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作 者:戴克胜[1,2] 朱振宇[1,2] 马涧泉[1,2]
机构地区:[1]中山医科大学生化教研室 [2]蚌埠医学院医检系
出 处:《中华微生物学和免疫学杂志》1998年第2期120-123,共4页Chinese Journal of Microbiology and Immunology
基 金:国家教委博士点基金
摘 要:目的EB病毒BHRF1基因克隆,其表达产物抑制CHO细胞凋亡功能的研究。方法以B95-8细胞株EBVDNA为模板设计一对引物,采用PCR技术扩增BHRF1基因,用目的基因内的两个单酶切点BamHⅠ、BglⅠ进行酶切鉴定。用引物上所引入的两个酶切位点NcoⅠ、SclⅠ酶切目的基因后定向连接到pBV221载体上,转入宿主菌DH5α经质粒抽提,单、双酶切鉴定,从所获克隆中筛选重组质粒克隆。温控诱导目的基因表达,SDS-PAGE及凝胶薄层扫描分析。采用缺血清培养方法建立CHO细胞凋亡模型。结果所得扩增产物长592bp与预期大小一致;筛选出的9个重组质粒克隆经SDS-PAGE和扫描表明重组蛋白表达量占菌体蛋白总量的2.5%。将含重组蛋白的菌体蛋白加入缺血清培养体系,通过与空白菌体蛋白对照表明,重组蛋白具有明显的抑制CHO细胞凋亡的能力。结论BHRF1蛋白具有有效控制血清缺乏所诱导的CHO细胞凋亡功能,这为BHRF1蛋白的广泛应用提供了依据。The BHRF1 gene was amplified from template DNA of B958 cell by polymerase chain reaction.The amplified fragment was about 592bp in length,and was identified with the method of digestion with two unique restriction endonucleases.PCRamplified fragment and plasmid pBV221 were restricted with NcoⅠ puls SalⅠ,and were orientally ligated by T4 DNA ligase. E.coli DH5α was transformed with recombinant plasmid.Nine positive recombinant colonies harbouring the inserted fragment were selected.The recombinant expressing plasmid was induced to expression.SDSPAGE assay showed that a 170kD protein was expressed as expected and the amount of this protein expressed was about 25% of the total bacterial proteins.CHO cells were cultured and induced apoptosis by being cultured with medium deficient in serum.Then,CHO cells were cultured in two kinds of serumdepleted media which were added by positive and negative strain proteins respectively for 72 hours.The results suggest that the recombinant protein has an effect of suppressing apoptosis.
分 类 号:R373.11[医药卫生—病原生物学]
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