Development, Optimization and Validation of a Sandwich ELISA for Detection of Recombinant Human Factor VII

Sarial, Sheila; Sonboli, Rozhan; Maleknia, Shayan; Ashori, Fatemeh; Rezaeiravesh, Sara; Nouri, Saeed; Abolhassan, Mohammadreza; Vaziri, Behrouz; Mahboudi, Fereidoun

doi:10.38150/sajeb.5(1).p26-31

SAJEB

2015

DOI: 10.38150/sajeb.5(1).p26-31

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Development, Optimization and Validation of a Sandwich ELISA for Detection of Recombinant Human Factor VII

Sheila Sarial¹,

Rozhan Sonboli²,

Shayan Maleknia³

et al.

Abstract: Recombinant human factor VII (rh-FVII) is produced by engineered BHK cells at low dose. Accordingly, establishment of a precise method is crucial to reliably measuring expression level of this protein during manufacturing pro-cesses. We developed and established a reproducible sandwich enzyme-linked immunosorbent assay (ELISA) method for measuring amount of FVII during biopharmaceutical in upstream and downstream processes of Aryo-Seven. A sandwich ELISA was designed using two different high affinity mon-oclon… Show more

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Determination of rFVII Concentration in Cell Culture Supernatant Using VIISelect Resin and RP-HPLC-UV

Khodadadian¹,

Zarezadeh²,

Behrouz³

et al. 2022

CPA

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Background: Recombinant activated human coagulation factor VIIa (rFVIIa), a vitamin K-dependent serine protease, was originally developed by Novo Nordisk® for the treatment of patients with FVII deficiency as well as patients with hemophilia A and B with inhibitors against FVIII or FIX. The gene for human FVII is cloned and expressed in baby hamster kidney (BHK) cells and the protein is secreted into the culture media, which is then converted to the active form during chromatographic purification steps. When secreted into the culture media, measuring the concentration levels of FVII is needed in order to monitor, control and optimize the production processes. However, because of the high complexity of such media, reliable analytical techniques are required for this purpose. Objective: This work focuses on the analytical application of VIISelect resin (GE Healthcare) as a highly selective adsorbent for cleanup and preconcentration of rFVII in culture supernatant before analysis by reversed phase high performance liquid chromatography (RP-HPLC). Method: Empty 1 ml SPE cartridges were packed with VIISelect resin. Four types of solutions were used for the sample preparation. The RP-HPLC separation was conducted on a C4 column with UV detection. Results: The method shows recoveries greater than 97% in culture medium with relative standard deviations (RSDs) of less than 2%. The limits of detection and quantification were 0.039 mg/L and 0.12 mg/L, respectively. Conclusion: The method showed better performance in terms of precision and accuracy for rFVIIa determination in cell culture supernatant compared with other techniques like ELISA and SDS-PAGE.

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Determination of rFVII Concentration in Cell Culture Supernatant Using VIISelect Resin and RP-HPLC-UV

Khodadadian¹,

Zarezadeh²,

Behrouz³

et al. 2022

CPA

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Optimization of HER2-based and cell-based ELISA for detection of trastuzumab biosimilar

Ahmadzadeh

Farshdari

Nematollahi

et al. 2020

Koomesh

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Introduction: ELISA is a sensitive, specific, reproducible and fast method to quantify the biological activity of antibodies. Trastuzumab is a humanized monoclonal antibody against HER2 receptors which prevents the initiation of downstream signaling pathway. Trastuzumab can be used as a positive control in the ELISA experiments for anti-HER2 antibodies. Additionaly, insufficient washing and blocking can be the cause of background in the ELISA experiment that is necessary to be optimized. As we do not want to waste antigen, it is also important to determine the last dilution of antigen that can give good titration curve for trastuzumab. The aim of this study was to optimize ELISA method for trastuzumab biosimilar (AryoTrust™, Aryogen pharmed). Materials and Methods: In this study, different variables including the number of washing cycle, the blocking agent and antigen concentration in HER2-based ELISA and the type of HER2 negative cell line and the blocking agent in cell-based ELISA were studied. Results: It was demonstrated that 5 times washing between different steps of HER2-based ELISA causes significant lower non-specific background as compared to 3 times washing. Moreover, the nonspecific binding was significantly lower in the presence of % 5 skim milk as blocking agent as compared to BSA %1 or BSA %3. In addition, the lowest HER2 concentration which gives good titration curve for trastuzumab was 0.1 μg/ml. In cellbased ELISA experiment, it was demonstrated that the use of MDA-MB-231 as negative HER2 cell line caused significant lower background than MCF-7. Furthermore, BSA 3% was chosen as proper blocking agent. Conclusion: The results of this study can be used for development of HER2 and cell-based ELISA for anti HER2 antibodies and its fragments.

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Development, Optimization and Validation of a Sandwich ELISA for Detection of Recombinant Human Factor VII

Cited by 2 publications

References 0 publications

Determination of rFVII Concentration in Cell Culture Supernatant Using VIISelect Resin and RP-HPLC-UV

Determination of rFVII Concentration in Cell Culture Supernatant Using VIISelect Resin and RP-HPLC-UV

Optimization of HER2-based and cell-based ELISA for detection of trastuzumab biosimilar

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