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一种用于筛选具有简单转基因整合和稳定转基因表达的转基因品系的新型T-DNA载体设计。

A novel T-DNA vector design for selection of transgenic lines with simple transgene integration and stable transgene expression.

作者信息

Chen Song, Helliwell Christopher A, Wu Li-Min, Dennis Elizabeth S, Upadhyaya Narayana M, Zhang Ren, Waterhouse Peter M, Wang Ming-Bo

机构信息

CSIRO Plant Industry, GPO Box 1600, Canberra, ACT 2601, Australia.

School of Biological Sciences, University of Wollongong, NSW 2522, Australia.

出版信息

Funct Plant Biol. 2005 Sep;32(8):671-681. doi: 10.1071/FP05072.

DOI:10.1071/FP05072
PMID:32689166
Abstract

Plants transformed with Agrobacterium frequently contain T-DNA concatamers with direct-repeat (d / r) or inverted-repeat (i / r) transgene integrations, and these repetitive T-DNA insertions are often associated with transgene silencing. To facilitate the selection of transgenic lines with simple T-DNA insertions, we constructed a binary vector (pSIV) based on the principle of hairpin RNA (hpRNA)-induced gene silencing. The vector is designed so that any transformed cells that contain more than one insertion per locus should generate hpRNA against the selective marker gene, leading to its silencing. These cells should, therefore, be sensitive to the selective agent and less likely to regenerate. Results from Arabidopsis and tobacco transformation showed that pSIV gave considerably fewer transgenic lines with repetitive insertions than did a conventional T-DNA vector (pCON). Furthermore, the transgene was more stably expressed in the pSIV plants than in the pCON plants. Rescue of plant DNA flanking sequences from pSIV plants was significantly more frequent than from pCON plants, suggesting that pSIV is potentially useful for T-DNA tagging. Our results revealed a perfect correlation between the presence of tail-to-tail inverted repeats and transgene silencing, supporting the view that read-through hpRNA transcript derived from i / r T-DNA insertions is a primary inducer of transgene silencing in plants.

摘要

用农杆菌转化的植物通常含有具有直接重复(d / r)或反向重复(i / r)转基因整合的T-DNA串联体,并且这些重复的T-DNA插入通常与转基因沉默相关。为了便于选择具有简单T-DNA插入的转基因株系,我们基于发夹RNA(hpRNA)诱导的基因沉默原理构建了一个二元载体(pSIV)。该载体的设计使得任何每个位点含有多个插入的转化细胞都应该产生针对选择标记基因的hpRNA,导致其沉默。因此,这些细胞应该对选择剂敏感并且再生的可能性较小。拟南芥和烟草转化的结果表明,与传统的T-DNA载体(pCON)相比,pSIV产生的具有重复插入的转基因株系要少得多。此外,转基因在pSIV植物中比在pCON植物中更稳定地表达。从pSIV植物中拯救植物DNA侧翼序列的频率明显高于从pCON植物中,这表明pSIV可能对T-DNA标签有用。我们的结果揭示了尾对尾反向重复的存在与转基因沉默之间的完美相关性,支持了这样一种观点,即源自i / r T-DNA插入的通读hpRNA转录本是植物中转基因沉默的主要诱导物。

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