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来自人胚胎肾细胞培养物的纤溶酶原激活剂。前激活剂的证据。

Plasminogen activator from human embryonic kidney cell cultures. Evidence for a proactivator.

作者信息

Nolan C, Hall L S, Barlow G H, Tribby I I

出版信息

Biochim Biophys Acta. 1977 Feb 28;496(2):384-400. doi: 10.1016/0304-4165(77)90321-x.

Abstract

The nature of the trypsin-activatable plasminogen activator produced by kidney cell cultures (Bernik, M.B (1973), J. Clin. Invest. 52, 823-834) was investigated using human embryonic kidney (HEK) cell cultures in serum-free medium. Plaminogen activator activity ratios (trypsin-activated/ untreated controls) in HEK cell-conditioned media were maximal (up to 3) during the first week of culture and remained nearly constant at approximatley 2 for the next 3-5 weeks, while the total plasminogen activator titer increased in a nearly linear manner. Therefore, coincident with progressive cell degeneration and death, the ratios decreased to near unity due to "spontaneous" activation of the enzyme, which was inhibited in cell-free conditioned media by the pancreatic trypsin inhibitor Kunitz and benzamidine. Since the activator is not inhibited by the trypsin inhibitor, it is concluded that a protease other than the plasminogen activator is responsible for the activation. Increases in the plasminogen activator titers (about 2-fold) were similarly obtained by culturing the cells in medium containing low concentrations (0.05-0.10 mug/ml) of trypsin for up to about 6 weeks. The presence of the trypsin inhibitor in HEK cells cultures decreased the rate of activation, resulting in higher activity ratios (up to 6), and the total plasminogen activator activity was reduced only minimally (less than 20%), if at all, by the highest concentration of the trypsin inhibitor (100 mug/ml) tested. Affinity chromatography of conditioned media with activity ratios of 1.6--2 separated the plasminogen activator into an active fraction and a fraction which was activated a minimum of 200-fold by trypsin and contained no measurable activity prior to activation. Gel filtration of crude conditioned media or partially purified activator separated the plasminogen activator into two peaks; both were trypsin-activatable, and their relative proportions varied with the isolated conditions. The results indicate the occurrence of a proenzyme form of the plasminogen activator in the culture media.

摘要

利用人胚肾(HEK)细胞在无血清培养基中培养,对肾细胞培养物产生的胰蛋白酶可激活的纤溶酶原激活剂的性质进行了研究(Bernik,M.B(1973年),《临床研究杂志》52,823 - 834)。在培养的第一周,HEK细胞条件培养基中的纤溶酶原激活剂活性比(胰蛋白酶激活的/未处理的对照)最大(高达3),并在接下来的3 - 5周内几乎保持在约2的恒定水平,而总纤溶酶原激活剂滴度以近似线性的方式增加。因此,随着细胞逐渐退化和死亡,由于该酶的“自发”激活,活性比降至接近1,而这种激活在无细胞条件培养基中被胰腺胰蛋白酶抑制剂库尼茨和苯甲脒所抑制。由于激活剂不受胰蛋白酶抑制剂的抑制,得出结论,负责激活的是纤溶酶原激活剂以外的一种蛋白酶。通过在含有低浓度(0.05 - 0.10微克/毫升)胰蛋白酶的培养基中培养细胞长达约6周,同样获得了纤溶酶原激活剂滴度的增加(约2倍)。HEK细胞培养物中胰蛋白酶抑制剂的存在降低了激活速率,导致更高的活性比(高达6),并且在测试的最高浓度(100微克/毫升)的胰蛋白酶抑制剂下,总纤溶酶原激活剂活性即使有降低也仅最小程度(小于20%)。对活性比为1.6 - 2的条件培养基进行亲和层析,将纤溶酶原激活剂分离为一个活性部分和一个被胰蛋白酶激活至少200倍且在激活前无可测量活性的部分。对粗制条件培养基或部分纯化的激活剂进行凝胶过滤,将纤溶酶原激活剂分离为两个峰;两者均为胰蛋白酶可激活的,并且它们的相对比例随分离条件而变化。结果表明在培养基中存在纤溶酶原激活剂的一种酶原形式。

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