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借助一种新型血红素加氧酶抗体测定培养的皮质神经元和星形胶质细胞中血红素加氧酶-1的差异表达。对氧化应激的反应。

Differential expression of heme oxygenase-1 in cultured cortical neurons and astrocytes determined by the aid of a new heme oxygenase antibody. Response to oxidative stress.

作者信息

Dwyer B E, Nishimura R N, Lu S Y

机构信息

Molecular Neurobiology Laboratory, Department of Veterans Affairs Medical Center, Sepulveda, CA 91343, USA.

出版信息

Brain Res Mol Brain Res. 1995 May;30(1):37-47. doi: 10.1016/0169-328x(94)00273-h.

DOI:10.1016/0169-328x(94)00273-h
PMID:7609642
Abstract

Heme oxygenase exists as two isoenzymes designated heme oxygenase-1 (HO-1) and heme oxygenase-2 (HO-2). HO-2 is made constitutively in many cell types whereas HO-1 is a stress protein inducible by heat, heavy metals, ultraviolet irradiation, and oxidative stress. Recombinant rat HO-1 was expressed in bacteria and antiserum designated HO-1713 was raised against the purified protein. HO-1713 detected recombinant rat HO-1 and recombinant rat HO-2. In rat tissues it detected HO-1 and a second, unidentified band designated HO-L (heme oxygenase-like immunoreactivity) which was not HO-2. Cultured rat cortical neurons and forebrain astrocytes were exposed to hydrogen peroxide (0.14-0.7 micromolar for 30 or 60 min). Neurons which contained little detectable HO-1 and which were sensitive to hydrogen peroxide at the high end of the dose curve failed to induce HO-1 by Western blot analysis. In contrast, cultured rat forebrain astrocytes which contained HO-1 under normal culture conditions and which were resistant to injury by hydrogen peroxide, increased their content of immunoreactive HO-1 by 7-fold within 3 h after exposure. Our results support a protective role for HO-1 in oxidative injury and suggest that the relative inability of neurons to increase HO-1 after oxidative stress may contribute to their selective vulnerability vis-a-vis astrocytes. They also suggest that differential expression of heme oxygenase in studies utilizing CNS cultures may alter normal cell physiology and cell survival.

摘要

血红素加氧酶以两种同工酶的形式存在,分别称为血红素加氧酶-1(HO-1)和血红素加氧酶-2(HO-2)。HO-2在许多细胞类型中组成性表达,而HO-1是一种应激蛋白,可被热、重金属、紫外线照射和氧化应激诱导。重组大鼠HO-1在细菌中表达,并针对纯化的蛋白制备了名为HO-1713的抗血清。HO-1713可检测重组大鼠HO-1和重组大鼠HO-2。在大鼠组织中,它可检测到HO-1和另一条未鉴定的条带,称为HO-L(血红素加氧酶样免疫反应性),其不是HO-2。培养的大鼠皮质神经元和前脑星形胶质细胞暴露于过氧化氢(0.14 - 0.7微摩尔,持续30或60分钟)。在剂量曲线高端对过氧化氢敏感且几乎检测不到HO-1的神经元,通过蛋白质印迹分析未能诱导出HO-1。相比之下,在正常培养条件下含有HO-1且对过氧化氢损伤有抗性的培养大鼠前脑星形胶质细胞,在暴露后3小时内其免疫反应性HO-1的含量增加了7倍。我们的结果支持HO-1在氧化损伤中具有保护作用,并表明神经元在氧化应激后相对无法增加HO-1可能导致它们相对于星形胶质细胞具有选择性易损性。它们还表明,在利用中枢神经系统培养物的研究中血红素加氧酶的差异表达可能会改变正常细胞生理学和细胞存活。

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