Sensitive amplified luminescent proximity homogeneous assay for the quantitative detection of CA242

We here developed a sensitive and stable amplified luminescent proximity homogeneous assay (AlphaLISA) method for fast quantification of CA242 in human serum. Donor and acceptor beads modified with carboxyl groups could be coupled with CA242 antibodies after activation in the AlphaLISA method. CA242...

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Veröffentlicht in:Journal of immunological methods 2023-06, Vol.517, p.113487-113487, Article 113487
Hauptverfasser: Chen, Jianye, Fu, Benqi, Xiang, Zhongyi, Chen, Xindong, Wang, Lu, Qin, Yuan, Zhao, Xueqin, Zhou, Xiumei, Liu, Pengfei, Huang, Biao
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container_title Journal of immunological methods
container_volume 517
creator Chen, Jianye
Fu, Benqi
Xiang, Zhongyi
Chen, Xindong
Wang, Lu
Qin, Yuan
Zhao, Xueqin
Zhou, Xiumei
Liu, Pengfei
Huang, Biao
description We here developed a sensitive and stable amplified luminescent proximity homogeneous assay (AlphaLISA) method for fast quantification of CA242 in human serum. Donor and acceptor beads modified with carboxyl groups could be coupled with CA242 antibodies after activation in the AlphaLISA method. CA242 was rapidly detected by the double antibody sandwich immunoassay. The method yielded good linearity (>0.996) and detection range (0.16–400 U/mL). The intra-assay precisions of CA242-AlphaLISA were between 3.43% and 6.81% (< 10%), and the inter-assay precisions were between 4.06% and 9.56% (< 15%). The relative recoveries ranged from 89.61% to 107.29%. Detection time for the CA242-AlphaLISA method was only 20 min. Moreover, results of CA242-AlphaLISA and time-resolved fluorescence immunoassay had satisfactory correlation and consistency (ρ = 0.9852). The method was successfully applied to the analysis of human serum samples. Meanwhile, serum CA242 has a good detection value in the identification and diagnosis of pancreatic cancer and the monitoring of disease degree. Furthermore, the proposed AlphaLISA method is expected to be an alternative to traditional detection methods, laying a good foundation for the further development of kits to detect other biomarkers in future studies. [Display omitted]
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Donor and acceptor beads modified with carboxyl groups could be coupled with CA242 antibodies after activation in the AlphaLISA method. CA242 was rapidly detected by the double antibody sandwich immunoassay. The method yielded good linearity (&gt;0.996) and detection range (0.16–400 U/mL). The intra-assay precisions of CA242-AlphaLISA were between 3.43% and 6.81% (&lt; 10%), and the inter-assay precisions were between 4.06% and 9.56% (&lt; 15%). The relative recoveries ranged from 89.61% to 107.29%. Detection time for the CA242-AlphaLISA method was only 20 min. Moreover, results of CA242-AlphaLISA and time-resolved fluorescence immunoassay had satisfactory correlation and consistency (ρ = 0.9852). The method was successfully applied to the analysis of human serum samples. Meanwhile, serum CA242 has a good detection value in the identification and diagnosis of pancreatic cancer and the monitoring of disease degree. 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Donor and acceptor beads modified with carboxyl groups could be coupled with CA242 antibodies after activation in the AlphaLISA method. CA242 was rapidly detected by the double antibody sandwich immunoassay. The method yielded good linearity (&gt;0.996) and detection range (0.16–400 U/mL). The intra-assay precisions of CA242-AlphaLISA were between 3.43% and 6.81% (&lt; 10%), and the inter-assay precisions were between 4.06% and 9.56% (&lt; 15%). The relative recoveries ranged from 89.61% to 107.29%. Detection time for the CA242-AlphaLISA method was only 20 min. Moreover, results of CA242-AlphaLISA and time-resolved fluorescence immunoassay had satisfactory correlation and consistency (ρ = 0.9852). The method was successfully applied to the analysis of human serum samples. Meanwhile, serum CA242 has a good detection value in the identification and diagnosis of pancreatic cancer and the monitoring of disease degree. Furthermore, the proposed AlphaLISA method is expected to be an alternative to traditional detection methods, laying a good foundation for the further development of kits to detect other biomarkers in future studies. 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Donor and acceptor beads modified with carboxyl groups could be coupled with CA242 antibodies after activation in the AlphaLISA method. CA242 was rapidly detected by the double antibody sandwich immunoassay. The method yielded good linearity (&gt;0.996) and detection range (0.16–400 U/mL). The intra-assay precisions of CA242-AlphaLISA were between 3.43% and 6.81% (&lt; 10%), and the inter-assay precisions were between 4.06% and 9.56% (&lt; 15%). The relative recoveries ranged from 89.61% to 107.29%. Detection time for the CA242-AlphaLISA method was only 20 min. Moreover, results of CA242-AlphaLISA and time-resolved fluorescence immunoassay had satisfactory correlation and consistency (ρ = 0.9852). The method was successfully applied to the analysis of human serum samples. Meanwhile, serum CA242 has a good detection value in the identification and diagnosis of pancreatic cancer and the monitoring of disease degree. 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subjects Amplified luminescent proximity homogeneous assay
Antibodies
CA242
Humans
Immunoassay - methods
Luminescent Measurements - methods
Pancreatic cancer
Quantitative detection
title Sensitive amplified luminescent proximity homogeneous assay for the quantitative detection of CA242
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