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影响Mos1水手转座子体外进化和转座的顺式和反式因子及其在功能基因组学中的潜力。

cis and trans factors affecting Mos1 mariner evolution and transposition in vitro, and its potential for functional genomics.

作者信息

Tosi L R, Beverley S M

机构信息

Department of Molecular Microbiology, Washington University Medical School, 660 South Euclid Avenue, St Louis, MO 63110, USA.

出版信息

Nucleic Acids Res. 2000 Feb 1;28(3):784-90. doi: 10.1093/nar/28.3.784.

Abstract

Mos1 and other mariner / Tc1 transposons move horizon-tally during evolution, and when transplanted into heterologous species can transpose in organisms ranging from prokaryotes to protozoans and vertebrates. To further develop the Drosophila Mos1 mariner system as a genetic tool and to probe mechanisms affecting the regulation of transposition activity, we developed an in vitro system for Mos1 transposition using purified transposase and selectable Mos1 derivatives. Transposition frequencies of nearly 10(-3)/target DNA molecule were obtained, and insertions occurred at TA dinucleotides with little other sequence specificity. Mos1 elements containing only the 28 bp terminal inverted repeats were inactive in vitro, while elements containing a few additional internal bases were fully active, establishing the minimal cis -acting requirements for transposition. With increasing transposase the transposition frequency increased to a plateau value, in contrast to the predictions of the protein over-expression inhibition model and to that found recently with a reconstructed Himar1 transposase. This difference between the 'natural' Mos1 and 'reconstructed' Himar1 transposases suggests an evolutionary path for down-regulation of mariner transposition following its introduction into a naïve population. The establishment of the cis and trans requirements for optimal mariner transposition in vitro provides key data for the creation of vectors for in vitro mutagenesis, and will facilitate the development of in vivo systems for mariner transposition.

摘要

Mos1及其他水手座/Tc1转座子在进化过程中进行水平转移,当被移植到异源物种中时,可在从原核生物到原生动物及脊椎动物等多种生物体中发生转座。为了进一步将果蝇Mos1水手座系统开发成一种遗传工具,并探究影响转座活性调控的机制,我们利用纯化的转座酶和可选择的Mos1衍生物开发了一种用于Mos1转座的体外系统。获得了接近10^(-3)/靶DNA分子的转座频率,并且插入发生在TA二核苷酸处,几乎没有其他序列特异性。仅含有28 bp末端反向重复序列的Mos1元件在体外无活性,而含有一些额外内部碱基的元件则完全有活性,从而确定了转座所需的最小顺式作用元件。随着转座酶浓度增加,转座频率增加至一个平稳值,这与蛋白质过表达抑制模型的预测相反,也与最近在重构的Himar1转座酶中发现的情况不同。“天然”Mos1转座酶与“重构”Himar1转座酶之间的这种差异暗示了水手座转座子引入新群体后其转座下调的一种进化途径。体外确定水手座最佳转座的顺式和反式作用元件要求,为创建体外诱变载体提供了关键数据,并将促进水手座转座体内系统的开发。

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