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体外培养的鳞状癌细胞系对甲状旁腺激素相关蛋白生成的调控

Regulation of parathyroid hormone-related protein production by a squamous carcinoma cell line in vitro.

作者信息

Merryman J I, Capen C C, McCauley L K, Werkmeister J R, Suter M M, Rosol T J

机构信息

Department of Veterinary Pathobiology, Ohio State University College of Veterinary Medicine, Columbus.

出版信息

Lab Invest. 1993 Sep;69(3):347-54.

PMID:8377475
Abstract

BACKGROUND

Humoral hypercalcemia of malignancy is a paraneoplastic syndrome associated with a variety of solid neoplasms including squamous cell carcinomas of various sites. Parathyroid hormone-related protein (PTHrP) is a newly recognized hormone that has been implicated as one of the major causative factors in the pathogenesis of this syndrome. A canine oral squamous carcinoma cell line (SCC 2/88) was used to investigate the regulation of production of PTHrP in response to agents that alter keratinocyte differentiation/proliferation in vitro.

EXPERIMENTAL DESIGN

SCC 2/88 cells grown in serum-free media were exposed to various factors and PTHrP production was measured by radioimmunoassay. This cell line spontaneously produced substantial amounts of PTHrP (up to 7,000 pg/ml) without the need for a fibroblast-feeder layer. Production of PTHrP decreased at cellular confluence, and with increasing passage number.

RESULTS

Epidermal growth factor, cholera toxin, calcium, 1,25-dihydroxyvitamin D, ionomycin, trans-retinoic acid, transforming growth factor-beta 1 and hydrocortisone stimulated production of PTHrP by SCC 2/88 cells to various degrees. Transforming growth factor-beta 1 was the most potent stimulator of PTHrP production, with a maximal stimulation of 25-fold over control. Monensin decreased PTHrP secretion as early as 6 hours post-treatment and by 48 hours, there was no detectable PTHrP in the conditioned cell culture medium. Calcium, cholera toxin, ionomycin, and transforming growth factor-beta 1 decreased keratinocyte proliferation as measured by cell counts at all doses tested.

CONCLUSIONS

The results of this study revealed that SCC 2/88 cells spontaneously produced substantial amounts of PTHrP under baseline conditions and that compounds known to affect keratinocyte differentiation/proliferation up-regulated production of PTHrP. These cells will be valuable to investigate the molecular regulation of PTHrP production by squamous cell carcinomas.

摘要

背景

恶性肿瘤体液性高钙血症是一种副肿瘤综合征,与多种实体瘤相关,包括不同部位的鳞状细胞癌。甲状旁腺激素相关蛋白(PTHrP)是一种新发现的激素,被认为是该综合征发病机制中的主要致病因素之一。使用犬口腔鳞状癌细胞系(SCC 2/88)在体外研究改变角质形成细胞分化/增殖的因子对PTHrP产生的调节作用。

实验设计

将在无血清培养基中生长的SCC 2/88细胞暴露于各种因子,通过放射免疫测定法测量PTHrP的产生。该细胞系在无需成纤维细胞饲养层的情况下自发产生大量PTHrP(高达7000 pg/ml)。PTHrP的产生在细胞汇合时以及传代次数增加时减少。

结果

表皮生长因子、霍乱毒素、钙、1,25 - 二羟维生素D、离子霉素、全反式维甲酸、转化生长因子 - β1和氢化可的松不同程度地刺激SCC 2/88细胞产生PTHrP。转化生长因子 - β1是PTHrP产生的最有效刺激物,最大刺激比对照高25倍。莫能菌素在处理后6小时就降低了PTHrP的分泌,到48小时时,条件性细胞培养基中检测不到PTHrP。在所有测试剂量下,通过细胞计数测量,钙、霍乱毒素、离子霉素和转化生长因子 - β1均降低了角质形成细胞的增殖。

结论

本研究结果表明,SCC 2/88细胞在基线条件下自发产生大量PTHrP,已知影响角质形成细胞分化/增殖的化合物上调了PTHrP的产生。这些细胞对于研究鳞状细胞癌产生PTHrP的分子调节将具有重要价值。

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