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构建蓝藻集胞藻 6803 中 D1 蛋白腔暴露区域的缺失:对 D1 插入和在类囊体膜中积累的影响,以及对光系统 II 组装的影响。

Constructed deletions in lumen-exposed regions of the D1 protein in the cyanobacterium Synechocystis 6803: Effects on D1 insertion and accumulation in the thylakoid membrane, and on Photosystem II assembly.

机构信息

Department of Biochemistry, The Arrhenius Laboratories, Stockholm University, S-10691, Stockholm, Sweden.

出版信息

Photosynth Res. 1996 Aug;49(2):131-40. doi: 10.1007/BF00117663.

Abstract

Modified forms of the D1 protein with deletions in lumen-exposed regions, were constructed in the cyanobacterium Synechocystis 6803 using site-directed mutagenesis. Integration and stability of the mutated D1 proteins in the thylakoid membrane were studied by immunoblot and pulse-chase analyses. It was found that in Δ(N325-E333), the D1 protein with a deletion in the C-terminal tail, could insert in the thylakoids to normal amounts but its stability in the membrane was dramatically reduced. Insertion of D1 in Δ(V58-D61) or Δ(D103-G109);G110R, with deletions in the A-B loop, was severely obstructed, For Δ(P350-T354), with a deletion in the processed region of the C-terminus of D1, no phenotypic effects were observed. The effects of failed D1 insertion or accumulation on Photosystem II assembly was monitored by immunoblot analysis. The conclusions from these experiments are that the extrinsic 33 kDa protein, CP43, and the β subunit of cytochrome b559 accumulate in the thylakoid membrane independently of the D1 protein, and that accumulation of the D2 protein and CP47 requires insertion but not necessarily accumulation of the D1 protein.

摘要

使用定点突变技术在蓝藻集胞藻 6803 中构建了 D1 蛋白在腔暴露区域缺失的修饰形式。通过免疫印迹和脉冲追踪分析研究了突变 D1 蛋白在类囊体膜中的整合和稳定性。结果发现,在 Δ(N325-E333)中,C 末端尾部缺失的 D1 蛋白可以正常插入类囊体,但在膜中的稳定性大大降低。在 Δ(V58-D61)或 Δ(D103-G109);G110R 中,A-B 环缺失的 D1 插入严重受阻。对于 Δ(P350-T354),在 D1 C 末端加工区域缺失,没有观察到表型效应。通过免疫印迹分析监测 D1 插入或积累失败对光系统 II 组装的影响。这些实验的结论是,外在的 33 kDa 蛋白 CP43 和细胞色素 b559 的β亚基独立于 D1 蛋白在类囊体膜中积累,而 D2 蛋白和 CP47 的积累需要插入而不一定需要 D1 蛋白的积累。

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