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小鼠腹腔巨噬细胞的5'-核苷酸酶活性。I. 驻留和炎症细胞群体中的合成与降解

5'-Nucleotidase activity of mouse peritoneal macrophages. I. Synthesis and degradation in resident and inflammatory populations.

作者信息

Edelson P J, Cohn Z A

出版信息

J Exp Med. 1976 Dec 1;144(6):1581-95. doi: 10.1084/jem.144.6.1581.

Abstract

Mouse resident peritoneal macrophages display sufficient 5'-nucleotidase activity to hydrolyze 58 nm AMP/min per cell protein. This activity increases approximately 163 nm AMP/min per mg after 72 h in culture. The enzyme is renewed in unstimulated cells with a half-time of 13.9 h. The activity is not reduced by treatment of intact cells with a variety of proteolytic enzymes, including trypsin, pronase, urokinase, and plasmin. Cells obtained from an inflammatory exudate have diminished or absent levels of enzyme activity. Endotoxin-elicited cells display enzyme activitiy of 20.9 nm AMP/min per mg, while thioglycollate-stimulated macrophages have no detectable activity. The reduced level of activity in endotoxin-stimulated cells is due to their elevated rate of enzyme degradation, with a half-time of 6.9 h. Their rate of enzyme synthesis is essentially normal. No evidence for latent enzyme activity could be obtained in thioglycollate-stimulated cells, nor do these cells produce any inhibition of normal cell enzyme activity. Serum deprivation reduces the enzyme activity of resident cells to about 45% of control activity. These conditions do not significantly affect the rate of enzyme synthesis, but again are explainable by an increase in the rate of enzyme degradation. Pinocytic rate is elevated in endotoxin-stimulated cells which show a more rapid rate of enzyme degradation than unstimulated cells do. However, in serum-free conditions, the rate of enzyme degradation is doubled with no change in the pinocytic rate of the cells.

摘要

小鼠腹腔常驻巨噬细胞表现出足够的5'-核苷酸酶活性,可水解每细胞蛋白每分钟58纳米的AMP。培养72小时后,该活性增加至每毫克每分钟约163纳米的AMP。在未受刺激的细胞中,该酶以13.9小时的半衰期更新。用包括胰蛋白酶、链霉蛋白酶、尿激酶和纤溶酶在内的多种蛋白水解酶处理完整细胞,该活性不会降低。从炎性渗出物中获得的细胞酶活性水平降低或缺失。内毒素诱导的细胞表现出的酶活性为每毫克每分钟20.9纳米的AMP,而巯基乙酸盐刺激的巨噬细胞则没有可检测到的活性。内毒素刺激细胞中活性水平的降低是由于其酶降解速率升高,半衰期为6.9小时。它们的酶合成速率基本正常。在巯基乙酸盐刺激的细胞中未获得潜在酶活性的证据,这些细胞也不会对正常细胞的酶活性产生任何抑制作用。血清剥夺使常驻细胞的酶活性降低至对照活性的约45%。这些条件不会显著影响酶合成速率,但同样可以通过酶降解速率的增加来解释。内毒素刺激的细胞中胞饮速率升高,其酶降解速率比未刺激的细胞更快。然而,在无血清条件下,酶降解速率加倍,而细胞的胞饮速率没有变化。

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