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人乳腺癌细胞的催乳素合成与分泌

Prolactin synthesis and secretion by human breast cancer cells.

作者信息

Ginsburg E, Vonderhaar B K

机构信息

Laboratory of Tumor Immunology and Biology, National Cancer Institute, NIH, Bethesda, Maryland 20892-1402, USA.

出版信息

Cancer Res. 1995 Jun 15;55(12):2591-5.

PMID:7780973
Abstract

A possible autocrine function of prolactin (Prl) in human breast cancer was explored by the addition of a panel of anti-human Prl mAbs to T47Dco and MCF7 human breast adenocarcinoma cells. mAb 631 and mAb 390 inhibited cell growth by 86 and 68%, respectively, in the estrogen receptor-negative T47Dco cells and by 20 and 71%, respectively, in the estrogen receptor-positive MCF7 cells. Conditioned medium prepared from T47Dco cells was assessed for the presence of Prl-like molecules by its ability to stimulate growth of Prl-responsive Nb2 rat lymphoma cells. Growth of Nb2 cells under the influence of human Prl or conditioned medium was abolished when either solution was pretreated with mAb 390, followed by Immunobead precipitation (Bio-Rad, Melville, NY). T47Dco cells secrete 0.7 microgram lactogen/ml over a 24-48-h period. With the use of reverse transcription-PCR, an expected 612-bp band was detected by ethidium bromide staining, and its similarity to pituitary Prl was confirmed by Southern blot analysis with the use of human Prl cDNA as a probe. A single M(r) 22,000 band, the dominant size of monomeric pituitary Prl, was found in immunoprecipitates of both cell extracts and conditioned medium from T47Dco cells labeled metabolically with [35S]cysteine. These data suggest that human breast cancer cells synthesize and secrete biologically active Prl.

摘要

通过向T47Dco和MCF7人乳腺腺癌细胞中添加一组抗人催乳素(Prl)单克隆抗体,探讨了催乳素(Prl)在人乳腺癌中可能的自分泌功能。在雌激素受体阴性的T47Dco细胞中,单克隆抗体631和单克隆抗体390分别将细胞生长抑制了86%和68%;在雌激素受体阳性的MCF7细胞中,分别抑制了20%和71%。通过其刺激Prl反应性Nb2大鼠淋巴瘤细胞生长的能力,评估了从T47Dco细胞制备的条件培养基中是否存在Prl样分子。当用单克隆抗体390预处理人Prl或条件培养基中的任何一种溶液,然后进行免疫珠沉淀(Bio-Rad,梅尔维尔,纽约)时,Nb2细胞在人Prl或条件培养基影响下的生长被消除。T47Dco细胞在24至48小时内分泌0.7微克催乳素/毫升。使用逆转录聚合酶链反应,通过溴化乙锭染色检测到预期的612碱基对条带,并通过使用人Prl cDNA作为探针的Southern印迹分析证实其与垂体Prl的相似性。在用[35S]半胱氨酸进行代谢标记的T47Dco细胞的细胞提取物和条件培养基的免疫沉淀物中,发现了一条单一的M(r)22,000条带,这是单体垂体Prl的主要大小。这些数据表明人乳腺癌细胞合成并分泌具有生物活性的Prl。

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