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光调节叶绿体反应中心蛋白D1的翻译延伸速率。

Light regulates the rate of translation elongation of chloroplast reaction center protein D1.

作者信息

Edhofer I, Mühlbauer S K, Eichacker L A

机构信息

Department of Botany, University of Munich, München, Germany.

出版信息

Eur J Biochem. 1998 Oct 1;257(1):78-84. doi: 10.1046/j.1432-1327.1998.2570078.x.

Abstract

Intact and lysed chloroplasts isolated from the day or night phase of seedling growth exhibit a higher rate of [35S]Met incorporation into the D1 protein in the light than in darkness. In the presence of the translation initiation inhibitor lincomycin, radiolabel incorporation remains unaffected for 7.5-10 min of the in vitro translation reaction, indicating that radiolabel incorporation is regulated by translation elongation. The rate of [35S]Met incorporation into D1-protein can be increased by addition of exogenous ATP to the in vitro translation reactions; however, ATP cannot replace light, and at physiological concentrations of stromal ATP (40 microM), the rate is at least 25-fold higher in the light than in darkness. This indicates that translation elongation is arrested in darkness. Separation of translation-elongation reactions into polysome-bound and membrane-integrated D1 proteins demonstrates that the rate of translation elongation is higher in the presence of light. In the light, less time is required to transiently radiolabel a D1 translation intermediate of about 17 kDa and to chase the translation intermediate into mature D1 protein. We propose that light regulates the enzymatic activity of the translation-elongation process in chloroplasts.

摘要

从幼苗生长的白天或黑夜阶段分离出的完整叶绿体和裂解叶绿体,在光照下比在黑暗中表现出更高的[35S]甲硫氨酸掺入D1蛋白的速率。在存在翻译起始抑制剂林可霉素的情况下,体外翻译反应7.5 - 10分钟内放射性标记掺入不受影响,这表明放射性标记掺入受翻译延伸调控。通过向体外翻译反应中添加外源ATP可提高[35S]甲硫氨酸掺入D1蛋白的速率;然而,ATP不能替代光照,在基质ATP的生理浓度(40微摩尔)下,光照下的速率比黑暗中至少高25倍。这表明黑暗中翻译延伸被阻断。将翻译延伸反应分为多核糖体结合的和膜整合的D1蛋白表明,光照下翻译延伸速率更高。在光照下,短暂放射性标记约17 kDa的D1翻译中间体并将其追踪为成熟D1蛋白所需的时间更短。我们提出,光照调节叶绿体中翻译延伸过程的酶活性。

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