TY - JOUR
T1 - Enhancing lysosome biogenesis attenuates BNIP3-induced cardiomyocyte death
AU - Xiucui, Ma
AU - Godar, Rebecca J.
AU - Liu, Haiyan
AU - Diwan, Abhinav
N1 - Funding Information:
Sigma, D1556) gradient (19%, 27% and 30%) and subjected to We thank Toni Gonzales for secretarial assistance and express our ultracentrifugation at 110,000 g for 2 h in a swinging bucket sincere gratitude to Douglas L. Mann, M.D., chief of cardiology rotor. Three-milliliter fractions were collected from the gradient; at Washington University School of Medicine, for his helpful and lysosomes, and mitochondria with mitochondria-associated-comments and support. membranes were recovered from the top and 3rd (from top) This study was supported by the NIH (HL107594), the fractions, respectively. The supernatant from the 20,000 g spin Department of Veterans Affairs (1 I01 BX000448-01) and the was subjected to ultracentrifugation at 100,000 g for 1 h to American Heart Association (0735135N Scientist Development recover endoplasmic reticulum rich fraction; with resultant Grant) all to A.D. The Hope Center Viral Vectors Core and Alafi supernatant concentrated as cytosol using Ultracel-10K protein Neuroimaging Core at Washington University are supported by filters (Millipore, UFC801024). P30 NS057105 and P01 NS032636 from the NIH.
PY - 2012/3
Y1 - 2012/3
N2 - Hypoxia-inducible pro-death protein BNIP3 (BCL-2/adenovirus E1B 19-kDa interacting protein 3), provokes mitochondrial permeabilization causing cardiomyocyte death in ischemia-reperfusion injury. Inhibition of autophagy accelerates BNIP3-induced cell death, by preventing removal of damaged mitochondria. We tested the hypothesis that stimulating autophagy will attenuate BNIP3-induced cardiomyocyte death. Neonatal rat cardiac myocytes (NRCMs) were adenovirally transduced with BNIP3 (or LacZ as control; at multiplicity of infection = 100); and autophagy was stimulated with rapamycin (100 nM). Cell death was assessed at 48 h. BNIP3 expression increased autophagosome abundance 8-fold and caused a 3.6-fold increase in cardiomyocyte death as compared with control. Rapamycin treatment of BNIP3-expressing cells led to further increase in autophagosome number without affecting cell death. BNIP3 expression led to accumulation of autophagosome-bound LC3-II and p62, and an increase in autophagosomes, but not autolysosomes (assessed with dual fluorescent mCherry-GFP-LC3 expression). BNIP3, but not the transmembrane deletion variant, interacted with LC3 and colocalized with mitochondria and lysosomes. However, BNIP3 did not target to lysosomes by subcellular fractionation, provoke lysosome permeabilization or alter lysosome pH. Rather, BNIP3-induced autophagy caused a decline in lysosome numbers with decreased expression of the lysosomal protein LAMP-1, indicating lysosome consumption and consequent autophagosome accumulation. Forced expression of transcription factor EB (TFEB) in BNIP3-expressing cells increased lysosome numbers, decreased autophagosomes and increased autolysosomes, prevented p62 accumulation, removed depolarized mitochondria and attenuated BNIP3-induced death. We conclude that BNIP3 expression induced autophagosome accumulation with lysosome consumption in cardiomyocytes. Forced expression of TFEB, a lysosomal biogenesis factor, restored autophagosome processing and attenuated BNIP3-induced cell death.
AB - Hypoxia-inducible pro-death protein BNIP3 (BCL-2/adenovirus E1B 19-kDa interacting protein 3), provokes mitochondrial permeabilization causing cardiomyocyte death in ischemia-reperfusion injury. Inhibition of autophagy accelerates BNIP3-induced cell death, by preventing removal of damaged mitochondria. We tested the hypothesis that stimulating autophagy will attenuate BNIP3-induced cardiomyocyte death. Neonatal rat cardiac myocytes (NRCMs) were adenovirally transduced with BNIP3 (or LacZ as control; at multiplicity of infection = 100); and autophagy was stimulated with rapamycin (100 nM). Cell death was assessed at 48 h. BNIP3 expression increased autophagosome abundance 8-fold and caused a 3.6-fold increase in cardiomyocyte death as compared with control. Rapamycin treatment of BNIP3-expressing cells led to further increase in autophagosome number without affecting cell death. BNIP3 expression led to accumulation of autophagosome-bound LC3-II and p62, and an increase in autophagosomes, but not autolysosomes (assessed with dual fluorescent mCherry-GFP-LC3 expression). BNIP3, but not the transmembrane deletion variant, interacted with LC3 and colocalized with mitochondria and lysosomes. However, BNIP3 did not target to lysosomes by subcellular fractionation, provoke lysosome permeabilization or alter lysosome pH. Rather, BNIP3-induced autophagy caused a decline in lysosome numbers with decreased expression of the lysosomal protein LAMP-1, indicating lysosome consumption and consequent autophagosome accumulation. Forced expression of transcription factor EB (TFEB) in BNIP3-expressing cells increased lysosome numbers, decreased autophagosomes and increased autolysosomes, prevented p62 accumulation, removed depolarized mitochondria and attenuated BNIP3-induced death. We conclude that BNIP3 expression induced autophagosome accumulation with lysosome consumption in cardiomyocytes. Forced expression of TFEB, a lysosomal biogenesis factor, restored autophagosome processing and attenuated BNIP3-induced cell death.
KW - Autophagy
KW - BNIP3
KW - Cardiomyocyte death
KW - Lysosomes
KW - TFEB
UR - http://www.scopus.com/inward/record.url?scp=84859151396&partnerID=8YFLogxK
U2 - 10.4161/auto.8.3.18658
DO - 10.4161/auto.8.3.18658
M3 - Article
C2 - 22302006
AN - SCOPUS:84859151396
SN - 1554-8627
VL - 8
SP - 297
EP - 309
JO - Autophagy
JF - Autophagy
IS - 3
ER -