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豚鼠粒细胞中唾液酸的测定与定位

The determination and localization of sialic acid in guinea-pig granulocytes.

作者信息

DePierre J W, Lazdins J, Karnovsky M L

出版信息

Biochem J. 1980 Nov 15;192(2):543-50. doi: 10.1042/bj1920543.

Abstract

When intact guinea-pig granulocytes (polymorphonuclear leucocytes) disrupted by sonication or with detergent were treated with neuraminidase from Vibrio cholerae, 3.1--3.2 nmol of sialic acid/10(7) cells was released. By using a chromatographic procedure for the specific determination of total cell sialic acid, this releasable portion was found to constitute 70% of the total sialate. All of the neuraminidase-releasable sialic acid of the cells could be removed by enzymic treatment of intact cells with neuraminidase. It thus seemed likely that the neuraminidase-releasable sialic acid is all on the cell surface. To make sure that the result was not due to entry of neuraminidase into the cells, the enzyme was bound covalently to Sepharose 6B, and intact polymorphonuclear leucocytes were treated with the bound enzyme. All of the neuraminidase-releasable sialic acid could still be removed, though more slowly. The cells remained intact and only 1.5--2% of the bound enzyme was released from the Sepharose during incubation. Freed enzyme could have been responsible, at the very most, for release of 18% of the sialic acid. Fractionation studies showed that the nucleus and cytoplasm contain low amounts of sialic acid and that the neuraminidase-releasable sialic acid distributes in a manner similar to the distribution of 5'-nucleotidase, an unambiguous marker for the plasma membrane in these cells. Thus neuraminidase-releasable sialate constitutes a clear marker for the membrane of polymorphonuclear leucocytes. Most of the neuraminidase-insensitive sialate was present in the granule fraction. Removal of sialic acid from intact polymorphonuclear leucocytes did not affect their ecto-AMPase, -ATPase and -p-nitrophenyl phosphatase activities.

摘要

当用超声处理或用去污剂破坏豚鼠完整的粒细胞(多形核白细胞)后,用霍乱弧菌的神经氨酸酶处理,每10⁷个细胞可释放出3.1 - 3.2 nmol的唾液酸。通过使用一种用于特异性测定总细胞唾液酸的色谱方法,发现这一可释放部分占总唾液酸的70%。用神经氨酸酶对完整细胞进行酶处理,可以去除细胞中所有可被神经氨酸酶释放的唾液酸。因此,似乎可被神经氨酸酶释放的唾液酸都在细胞表面。为确保结果不是由于神经氨酸酶进入细胞所致,将该酶共价结合到琼脂糖6B上,并用结合的酶处理完整的多形核白细胞。所有可被神经氨酸酶释放的唾液酸仍然可以被去除,只是速度较慢。细胞保持完整,在孵育过程中,只有1.5 - 2%的结合酶从琼脂糖中释放出来。最多只有18%的唾液酸释放可能是由游离酶造成的。分级分离研究表明,细胞核和细胞质中唾液酸含量较低,可被神经氨酸酶释放的唾液酸的分布方式与5'-核苷酸酶(这些细胞中质膜的明确标记物)的分布相似。因此,可被神经氨酸酶释放的唾液酸是多形核白细胞膜的一个明确标记物。大部分对神经氨酸酶不敏感的唾液酸存在于颗粒部分。从完整的多形核白细胞中去除唾液酸并不影响其胞外腺苷酸酶、ATP酶和对硝基苯磷酸酶的活性。

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本文引用的文献

1
Metabolic basis of phagocytic activity.吞噬活性的代谢基础。
Physiol Rev. 1962 Jan;42:143-68. doi: 10.1152/physrev.1962.42.1.143.
2
4
The surface structure of erythrocytes from some animal sources.一些动物来源的红细胞的表面结构。
Arch Biochem Biophys. 1963 Mar;100:493-502. doi: 10.1016/0003-9861(63)90117-6.

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