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Biosynthesis and regulation of rat alpha 1-inhibitor3 a negative acute-phase reactant of the macroglobulin family.

机译:大鼠α1抑制剂3(巨球蛋白家族的阴性急性期反应物)的生物合成和调控。

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摘要

The biosynthesis of rat alpha 1-inhibitor3, a negative acute-phase reactant specifically found in rodents, was studied in vitro in a cell-free translation system from rabbit reticulocytes, in rat hepatocyte primary cultures and in vivo by immunocytochemistry using normal and turpentine-injected rats. By sucrose-gradient centrifugation and subsequent translation of the fractionated RNA in vitro it was found that the mRNA coding for alpha 1-inhibitor3 exhibited a size of about 28S. For the alpha 1-inhibitor3 translated in vitro an apparent Mr of 155,000 was determined. A continuous decrease in the level of alpha 1-inhibitor3 in serum during experimental inflammation induced by turpentine injection was demonstrated by means of quantitative 'rocket' immunoelectrophoresis. This result agrees with the observation by immunocytochemistry of a drastic decrease in alpha 1-inhibitor3 levels in hepatocytes 24 h after turpentine injection. At that time alpha 1-inhibitor3 is mainly located in the Golgi apparatus, whereas it is also present in the membranes of the rough and smooth endoplasmic reticulum when normal liver is used. All hepatocytes, but no other hepatic cells, contain alpha 1-inhibitor3. When hepatocyte primary cultures were labelled with [35S]methionine and alpha 1-inhibitor3 was immunoprecipitated from the hepatocyte medium and the supernatant of homogenized cells, two different forms of alpha 1-inhibitor3 were found. The intracellular form of alpha 1-inhibitor3, with an apparent Mr of 173,000, is characterized by oligosaccharide side chains of the high-mannose type. The form of alpha 1-inhibitor3 in the medium exhibited an Mr of 186,000 and carried carbohydrate side chains of the complex type. After labelling hepatocytes with radioactive sugars, [3H]mannose was found in both forms of alpha 1-inhibitor3, whereas [3H]fucose and [3H]galactose were incorporated only into the form found in the medium. In the presence of tunicamycin an unglycosylated alpha 1-inhibitor3 with an apparent Mr of 154,000 was found in cells and in the medium. In a pulse-chase experiment it was shown that inhibition of glycosylation by tunicamycin resulted in a marked delay of secretion of alpha 1-inhibitor3. Thus the oligosaccharide side chains of alpha 1-inhibitor3 play an important role during its transport into the medium.
机译:大鼠α1抑制剂3(一种在啮齿动物中特别发现的负急性期反应物)的生物合成是在兔网织细胞的无细胞翻译系统中,大鼠肝细胞原代培养物中以及使用正常和松节油的免疫细胞化学方法在体内进行的研究。注射大鼠。通过蔗糖梯度离心和随后的体外分离RNA的翻译,发现编码α1-抑制剂3的mRNA显示出约28S的大小。对于体外翻译的α1-抑制剂3,确定的表观先生为155,000。通过定量“火箭”免疫电泳证实了松节油注射引起的实验性炎症期间血清中α1-抑制物3水平的持续降低。该结果与通过免疫细胞化学观察到的松节油注射后24 h肝细胞中的α1-inhibitor3水平急剧下降是一致的。那时,α1-抑制剂3主要位于高尔基体中,而当使用正常肝脏时,α1-抑制剂3也存在于粗糙而光滑的内质网的膜中。所有的肝细胞,但没有其他肝细胞,都含有α1抑制剂3。当用[35S]蛋氨酸标记肝细胞原代培养物,并从肝细胞培养基和匀浆细胞的上清液中免疫沉淀出α1-抑制剂3时,发现了两种不同形式的α1-抑制剂3。 α1抑制剂3的细胞内形式具有173,000的明显Mr,其特征在于高甘露糖类型的寡糖侧链。介质中的α1-抑制剂3形式的Mr为186,000,带有复杂类型的碳水化合物侧链。用放射性糖标记肝细胞后,发现[3H]甘露糖以两种形式的α1-抑制剂3出现,而[3H]岩藻糖和[3H]半乳糖仅掺入培养基中发现的形式。在衣霉素存在的情况下,在细胞和培养基中发现具有明显的154,000 Mr的未糖基化的α1抑制剂3。在脉冲追踪实验中显示,衣霉素抑制糖基化会明显延迟α1抑制剂3的分泌。因此,α1抑制剂3的寡糖侧链在其转运至培养基期间起着重要作用。

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