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Multiple calcium-activated neutral proteinases (CANP) in mouse retinal ganglion cell neurons: specificities for endogenous neuronal substrates and comparison to purified brain CANP

机译：小鼠视网膜神经节细胞神经元中的多种钙激活中性蛋白酶（CAMP）：内源性神经元底物的特异性和与纯化的脑CAMP的比较

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Calcium-activated neutral proteinases (CANPs) and their specificities for axonally transported proteins were studied within intact axons of mouse retinal ganglion cell (RGC) neurons in vitro. Two CANP activities with markedly different properties were identified. CANP B, at endogenous calcium levels, selectively cleaved the 145,000 Da (145 kDa) neurofilament protein subunit to yield 143 and 140 kDa neurofilament proteins that are also major constituents of the axonal cytoskeleton. This process represents a posttranslational modification of the neurofilament protein subunit rather than the initial step in its degradation (Nixon et al., 1982, 1983). A second calcium-activated neutral proteinase activity, CANP A, appeared only when calcium levels in the incubating medium were 100 microM or higher. CANP A degraded most proteins in RGC axons but acted considerably more rapidly on high- molecular-weight species. In particular, a 290–320 kDa protein in the Group IV (SCb) phase of axoplasmic transport was degraded 3 X faster than other major axonal proteins, including neurofilament proteins and fodrin. When maximally expressed, CANP A activity represented an enormous proteolytic potential in RGC axons--more than 50% of the total axonal content of proteins larger than 60 kDa could be hydrolyzed within 5 min. The calcium requirements, inhibitor profile, and substrate specificity of CANP A were similar to those of mCANP, the major CANP of mouse brain purified to homogeneity, suggesting that these enzymes may be the same or highly related proteins. The existence in a single neuron type of two CANP activities with markedly different substrate specificities and enzymatic properties emphasizes the possible functional diversity of calcium-activated neutral proteinases in neurons. These functions include the posttranslational modification, as well as degradation of neuronal proteins.

机译：钙激活中性蛋白酶（CANPs）及其对轴突转运蛋白的特异性在体外小鼠视网膜神经节细胞（RGC）神经元的完整轴突中进行了研究。确定了两个具有明显不同特性的CANP活动。在内源性钙水平下，CNP B选择性切割145,000 Da（145 kDa）神经丝蛋白亚基，产生143和140 kDa神经丝蛋白，它们也是轴突细胞骨架的主要成分。这个过程代表了神经丝蛋白亚基的翻译后修饰，而不是其降解的第一步（Nixon et al。，1982，1983）。仅当孵育培养基中的钙水平为100 microM或更高时，才会出现第二个钙激活的中性蛋白酶活性CANPA。 CANP A降解了RGC轴突中的大多数蛋白质，但对高分子量物种的作用明显更快。特别是，在轴质运输的第IV组（SCb）期中，一种290-320 kDa的蛋白质比其他主要的轴突蛋白质（包括神经丝蛋白质和草丁膦）降解的速度快了3倍。当最大程度表达时，CNP A活性代表了RGC轴突中巨大的蛋白水解潜力-大于60 kDa的蛋白质的总轴突含量中有50％以上可以在5分钟内水解。 CANP A的钙需求量，抑制剂谱和底物特异性与纯化至均质的小鼠脑主要CANP mCANP相似，表明这些酶可能是相同或高度相关的蛋白质。在单个神经元类型中，两种具有明显不同的底物特异性和酶性质的CANP活性的存在，强调了神经元中钙激活的中性蛋白酶的可能功能多样性。这些功能包括翻译后修饰以及神经元蛋白质的降解。

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期刊名称 The Journal of Neuroscience
作者
RA Nixon; R Quackenbush; A Vitto;
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年(卷),期 1986(6),5
年度 1986
页码 1252–1263
总页数 12
原文格式 PDF
正文语种
中图分类神经科学;
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机译：视网膜神经节细胞神经元和视神经胶质中钙激活的中性蛋白酶（CAMP）引起的纤维蛋白降解：神经元中CANP活性的优先定位
6. Multiple calcium-activated neutral proteinases (CANP) in mouse retinal ganglion cell neurons: specificities for endogenous neuronal substrates and comparison to purified brain CANP [O] . RA Nixon, R Quackenbush, A Vitto 1986

机译：小鼠视网膜神经节细胞神经元的多种钙激活中性蛋白酶（营地）：内源神经元底物的特异性及其与纯化的脑卡

Multiple calcium-activated neutral proteinases (CANP) in mouse retinal ganglion cell neurons: specificities for endogenous neuronal substrates and comparison to purified brain CANP

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