Control (CTR) or expressing wild-type NDPK-D (WT) or mutant NDPK-D (BD, KD) had been labeled with one hundred nM Mitotracker Green. Representative confocal photos are shown with each other with a 2.7-fold magnified detail to the ideal. Scale bar, 20 m. Further file 14: Fig. S8. NME4 expression is decreased in human breast tumor cell lines with the triple-negative phenotype. NME4 mRNASupplementary InformationThe on the web version consists of supplementary material out there at https://doi. org/10.1186/s12915-021-01155-5. Additional file 1: Fig. S1. NDPK protein expression, kinase activity, and subcellular localization in HeLa clones. HeLa cells had been stably transfected with empty vector pcDNA4TO (CTR) or constructs for expression of NDPK-D WT (WT), CL-binding deficient R90D (BD) or kinase dead H151N (KD). A) Immunoblot detection of NDPK-D (NME4) in extracts with the transfected HeLa cells with -tubulin as loading manage. B) NDP kinase activity in purified HeLa mitochondria. Values are indicates SEM (n=3). C) HeLa TLR4 Agonist manufacturer clones stably transfected with empty vector (CTR), or expressing NDPK-D WT, BD or KD mutants, displaying identical labeling of mitochondrion-selective dye MitoTracker Red CMXRos (red) and immunolabeled NDPK-D (green). Mitochondrial network particulars are indicated by faint line boxes magnified in bold line boxes. Scale bar, 10 m. D) Immunoblot detection of NDPK-A (NME1) and NDPK-B (NME2) in extracts with the transfected HeLa cells with -tubulin as loading manage. Added file 2: Film 1. Videomicroscopy of control HeLa clones. Further file three: Film two. Videomicroscopy of wild-type NDPK-D HeLa clones. More file 4: Film 3. Videomicroscopy of membrane-binding deficient NDPK-D mutant HeLa clones. Additional file 5: Movie four. Videomicroscopy of kinase-dead NDPK-D mutant HeLa clones. More file 6: Fig. S2. Invasion assay of HeLa cells depleted for NDPK-A. A) Phase-contrast microscopy of control (scramble, Scr) and NDPK-A-depleted HeLa cells 72 h post-transfection. Note: Silenced cells are scattered as compared to handle. B) Manage siRNA and NDPK-A depleted (siNME1-1, siNME1-2) HeLa cells were tested for their ability to invade native form I collagen in a 24 h invasion assay. Data are implies SEM (2 independent experiments). C) Activation status of Rac1 (Rac1-GTP) and PAK (phosphorylated PAK, pPAK) of NDPK-A depleted (siNME1-1, siNME1-2) HeLa cells as when compared with total Rac1 and PAK protein, and NDPK-A protein levels. p 0.01.Lacombe et al. BMC Biology(2021) 19:Page 26 oflevels were measured by RT PCR in normal-like human breast cell lines, in hormone receptor-positive (HR+) human breast tumor cell lines, and in triple-negative (TN) human breast tumor cell lines. Each data point represents a single cell line. 3 independent analyses have been performed for every cell line. Information are expressed as signifies SEM. p 0.001, p 0.01. More file 15: Fig. S9. NDPK-D protein expression and mitochondrial localization in NPY Y4 receptor Agonist Formulation MDA-MB-231 clones. A) Immunoblot detection of NDPK-D from MDA-MB-231 cells stably transfected with empty pcDNA4TO (CTR) or constructs for expression of NDPK-D WT, BD or KD. Alpha-tubulin was used as loading control. B) MDA-MB-231 clones stably transfected with empty vector (CTR), or expressing NDPK-D WT or mutants BD or KD, displaying labeling of mitochondrion-selective dye MitoTracker Red CMXRos (red) and immunolabeled NDPK-D (green). Mitochondrial network particulars are indicated by faint line boxes magnified in bold line boxes. Scale bar, ten m. Further file 1.