2-十四烷基缩水甘油酸、2-十四烷基缩水甘油辅酶A和2-十四烷基缩水甘油肉碱对肝脏肉碱棕榈酰转移酶的体内外作用
Action in vivo and in vitro of 2-tetradecylglycidic acid, 2-tetradecylglycidyl-CoA and 2-tetradecylglycidylcarnitine on hepatic carnitine palmitoyltransferase.
作者信息
Brady P S, Brady L J
出版信息
Biochem J. 1986 Sep 15;238(3):801-9. doi: 10.1042/bj2380801.
The effects of 2-tetradecylglycidic acid (TDGA), TDGA-CoA and TDGA-carnitine were examined in purified hepatic CPT (carnitine palmitoyltransferase) and in hepatic mitochondria and inverted submitochondrial vesicles derived from Sprague-Dawley rats. Since TDGA has been reported as a specific inhibitor of carnitine palmitoyltransferase-A (CPT-A), the focus was on kinetics and inhibition of CPT-A, and the relationship of this key enzyme to beta-oxidation. After administration of TDGA in vivo to overnight-starved rats, the Vmax. of CPT in intact mitochondria and in inverted vesicles (CPT-B) was depressed by 66%. The S0.5 for palmitoyl-CoA and Km for carnitine were unchanged. The I50 (concn. giving 50% inhibition) for malonyl-CoA was significantly increased from 20 to 141 microM in intact mitochondria, but unchanged (199 versus 268 microM) in inverted vesicles. The addition in vitro of TDGA-CoA (0-1.0 microM) gave I50 values of 0.29 and 0.27 microM (S.E.M. = 0.19) in intact mitochondria from fed and 48 h-starved rats, and 0.81 and 1.57 microM (S.E.M. = 0.29) for inverted vesicles derived from fed and starved rats. Addition in vitro of TDGA-carnitine to mitochondria from starved rats yielded an I50 value of 27.7 mM (S.E.M. = 12.2) for L-[methyl-14C]carnitine release from palmitoyl-L-[methyl-14C]carnitine and 0.64 mM (S.E.M. = 0.07) for palmitoyl-L-[methyl-14C]carnitine formation from L-[methyl-14C]carnitine in intact mitochondria. Inverted vesicles were not measurably sensitive to TDGA-carnitine up to 500 microM for the assay of L-[methyl-14C]carnitine release, but were as sensitive as intact mitochondria when inhibition was determined in the direction of palmitoyl-L-[methyl-14C]carnitine formation (I50 = 0.54 +/- 0.07 microM). When TDGA-CoA was added to intact mitochondria, then incubated for 5 min at room temperature and subsequently washed out, Vmax. of CPT decreased from 5.8 to 3.5 (S.E.M. = 0.6) in intact mitochondria, and from 17.2 to 6.3 (S.E.M. = 4.8) in inverted vesicles. The Km for L-carnitine and the S0.5 for palmitoyl-CoA increased 2-fold with TDGA-CoA pretreatment in both intact mitochondria and inverted vesicles. Detergent solubilization (0.05% Triton X-100) resulted in a complete loss of TDGA-CoA sensitivity (up to 1.0 microM measured). Sonicated mitochondria exhibited an I50 of 0.72 +/- 0.03 microM.(ABSTRACT TRUNCATED AT 400 WORDS)
在纯化的肝脏肉碱棕榈酰转移酶(CPT)以及源自Sprague-Dawley大鼠的肝脏线粒体和反向亚线粒体小泡中,研究了2-十四烷基缩水甘油酸(TDGA)、TDGA-辅酶A和TDGA-肉碱的作用。由于TDGA已被报道为肉碱棕榈酰转移酶-A(CPT-A)的特异性抑制剂,研究重点在于CPT-A的动力学和抑制作用,以及这种关键酶与β-氧化的关系。给过夜禁食的大鼠体内注射TDGA后,完整线粒体和反向小泡(CPT-B)中CPT的Vmax降低了66%。棕榈酰辅酶A的S0.5和肉碱的Km未发生变化。完整线粒体中丙二酰辅酶A的I50(产生50%抑制的浓度)从20显著增加至141 microM,但反向小泡中未改变(199对268 microM)。体外添加TDGA-辅酶A(0 - 1.0 microM)时,喂食大鼠和饥饿48小时大鼠的完整线粒体中I50值分别为0.29和0.27 microM(标准误 = 0.19),喂食大鼠和饥饿大鼠来源的反向小泡的I50值分别为0.81和1.57 microM(标准误 = 0.29)。体外向饥饿大鼠的线粒体中添加TDGA-肉碱,对于从棕榈酰-L-[甲基-14C]肉碱释放L-[甲基-14C]肉碱,I50值为27.7 mM(标准误 = 12.2),对于完整线粒体中由L-[甲基-14C]肉碱形成棕榈酰-L-[甲基-14C]肉碱,I50值为0.64 mM(标准误 = 0.07)。对于L-[甲基-14C]肉碱释放的测定,高达500 microM时反向小泡对TDGA-肉碱无明显敏感性,但在测定棕榈酰-L-[甲基-14C]肉碱形成方向的抑制作用时,其与完整线粒体一样敏感(I50 = 0.54 +/- 0.07 microM)。当将TDGA-辅酶A添加到完整线粒体中,在室温下孵育5分钟,随后洗脱,完整线粒体中CPT的Vmax从5.8降至3.5(标准误 = 0.6),反向小泡中从17.2降至6.3(标准误 = 4.8)。在完整线粒体和反向小泡中,经TDGA-辅酶A预处理后,L-肉碱的Km和棕榈酰辅酶A的S0.5均增加了2倍。去污剂溶解(0.05% Triton X-100)导致对TDGA-辅酶A的敏感性完全丧失(测定高达1.0 microM时)。超声处理的线粒体的I50为0.72 +/- 0.03 microM。(摘要截短至400字)
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