A novel technique for protein immobilization onto CrAsH-modified surfaces is presented. This approach enables an efficient, reversible and fluorogenic immobilization of proteins. Moreover, expressed proteins can also be directly immobilized from cellular lysates without prior purification. The immobilized proteins are suitable for protein-protein interaction studies and the fluorescence enhancement upon immobilization can be employed for the direct detection of the immobilized protein without the need for secondary detection methods.
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CSIC, Inst Catalysis, Dept Biocatalysis, Marie Curie 2, Madrid 28049, Spain
CSIC, Inst Food Sci Technol & Nutr ICTAN, Bacterial Biotechnol, Juan de la Cierva 3, Madrid 28006, SpainCSIC, Inst Catalysis, Dept Biocatalysis, Marie Curie 2, Madrid 28049, Spain
Brabcova, Jana
Andreu, Alicia
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CSIC, Inst Catalysis, Dept Biocatalysis, Marie Curie 2, Madrid 28049, SpainCSIC, Inst Catalysis, Dept Biocatalysis, Marie Curie 2, Madrid 28049, Spain
Andreu, Alicia
Aguilera, David
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CSIC, Inst Catalysis, Dept Biocatalysis, Marie Curie 2, Madrid 28049, SpainCSIC, Inst Catalysis, Dept Biocatalysis, Marie Curie 2, Madrid 28049, Spain
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CSIC, Inst Food Sci Technol & Nutr ICTAN, Bacterial Biotechnol, Juan de la Cierva 3, Madrid 28006, SpainCSIC, Inst Catalysis, Dept Biocatalysis, Marie Curie 2, Madrid 28049, Spain
Munoz, Rosario
Palomo, Jose M.
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CSIC, Inst Catalysis, Dept Biocatalysis, Marie Curie 2, Madrid 28049, SpainCSIC, Inst Catalysis, Dept Biocatalysis, Marie Curie 2, Madrid 28049, Spain