Gfp mouse antibody

CREST was detected in pre-cleared lysates separated by SDS-PAGE and blotted as described previously [96 (link)]. For analysis of proteins in total lysate vs. supernatant and pellet, the pellet from 90 μg of total lysate centrifuged at 50K rpm for 6 min was resuspended in water to the initial volume of total lysate centrifuged. The same sample volumes of total lysate, supernatant and pellet were then separated by SDS-PAGE. Blots were developed with GFP mouse antibody from Roche Applied Science (Indianapolis, IN) and PGK antibody from life technologies (Frederick, MD).

The following antibodies were used: VAMP2 rabbit antibody (#104202; Synaptic System), SV2 mouse antibody (Developmental Studies Hybridoma Bank), Flag M2 mouse antibody (#1804; Sigma-Aldrich), tubulin mouse antibody (#t9026; Sigma-Aldrich), mCherry rabbit antibody (#5993; BioVision), Myc mouse antibody (9E10; Santa Cruz), Hrs rabbit antibody (D7T5N; Cell Signaling), Hrs mouse antibody (ab56468; Abcam), GFP mouse antibody (#11814460001; Roche), KIF13A rabbit antibody (PA5-30874; Thermo Fisher Scientific), KIF13B mouse antibody (6E11; Santa Cruz), neurofilament and β-actin mouse antibodies (2H3 and 8-7A5; Developmental Studies Hybridoma Bank). Pharmacological agents were used in the following concentrations and time courses: cycloheximide (Calbiochem, 0.2 μg/μl, 24 h), bicuculline (Sigma-Aldrich, 40 μM, 5 min-2h or 20 h), 4-aminopyridine (Tocris Bioscience, 50 μM, 5 min-2h or 20 h), BDNF (R&D Systems, 50 ng/ml, 1 h), TTX (Tocris Bioscience, 0.5 μM, 2 h), Rapamycin analogue linker drug (AP21967; Clontech, 100 nM, 3 h), SAR405 (Millipore Sigma-Aldrich, 1 μM, 24 h), and Janelia Fluor 549 SNAPtag ligand (Janelia Research Campus, 200 nM, 30 min). Unless otherwise indicated, all other chemicals were purchased from Sigma-Aldrich.