Electrochemical immunoassay of membrane P-glycoprotein by immobilization of cells on gold nanoparticles modified on a methoxysilyl-terminated butyrylchitosan matrix
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作者:
Du, D
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机构:Nanjing Univ, Key Lab Analyt Chem Life Sci, Educ Minist China, Dept Chem, Nanjing 210093, Peoples R China
Du, D
Ju, HX
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Nanjing Univ, Key Lab Analyt Chem Life Sci, Educ Minist China, Dept Chem, Nanjing 210093, Peoples R ChinaNanjing Univ, Key Lab Analyt Chem Life Sci, Educ Minist China, Dept Chem, Nanjing 210093, Peoples R China
Ju, HX
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Zhang, XJ
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机构:Nanjing Univ, Key Lab Analyt Chem Life Sci, Educ Minist China, Dept Chem, Nanjing 210093, Peoples R China
Zhang, XJ
Chen, J
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机构:Nanjing Univ, Key Lab Analyt Chem Life Sci, Educ Minist China, Dept Chem, Nanjing 210093, Peoples R China
Chen, J
Cai, J
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机构:Nanjing Univ, Key Lab Analyt Chem Life Sci, Educ Minist China, Dept Chem, Nanjing 210093, Peoples R China
Cai, J
Chen, HY
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机构:Nanjing Univ, Key Lab Analyt Chem Life Sci, Educ Minist China, Dept Chem, Nanjing 210093, Peoples R China
Chen, HY
机构:
[1] Nanjing Univ, Key Lab Analyt Chem Life Sci, Educ Minist China, Dept Chem, Nanjing 210093, Peoples R China
[2] Univ S Florida, Dept Chem, Tampa, FL 33620 USA
A strategy to detect P-glycoprotein (P-gp) on cell membrane and quantify the cell number using electrochemical immunoassay was developed by effective surface immunoreactions and immobilization of cells on a highly hydrophilic interface, which was constructed by adsorption of colloidal gold nanoparticles on a methoxysilyl-terminated (Mos) butyrylchitosan modified glassy carbon electrode (Au-CS/GCE). Atomic force microscopy studies proved that the nanoparticles adsorbed on Mos-butyrylchitosan were efficient in preventing the cell leakage and retaining the activity of immobilized living K562/ADM leukemic cells. The incubation with P-gp monoclonal antibody and then the secondary alkaline phosphatase (AP) conjugated antibody introduced AP onto the K562/ADM cell immobilized on Au-CS/GCE. The bound AP led to an amperometric response of I-naphthyl phosphate. Under optimal conditions the response was proportional to the logarithm of cell concentration in the range from 5.0 x 10(4) to 1.0 X 10(7) cells mL(-1) with a detection limit of 1.0 X 10(4) cells mL(-1). The results were comparable to flow cytometric analysis of P-gp expression. This proposed method was practical, convenient, and significant in the clinic and cytobiology.