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作 者:王燕妮[1] 肖谷田[2] 毕惠祥 李明 金丽娟 李英杰 谢毅[2]
机构地区:[1]遵义医学院免疫学教研室,遵义563003 [2]复旦大学遗传工程国家重点实验室,上海200433 [3]第一军医大学疟疾免疫研究室,广州510515
出 处:《中国寄生虫学与寄生虫病杂志》1997年第1期21-25,共5页Chinese Journal of Parasitology and Parasitic Diseases
基 金:上海青年科技启明星计划资助
摘 要:目的 :构建恶性疟原虫 c DNA表达文库。方法 :采用“一步法”提取红内期恶性疟原虫12 2 4 μg RNA,经 Oligo( d T)纤维素柱纯化得到 35.84 μg poly ( A) +m RNA。取 10 μg m RNA反转录得到 1.75μg平端双链 c DNA,与含 Eco RI,Not I,Sal I酶切位点的衔接头连接后 ,经分级分离柱纯化回收到 2 0 0 ng大小主要在 50 0 bp- 7kb左右的 c DNA片段。取 50 ng c DNA与λgt11噬菌体臂连接后体外包装 ,完成建库。并采用 PCR方法初步鉴定该文库。结果 :已构建一个含 10 6个重组子的 c DNA表达文库。结论 :文库容量及插入 c DNA片段的大小适合于进一步研究。AIM:To construct a c DNA expression library from erythrocytic Plasmodium falci- parum(FCC/HN) .METHODS:1 2 2 4μg total RNA and35 .84μg poly(A) +m RNA have been successively obtained from the blood- stage Plasmodium falciparum mainly consisting of trophozoites using“single- step method”and by chromatography on oligo- (d T) cellulose. With the reverse transcriptase(M- MLV) ,1 0 μg m RNA was synthesized into1 .75 μg blunt c DNA.After the c DNA was ligated to Eco R I(Not I,Sal I) adapter and purified by fraction- ation,2 0 0 ng c DNA of about5 0 0 bp- 7kb was collected.Of which5 0 ng c DNA was ligated intoλgt1 1 phage particles and was packaged with the packagen extract system in vitro. This library was characterized primarily by PCR.RESUL TS:A c DNA library containing1 0 6re- combinants has been constructed.CONCLUSION:The capacity of this library and the size of c DNA is suitable for further study.
分 类 号:R382.31[医药卫生—医学寄生虫学]
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