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N-糖基化对鲍伊斯黑色素瘤和人结肠成纤维细胞源性组织纤溶酶原激活物体外活性的影响。

Effects of N-glycosylation on in vitro activity of Bowes melanoma and human colon fibroblast derived tissue plasminogen activator.

作者信息

Wittwer A J, Howard S C, Carr L S, Harakas N K, Feder J, Parekh R B, Rudd P M, Dwek R A, Rademacher T W

机构信息

Department of Cell Culture and Biochemistry, Monsanto Company, St. Louis, Missouri 63167.

出版信息

Biochemistry. 1989 Sep 19;28(19):7662-9. doi: 10.1021/bi00445a022.

DOI:10.1021/bi00445a022
PMID:2514792
Abstract

Tissue-type plasminogen activator (t-PA), when isolated from human colon fibroblast (hcf) cells, is N-glycosylated differently than when isolated from the Bowes melanoma (m) cell line (Parekh et al., 1988). Both hcf- and m-t-PA can be separated into type I t-PA (with three occupied N-glycosylation sequons, at Asn-117, -184, and -448) and type II t-PA (with two occupied sequons, at Asn-117 and -448). Oligosaccharide analysis of each of these types of t-PA indicates that hcf-t-PA and m-t-PA have no glycoforms in common, despite having the same primary amino acid sequence. We have therefore compared in vitro the enzymatic activities and fibrin binding of type I and type II hcf- and m-t-PA with those of aglycosyl t-PA isolated from tunicamycin-treated cells. Plasminogen activation kinetics were determined by using an indirect amidolytic assay with Glu-plasminogen and a chromogenic plasmin substrate. In the absence of stimulator, there was little difference in activity between type I and type II t-PA, but the activity of aglycosyl t-PA was 2-4-fold higher than that of the corresponding glycosylated t-PA. In the presence of a fibrinogen fragment stimulator, the Kcat value of type II t-PA was approximately 5-fold that of type I t-PA from the same cell line, while the Km values for activation of Glu-plasminogen were similar (0.13-0.18 microM). The stimulated activity of glycosyl t-PA was similar to that of type II t-PA.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

组织型纤溶酶原激活剂(t-PA),从人结肠成纤维细胞(hcf)中分离出来时,其N-糖基化情况与从鲍伊斯黑色素瘤(m)细胞系中分离出来时不同(帕雷克等人,1988年)。hcf-t-PA和m-t-PA都可分为I型t-PA(在天冬酰胺-117、-184和-448处有三个被占据的N-糖基化序列)和II型t-PA(在天冬酰胺-117和-448处有两个被占据的序列)。对这些类型的t-PA进行的寡糖分析表明,尽管hcf-t-PA和m-t-PA具有相同的一级氨基酸序列,但它们没有共同的糖型。因此,我们在体外比较了I型和II型hcf-t-PA和m-t-PA与从衣霉素处理的细胞中分离出的无糖基t-PA的酶活性和纤维蛋白结合情况。通过使用含谷氨酸纤溶酶原和发色纤溶酶底物的间接酰胺水解测定法来确定纤溶酶原激活动力学。在没有刺激剂的情况下,I型和II型t-PA之间的活性差异很小,但无糖基t-PA的活性比相应的糖基化t-PA高2至4倍。在存在纤维蛋白原片段刺激剂的情况下,来自同一细胞系的II型t-PA的Kcat值约为I型t-PA的5倍,而激活谷氨酸纤溶酶原的Km值相似(0.13 - 0.18微摩尔)。糖基化t-PA的刺激活性与II型t-PA相似。(摘要截选至250字)

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