研究目的
Determination of PPi and PPase in biological fluids for clinical diagnosis and therapy of arthritic diseases.
研究成果
The study successfully developed a fluorescent assay for PPi and PPase activity detection with specific and accurate results, demonstrating potential for clinical diagnosis and therapy of arthritic diseases.
研究不足
The detection limits and sensitivity may need further improvement for clinical applications.
1:Experimental Design and Method Selection:
The study utilized FeCo-LDH as a peroxidase mimic to catalyze the formation of fluorescent PDA from dopamine in the presence of low-concentration H2O
2:Sample Selection and Data Sources:
The study focused on the detection of PPi and PPase activity in biological fluids.
3:List of Experimental Equipment and Materials:
FeCo-LDH, dopamine, H2O2, PPi, PPase, and other chemicals were used.
4:Experimental Procedures and Operational Workflow:
The formation of fluorescent PDA was monitored, and its interaction with Fe3+ and PPi was studied. PPase activity was detected based on the hydrolysis of PPi.
5:Data Analysis Methods:
Fluorescence spectra were measured to analyze the interaction and detection limits.
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FeCo-LDH
Peroxidase mimic to facilitate the in situ formation of fluorescent PDA
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Polydopamine (PDA)
Fluorescent label for PPi and PPase activity detection
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H2O2
Oxidizing agent for the formation of fluorescent PDA
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Dopamine (DA)
Precursor for the formation of fluorescent PDA
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Fe3+
Quencher of fluorescent PDA and coordinator with PPi
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PPi
Target for detection, coordinates with Fe3+
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PPase
Enzyme that catalyzes the hydrolysis of PPi
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