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建立了能表达基因重组NT 3的中国仓鼠卵巢 (CHO)细胞系 ;通过Southernblot分析表明克隆细胞染色体中有明显的NT 3基因插入 ;用DotELISA和Westernblot实验证实了目的蛋白的表达及其分子量约为 1 4ku .利用EIA方法测定了阳性细胞株表达NT 3的量平均为 2 1 0 0ng/( 1 0 6细胞·48h) ;rNT 3可促进鸡E8背根神经节神经突起生长 ,其长度与rNT 3浓度有明显的量效关系 ;rNT 3的EC5 0 值为 1 6 .7ng/mL ;单克隆抗体 3W3可中和所表达的rNT 3的生物活性 .  相似文献   
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The CHO cell line stably producing recombinant rat NT-3 was established. The insertion of rNT-3 cDNA into transferred cell gonome was analyzed with Southern blot. The expressed protein was identified by Dot ELISA (enzyme-linked immunosorbent assay) and Western blot. Western blot showed a clear specifie band of about 14 ku for NT-3. The mean level of rNT-3 in four NT-3eDNA/CHO cell lines was about 2 100 ng/10~6 cells/48 h determined by EIA. The conditioned-medium (CM) of NT-3cDNA/CHO cells could promote the fiber outgrowth of the dissociated dorsal root ganglion of 8-day-old chick embryos, which shows a dose-response relationship. A half-maximal concentration of the biological activity (EC50) of the recombinant protein was approximately 16.7 ng/mL. The MoAb 3W3 of NT-3 could neutralize the biological activity of the rNT-3.  相似文献   
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