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来自甘蓝型油菜的extA伸展蛋白基因的启动子区域控制着对创伤和拉伸应力的响应激活。

Promoter regions of the extA extensin gene from Brassica napus control activation in response to wounding and tensile stress.

作者信息

Elliott K A, Shirsat A H

机构信息

School of Biological Sciences, University of Wales, Bangor, Gwynedd, UK.

出版信息

Plant Mol Biol. 1998 Jul;37(4):675-87. doi: 10.1023/a:1005918816630.

Abstract

To identify controlling cis acting promoter regions in the B. napus extA extensin gene, expression in transgenic tobacco of 5' - 159, -433, -664, -789 and -940 bp promoter truncations linked to the uidA (B-glucuronidase) reporter coding sequence were analysed. The - 159 and -433 bp truncations directed non specific expression in all cell types within the plant. An activator region which increased expression levels 10 fold in all cell types was located between - 159 to -433 bp. A repressor region was found between -664 to -789 bp; removal of this region resulted in a 15 fold increase in expression. Histochemical analysis showed that transgenics containing the -664, -789 and -940 bp truncations directed expression of the fusion gene only in the phloem. A negative regulatory region located between -433 to -664 bp repressed expression in non-phloem cell types. In areas of the plant subject to tensile stress, the repression exerted by the negative regulatory region was overcome, allowing expression in all cell types. The quantitative repressor and activator regions which controlled absolute expression levels in all cell types were separate from the negative regulatory region which controlled cell type specific expression in response to tensile stress. A wound responsive region was found to be located between -940 to -3500 bp. Thus, the extA gene is under complex control, being regulated by 4 sets of positively and negatively acting cis regions, which control wound inducibility, activation in response to tensile stress, and quantitative expression levels.

摘要

为了鉴定甘蓝型油菜extA伸展蛋白基因中的顺式作用启动子控制区域,分析了与uidA(β-葡萄糖醛酸酶)报告基因编码序列相连的5' - 159、-433、-664、-789和-940 bp启动子截短体在转基因烟草中的表达情况。-159和-433 bp截短体在植物的所有细胞类型中都引导非特异性表达。在-159至-433 bp之间定位到一个在所有细胞类型中使表达水平提高10倍的激活区域。在-664至-789 bp之间发现了一个抑制区域;去除该区域导致表达增加15倍。组织化学分析表明,含有-664、-789和-940 bp截短体的转基因仅在韧皮部引导融合基因的表达。位于-433至-664 bp之间的一个负调控区域抑制非韧皮部细胞类型中的表达。在植物受到拉伸应力的区域,负调控区域施加的抑制作用被克服,从而允许在所有细胞类型中表达。控制所有细胞类型中绝对表达水平的定量抑制和激活区域与响应拉伸应力控制细胞类型特异性表达的负调控区域是分开的。发现一个创伤响应区域位于-940至-3500 bp之间。因此,extA基因受到复杂的调控,由4组正向和负向作用的顺式区域调控,这些区域控制创伤诱导性、对拉伸应力的激活以及定量表达水平。

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