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在生理离子强度和pH值下从髓鞘膜解离的碱性蛋白被切割成三个主要片段。

Basic protein dissociating from myelin membranes at physiological ionic strength and pH is cleaved into three major fragments.

作者信息

Glynn P, Chantry A, Groome N, Cuzner M L

出版信息

J Neurochem. 1987 Mar;48(3):752-9. doi: 10.1111/j.1471-4159.1987.tb05581.x.

Abstract

Experiments were performed with isolated human myelin membrane preparations to analyse factors that may modulate association of myelin basic protein (MBP) with the membranes and could contribute to demyelinating processes. Transfer of membranes (5 mg protein ml-1) at 37 degrees C and pH 7.4 from a hypotonic medium, in which they were relatively stable, to one of physiological ionic strength produced three major effects: (1) initial dissociation of MBP from the membranes by a nonenzymatic process that was doubled in the presence of millimolar Ca2+/Mg2+; (2) within 10 min, the appearance in the medium of three major MBP fragments (14.4, 10.3, and 8.4 kilodaltons); and (3) progressive acidification of dissociated MBP and its fragments, probably due to deamidation. Between 1 and 6 h a steady state was apparent in which protein equivalent to 15% of the MBP originally bound to the membranes was found in the medium. The three major MBP fragments formed two-thirds of this solubilised material and appeared metabolically stable for 24 h. The kinetics of peptide formation suggested that dissociated, rather than membrane-bound, MBP was cleaved by myelin-associated neutral proteases. Two-dimensional electrophoresis and immunoblotting using two monoclonal antibodies indicated that proteolysis occurred in the vicinity of residues 35 and 75. Evidence was also obtained for removal of C-terminal arginines and relatively rapid deamidation in the C-terminal half of MBP. These modifications of MBP might also occur if extracellular fluid gained access to the compacted cytoplasmic space of the myelin sheath.

摘要

采用分离的人髓磷脂膜制剂进行实验,以分析可能调节髓磷脂碱性蛋白(MBP)与膜结合并可能导致脱髓鞘过程的因素。在37℃和pH 7.4条件下,将膜(5mg蛋白质/ml-1)从相对稳定的低渗介质转移到生理离子强度的介质中,产生了三个主要影响:(1)MBP通过非酶过程从膜上初始解离,在存在毫摩尔浓度的Ca2+/Mg2+时,解离作用增强一倍;(2)在10分钟内,介质中出现三种主要的MBP片段(14.4、10.3和8.4千道尔顿);(3)解离的MBP及其片段逐渐酸化,可能是由于脱酰胺作用。在1至6小时之间,出现了一种稳定状态,此时在介质中发现了相当于最初与膜结合的MBP的15%的蛋白质。这三种主要的MBP片段占这种溶解物质的三分之二,并且在24小时内代谢稳定。肽形成的动力学表明,解离的而非膜结合的MBP被髓磷脂相关中性蛋白酶切割。使用两种单克隆抗体进行的二维电泳和免疫印迹表明,蛋白水解发生在残基35和75附近。还获得了关于去除MBP C末端精氨酸以及MBP C末端一半区域相对快速脱酰胺的证据。如果细胞外液进入髓鞘紧密的细胞质空间,MBP的这些修饰也可能发生。

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