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一种高频生产重组杆状病毒表达载体的方法。

A method for producing recombinant baculovirus expression vectors at high frequency.

作者信息

Kitts P A, Possee R D

机构信息

NERC Institute of Virology and Environmental Microbiology, Oxford, UK.

出版信息

Biotechniques. 1993 May;14(5):810-7.

PMID:8512707
Abstract

A system has been developed that can generate recombinant baculovirus expression vectors at frequencies approaching 100%. This system provides a selection for recombinant viruses by using the essential gene downstream of the Autographa californica nuclear polyhedrosis virus (AcMNPV) polyhedrin expression locus. Two AcMNPV derivatives were constructed in which the expression locus and part of the downstream gene are flanked by restriction sites. The parental viruses are viable; however, restriction of the viral DNAs removes an essential piece of the viral genome. Transfer vectors carry a copy of the missing sequences downstream from the site into which foreign genes are inserted for expression; hence, recombination between a transfer vector and the restricted viral DNA can restore the integrity of the essential gene. Such recombination events also transfer any foreign gene present in the expression locus of the transfer vector to the viral genome. Recombinant viruses therefore have a selective advantage over nonrecombinant viral DNAs. Consequently, a high proportion of the viruses obtained by co-transfecting transfer vector DNA and restricted viral DNA of one of these new viruses expresses the target gene from the transfer vector. This system greatly reduces the time needed to make recombinant baculovirus expression vectors.

摘要

已经开发出一种系统,该系统能够以接近100%的频率产生重组杆状病毒表达载体。该系统通过利用苜蓿银纹夜蛾核型多角体病毒(AcMNPV)多角体蛋白表达位点下游的必需基因来筛选重组病毒。构建了两种AcMNPV衍生物,其中表达位点和部分下游基因两侧为限制性酶切位点。亲本病毒是有活力的;然而,对病毒DNA的酶切会去除病毒基因组的一个必需片段。转移载体携带缺失序列的一个拷贝,该序列位于插入外源基因进行表达的位点下游;因此,转移载体与经酶切的病毒DNA之间的重组可以恢复必需基因的完整性。这种重组事件还会将转移载体表达位点中存在的任何外源基因转移到病毒基因组中。因此,重组病毒相对于非重组病毒DNA具有选择优势。因此,通过共转染转移载体DNA和这些新病毒之一的经酶切的病毒DNA获得的病毒中,很大一部分表达来自转移载体的靶基因。该系统大大减少了制备重组杆状病毒表达载体所需的时间。

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