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经5-氮杂胞苷处理后转基因拟南芥中Ac转座元件的体细胞切除

Somatic excision of the Ac transposable element in transgenic Arabidopsis thaliana after 5-azacytidine treatment.

作者信息

Scortecci K C, Dessaux Y, Petit A, Van Sluys M A

机构信息

Depto. de Botânica-IBUSP, C.P. 11461, São Paulo/SP, Brazil.

出版信息

Plant Cell Physiol. 1997 Mar;38(3):336-43. doi: 10.1093/oxfordjournals.pcp.a029171.

DOI:10.1093/oxfordjournals.pcp.a029171
PMID:9150605
Abstract

We have introduced the maize Ac transposable element in Arabidopsis thaliana and found that after three selfing generations, the element is immobile and extensively methylated. Moreover, the nopaline synthase (nos) gene present on the same transferred T-DNA, was active early after transformation and regeneration, but inactive in most of the S1 progeny. We used 5-azacytidine (5AzaC) to determine whether a reduction in the methylation would affect both Ac transposition and expression of the nos gene. After treatment with 5AzaC doses from 0.3 mM to 1.0 mM, approximately 25% of the plants produced detectable amounts of nopaline, indicating that the nos gene was reactivated. Using the polymerase chain reaction (PCR) to detect the empty donor site left by Ac transposition, we demonstrated that 5AzaC also activates Ac excision in the transgenic plants. Approximately 13% of the 5AzaC treated plants (doses from 0.1 mM to 1.0 mM) were shown to have empty donor sites due to Ac excision. None of the plants cultivated in the absence of 5AzaC showed evidence for Ac transposition or reactivation of the nos gene. Further analysis using Southern blot indicate that some demethylation occurred in the genome of individual plants. These results may represent demethylation in few cells during development which may be sufficient to reactivate in these cells the expression of the nos and Ac transposase transgenes, the latter promoting Ac transposition in somatic cells.

摘要

我们已将玉米Ac转座因子导入拟南芥,发现经过三代自交后,该因子不再移动且发生了广泛的甲基化。此外,存在于同一转移T-DNA上的胭脂碱合成酶(nos)基因,在转化和再生后早期具有活性,但在大多数S1后代中无活性。我们使用5-氮杂胞苷(5AzaC)来确定甲基化程度的降低是否会影响Ac转座以及nos基因的表达。用0.3 mM至1.0 mM剂量的5AzaC处理后,约25%的植株产生了可检测量的胭脂碱,表明nos基因被重新激活。利用聚合酶链反应(PCR)检测Ac转座后留下的空供体位点,我们证明5AzaC也能激活转基因植株中的Ac切除。约13%经5AzaC处理的植株(剂量为0.1 mM至1.0 mM)因Ac切除而显示有空供体位点。在未使用5AzaC培养的植株中,没有一株显示出Ac转座或nos基因重新激活的证据。使用Southern杂交的进一步分析表明,个别植株的基因组中发生了一些去甲基化。这些结果可能代表发育过程中少数细胞中的去甲基化,这可能足以在这些细胞中重新激活nos和Ac转座酶转基因的表达,后者促进体细胞中的Ac转座。

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