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在HeLa细胞复制周期中核苷摄取的波动以及核苷转运抑制剂硝基苄硫基肌苷的结合情况。

Fluctuations in nucleoside uptake and binding of the inhibitor of nucleoside transport, nitrobenzylthioinosine, during the replication cycle of HeLa cells.

作者信息

Cass C E, Dahlig E, Lau E Y, Lynch T P, Paterson A R

出版信息

Cancer Res. 1979 Apr;39(4):1245-52.

PMID:421208
Abstract

Binding of the potent nucleoside transport inhibitor 6-[(4-nitrobenzyl)thio]-9-beta-D-ribofuranosylpurine (NBMPR) and rates of uptake of several nucleosides were examined at 4-hr intervals during the replication cycle of HeLa S3 cells. Monolayer cultures of synchronous cells, obtained by mitotic detachment, were assayed for high-affinity binding of NBMPR and for rates of uptake of thymidine, uridine, cytidine, adenosine, inosine, and guanosine. The number of NBMPR binding sites per cell doubled between 4 and 16 hr after detachment (late G1 and S phase); during this interval, V max 'S for uptake of cytidine and adenosine doubled, and for uridine and thymidine uptake increased about 4- and 8-fold, respectively. Rates of inosine and guanosine uptake at extracellular concentrations below saturation increased 2-fold between G1 and S phase of the cell cycle. Km 'S for cellular uptake of thymidine, uridine, cytidine, and adenosine did not change with progress through the cycle. The results presented suggest that changes in nucleoside uptake during the HeLa cell cycle were due, in part, to changes in the activity of NBMPR-sensitive transport elements in the membrane.

摘要

在HeLa S3细胞的复制周期中,每隔4小时检测一次强效核苷转运抑制剂6-[(4-硝基苄基)硫代]-9-β-D-呋喃核糖基嘌呤(NBMPR)的结合情况以及几种核苷的摄取速率。通过有丝分裂分离获得的同步细胞单层培养物,用于检测NBMPR的高亲和力结合以及胸苷、尿苷、胞苷、腺苷、肌苷和鸟苷的摄取速率。每个细胞的NBMPR结合位点数量在分离后4至16小时(G1晚期和S期)之间增加了一倍;在此期间,胞苷和腺苷摄取的Vmax增加了一倍,尿苷和胸苷摄取分别增加了约4倍和8倍。在细胞周期的G1期和S期之间,细胞外浓度低于饱和时的肌苷和鸟苷摄取速率增加了2倍。细胞摄取胸苷、尿苷、胞苷和腺苷的Km值在整个周期中没有变化。呈现的结果表明,HeLa细胞周期中核苷摄取的变化部分归因于膜中NBMPR敏感转运元件活性的变化。

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