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4 protocols using ly333531

1

Signal Pathway Protein Detection

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Western blots were performed as previously described [9 (link)]. Antibodies for AKT, GSK3, S6, 4EBP1, S6K1, GAPDH, vinculin, and STAT3 were purchased from Cell Signaling Technology. PRAS40 antibody was purchased from Invitrogen. BLNK antibody was purchased from BD Biosciences. GSK690693, MK2206, everolimus, rapamycin, PF-4708671, AT7867, GS-9973, and ibrutinib were purchased from Selleck. LY-333531 was purchased from Tocris. AZD2014, AZD5363, AZD1208, and C21H25ClN4O2 were synthesized by AstraZeneca.
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2

Adipocyte Lipolysis Regulation Assay

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Antibodies: pPKA and pPKC substrate specific antibodies; PLIN1 and pHSL (S660): from Cell Signaling Technology. CGI-58, HSL, GST and β-Actin: from Santa Cruz Biotechnology. Myc: from Roche. IP6K1: from Genetex. Plasmid construct: pT7T3D-PacI-PLIN1 construct was purchased from GE Healthcare/Open Biosystems. Reagents and Kits: Glycerol, FFA and TAG assay kits: from Cayman Chemicals; insulin Elisa kit from Crystal Chem; BCA protein assay kit: Pierce Biotechnology; Jetprime transfection reagent from Polypus; RetroX concentrator: from Clontech; Cyclic AMP from Cell Signaling; protein A/G beads from EMD Millipore. Pharmacologic modulators: Forskolin/FSK (Cell Signaling), isoproterenol (Sigma), CL316243 (Sigma); Rottlerin, LY333531 and GF109203X (Tocris). Protease plus phosphatase inhibitor tablets; Thermo Scientific, Waltham, MA. Unless otherwise stated, all the chemicals are purchased from Sigma Aldrich.
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3

PKC Inhibitors and Calcium Signaling

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All pharmacological agents were obtained from Sigma–Aldrich unless otherwise indicated. Stock solutions of adiponectin, the PKCβ1 inhibitory peptide (PKCβ1-IP, Santa Cruz Biotechnology), the PKCβ2 inhibitory peptide (PKCβ2-IP, Santa Cruz Biotechnology) and GDP-β-S were prepared with double deionized water (Merck Milli-Q). Stock solutions of CX-4945 (Selleck), TBB (Abcam), nitrendipine, KT-5720 (Calbiochem), GF109203X, Bisindolylmaleimide V, Gö6976 (Tocris Bioscience), LY333531 (Tocris Bioscience), HBDDE, TTA-P2 (Alomone Labs), and Z941 (from T.P. Snutch) were prepared in dimethyl sulfoxide (DMSO). The DMSO concentration in each medium was less than 0.05% and did not have significant effects on IT.
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4

High-throughput screening for EMT inhibitors

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MCF10A cells were infected with a retrovirus encoding mouse Twist1 or control cDNA, and after allowing 14 days for EMT reprogramming, the cells were seeded into 384-well plates and screened against a chemical library of 20,000 chemical compounds including FDA-approved drugs, kinase inhibitors, chromatin modifiers, and a set of structurally diverse compounds (enamine) with unknown activity. The screen was performed in duplicate with 3 days of drug incubation at a concentration of 5–10 μM, depending on the compound. Quantification of viable cells was performed with Celltiter Glo (Promega). The toxic cardiac glycoside sanguinarine (Sigma-Aldrich, Darmstadt, Germany) was used as a positive control and vehicle (DMSO) as a negative control. Celltiter Glo signals were normalized per plate, and hit selection was based on a z-score threshold (z-score < −2.12) derived from the distribution of positive and negative controls. Jaccard indices were calculated from the structures of the hit compounds and were then clustered using Tanimoto similarity and distance.
PKC412 (Novartis), R406, AB1010 (masitinib), OSI-930, sunitinib, and MLN518 were obtained from Selleckchem. Go6976 and LY333531 were purchased from Tocris Bioscience. BAY61-6306 was obtained from Sigma-Aldrich. For the in vivo experiments, PKC412 was kindly provided by Novartis.
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