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用番红法测定离子载体和代谢抑制剂对分离的肝细胞线粒体内膜电位的影响。

Effects of ionophores and metabolic inhibitors on the mitochondrial membrane potential within isolated hepatocytes as measured with the safranine method.

作者信息

Akerman K E, Järvisalo J O

出版信息

Biochem J. 1980 Oct 15;192(1):183-90. doi: 10.1042/bj1920183.

DOI:10.1042/bj1920183
PMID:7305896
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1162321/
Abstract

A difference spectrum with a peak of absorbance at 526nm appears slowly upon addition of valinomycin or KCN in combination with oligomycin to a hepatocyte suspension in the presence of safranine. When the cells are incubated at 37 degrees C in a medium containing safranine, a slow decrease in the absorbance occurs at the wavelength pair 524-484 nm. The change in absorbance is completed within 20-30 min after additions of cells to a medium containing safranine. At this time the safranine concentration of the outer medium is considerably decreased. The safranine signal is completely reversed by valinomycin, carbonyl cyanide p-trifluoromethoxyphenyl-hydrazone or KCN in combination with oligomycin. None of these treatments have any immediate effect on cellular ATP concentrations or the 36Cl- equilibrium potential across the plasma membrane. In the presence of iodoacetate a slow reversal of the trace can be induced upon addition of KCN, but not of oligomycin alone. Rotenone, in combination with oligomycin, does not reverse the safranine signal except when both KF and iodoacetate are present, in which case a slow reversal is seen. A subsequent addition of duroquinone brings back the signal to the same level as in the presence of rotenone alone. The results indicate that the spectral response of safranine in the presence of isolated hepatocytes is a result of a slow penetration of safranine into intracellular mitochondria, where aggregation of safranine molecules occurs as a response to the mitochondrial membrane potential.

摘要

在藏红存在的情况下,向肝细胞悬液中加入缬氨霉素或氰化钾并结合寡霉素后,会缓慢出现一个在526nm处有吸光度峰值的差示光谱。当细胞在含有藏红的培养基中于37℃孵育时,在524 - 484nm波长对处吸光度会缓慢下降。将细胞加入含有藏红的培养基后,吸光度的变化在20 - 30分钟内完成。此时外部培养基中的藏红浓度显著降低。缬氨霉素、羰基氰对三氟甲氧基苯腙或氰化钾与寡霉素的组合可使藏红信号完全逆转。这些处理均对细胞内ATP浓度或质膜两侧的³⁶Cl⁻平衡电位没有任何即时影响。在碘乙酸存在的情况下,加入氰化钾可诱导信号缓慢逆转,但单独加入寡霉素则不行。鱼藤酮与寡霉素组合不会使藏红信号逆转,除非同时存在氟化钾和碘乙酸,在这种情况下会出现缓慢逆转。随后加入杜醌可使信号恢复到仅存在鱼藤酮时的相同水平。结果表明,在分离的肝细胞存在的情况下,藏红的光谱响应是藏红缓慢渗透到细胞内线粒体的结果,在那里藏红分子会因线粒体膜电位而发生聚集。

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