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Time-resolved flow-flash FT-IR difference spectroscopy: the kinetics of CO photodissociation from myoglobin revisited

机译:时间分辨的流动闪光FT-IR差异光谱:肌红蛋白引起的CO光解离动力学

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摘要

Fourier-transform infrared (FT-IR) difference spectroscopy has been proven to be a significant tool in biospectroscopy. In particular, the step-scan technique monitors structural and electronic changes at time resolutions down to a few nanoseconds retaining the multiplex advantage of FT-IR. For the elucidation of the functional mechanisms of proteins, this technique is currently limited to repetitive systems undergoing a rapid photocycle. To overcome this obstacle, we developed a flow-flash experiment in a miniaturised flow channel which was integrated into a step-scan FT-IR spectroscopic setup. As a proof of principle, we studied the rebinding reaction of CO to myoglobin after photodissociation. The use of microfluidics reduced the sample consumption drastically such that a typical step-scan experiment takes only a few 10 ml of a millimolar sample solution, making this method particularly interesting for the investigation of biological samples that are only available in small quantities. Moreover, the flow cell provides the unique opportunity to assess the reaction mechanism of proteins that cycle slowly or react irreversibly. We infer that this novel approach will help in the elucidation of molecular reactions as complex as those of vectorial ion transfer in membrane proteins. The potential application to the oxygen splitting reaction of cytochrome c oxidase is discussed.
机译:傅里叶变换红外(FT-IR)差异光谱已被证明是生物光谱中的重要工具。特别地,步进扫描技术以低至几纳秒的时间分辨率监视结构和电子变化,从而保留了FT-IR的多重优势。为了阐明蛋白质的功能机制,该技术目前仅限于经历快速光循环的重复系统。为了克服这一障碍,我们在小型流动通道中开发了流动闪光实验,该实验已集成到步进扫描FT-IR光谱仪中。作为原理的证明,我们研究了光解离后CO与肌红蛋白的重新结合反应。微流体技术的使用极大地减少了样品的消耗,因此典型的步进扫描实验只需几毫升10毫摩尔的样品溶液,这使得该方法对于仅少量获取的生物样品的研究尤为有趣。此外,流通池为评估缓慢循环或不可逆反应的蛋白质的反应机理提供了独特的机会。我们推断,这种新颖的方法将有助于阐明与膜蛋白中的矢量离子转移一样复杂的分子反应。讨论了细胞色素c氧化酶在氧裂解反应中的潜在应用。

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