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利用选择性同位素标记和红外光谱技术解析植物隐花色素光解酶同源区的光诱导构象变化。

Light-Induced Conformational Changes in the Plant Cryptochrome Photolyase Homology Region Resolved by Selective Isotope Labeling and Infrared Spectroscopy.

机构信息

Physical and Biophysical Chemistry, Department of Chemistry, Bielefeld University, Bielefeld, Germany.

Proteome and Metabolome Research (Bio 27), Department of Biology, Bielefeld University, Bielefeld, Germany.

出版信息

Photochem Photobiol. 2017 May;93(3):881-887. doi: 10.1111/php.12750.

Abstract

Plant cryptochromes are photoreceptors that regulate flowering, circadian rhythm and photomorphogenesis in response to blue and UV-A light. It has been demonstrated that the oxidized flavin cofactor is photoreduced to the neutral radical state via separate electron and proton transfer. Conformational changes have been found in the C-terminal extension, but few studies have addressed the changes in secondary structure in the sensory photolyase homology region (PHR). Here, we investigated the PHR of the plant cryptochrome from the green alga Chlamydomonas reinhardtii by light-induced infrared difference spectroscopy in combination with global C and N isotope labeling. Assignment of the signals is achieved by establishing a labeling strategy for cryptochromes that preserves the flavin at natural abundance. We demonstrate by UV/vis spectroscopy that the integrity of the sample is maintained and by mass spectrometry that the global labeling was highly efficient. As a result, difference bands are resolved at full intensity that at natural abundance are compensated by the overlap of flavin and protein signals. These bands are assigned to prominent conformational changes in the PHR by blue light illumination. We postulate that not only the partial unfolding of the C-terminal extension but also changes in the PHR may mediate signaling events.

摘要

植物隐花色素是光受体,可响应蓝光和 UV-A 光来调节开花、昼夜节律和光形态发生。已经证明,氧化的黄素辅因子通过单独的电子和质子转移被光还原为中性自由基状态。已经在 C 末端延伸部分发现了构象变化,但很少有研究涉及感光光解酶同源区(PHR)中的二级结构变化。在这里,我们通过光诱导的中红外差光谱结合全局 C 和 N 同位素标记研究了来自绿藻衣藻的植物隐花色素的 PHR。通过建立一种保持黄素天然丰度的隐花色素标记策略来实现信号的分配。我们通过紫外/可见光谱证明了样品的完整性得以保持,通过质谱证明了全局标记的高效性。结果,在天然丰度下由黄素和蛋白质信号重叠补偿的强度完全的差分带得到解析。这些带通过蓝光照射被分配到 PHR 中的显著构象变化。我们假设,不仅 C 末端延伸部分的部分展开,而且 PHR 的变化也可能介导信号事件。

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