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Mucus glycoprotein secretion by tracheal explants: effects of pollutants.

机译:气管外植体分泌的粘液糖蛋白:污染物的影响。

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摘要

Tracheal slices incubated with radioactive precursors in tissue culture medium secrete labeled mucus glycoproteins into the culture medium. We have used an in vivtro approach, a combined method utilizing exposure to pneumotoxins in vivo coupled with quantitation of mucus secretion rates in vitro, to study the effects of inhaled pollutants on mucus biosynthesis by rat airways. In addition, we have purified the mucus glycoproteins secreted by rat tracheal explants in order to determine putative structural changes that might by the basis for the observed augmented secretion rates after exposure of rats to H2SO4 aerosols in combination with high ambient levels of ozone. After digestion with papain, mucus glycoproteins secreted by tracheal explants may be separated into five fractions by ion-exchange chromatography, with recovery in high yield, on columns of DEAE-cellulose. Each of these five fractions, one neutral and four acidic, migrates as a single unique spot upon cellulose acetate electrophoresis at pH values of 8.6 and 1.2. The neutral fraction, which is labeled with [3H] glucosamine, does not contain radioactivity when Na2 35SO4 is used as the precursor. Acidic fractions I-IV are all labeled with either 3H-glucosamine or Na2 35SO4 as precursor. Acidic fraction II contains sialic acid as the terminal sugar on its oligosaccharide side chains, based upon its chromatographic behavior on columns of wheat-germ agglutinin-Agarose. Treatment of this fraction with neuraminidase shifts its elution position in the gradient to a lower salt concentration, coincident with acidic fraction I. After removal of terminal sialic acid residues with either neuraminidase or low pH treatment, the resultant terminal sugar on the oligosaccharide side chains is fucose. These results are identical with those observed with mucus glycoproteins secreted by cultured human tracheal explants and purified by these same techniques.
机译:在组织培养基中与放射性前体一起孵育的气管切片将标记的粘液糖蛋白分泌到培养基中。我们使用了一种体内方法,一种结合了体内暴露于肺炎毒素的方法,并结合了体外对粘液分泌速率的定量研究来研究吸入污染物对大鼠气道粘液生物合成的影响。另外,我们已经纯化了大鼠气管外植体分泌的粘液糖蛋白,以便确定可能的结构变化,这些变化可能是根据大鼠暴露于H2SO4气溶胶并与高环境臭氧水平相结合后观察到的分泌率增加而确定的。用木瓜蛋白酶消化后,可将气管外植体分泌的粘液糖蛋白通过离子交换色谱在DEAE-纤维素柱上分离成五个部分,并以高收率回收。在乙酸纤维素电泳时,这五个级分中的每个(一个中性和四个酸性)都作为单个唯一的斑点迁移,pH值为8.6和1.2。当使用Na2 35SO4作为前体时,标有[3H]葡糖胺的中性馏分不包含放射性。酸性馏分I-IV均用3H-葡萄糖胺或Na2 35SO4作为前体标记。根据其在小麦胚芽凝集素-琼脂糖柱上的色谱行为,酸性级分II的寡糖侧链上含有唾液酸作为末端糖。用神经氨酸酶处理该级分会将其洗脱位置移至较低的盐浓度,与酸性级分I一致。用神经氨酸酶或低pH处理去除末端唾液酸残基后,寡糖侧链上的最终末端糖为岩藻糖。这些结果与通过培养的人气管外植体分泌并通过这些相同技术纯化的粘液糖蛋白观察到的结果相同。

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  • 作者

    Last, J A; Kaizu, T;

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  • 年度 1980
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  • 原文格式 PDF
  • 正文语种 {"code":"en","name":"English","id":9}
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