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眼虫叶绿体早期发育相关事件:VII. 铁氧还蛋白-NADP 还原酶系统还原氯霉素的还原剂来源的光控作用。

Events Surrounding the Early Development of Euglena Chloroplasts: VII. Photocontrol of the Source Of Reducing Power for Chloramphenicol Reduction by the Ferredoxin-NADP Reductase System.

机构信息

Institute for Photobiology of Cells and Organelles, Brandeis University, Waltham, Massachusetts 02154.

出版信息

Plant Physiol. 1976 Apr;57(4):594-601. doi: 10.1104/pp.57.4.594.

Abstract

d(-)threo-Chloramphenicol blocks chlorophyll and plastid protein synthesis in Euglena. During chloroplast development in white light, but not in red, the cells escape from chloramphenicol inhibition and chlorophyll formation is restored. Concomitantly, chloramphenicol is reduced. Reduction of chloramphenicol in an enzyme extract from Euglena requires NADPH and ferredoxin for maximal activity. Methyl viologen replaces ferredoxin, and when chemically reduced, ferredoxin or methyl viologen reduces chloramphenicol directly. This suggests that the enzyme involved is ferredoxin-NADP reductase. In agreement, crude extracts from wild type and W(3)BUL, a mutant lacking detectable plastids and plastid DNA, when separated on acrylamide gels, show a single band which reduces methyl viologen with NADPH, and its mobility is similar in wild type and in mutant W(3)BUL. The reductase is inducible by light and increases 3-fold in wild type in white or red light and 1.5-fold in W(3)BUL in white light. DCMU does not block chloramphenicol reduction in vivo indicating that electrons originate from sources other than photosynthetic electron transport. We infer that chloramphenicol is reduced by ferredoxin which receives electrons via ferredoxin-NADP reductase. The limiting step is not the enzyme but the source of reducing power which can be supplied from the cytoplasm, probably under control of the blue light receptor. Ferredoxin and ferredoxin NADP reductase appear to be coded in the nuclear genome, synthesized on cytoplasmic ribosomes, and join a group of enzymes which cannot be precisely localized, since they may be active anywhere from their site of synthesis in the cytoplasm to their place of deposition in the chloroplast.

摘要

d(-)苏- 氯霉素阻止衣藻中的叶绿素和质体蛋白合成。在白光下进行叶绿体发育时,但不在红光下,细胞逃避氯霉素的抑制,并且恢复叶绿素的形成。同时,氯霉素被还原。来自衣藻的酶提取物还原氯霉素需要 NADPH 和铁氧还蛋白才能达到最大活性。甲基紫精替代铁氧还蛋白,并且当化学还原时,铁氧还蛋白或甲基紫精直接还原氯霉素。这表明涉及的酶是铁氧还蛋白-NADP 还原酶。一致地,野生型和 W(3)BUL 的粗提取物,一种缺乏可检测的质体和质体 DNA 的突变体,当在丙烯酰胺凝胶上分离时,显示出一种与 NADPH 还原甲基紫精的单一带,并且其迁移率在野生型和突变体 W(3)BUL 中相似。该还原酶可被光诱导,并且在白光或红光中野生型增加 3 倍,在白光中 W(3)BUL 增加 1.5 倍。DCMU 不会在体内阻断氯霉素的还原,表明电子源不是来自光合电子传递。我们推断氯霉素被铁氧还蛋白还原,铁氧还蛋白通过铁氧还蛋白-NADP 还原酶接收电子。限速步骤不是酶,而是还原力的来源,它可以从细胞质供应,可能受蓝光受体的控制。铁氧还蛋白和铁氧还蛋白 NADP 还原酶似乎编码在核基因组中,在细胞质核糖体上合成,并加入一组不能精确定位的酶,因为它们可能在从细胞质中合成它们的位置到它们在叶绿体中的沉积位置的任何地方都具有活性。

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Ferredoxin biosynthesis in Euglena gracilis.纤细裸藻中的铁氧化还原蛋白生物合成
Biochim Biophys Acta. 1976 Aug 2;442(1):76-87. doi: 10.1016/0005-2787(76)90178-7.

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