A method for detecting trypsin and its inhibitors based on phosphorescent copper nanoclusters
A trypsin inhibition and trypsin technology, applied in the field of biosensing, can solve the problems of low detection limit, complicated operation and high price, and achieve the effects of fast reaction, simple synthesis and high sensitivity
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Embodiment 1
[0040]Example 1: At room temperature, take DMF and deionized water to prepare a mixed solution, and the volume ratio of DMF / water is 2:1. Add 20 μL of glutathione (0.2M) to 480 μL of mixed solvent and shake gently until uniform. Take the copper sulfate solution and add it into a glass bottle, so that the copper ion concentration in the mixed solution is 500 μM, put it into a 20° C. shaking box, stir and shake at a slow speed for 1 minute, and form phosphorescent copper nanoclusters. The prepared phosphorescent copper nanoclusters were measured by ultraviolet-visible spectrophotometer and fluorescence spectrophotometer to draw absorption spectrum curve and fluorescence spectrum curve, and the phosphorescence lifetime and fitting curve of copper nanoclusters were drawn by lifetime detection. like figure 1 , figure 2 and image 3 .
Embodiment 2
[0041] Example 2: At room temperature, take DMF and deionized water to prepare a mixed solution, and the volume ratio of DMF / water is 2:1. Add 20 μL of glutathione (0.2M) to 480 μL of mixed solvent and shake gently until uniform. Take the copper sulfate solution and add it into a glass bottle, so that the copper ion concentration in the mixed solution is 500 μM, put it into a 20° C. shaking box, stir and shake at a slow speed for 1 minute, and form phosphorescent copper nanoclusters. A certain amount of copper nanoclusters was freeze-dried, and characterized by transmission electron microscopy (TEM) and X-ray photoelectric spectroscopy (XPS). like Figure 4 , Figure 5 and Figure 6 .
Embodiment 3
[0042] Example 3: Cytochrome C solution (2 mg / mL) was prepared with prepared Tris-HCl (50 mM, pH 8.9) buffer. The absorption spectrum curve is drawn by UV-Vis spectrophotometer measurement, such as Figure 7 .
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