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蓝藻聚球藻通过交换光系统II反应中心的D1蛋白来抵抗UV-B。

The cyanobacterium Synechococcus resists UV-B by exchanging photosystem II reaction-center D1 proteins.

作者信息

Campbell D, Eriksson M J, Oquist G, Gustafsson P, Clarke A K

机构信息

Department of Plant Physiology, University of Umeâ, S-901 87 Umeâ, Sweden.

出版信息

Proc Natl Acad Sci U S A. 1998 Jan 6;95(1):364-9. doi: 10.1073/pnas.95.1.364.

Abstract

Current ambient UV-B levels can significantly depress productivity in aquatic habitats, largely because UV-B inhibits several steps of photosynthesis, including the photooxidation of water catalyzed by photosystem II. We show that upon UV-B exposure the cyanobacterium Synechococcus sp. PCC 7942 rapidly changes the expression of a family of three psbA genes encoding photosystem II D1 proteins. In wild-type cells the psbAI gene is expressed constitutively, but strong accumulations of psbAII and psbAIII transcripts are induced within 15 min of moderate UV-B exposure (0.4 W/m2). This transcriptional response causes an exchange of two distinct photosystem II D1 proteins. D1:1 is encoded by psbAI, but on UV-B exposure, it is largely replaced by the alternate D1:2 form, encoded by both psbAII and psbAIII. The total content of D1 and other photosystem II reaction center protein, D2, remained unchanged throughout the UV exposure, as did the content and composition of the phycobilisome. Wild-type cells suffered only slight transient inhibition of photosystem II function under UV-B exposure. In marked contrast, under the same UV-B treatment, a mutant strain expressing only psbAI suffered severe (40%) and sustained inhibition of photosystem II function. Another mutant strain with constitutive expression of psbAII and psbAIII was almost completely resistant to the UV-B treatment, showing no inhibition of photosystem II function and only a slight drop in electron transport. In Synechococcus the rapid exchange of alternate D1 forms, therefore, accounts for much of the cellular resistance to UV-B inhibition of photosystem II activity and photosynthetic electron transport. This molecular plasticity may be an important element in community-level responses to UV-B, where susceptibility to UV-B inhibition of photosynthesis changes diurnally.

摘要

当前的环境UV-B水平会显著降低水生栖息地的生产力,主要是因为UV-B会抑制光合作用的几个步骤,包括光系统II催化的水的光氧化。我们发现,在暴露于UV-B时,蓝藻聚球藻属PCC 7942会迅速改变编码光系统II D1蛋白的三个psbA基因家族的表达。在野生型细胞中,psbAI基因持续表达,但在中等强度的UV-B暴露(0.4 W/m2)15分钟内,psbAII和psbAIII转录本会大量积累。这种转录反应导致两种不同的光系统II D1蛋白发生交换。D1:1由psbAI编码,但在UV-B暴露时,它会被由psbAII和psbAIII编码的另一种D1:2形式大量取代。在整个UV暴露过程中,D1和其他光系统II反应中心蛋白D2的总含量保持不变,藻胆体的含量和组成也是如此。野生型细胞在UV-B暴露下仅受到轻微的短暂光系统II功能抑制。与之形成鲜明对比的是,在相同的UV-B处理下,仅表达psbAI的突变株受到严重(40%)且持续的光系统II功能抑制。另一个组成型表达psbAII和psbAIII的突变株几乎完全抵抗UV-B处理,光系统II功能未受抑制,电子传递仅略有下降。因此,在聚球藻中,交替的D1形式的快速交换是细胞对UV-B抑制光系统II活性和光合电子传递产生抗性的主要原因。这种分子可塑性可能是群落水平对UV-B反应的一个重要因素,在这种反应中,光合作用对UV-B抑制的敏感性会随昼夜变化。

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