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大鼠肝脏溶酶体唾液酸酶。溶解、底物特异性及与胞质唾液酸酶的比较。

Rat-liver lysosomal sialidase. Solubilization, substrate specificity and comparison with the cytosolic sialidase.

作者信息

Miyagi T, Tsuiki S

出版信息

Eur J Biochem. 1984 May 15;141(1):75-81. doi: 10.1111/j.1432-1033.1984.tb08159.x.

DOI:10.1111/j.1432-1033.1984.tb08159.x
PMID:6723666
Abstract

Purified liver lysosomes, prepared from rats previously injected with Triton WR-1339, exhibited sialidase activity towards sialyllactose, fetuin, submaxillary mucin (bovine) and gangliosides, and could be disrupted hypotonically with little loss in these activities. After centrifugation, the activities with sialyllactose and fetuin were largely recovered in the supernatant, demonstrating that they were originally in the intralysosomal space. The activities towards submaxillary mucin and gangliosides, on the other hand, remained in the pellet. In the supernatant, activity with fetuin or orosomucoid was markedly reduced by protease inhibitors, suggesting that proteolysis of these glycoproteins may be prerequisite to sialidase activity. The intralysosomal sialidase was solubilized from the mitochondrial-lysosomal fraction of rat liver and partially purified by Sephadex G-200, or Sephadex G-200 followed by CM-cellulose. The enzyme was maximally active at pH 4.7 with sialyllactose as substrate and had a minimum relative molecular mass of 60 000 +/- 5000 by gel filtration; it hydrolyzed a variety of sialooligosaccharides , those containing (alpha 2----3)sialyl linkages being better substrates than those with (alpha 2----6)sialyl linkages. The enzyme failed to attack submaxillary mucin and gangliosides. It was also inactive towards fetuin, orosomucoid and transferrin but capable of hydrolyzing glycopeptides from pronase digest of fetuin. In contrast to the intralysosomal sialidase, the sialidase partially purified from rat liver cytosol by (NH4)2SO4 fractionation followed by chromatography on DEAE-cellulose and CM-cellulose hydrolyzed fetuin and orosomucoid to the extent about half that for sialyllactose. The enzyme was maximally active at pH 5.8 and had a relative molecular mass of approximately 60 000. It also hydrolyzed gangliosides but not submaxillary mucin.

摘要

从预先注射曲拉通WR - 1339的大鼠中制备的纯化肝溶酶体,对唾液乳糖、胎球蛋白、下颌下粘蛋白(牛)和神经节苷脂表现出唾液酸酶活性,并且可以通过低渗处理使其破裂,而这些活性几乎没有损失。离心后,唾液乳糖和胎球蛋白的活性大部分在上清液中恢复,表明它们最初存在于溶酶体内腔。另一方面,对下颌下粘蛋白和神经节苷脂的活性仍保留在沉淀中。在上清液中,蛋白酶抑制剂可显著降低胎球蛋白或血清类粘蛋白的活性,这表明这些糖蛋白的蛋白水解可能是唾液酸酶活性的先决条件。溶酶体内的唾液酸酶从大鼠肝脏的线粒体 - 溶酶体部分中溶解出来,并通过葡聚糖凝胶G - 200或先经葡聚糖凝胶G - 200再经CM - 纤维素进行部分纯化。以唾液乳糖为底物时,该酶在pH 4.7时活性最高,通过凝胶过滤法测得其最小相对分子质量为60000±5000;它能水解多种唾液寡糖,含有(α2→3)唾液酸连接键的比含有(α2→6)唾液酸连接键的是更好的底物。该酶不能作用于下颌下粘蛋白和神经节苷脂。它对胎球蛋白、血清类粘蛋白和转铁蛋白也无活性,但能够水解胎球蛋白经链霉蛋白酶消化后的糖肽。与溶酶体内的唾液酸酶相比,通过硫酸铵分级分离,然后在DEAE - 纤维素和CM - 纤维素上进行层析从大鼠肝细胞溶质中部分纯化得到的唾液酸酶,对胎球蛋白和血清类粘蛋白的水解程度约为对唾液乳糖水解程度的一半。该酶在pH 5.8时活性最高,相对分子质量约为60000。它也能水解神经节苷脂,但不能水解下颌下粘蛋白。

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