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Inactive proenzyme to tissue-type plasminogen activator from human melanoma cells identified after affinity purification with a monoclonal antibody.

机译:使用单克隆抗体进行亲和纯化后人黑素瘤细胞的组织型纤溶酶原激活物的酶原失活。

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摘要

The human 66 000 mol. wt. plasminogen activator (HPA66; tissue-type plasminogen activator) has been purified from melanoma cells by a one-step affinity method with a monoclonal antibody. HPA66 purified in this way consists mainly of a one-polypeptide chain form with small amounts (15%) of a form containing two polypeptide chains held together by one or more disulphide bridges. The one-chain form was converted to the two-chain form by catalytic amounts of plasmin. During the conversion, the enzyme activity of HPA66, as measured by an [125I]plasminogen conversion assay and with a chromogenic substrate, increased linearly with the percentage of the two-chain form. A linear regression analysis showed that all enzyme activity could be accounted for by the two-chain form, while the one-chain form had no measurable enzyme activity (detection limit approximately 5% of the activity of the two-chain form). Together with previous findings of inactive proenzymes to murine and human approximately 50 000 mol. wt. (urokinase-type) plasminogen activators, these findings indicate that plasminogen activators are generally formed from inactive one-chain proenzymes which are converted to active two-chain enzymes by limited proteolysis, thus demonstrating a third step in a cascade reaction leading to extracellular proteolysis.
机译:人类66 000 mol。重量纤溶酶原激活物(HPA66;组织型纤溶酶原激活物)已通过单克隆抗体的一步亲和法从黑素瘤细胞中纯化出来。以这种方式纯化的HPA66主要由一种多肽链形式组成,少量(15%)的形式包含通过一条或多条二硫键连接在一起的两条多肽链。通过催化量的纤溶酶将单链形式转化为两链形式。在转化过程中,HPA66的酶活性(通过[125I]纤溶酶原转化测定法和发色底物测得)随双链形式的百分比线性增加。线性回归分析表明,所有酶的活性都可以由双链形式解释,而单链形式没有可测量的酶活性(检测极限约为双链形式活性的5%)。连同先前对鼠和人的无活性酶的发现,大约有5万摩尔。重量(尿激酶型)纤溶酶原激活物,这些发现表明纤溶酶原激活物通常由无活性的单链酶形成,这些酶通过有限的蛋白水解作用转化为有活性的两链酶,因此证明了级联反应的第三步导致细胞外蛋白水解。

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