration on the gel. (F, G) Co-immunoprecipitation of IP3R1 and calcineurin B from solubilised colonic smooth muscle. Immunoprecipitations were performed as above using rabbit anti-IP3R1 antibody, and immunoblots probed for the presence of IP3R1 (F) and calcineurin B (G). Lane 1 in each panel is the immunoprecipitated protein from colon, lane 2 is solubilised preparation plus protein G without antibody, lane 3 antibody alone, lane 4 the positive control (10 µg solubilised supernatant in each case). Arrows indicate the position of molecular-mass markers run in parallel. The detection of a band at 19 kDa indicates that calcineurin B is present and associated with IP3R1. These data are representative of six experiments. (H, I) Co-immunoprecipitation of IP3R1 and calcineurin A from solubilised colonic smooth muscle. Immunoprecipitations were performed as above using rabbit anti-IP3R1 antibody and immunoblots were probed for the presence of IP3R1 (H) and calcineurin A (I). Lane 1 in each panel is the immunoprecipitated protein from colon, lane 2 the solubilised preparation plus protein G without antibody, lane 3 the antibody alone and lane 4 the positive control (10 µg solubilised supernatant in each case). Arrows on the right indicate the position of molecular-mass markers run in parallel. The detection of a band at 55 kDa indicates that calcineurin A is present and associated with IP3R1. This data is representative of two experiments.
|
CiteULike 
Complore 
Connotea 
Del.icio.us 
Digg 
Reddit 
Technorati 
Twitter What's this?
) increased [Ca2+]c as indicated by F/F0. Rapamycin (10 µM, n=7) significantly reduced (P<0.05) the IP3-evoked [Ca2+]c transients. (B) Rapamycin (10 µM, n=10, P<0.01) significantly increased the Ca2+ rise evoked by caffeine (CAF, 10 mM) following activation of RyR.
