Ab110410

Cells were lysed in Lamelli buffer and samples were separated by SDS polyacrylamide gel electrophoresis. Nitrocellulose or PVDF membranes were probed with antibodies for BMAL1 (14020S, CST), TOM20 (sc-11415, Santa Cruz), β-Actin (4967S, CST) Pro-IL1β (AF-401-NA, CST), Complex II WB Antibody Cocktail (ab110410, Abcam) HIF-1α (14179, CST), GLUT1 (12939, CST), PDHα (3205S, CST), PKM2 (4053, CST), α-Tubulin (3873, CST), Histone H3 (4499, CST), and pSTAT3-Tyr705 (9145, CST). Bands were visualized using an Amersham 680 Imager (GE Healthcare). Densitometry quantification was performed according to the following protocol: http://www.yorku.ca/yisheng/Internal/Protocols/ImageJ.pdf.

Protein levels of interest were determined by Western blot analysis according to a protocol described elsewhere [20 (link)]. Cells were treated with NTG in the 6-well plate, and the whole-cell lysates were quantified with a BCA kit (P0012, Beyotime, Shanghai, China). The protein sample (30 μg/sample) was loaded in each lane of the gel. The primary antibodies to pAMPK (α1T183 + α2T172, ab133448), pPDE1a (Ser297, ab177461), Citrate synthase (ab129095), IDH2 (ab131263), MDH2 (ab181873), Complex I (NDUFB8, ab110242), Complex II (ab110410), Complex III (UQCRC2, ab14745), Complex IV (COX IV, ab16056) and β-tubulin (ab6046) were obtained from Abcam (Cambridge, MA, USA). Antibody to ATP5A1 (495240) was from Invitrogen (Camarillo, CA, USA). β-tubulin was used as the internal control. The signal was collected with a Chemiluminescence gel imager (Amersham Imager 600, GE Healthcare, Chicago, IL, USA) and the images were quantified with the Image J software.