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Tissue culture-induced DNA methylation variation in maize.

机译:组织培养诱导的玉米DNA甲基化变异。

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摘要

Twenty-one progeny lines derived from tissue cultures of two embryo sources of maize inbred strain A188 were examined for DNA methylation changes. Total DNA was cut with the isoschizomers Hpa II and Msp I and probed with 18 single-copy Pst I genomic clones and two cDNA clones. Eight of these probes could detect both increases and decreases in methylation. With these probes 39% of the families were found to contain an altered methylation pattern. All changes represented a decrease in methylation. The other 12 probes could detect only increases in methylation; no methylation variation was seen with these probes. Fifteen percent of the methylation changes were homozygous in the original regenerated plant. Changes were stably inherited upon two generations of self-pollination. No sequence variation was observed in Msp I-digested DNA from the same 21 progeny lines. Certain probes detected methylation changes much more often than others. Our study provides evidence that demethylation occurs at a high frequency and could be an important cause of tissue culture-induced variation. Occurrence of the frequent homozygous alterations in original regenerated plants implies a non-random mutational mechanism.
机译:检查了来自玉米自交系A188的两个胚胎来源的组织培养物中的二十一个后代系的DNA甲基化变化。用等分异构体Hpa II和Msp I切割总DNA,并用18个单拷贝Pst I基因组克隆和两个cDNA克隆进行探测。这些探针中的八个可以检测到甲基化的增加和减少。使用这些探针,发现39%的家族含有改变的甲基化模式。所有变化代表甲基化的减少。其他12个探针只能检测到甲基化的增加。这些探针未见甲基化变化。在原始的再生植物中,有15%的甲基化变化是纯合的。变化是两代自花传粉的稳定遗传。在来自相同21个后代系的Msp I消化的DNA中未观察到序列变异。某些探针检测到甲基化变化的频率要高于其他探针。我们的研究提供了证据,表明去甲基化的频率很高,并且可能是组织培养物诱导的变异的重要原因。在原始再生植物中频繁发生的纯合子改变暗示着一种非随机的突变机制。

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