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固氮根瘤中特异性诱导的植物基因的调控:顺式作用元件和反式作用因子在豆血红蛋白基因表达中的作用

Regulation of plant genes specifically induced in nitrogen-fixing nodules: role of cis-acting elements and trans-acting factors in leghemoglobin gene expression.

作者信息

de Bruijn F J, Felix G, Grunenberg B, Hoffmann H J, Metz B, Ratet P, Simons-Schreier A, Szabados L, Welters P, Schell J

机构信息

Max-Planck-Institut für Züchtungsforschung, Köln, FRG.

出版信息

Plant Mol Biol. 1989 Sep;13(3):319-25. doi: 10.1007/BF00025320.

Abstract

Transgenic alfalfa plants harboring a gene fusion between the soybean leghemoglobin (lbc3) promoter region and the chloramphenicol acetyl transferase (cat) gene were used to determine the influence of rhizobial mutants on lb gene expression in nodules. The promoter region of the Sesbania rostrata glb3 (Srglb3) leghemoglobin gene was examined for the presence of conserved motifs homologous to binding site 1 and 2 of the soybean lbc3 promoter region, found to interact with a trans-acting factor present in soybean nodule nuclear extracts (Jensen EO, Marcker KA, Schell J, de Bruijn FJ, EMBO J 7:1265-1271, 1988). Subfragments of the S. rostrata glb3 (Srglb3) promoter region were examined for binding to trans-acting factors from nodule nuclear extracts. In addition to the binding sites previously identified (Metz BA, Welters P, Hoffmann HJ, Jensen EO, Schell J, de Bruijn FJ, Mol Gen Genet 214: 181-191), several other sites were found to interact with trans-acting factors. In most cases the same trans-acting factor(s) were shown to be involved. One fragment (202) was found to bind specifically to a different factor (protein) which was extremely heat-resistant (100 degrees C). The appearance of this factor was shown to be developmentally regulated since the expected protein-DNA complexes were first observed around 12 days after infection, concomitant with the production of leghemoglobin proteins. Fragments of the Srglb3 5' upstream region were fused to the beta-glucuronidase reporter gene with its own CAAT and TATA box region or those of the cauliflower mosaic virus 35S and nopaline synthase (nos) promoters.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

携带大豆豆血红蛋白(lbc3)启动子区域与氯霉素乙酰转移酶(cat)基因之间基因融合的转基因苜蓿植株,被用于确定根瘤菌突变体对根瘤中lb基因表达的影响。对刺槐(Sesbania rostrata)glb3(Srglb3)豆血红蛋白基因的启动子区域进行检查,以寻找与大豆lbc3启动子区域结合位点1和2同源的保守基序,已发现这些基序可与大豆根瘤核提取物中存在的反式作用因子相互作用(Jensen EO,Marcker KA,Schell J,de Bruijn FJ,《欧洲分子生物学组织杂志》7卷:1265 - 1271页,1988年)。对刺槐glb3(Srglb3)启动子区域的亚片段进行检查,以确定其与根瘤核提取物中的反式作用因子的结合情况。除了先前鉴定出的结合位点(Metz BA,Welters P,Hoffmann HJ,Jensen EO,Schell J,de Bruijn FJ,《分子与普通遗传学》214卷:181 - 191页)外,还发现了其他几个可与反式作用因子相互作用的位点。在大多数情况下,显示涉及相同的反式作用因子。发现一个片段(202)可特异性结合一种不同的因子(蛋白质),该因子具有极高的耐热性(100摄氏度)。由于预期的蛋白质 - DNA复合物在感染后约12天首次观察到,同时伴有豆血红蛋白蛋白的产生,因此表明该因子的出现受发育调控。将Srglb3 5'上游区域的片段与带有自身CAAT和TATA盒区域的β - 葡萄糖醛酸酶报告基因融合,或与花椰菜花叶病毒35S和胭脂碱合酶(nos)启动子的片段融合。(摘要截短于250字)

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