Cogoni C, Irelan J T, Schumacher M, Schmidhauser T J, Selker E U, Macino G
Dipartimento di Biopatologia Umana, Sezione di Biologia Cellulare, Policlinico Umberto 1, Università di Roma La Sapienza, Italy.
EMBO J. 1996 Jun 17;15(12):3153-63.
The molecular mechanisms involved in transgene-induced gene silencing ('quelling') in Neurospora crassa were investigated using the carotenoid biosynthetic gene albino-1 (al-1) as a visual marker. Deletion derivatives of the al-1 gene showed that a transgene must contain at least approximately 132 bp of sequences homologous to the transcribed region of the native gene in order to induce quelling. Transgenes containing only al-1 promoter sequences do not cause quelling. Specific sequences are not required for gene silencing, as different regions of the al-1 gene produced quelling. A mutant defective in cytosine methylation (dim-2) exhibited normal frequencies and degrees of silencing, indicating that cytosine methylation is not responsible for quelling, despite the fact that methylation of transgene sequences frequently is correlated with silencing. Silencing was shown to be a dominant trait, operative in heterokaryotic strains containing a mixture of transgenic and non-transgenic nuclei. This result indicates that a diffusable, trans-acting molecule is involved in quelling. A transgene-derived, sense RNA was detected in quelled strains and was found to be absent in their revertants. These data are consistent with a model in which an RNA-DNA or RNA-RNA interaction is involved in transgene-induced gene silencing in Neurospora.
利用类胡萝卜素生物合成基因白化-1(al-1)作为视觉标记,研究了粗糙脉孢菌中转基因诱导的基因沉默(“抑制”)所涉及的分子机制。al-1基因的缺失衍生物表明,转基因必须包含至少约132 bp与天然基因转录区域同源的序列,才能诱导抑制。仅包含al-1启动子序列的转基因不会引起抑制。基因沉默不需要特定序列,因为al-1基因的不同区域都能产生抑制。一个胞嘧啶甲基化缺陷的突变体(dim-2)表现出正常的沉默频率和程度,这表明胞嘧啶甲基化与抑制无关,尽管转基因序列的甲基化经常与沉默相关。抑制被证明是一种显性性状,在含有转基因和非转基因核混合物的异核体菌株中起作用。这一结果表明,一种可扩散的反式作用分子参与了抑制。在被抑制的菌株中检测到了转基因来源的正义RNA,而在其回复突变体中未发现。这些数据与一个模型一致,即RNA-DNA或RNA-RNA相互作用参与了粗糙脉孢菌中转基因诱导的基因沉默。
