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淋巴细胞产生的调节因子。II. 与抑制DNA聚合酶α活性的因子相关的细胞DNA合成抑制

Regulatory factors produced by lymphocytes. II. Inhibition of cellular DNA synthesis associated with a factor inhibiting DNA polymerase alpha activity.

作者信息

Lee S C, Lucas Z J

出版信息

J Immunol. 1977 Jan;118(1):88-97.

PMID:299764
Abstract

Supernatants of phytohemagglutinin-stimulated human tonsil cells contain two growth inhibitory factors. These factors, called inhibitors of DNA synthesis (IDS), reduce (3)H-thymidine incorporation into mitogen-stimulated lymphocytes and into growing HeLa cells. By Sephadex chromatography, these factors have volumes of distribution corresponding to about 80,000 and 40,000 daltons. Both factors inhibit the activity of calf thymus DNA polymerase alpha in cell-free assays (termed inhibitor of DNA polymerase, IDP). The larger factor, which is chromatographically separable from alpha-lymphotoxin (alpha-LT), is completely inactivated by heating at 70 degrees C for 15 min. This treatment does not destroy alpha-LT. Using supernatants from PHA-stimulated tonsil cells cultured for 5 days in serum-free medium, we attained a 150-fold purification with a succession of molecular sieving, ion exchange, and adsorption chromatographic procedures. Although not purified to homogeneity, the extensive copurification of IDS and IDP activities and their identical heat inactivation profiles suggest that they are the same entity. IDP separated free of alpha-LT inhibits thymidine incorporation into HeLa cells without causing cell death. alpha-LT purified free of IDS does not inhibit thymidine incorporation into HeLa cells, not even at concentrations 7000 times that necessary to kill 50% of growth-inhibited L cell cultures.

摘要

植物血凝素刺激的人扁桃体细胞的上清液中含有两种生长抑制因子。这些因子被称为DNA合成抑制剂(IDS),可减少(3)H-胸腺嘧啶核苷掺入有丝分裂原刺激的淋巴细胞和生长中的HeLa细胞。通过葡聚糖凝胶色谱法,这些因子的分布体积分别对应于约80,000和40,000道尔顿。在无细胞试验中,这两种因子均抑制小牛胸腺DNA聚合酶α的活性(称为DNA聚合酶抑制剂,IDP)。较大的因子在色谱上可与α-淋巴毒素(α-LT)分离,在70℃加热15分钟可使其完全失活。这种处理不会破坏α-LT。使用在无血清培养基中培养5天的PHA刺激的扁桃体细胞的上清液,我们通过一系列分子筛分、离子交换和吸附色谱程序实现了150倍的纯化。尽管未纯化至同质,但IDS和IDP活性的广泛共纯化及其相同的热失活曲线表明它们是同一实体。不含α-LT的IDP可抑制胸腺嘧啶核苷掺入HeLa细胞而不引起细胞死亡。不含IDS纯化的α-LT即使在杀死50%生长受抑制的L细胞培养物所需浓度的7000倍时,也不抑制胸腺嘧啶核苷掺入HeLa细胞。

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