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再生大鼠肝脏中的唾液酸转移酶活性

Sialyltransferase activity in regenerating rat liver.

作者信息

Serafini-Cessi F

出版信息

Biochem J. 1977 Sep 15;166(3):381-6. doi: 10.1042/bj1660381.

Abstract

Liver microsomal fractions catalyse the transfer of sialic acid from CMP-N-acetyl-neuraminic acid to various exogenous acceptors such as desialylated fetuin, desialylated human Tamm-Horsfall glycoprotein and desialylated bovine submaxillary-gland mucin. An increase in the rate of incorporation of sialic acid into desialylated glycoproteins was found after a lag period (7h) in regenerating liver. The increase was maximum 24h after partial hepatectomy for all acceptors tested. At later times after operation the sialyltransferase activity remained high only for desialylated fetuin. No soluble factors from liver or serum of partially hepatectomized animals influenced the activity of the sialyltransferases bound to the microsomal fraction. The sensitivity of sialyltransferases to activation by Triton X-100, added to the incubation medium, was unchanged in the microsomal preparation from animals 24h after sham operation or partial hepatectomy. The full activity of sialyltransferases towards the various desialylated acceptors showed some differences. Human Tamm-Horsfall glycoprotein was a good acceptor of sialic acid only when desialylated by mild acid hydrolysis. After this treatment, but not after enzymic hydrolysis, a decrease in molecular weight of human Tamm-Horsfall glycoprotein was observed. Further, the sialyltransferase activity as a function of incubation temperature gave different curves according to the acceptor used. The relationship between the biosynthesis of glycoproteins by regenerating liver and the sialyltransferase activity of microsomal fraction after partial hepatectomy is discussed.

摘要

肝微粒体组分催化唾液酸从CMP-N-乙酰神经氨酸转移至各种外源性受体,如去唾液酸胎球蛋白、去唾液酸人Tamm-Horsfall糖蛋白和去唾液酸牛颌下腺粘蛋白。在再生肝中,经过一段延迟期(7小时)后,发现唾液酸掺入去唾液酸糖蛋白的速率增加。对于所有测试的受体,在部分肝切除术后24小时增加量最大。术后较晚时间,唾液酸转移酶活性仅对去唾液酸胎球蛋白保持较高水平。部分肝切除动物的肝脏或血清中的可溶性因子不影响与微粒体组分结合的唾液酸转移酶的活性。在假手术或部分肝切除术后24小时的动物微粒体制备物中,添加到孵育培养基中的Triton X-100对唾液酸转移酶的激活敏感性未发生变化。唾液酸转移酶对各种去唾液酸受体的完全活性存在一些差异。人Tamm-Horsfall糖蛋白仅在经温和酸水解去唾液酸后才是唾液酸的良好受体。经过这种处理后,但酶解后未观察到,人Tamm-Horsfall糖蛋白的分子量降低。此外,根据所用受体的不同,唾液酸转移酶活性作为孵育温度的函数给出不同的曲线。本文讨论了再生肝中糖蛋白的生物合成与部分肝切除后微粒体组分的唾液酸转移酶活性之间的关系。

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本文引用的文献

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