Abstract
In recent years, real-time observations of molecules have been required to understand their behavior and function. To date, we have reported two different time-resolved observation methods: diffracted x-ray tracking and diffracted x-ray blinking (DXB). The former monitors the motion of diffracted spots derived from nanocrystals labeled onto target molecules, and the latter measures the fluctuation of the diffraction intensity that is highly correlated with the target molecular motion. However, these reports use a synchrotron x-ray source because of its high average flux, resulting in a high time resolution. Here, we used a laboratory x-ray source and DXB to measure the internal molecular dynamics of three different systems. The samples studied were bovine serum albumin (BSA) pinned onto a substrate, antifreeze protein (AFP) crystallized as a single crystal, and poly{2-(perfluorooctyl)ethyl acrylate} (PC8FA) polymer between polyimide sheets. It was found that not only BSA but also AFP and PC8FA molecules move in the systems. In addition, the molecular motion of AFP molecules was observed to increase with decreasing temperature. The rotational diffusion coefficients (DR) of BSA, AFP, and PC8FA were estimated to be 0.73 pm2/s, 0.65 pm2/s, and 3.29 pm2/s, respectively. Surprisingly, the DR of the PC8FA polymer was found to be the highest among the three samples. This is the first report that measures the molecular motion of a single protein crystal and polymer by using DXB with a laboratory x-ray source. This technique can be applied to any kind of crystal and crystalline polymer and provides atomic-order molecular information.
Highlights
Dynamic information within a protein molecule is essential for understanding and controlling the function of that molecule
The former monitors the motion of diffracted spots derived from nanocrystals labeled onto target molecules, and the latter measures the fluctuation of the diffraction intensity that is highly correlated with the target molecular motion
bovine serum albumin (BSA) was chosen for the first sample of diffracted x-ray blinking (DXB) with a laboratory xray source because this 66 kDa globular protein is widely used for a wide variety of experiments as a control
Summary
Dynamic information within a protein molecule is essential for understanding and controlling the function of that molecule. Since the DXT/DXB measurement targets a noncrystalline system such as single protein molecules, it requires gold nanocrystal labeling. The first example of our laboratory-DXB is bovine serum albumin (BSA) labeled with commercially available gold colloids This measurement shows that DXB using commercially available colloidal gold with a laboratory x-ray light source is possible to monitor the protein motion. Laboratory x-ray sources cannot provide sufficient flux, so time-resolved x-ray diffraction image data must be carefully statistically processed to extract useful dynamic information
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