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利用转座的P因子构建具有明确端点的果蝇缺失突变体并进行特性分析。

Construction and characterization of deletions with defined end points in Drosophila using P elements in trans.

作者信息

Paré Adam C, Dean Derek M, Ewer John

机构信息

Entomology Department, Cornell University, Ithaca, New York 14853, USA.

出版信息

Genetics. 2009 Jan;181(1):53-63. doi: 10.1534/genetics.108.094193. Epub 2008 Nov 3.

Abstract

We used P-element transposase-mediated "male recombination" between two P elements in trans to create genetic deletions that removed a number of loci, including the gene encoding the neuropeptide crustacean cardioactive peptide (CCAP). Two classes of recombinant chromosomes were produced. Approximately one-quarter were viable when homozygous or hemizygous, whereas the remaining lines caused homozygous and hemizygous lethality. Preliminary analyses using PCR and CCAP immunohistochemistry suggested that, whereas the DNA of the viable lines was largely intact, most lethal lines contained chromosomal deletions that were roughly bounded by the insertion sites of the two P elements used. Southern blot analyses of select lethal lines showed that the DNA flanking the deletion was indeed grossly intact whereas the intervening DNA could not be detected. Sequencing across the deletion in three of these lethal lines identified a single line bearing intact genomic DNA on either side of the deletion separated by 30 bp of P-element DNA. The method described here suggests a simple procedure for creating deletions with defined end points. Importantly, it can use preexisting P-element insertion strains and does not rely on the use of transposable elements that are engineered to cause specific DNA rearrangements.

摘要

我们利用P因子转座酶介导的反式排列的两个P因子之间的“雄性重组”来产生基因缺失,这些缺失去除了多个基因座,包括编码神经肽甲壳动物心脏活性肽(CCAP)的基因。产生了两类重组染色体。大约四分之一在纯合或半合状态下是存活的,而其余的品系则导致纯合和半合致死。使用PCR和CCAP免疫组织化学的初步分析表明,虽然存活品系的DNA基本完整,但大多数致死品系含有染色体缺失,这些缺失大致由所用的两个P因子的插入位点界定。对选定致死品系的Southern印迹分析表明,缺失侧翼的DNA确实基本完整,而中间的DNA无法检测到。对其中三个致死品系的缺失区域进行测序,确定了一个品系,其缺失两侧的基因组DNA完整,中间由30 bp的P因子DNA隔开。这里描述的方法提出了一种创建具有确定端点的缺失的简单程序。重要的是,它可以使用预先存在的P因子插入菌株,并且不依赖于使用经过工程改造以引起特定DNA重排的转座元件。

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