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玉米中Mu转座因子的分子与遗传特征:在愈伤组织培养和再生植株中的行为

Molecular and genetic characterization of Mu transposable elements in Zea mays: behavior in callus culture and regenerated plants.

作者信息

Planckaert F, Walbot V

机构信息

Department of Biological Sciences, Stanford University, California 94305-5020.

出版信息

Genetics. 1989 Nov;123(3):567-78. doi: 10.1093/genetics/123.3.567.

Abstract

Active Mutator lines of maize (Zea mays L.) have a high mutation rate and contain multiple hypomethylated 1.4-kb and 1.7-kb Mu transposable elements. Correlated with the inactivation of the Mutator system, these Mu elements cease to transpose and become more methylated. To determine whether the shock of tissue culture can affect Mutator activities, F1 progenies of outcrosses between active or inactive Mutator stocks and inbred line A188 were used to initiate embryogenic callus cultures. HinfI restriction digestion of genomic DNA isolated from 3-5-month-old cultures demonstrated that there is a very good correlation between the modification state of Mu elements in the cultures and the Mutator parent. Despite the dedifferentiation and rapid proliferation characteristic of tissue culture, the Mutator activity state is relatively stable during an extended tissue culture period. Cultures established from inactive Mutator lines were not reactivated; cultures established from active lines maintained a high Mu copy number, and most Mu elements remained unmodified. In contrast, weakly active Mutator parents gave rise to cultures in which Mu element modification could switch between low and high methylation during the culture period. Evidence for transposition was investigated with EcoRI digestion of genomic DNA isolated at different times during culture. The appearance of novel Mu-hybridizing fragments and a strong background hybridization are interpreted as evidence that transposition events occur during culture. Plants regenerated from such active cultures transmitted Mutator activity to their progeny.

摘要

玉米(Zea mays L.)的活跃突变体系具有高突变率,并且包含多个低甲基化的1.4 kb和1.7 kb Mu转座元件。与突变体系的失活相关,这些Mu元件停止转座并变得更加甲基化。为了确定组织培养的刺激是否会影响突变体活性,将活跃或不活跃突变体库与自交系A188杂交的F1后代用于启动胚性愈伤组织培养。对从3至5个月大的培养物中分离的基因组DNA进行HinfI酶切分析表明,培养物中Mu元件的修饰状态与突变体亲本之间存在很好的相关性。尽管组织培养具有去分化和快速增殖的特性,但在延长的组织培养期内,突变体活性状态相对稳定。从不活跃突变体系建立的培养物没有重新激活;从活跃体系建立的培养物保持了较高的Mu拷贝数,并且大多数Mu元件仍未修饰。相比之下,弱活跃的突变体亲本产生的培养物中,Mu元件的修饰在培养期间可在低甲基化和高甲基化之间转换。通过对培养期间不同时间分离的基因组DNA进行EcoRI酶切来研究转座证据。新的Mu杂交片段的出现和强烈的背景杂交被解释为转座事件在培养期间发生的证据。从这种活跃培养物再生的植株将突变体活性传递给了它们的后代。

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