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莱茵衣藻叶绿体psaB基因表达中3'非编码序列的功能及终止密码子的使用情况

Function of 3' non-coding sequences and stop codon usage in expression of the chloroplast psaB gene in Chlamydomonas reinhardtii.

作者信息

Lee H, Bingham S E, Webber A N

机构信息

Department of Botany, Arizona State University, Tempe 85287-1601, USA.

出版信息

Plant Mol Biol. 1996 May;31(2):337-54. doi: 10.1007/BF00021794.

Abstract

The rate of mRNA decay is an important step in the control of gene expression in prokaryotes, eukaryotes and cellular organelles. Factors that determine the rate of mRNA decay in chloroplasts are not well understood. Chloroplast mRNAs typically contain an inverted repeat sequence within the 3' untranslated region that can potentially fold into a stem-loop structure. These stem-loop structures have been suggested to stabilize the mRNA by preventing degradation by exonuclease activity, although such a function in vivo has not been clearly established. Secondary structures within the translation reading frame may also determine the inherent stability of an mRNA. To test the function of the inverted repeat structures in chloroplast mRNA stability mutants were constructed in the psaB gene that eliminated the 3' flanking sequences of psaB or extended the open reading frame into the 3' inverted repeat. The mutant psaB genes were introduced into the chloroplast genome of Chlamydomonas reinhardtii. Mutants lacking the 3' stem-loop exhibited a 75% reduction in the level of psaB mRNA. The accumulation of photosystem I complexes was also decreased by a corresponding amount indicating that the mRNA level is limiting to PsaB protein synthesis. Pulse-chase labeling of the mRNA showed that the decay rate of the psaB mRNA was significantly increased demonstrating that the stem-loop structure is required for psaB mRNA stability. When the translation reading frame was extended into the 3' inverted repeat the mRNA level was reduced to only 2% of wild-type indicating that ribosome interaction with stem-loop structures destabilizes chloroplast mRNAs. The non-photosynthetic phenotype of the mutant with an extended reading frame allowed us to test whether infrequently used stop codons (UAG and UGA) can terminate translation in vivo. Both UAG and UGA are able to effectively terminate PsaB synthesis although UGA is never used in any of the Chlamydomonas chloroplast genes that have been sequenced.

摘要

mRNA 衰变率是原核生物、真核生物和细胞器中基因表达调控的重要步骤。决定叶绿体中 mRNA 衰变率的因素尚未完全明确。叶绿体 mRNA 通常在 3' 非翻译区包含一个反向重复序列,该序列可能折叠成茎环结构。尽管这种功能在体内尚未明确确立,但这些茎环结构被认为通过防止核酸外切酶活性降解来稳定 mRNA。翻译阅读框内的二级结构也可能决定 mRNA 的固有稳定性。为了测试反向重复结构在叶绿体 mRNA 稳定性中的功能,构建了 psaB 基因突变体,该突变体消除了 psaB 的 3' 侧翼序列或将开放阅读框延伸到 3' 反向重复序列中。将突变的 psaB 基因导入莱茵衣藻的叶绿体基因组。缺乏 3' 茎环的突变体中 psaB mRNA 水平降低了 75%。光系统 I 复合物的积累也相应减少,表明 mRNA 水平限制了 PsaB 蛋白的合成。对 mRNA 的脉冲追踪标记显示,psaB mRNA 的衰变率显著增加,表明茎环结构是 psaB mRNA 稳定性所必需的。当翻译阅读框延伸到 3' 反向重复序列中时,mRNA 水平降至野生型的仅 2%,表明核糖体与茎环结构的相互作用会使叶绿体 mRNA 不稳定。具有延伸阅读框的突变体的非光合表型使我们能够测试不常用的终止密码子(UAG 和 UGA)是否能在体内终止翻译。尽管在已测序的任何衣藻叶绿体基因中都从未使用过 UGA,但 UAG 和 UGA 都能够有效终止 PsaB 的合成。

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