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Low charge and reduced mobility of membrane protein complexes has implications for calibration of collision cross section measurements

机译:膜蛋白复合物的低电荷和降低的迁移率对碰撞截面测量的校准具有影响

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摘要

Ion mobility mass spectrometry of integral membrane proteins provides valuable insights into their architecture and stability. Here we show that due to their lower charge the average mobility of native-like membrane protein ions is approximately 30 % lower than that of soluble proteins of similar mass. This has implications for drift time measurements, made on travelling wave ion mobility mass spectrometers, which have to be calibrated to extract collision cross sections (Ω). Common calibration strategies employ unfolded or native-like soluble protein standards with masses and mobilities comparable to the protein of interest. We compare Ω values for membrane proteins, derived from standard calibration protocols using soluble proteins, to values measured using an RF-confined drift tube. Our results demonstrate that, while common calibration methods underestimate Ω for native-like or unfolded membrane protein complexes, higher mass soluble calibration standards consistently yield more accurate Ω values. These findings enable us to obtain directly structural information for highly charge-reduced complexes by travelling wave ion mobility mass spectrometry.
机译:整体膜蛋白的离子淌度质谱为他们的结构和稳定性提供了宝贵的见解。在这里我们表明,由于它们的电荷较低,天然类膜蛋白离子的平均迁移率比质量相似的可溶性蛋白低约30%。这对在行波离子迁移率质谱仪上进行的漂移时间测量有影响,必须对其进行校准以提取碰撞截面(Ω)。常见的校准策略采用质量和迁移率与目标蛋白质相当的未折叠或类似天然的可溶性蛋白质标准品。我们将使用可溶蛋白的标准校准方案得出的膜蛋白的Ω值与使用RF限制的漂移管测得的值进行比较。我们的结果表明,尽管普通校准方法低估了天然样或未折叠膜蛋白复合物的Ω,但质量较高的可溶性校准标准品始终能产生更准确的Ω值。这些发现使我们能够通过行波离子迁移率质谱法直接获得高度减少电荷的配合物的结构信息。

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