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慢性吗啡暴露对大鼠突触质膜亚蛋白质组的影响:基于同位素编码亲和标签和液相色谱/质谱的定量蛋白质谱研究

Effect of chronic morphine exposure on the synaptic plasma-membrane subproteome of rats: a quantitative protein profiling study based on isotope-coded affinity tags and liquid chromatography/mass spectrometry.

作者信息

Prokai Laszlo, Zharikova Alevtina D, Stevens Stanley M

机构信息

Department of Medicinal Chemistry, University of Florida, Gainesville, Florida 32610-0485, USA.

出版信息

J Mass Spectrom. 2005 Feb;40(2):169-75. doi: 10.1002/jms.736.

Abstract

The effect of chronic morphine exposure on the synaptic plasma-membrane subproteome in rats was studied by the isotope-coded affinity tag (ICAT) method coupled with capillary reversed-phase liquid chromatography/electrospray ionization mass spectrometry and tandem mass spectrometry. ICAT-labeled tryptic peptides of synaptic membrane proteins were successfully identified using tandem mass spectrometry in conjunction with protein database searching. Several important synaptic plasma-membrane proteins displayed significant regulation changes as a result of chronic morphine exposure in vivo. In particular, an integral membrane protein Na(+)/K+ ATPase (alpha-subunit) involved in regulation of the cell membrane potential by controlling sodium and potassium ion permeability was downregulated by 39 +/- 2%. This result was in excellent agreement with the reduction in electrogenic Na+, K+ pumping due to about 40% downregulation of Na(+)/K+ ATPase alpha3-isoform in myenteric S-neurons of morphine-exposed guinea-pigs measured by others via immunohistochemistry. The decrease in the abundance of non-erythroid alpha II-spectrin in the synaptic plasma-membrane fraction was also observed, which was hypothetically associated with the breakdown of the protein due to the upregulation of the proteolytic enzyme caspase-3 upon chronic morphine exposure.

摘要

采用同位素编码亲和标签(ICAT)法结合毛细管反相液相色谱/电喷雾电离质谱和串联质谱,研究了慢性吗啡暴露对大鼠突触质膜亚蛋白质组的影响。通过串联质谱结合蛋白质数据库搜索,成功鉴定了突触膜蛋白的ICAT标记胰蛋白酶肽段。由于体内慢性吗啡暴露,几种重要的突触质膜蛋白表现出显著的调节变化。特别是,一种通过控制钠和钾离子通透性参与调节细胞膜电位的整合膜蛋白Na(+)/K+ ATP酶(α亚基)下调了39±2%。这一结果与其他研究人员通过免疫组织化学测量发现的吗啡暴露豚鼠肠肌间S神经元中Na(+)/K+ ATP酶α3亚型下调约40%导致的电致Na+、K+泵浦减少高度一致。在突触质膜组分中还观察到非红细胞α II-血影蛋白丰度的降低,推测这与慢性吗啡暴露后蛋白水解酶caspase-3上调导致的蛋白质降解有关。

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