RESUMO
OBJECTIVES: Quantitative detection of interleukin-6 (IL-6) in serum and plasma can help monitor immune responses and the development of acute inflammation to guide patient management. We developed an IL-6 immunoassay for use with the automated ARCHITECT system for detecting an increase in the inflammatory response. METHODS: Immunized mouse sera were tested and selected B-cells were harvested for fusion with myeloma cells. A panel of monoclonal antibodies were produced, from which capture and detection monoclonal antibodies for the prototype IL-6 immunoassay were selected and screened on the ARCHITECT instrument. The antibody pair that most effectively captured and detected IL-6 was selected to develop a prototype IL-6 immunoassay. Calibrator and panel preparations using an internal recombinant IL-6 standard were compared to serum panels prepared with the IL-6 International Standard 89/548. Assay specificity and spike recovery were determined, and assay sensitivity was compared with the Roche EUA Elecsys IL-6 assay run on the cobas analyzer. RESULTS: Twenty-one antibodies in 441 antibody pairs were screened. The prototype IL-6 assay showed high sensitivity with an estimated limit of detection of 0.317 pg/mL and limit of quantitation of <1.27. Spike recovery was 90%-110% in serum and plasma. The internal recombinant human IL-6 calibrator showed excellent stability for 63 days at 2-8 °C. The prototype IL-6 immunoassay was specific for IL-6, exhibited no cross reactivity to related cytokines and interleukins, and was 10-fold more sensitive than the Elecsys IL-6 assay. CONCLUSIONS: The prototype ARCHITECT IL-6 automated immunoassay is a reliable and robust method for the quantitative determination of IL-6 in human serum and plasma.
Assuntos
Testes Imunológicos , Interleucina-6 , Animais , Anticorpos Monoclonais , Humanos , Imunoensaio/métodos , Fatores Imunológicos , Camundongos , Sensibilidade e EspecificidadeRESUMO
DNA immunization offers the advantage of allowing for the initiation of animal immunogenicity studies while work to produce and purify the protein of interest is completed. In this study, we sought to evaluate in vivo electroporation (EP) as a means to enhance the antigen-specific immune response from DNA immunization. Mice were immunized thrice with DNA encoding the protein of interest through intramuscular (IM) or intradermal (ID) injections. Test animals were administered an electrical pulse into the muscle or dermis at the site of injection immediately following immunization. In addition, cardiotoxin was injected into the muscle of a subset of test animals 5 days before each DNA injection. Nine weeks following the final DNA immunization, mice were immunized with the encoded purified protein emulsified in Freund's adjuvant. Sera from EP mice taken 2 weeks following the final DNA immunization showed a significant enhancement in antibody response. Specifically, those mice treated with cardiotoxin, immunized IM and given EP showed a strong response, but this was only observed versus solid phase and not solution phase antigen, suggesting the resulting antibody was of low titer and affinity. Similar testing following the protein immunization revealed a significant improvement in relative affinity versus sera taken following DNA immunization. Our results suggest EP can enhance the immune response elicited by DNA immunization.
RESUMO
Mouse-human chimeric antibodies (cAbs) against hepatitis C virus (HCV) core, NS3 (nonstructural), NS4, and NS5 antigens were developed as quality control (QC) reagents to replace the use of human sera/plasma for Abbott HCV immunoassays. The cAb retains the mouse monoclonal antibody (MAb) specificity and affinity but still reacts in the existing HCV assay format, which measures human anti-HCV immunoglobulin. Mouse heavy-chain (V(H)) and light-chain (V(L)) variable regions of anti-HCV core, NS3, NS4, and NS5 antigens were PCR amplified from hybridoma lines and then cloned with human IgG1 heavy-chain (C(H)) and light-chain (C(L)) constant regions, respectively. A single mammalian expression plasmid containing both heavy-chain and light-chain immunoglobulin genes was constructed and transfected into dihydrofolate reductase (DHFR)-deficient Chinese hamster ovary (CHO) cells. The transfected CHO cells were selected using hypoxanthine- and thymidine-free medium and screened by an enzyme immunoassay (EIA). The clone secreting the highest level of antibody was isolated from the CHO transfectants and further subcloned. Each cAb-expressing CHO cell line was weaned into serum-free medium, and the cAb was purified by protein A affinity chromatography. The levels of cAb production for the various CHO cell lines varied from 10 to 20 mg/liter. Purified anti-HCV cAbs were tested with Abbott HCV immunoassays and showed reactivity. Moreover, yeast surface display combined with alanine-scanning mutagenesis was used to map the epitope at the individual amino acid level. Our results suggest that these HCV cAbs are ideal controls, calibrators, and/or QC reagents for HCV assay standardization.
