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一般描述
原癌基因fos与细胞的生长,分化和发育有关。Fos是由大量刺激物诱导的,包括有丝分裂原,分化特异性药物,药理药物等。62,000道尔顿fos蛋白的诱导是快速但短暂的。fos蛋白与39,000道尔顿蛋白相关,该蛋白已被鉴定为jun原癌基因(c-jun)的蛋白产物。Fos/Jun蛋白复合物与DNA中称为AP-1结合位点的序列元件特异性结合。
可识别HepG2、NIH3T3和MCF-7细胞中的~50-62 kDa c-Fos蛋白。
蛋白A纯化的兔多克隆抗体。可识别v-fos和~50-62 kDa c-fos蛋白。
该抗c-Fos(Ab-2)(4-17)兔pAb经验证可用于冰冻切片、免疫印迹、IF、IP、石蜡切片,以检测c-Fos(Ab-2)(4-17)。
免疫原
人
对应于人c-Fos氨基酸4-17的合成肽(SGFNADYEASSSRC)(目录号PP10)
应用
冰冻切片(5-10 µg/ml)
免疫印迹(1-5 µg/ml)
免疫荧光(1-5 µg/ml)
免疫沉淀(1-2 µg/反应)
石蜡切片(5-10 µg/ml,需要胃蛋白酶或加热预处理)
自由浮动切片(不建议使用)
免疫印迹(1-5 µg/ml)
免疫荧光(1-5 µg/ml)
免疫沉淀(1-2 µg/反应)
石蜡切片(5-10 µg/ml,需要胃蛋白酶或加热预处理)
自由浮动切片(不建议使用)
包装
请参考特定浓度批号的标签。
警告
毒性:高毒性(H)
外形
溶于0.05 M磷酸钠缓冲液,含0.2%明胶。
分析说明
阳性对照
HepG2、NIH 3T3细胞、MCF-7细胞、结肠或乳腺腺癌组织
HepG2、NIH 3T3细胞、MCF-7细胞、结肠或乳腺腺癌组织
其他说明
DeTogni, P., et al. 1988.Cell Biol.8, 2251.
Rouscher III, F.J., et al. 1988.Science240, 1010.
Sassone-Corsi, P., et al. 1988.Cell54, 553.
Verma, I.M. and Graham, W.R.1987.Cancer Res.49, 29.
Verma, I.M. and Sassone-Corsi, P. 1987.Cell51, 513.
Muller, R. 1986.Biochim.Biophys.Acta823, 207.
Verma, I. 1986.Trends Genet.2, 93.
Greenberg, M. and Ziff, E. 1984.Nature (London), 311, 433.
Rouscher III, F.J., et al. 1988.Science240, 1010.
Sassone-Corsi, P., et al. 1988.Cell54, 553.
Verma, I.M. and Graham, W.R.1987.Cancer Res.49, 29.
Verma, I.M. and Sassone-Corsi, P. 1987.Cell51, 513.
Muller, R. 1986.Biochim.Biophys.Acta823, 207.
Verma, I. 1986.Trends Genet.2, 93.
Greenberg, M. and Ziff, E. 1984.Nature (London), 311, 433.
对于凝胶阻滞分析,使用目录编号PC05L重悬于100 µl缓冲液中。免疫原,c-fos(肽-2),目录编号PP10也可用于竞争研究(请参见下面的Murphy等人)。在单个系统中,应对抗体进行滴定以获得最佳结果。
法律信息
CALBIOCHEM is a registered trademark of Merck KGaA, Darmstadt, Germany
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储存分类代码
10 - Combustible liquids
WGK
nwg
法规信息
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