Western Blot Analysis of Cellular Biomolecules

Blood inside organs were removed by rinsing tissues with PBS. Tissues were snap-frozen under liquid nitrogen. Tissues were homogenized in RIPA buffer (Sigma) with protease (Roche), deacetylase (nicotinamide, Tricostatin A) and phosphatase inhibitors (Roche)^{7 (link)}. Protein concentrations of samples were determined by Lowry assay and each amount of protein (30–50 ug per sample) were loaded for SDS-PAGE. Antibodies from the following companies were used for Western blot analysis: Phospho-H2Ax (1:500, NBP1-19255-Novus Biological), PAR (1:500, AM80100UG-Millipore), actin (1:5000, sc-8432-Santa Cruz), nitrotyrosine (1:500, 06-284-Millipore) acetyl-lysine (1:1000, 9441-Cell signaling), HIF1a (1:400, 14179-Cell Signaling), GLUT1 (1:500, ab652-Abcam), PDK4 (1:1000, 3820-Cell Signaling), LDHA (1:1000, 3582-Cell Signaling), SDHA (1:10000, ab14715-Abcam), Ndufs4 (1:1000, ab87399-Abcam,), SOD2 (1:1000, ab16956-Abcam) SOD2-Ac (1:1000, ab137037-Abcam), GDH (1:1000, 12793-Cell Signaling). Blots were blocked in 5% BSA-TBST. Antibodies were diluted in 5% BSA-TBST. Protein bands were visualized with chemiluminescence assay (Pierce) with secondary antibodies coupled with HRP. The protein abundance was analyzed by densitometry with ImageJ. SDHA or actin were used as a loading control for quantification.

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Lee C.F., Caudal A., Abell L., Nagana Gowda G.A, & Tian R. (2019). Targeting NAD+ Metabolism as Interventions for Mitochondrial Disease. Scientific Reports, 9, 3073.

Publication 2019

RIPA buffer protease phosphatase inhibitors AM80100UG sc-8432 acetyl-lysine HIF1a ab14715 ab87399 ab16956

Actin Antibodies Assay Biological Blood Buffer Chemiluminescence assay Densitometry Frozen Glut1 Hif1a Inhibitors Ldha Lysine Nicotinamide Nitrogen Nitrotyrosine Novus Pdk4 Phosphatase Protease Protein Ripa Sds page Sod2 Tissues Tricostatin Western blot analysis

Corresponding Organization :

Other organizations : University of Washington

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Variable analysis

independent variables

Removal of blood inside organs by rinsing tissues with PBS
Snap-freezing of tissues under liquid nitrogen
Homogenization of tissues in RIPA buffer with protease, deacetylase, and phosphatase inhibitors

dependent variables

Protein concentrations of samples
Protein abundance analyzed by densitometry with ImageJ

control variables

Protein loading amount (30-50 μg per sample)
SDHA or actin used as loading controls for quantification

positive controls

None explicitly mentioned

negative controls

None explicitly mentioned

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