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Studies on the Mechanism of Regulation of the mRNA Level for a Soybean Storage Protein Subunit by Exogenous l-Methionine

机译:外源L-蛋氨酸调节大豆贮藏蛋白亚基mRNA水平的机理研究

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摘要

In previous studies (GL Creason et al. 1983 Biochem Biophys Res Commun 117: 658-662; LP Holowach et al. 1984 Plant Physiol 74: 576-583), we have shown that when soybean (Glycine max L. Merrill cv Provar) cotyledons are cultured in medium supplemented with l-methionine, the β-subunit of 7S protein and β-mRNA are absent. We have carried out further studies on the mechanism of the methionine action. In one experiment, cotyledons were cultured for 16 days with or without methionine. After 4 days, some cotyledons were transferred from methionine-supplemented to basal (no methionine) medium and vice versa. In basal medium, β-subunit was detected at 4 days whereas in methionine-supplemented medium, no β-subunit was present. When cotyledons were transferred from basal to methionine-supplemented medium, the β-subunit increased within a 4 day period and then remained constant (on a per cotyledon basis). This result indicated that methionine was not acting by accelerating the degradation of the β-subunit. Four days after transfer from supplemented to basal medium cotyledons contained β-subunit, thus demonstrating that the inhibition was reversible. During this time, the uncombined methionine declined from 7 to 1.5 μmoles methionine per gram fresh weight. When β-mRNA was measured by in vitro translation, functional β-mRNA was absent in tissue that was not accumulating β-subunit. The messenger RNA for the β-subunit had a half-life of about 1 day in the presence of methionine. Hybridization of cotyledon mRNA with cDNA complementary to β-mRNA revealed that the 1700 nucleotide β-mRNA was not present in supplemented cotyledons. Thus, expression of the β-subunit gene is controlled at the level of transcription, RNA processing, or RNA turnover, rather than at the level of translation.
机译:在以前的研究中(GL Creason等人,1983 Biochem Biophys Res Commun 117:658-662; LP Holowach等人,1984 Plant Physiol 74:576-583),我们已经证明当大豆时(Glycine max L. Merrill cv Provar)子叶在补充有L-蛋氨酸的培养基中培养,不存在7S蛋白的β亚基和β-mRNA。我们对蛋氨酸的作用机理进行了进一步的研究。在一个实验中,将子叶在有或没有蛋氨酸的情况下培养16天。 4天后,将部分子叶从补充蛋氨酸的培养基转移到基础培养基(无蛋氨酸),反之亦然。在基础培养基中,第4天检测到β亚基,而在补充蛋氨酸的培养基中没有β亚基。当子叶从基础培养基转移至蛋氨酸补充培养基时,β亚基在4天的时间内增加,然后保持恒定(以每个子叶为基础)。该结果表明蛋氨酸不通过促进β-亚基的降解起作用。从补充子叶​​向基础培养基子叶转移后四天,其子叶中含有β-亚基,因此表明抑制作用是可逆的。在此期间,未结合的蛋氨酸从每克鲜重7摩尔摩尔降至1.5摩尔摩尔蛋氨酸。当通过体外翻译测量β-mRNA时,在不积累β-亚基的组织中不存在功能性β-mRNA。在蛋氨酸存在下,β-亚基的信使RNA的半衰期约为1天。子叶mRNA与互补于β-mRNA的cDNA杂交表明,在补充的子叶中不存在1700个核苷酸的β-mRNA。因此,β-亚基基因的表达被控制在转录,RNA加工或RNA周转的水平上,而不是在翻译的水平上。

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