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[从皱果苋中克隆AHA基因及其在转基因烟草植株中的抗蚜效果]

[Cloning of AHA gene from Amaranthus hypochondriacus and it's aphid inhibitory effect in transgenic tabacco plants].

作者信息

Zhou Y G, Tian Y C, Mang K Q

机构信息

Institute of Microbiology, Chinese Academy of Sciences, Beijing 100080, China.

出版信息

Sheng Wu Gong Cheng Xue Bao. 2001 Jan;17(1):34-9.

PMID:11330184
Abstract

Using total DNA isolated from Amaranthus hypochondriacus as template, Amaranthus hypochondriacus agglutinin AHA gene was amplified by PCR and cloned. Sequence analysis results showed that this gene is consisted of 2453 base pairs including one 1538 bp intron and two exons of 212 bp and 703 bp respectively. After inverse PCR amplification, coding region of AHA gene was obtained. AHA gene with it's intron (AHAg) and withou intron (AHAc) were inserted downstream of 35S promotor in the binary vector pBin438 resulting in the construction of two plant expression vectors pBAHAg and pBAHAc repectively. Leave explants of Nicotinana tabacum var. SR1 were transformed with A. tumefaciens LBA4404 harbouring the above expression vectors. Results from PCR and Southern blot analysis showed that AHA genes were inserted into the genome of transformed tobacco plants. Immunodot blot analysis indicated that AHA was expressed in transgenic plants. The results from insect bioassay with peach aphid (Mizus persicae) showed that the transgenic plants of pBAHAg and pBAHAc were aphid resistant, evidenced by a 57%-48% reduction in insect population density, some plants were more than 85%. The aphid resistance of transgenic plants transformed with AHAg gene as judged by aphid inhibition rate was higher than that of plants transormed with AHAc gene indicating that the intron in AHAg may be favorable for expression of AHA in transgenic plants.

摘要

以从皱果苋中分离得到的总DNA为模板,通过PCR扩增并克隆了皱果苋凝集素AHA基因。序列分析结果表明,该基因由2453个碱基对组成,包括一个1538 bp的内含子和两个分别为212 bp和703 bp的外显子。经反向PCR扩增后,获得了AHA基因的编码区。将带有内含子的AHA基因(AHAg)和无内含子的AHA基因(AHAc)分别插入二元载体pBin438的35S启动子下游,分别构建了两个植物表达载体pBAHAg和pBAHAc。用携带上述表达载体的根癌农杆菌LBA4404转化烟草品种SR1的离体叶片外植体。PCR和Southern杂交分析结果表明,AHA基因已插入到转化烟草植株的基因组中。免疫斑点印迹分析表明,AHA在转基因植株中表达。用桃蚜进行昆虫生物测定的结果表明,pBAHAg和pBAHAc的转基因植株具有抗蚜性,昆虫种群密度降低了57%-48%,有些植株超过85%。以蚜虫抑制率判断,转AHAg基因的转基因植株的抗蚜性高于转AHAc基因的植株,表明AHAg中的内含子可能有利于AHA在转基因植株中的表达。

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