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胞外5'-核苷酸酶可提供丝裂原刺激的人T细胞和快速分裂的人B淋巴母细胞的全部嘌呤需求。

Ecto-5'-nucleotidase can provide the total purine requirements of mitogen-stimulated human T cells and rapidly dividing human B lymphoblastoid cells.

作者信息

Thompson L F

出版信息

J Immunol. 1985 Jun;134(6):3794-7.

PMID:2985697
Abstract

The ability of mitogen-stimulated human T cells or rapidly dividing human B lymphoblastoid cells to drive their total purine requirements from inosine 5'-monophosphate, inosine, or hypoxanthine was compared. Inosine 5'-monophosphate first must be converted to inosine by the action of the enzyme ecto-5'-nucleotidase before it can be transported into the cell; inosine and hypoxanthine, however, can be transported directly. Mitogen-stimulated human peripheral blood T cells were treated with aminopterin to inhibit purine synthesis de novo and to make the cells dependent on an exogenous purine source. Thymidine was added as a source of pyrimidines. Under these conditions, 30 microM inosine 5'-monophosphate, inosine, and hypoxanthine showed comparable abilities to support [3H]thymidine incorporation into DNA or [3H]leucine incorporation into protein at rates equal to that of untreated control cultures. Similar results were found when azaserine was used to inhibit purine synthesis de novo, and thus DNA synthesis. In parallel experiments with the rapidly dividing human B lymphoblastoid cell line WI-L2, treatment with aminopterin (plus thymidine) inhibited the growth rate by greater than 95%. The normal growth rate was restored by the addition of 30 microM inosine 5'-monophosphate, inosine, or hypoxanthine to the medium. However, in similar experiments with cell line 1254, a derivative of WI-L2 which lacks detectable ecto-5'-nucleotidase activity, inosine and hypoxanthine (plus thymidine), but not inosine 5'-monophosphate (and thymidine) were able to restore the growth inhibition due to aminopterin. These results show that the catalytic activity of ecto-5'-nucleotidase is sufficient to meet the total purine requirements of mitogen-stimulated human T cells or rapidly dividing human B lymphoblastoid cells, and suggest that this enzyme may be important for purine salvage when rates of purine synthesis de novo are limited and/or an extracellular source of purine nucleotides is available.

摘要

比较了丝裂原刺激的人T细胞或快速分裂的人B淋巴母细胞从5'-单磷酸肌苷、肌苷或次黄嘌呤满足其总嘌呤需求的能力。5'-单磷酸肌苷必须先通过ecto-5'-核苷酸酶的作用转化为肌苷,才能被转运到细胞内;而肌苷和次黄嘌呤则可以直接转运。用氨甲蝶呤处理丝裂原刺激的人外周血T细胞,以抑制嘌呤从头合成,使细胞依赖外源性嘌呤来源。添加胸苷作为嘧啶来源。在这些条件下,30微摩尔的5'-单磷酸肌苷、肌苷和次黄嘌呤在支持[3H]胸苷掺入DNA或[3H]亮氨酸掺入蛋白质方面表现出相当的能力,其速率与未处理的对照培养物相当。当用重氮丝氨酸抑制嘌呤从头合成从而抑制DNA合成时,也得到了类似的结果。在对快速分裂的人B淋巴母细胞系WI-L-2进行的平行实验中,用氨甲蝶呤(加胸苷)处理使生长速率降低了95%以上。向培养基中添加30微摩尔的5'-单磷酸肌苷、肌苷或次黄嘌呤可恢复正常生长速率。然而,在对WI-L-2的衍生物细胞系1254进行的类似实验中,该细胞系缺乏可检测到的ecto-5'-核苷酸酶活性,肌苷和次黄嘌呤(加胸苷)能够恢复因氨甲蝶呤导致的生长抑制,而5'-单磷酸肌苷(和胸苷)则不能。这些结果表明,ecto-5'-核苷酸酶的催化活性足以满足丝裂原刺激的人T细胞或快速分裂的人B淋巴母细胞的总嘌呤需求,并表明当嘌呤从头合成速率有限和/或有细胞外嘌呤核苷酸来源时,该酶对于嘌呤补救可能很重要。

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