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凝集素激活对人淋巴细胞唾液酸转移酶活性的影响。

Effects of lectin activation on sialyltransferase activities in human lymphocytes.

作者信息

Basu S K, Whisler R L, Yates A J

出版信息

Biochemistry. 1986 May 6;25(9):2577-81. doi: 10.1021/bi00357a044.

DOI:10.1021/bi00357a044
PMID:3718965
Abstract

The effects of phytohemagglutinin (PHA) stimulation on the activities of sialyltransferase 1 (SAT-1), and sialyltransferase 3 (SAT-3), in human lymphocytes were investigated in vitro. For SAT-1 and SAT-3, respectively, the apparent Km values with variable CMP-NeuAc concentrations were 0.19 and 0.015 mM and with variable LacCer were 0.075 and 0.17 mM. Progressive increases in the activities of SAT-1 and SAT-3 were detected in lymphocytes stimulated with PHA, whereas no increase was observed in control lymphocytes incubated in culture medium alone. These increased activities occurred within 18-36 h of incubation and preceded optimum lymphocyte proliferation. Intact lymphocytes were needed for the lectin-stimulated increase of sialyltransferase activities because neither concanavalin A nor phytohemagglutinin added to the broken cell preparation modulated SAT-1 activity. The glycolipid products formed as a result of these enzymatic reactions in the presence of endogenous and exogenous acceptors were tentatively identified by thin-layer chromatography and autofluorography. The addition of exogenous LacCer to the SAT-1 assay resulted in the radiolabeling of a small amount of ganglioside GM1b (3.4%), but GM3 was the major labeled product (96%). When GgOse4Cer was added to the SAT-3 assay, 32% GM3 and 24.6% GM1b were detected while 44% consisted of glycolipids not labeled in assays performed without exogenous acceptors. Of the radioactivity transferred to endogenous acceptors, 81.3% was in GM3 and 14.6% in GM1b. These results demonstrate that the modulation of sialyltransferase activity occurs earlier than cellular activation.

摘要

在体外研究了植物血凝素(PHA)刺激对人淋巴细胞中唾液酸转移酶1(SAT-1)和唾液酸转移酶3(SAT-3)活性的影响。对于SAT-1和SAT-3,在CMP-神经氨酸浓度可变时,其表观Km值分别为0.19和0.015 mM,在乳糖神经酰胺浓度可变时,其表观Km值分别为0.075和0.17 mM。在用PHA刺激的淋巴细胞中检测到SAT-1和SAT-3的活性逐渐增加,而在仅在培养基中孵育的对照淋巴细胞中未观察到增加。这些增加的活性在孵育18 - 36小时内出现,并先于最佳淋巴细胞增殖。凝集素刺激的唾液酸转移酶活性增加需要完整的淋巴细胞,因为添加到破碎细胞制剂中的刀豆球蛋白A和植物血凝素均未调节SAT-1活性。通过薄层色谱和放射自显影初步鉴定了在内源性和外源性受体存在下这些酶促反应形成的糖脂产物。向SAT-1测定中添加外源性乳糖神经酰胺导致少量神经节苷脂GM1b(3.4%)被放射性标记,但GM3是主要的标记产物(96%)。当向SAT-3测定中添加GgOse4Cer时,检测到32%的GM3和24.6%的GM1b,而44%由在没有外源性受体的测定中未被标记的糖脂组成。转移到内源性受体的放射性中,81.3%存在于GM3中,14.6%存在于GM1b中。这些结果表明唾液酸转移酶活性的调节比细胞活化更早发生。

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