senox is often a clinically established drug for the therapy of acute promylocytic leukemia APL 19 , and also potentially helpful against other hematological malignancies 20 . Nonetheless its efficacy is often limited by the requirement of high doses to efficiently Icotinib induce apoptosis, pointing to the necessity of introducing sensitizing approaches. An earlier report indicated that 2 DG did not have an effect on ATO toxicity in numerous tumor cell models 12 . Nevertheless we lately showed that lonidamine, a glycolytic inhibitor 21 improved the apoptotic efficacy of ATO in leukemia cells 22 . With this precedents in mind, in the present report we examine the capacity of 2 DG to cooperate with ATO and other antitumor drugs to induce apoptosis in HL60 and other human myeloid leukemia cell lines, also as the behavior of aspects like ATP levels, oxidative anxiety, mitochondrial dysfunction, and protein kinase signaling pathways, essential for apoptosis regulation and execution.
The results indicate that ATO and 2 DG efficaciously cooperate to induce apoptosis by mechanisms involving attenuation by ATO of 2 DG provoked IGF 1R, MEK ERK and Akt mTOR activation, also as occasional inactivation by 2 DG with the LKB 1 AMPK pathway. 2. Supplies and techniques . Reagents and antibodies All components for Icotinib cell culture were obtained from Invitrogen, Inc. Carlsbad, CA, USA . 4,6 diamino 2 phenylindole DAPI was obtained from Serva Heidelberg, Germany . Dichlorodihydrofluorescein diacetate H2DCFDA and monochlorobimane were obtained from Molecular Probes, Inc. Eugene, OR, USA .
Dihydroethidium DHE, supplied as a 5 mM solution in dimethyl sulfoxide was obtained from Invitrogen, Inc. Lonafarnib The kinase inhibitors Compound C AMPK inhibitor, CC , 1,4 Diamino 2,3 dicyano 1,4 bis 2 aminophenylthio butadiene U0126 , 2 4 Morpholinyl 8 phenyl 4H 1 benzopyran 4 one LY294002 , triciribine Akt inhibitor V, AktiV , N 2 Methoxy 5 chlorophenyl N0 2methylquinilin 4 yl urea IGF 1R inhibitor, PQ401 , and the caspase inhibitor Z Val Ala Asp OMe CH2F z VAD fmk Ribonucleotide , were obtained from Calbiochem Darmstad, Germany . Rabbit anti human AMPKa, p44 42 MAPK, phospho p44 p42 MAPK Thr202 Tyr204 , Akt, phospho Akt Ser473 , phospho mTOR Ser2448 , phospho S6 ribosomal protein Ser235 236 rpS6 , HtrA2, and caspase 3 polyclonal antibodies pAbs , rabbit anti human phospho AMPKa Thr172 , phospho LKB1 Ser428 C6743 , and mTOR 7C10 monoclonal antibodies mAbs , and mouse anti human phosphop70 S6 kinase Thr389 1A5 p70S6K mAb, were obtained from Cell Signaling Technology Inc Danvers, MA, USA .
Mouse antipigeon cytochrome c mAb clone 7H8.2C12 was obtained from BD PharMingen San Diego, CA, USA . Rabbit anti human phospho IGF 1R Tyr1165 1166 , Bax N 20 , and caspase 9 p35 H 170 pAbs; and goat anti human Bid C 20 pAb, were obtained from Santa Cruz Biotechnology, Inc. Santa Cruz, CA, USA . Mouse anti XIAP clone 2F1 mAb was obtained from MBL International Corporation Woburn, Lonafarnib MA, USA . Peroxidase conjugated immunoglobulin G antibodies were obtained from DAKO Diagnostics, S.A. Barcelona, Spain . Tiny interfering RNA siRNA against AMPK AMPK1 2 siRNA h and manage Icotinib scramble siRNA were obtained from Santa Cruz Biotechnology, Inc.
All other non talked about reagents and antibodies were from Sigma Madrid, Spain Cells and treatment options The human cell lines HL60 and U937 acute myeloid leukemia, AML , NB4 acute promyelocytic leukemia, APL , and THP 1 promonocytic leukemia were grown in normal RPMI 1640 medium containing 2.05 mM L glutamine Lonafarnib and 11.11 mM Lglucose supplemented with 10 v v heat inactivated calf serum, 0.2 sodium bicarbonate and antibiotics in a humidified 5 CO2 atmosphere at 37 8C. Cells were routinely maintained under logarithmic growth by passing them each 2 3 days. Under these conditions, HL60, U937, and NB4 cells exhibited an approximate doubling time of 18 h, and THP 1 of 24 36 h. Except when essential, to avoid manipulations which could per se have an effect on basal kinase activation, 24 h prior to treatment options the cells were adjusted at 105 for 16 24 h treatment options or 2 105 for 0.
5 8 h treatment options cells ml working with a mixture of conditioned and fresh medium, and after that remained undisturbed until the time of drug administration. Icotinib To check the attainable influence of cell culture conditions, in some experiments the culture medium was re supplemented with 2 mM glutamine and 1 mM pyruvate, or the serum concentration was decreased ranging from 0 to 5 . For Lonafarnib glucose deprivation, the cells were extensively washed with phosphate buffered saline PBS and after that seeded at the suitable concentration in glucoselacking RPMI medium supplemented with 10 v v serum. For experiments with IGF 1, 16 h prior to treatment options the cells were washed and seeded in normal RPMI medium supplemented with 1 v v serum. Human peripheral blood lymphocytes PBLs obtained from healthy donors were isolated, cultured and stimulated to proliferate by sequential therapy with phytohemagluttining and human interleukin 2 IL 2 , as previously described 22 .
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