Production and characterization of anti-porcine CXCL10 monoclonal antibodies

Taylor Hailstock,Chaohui Dai, Jovan Aquino, Kristen E. Walker, Shannon Chick,Jean N. Manirarora,Raksha Suresh,Veerupaxagouda Patil, Gourapura J. Renukaradhya,Yvonne B. Sullivan, Joanna Labresh,Joan K. Lunney

CYTOKINE(2024)

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摘要
Research on C-X-C motif chemokine ligand 10 (CXCL10) has been widely reported for humans and select animal species, yet immune reagents are limited for pig chemokines. Our goal is to provide veterinary immunologists and the biomedical community with new commercial immune reagents and standardized assays. Recombinant porcine CXCL10 (rPoCXCL10) protein was produced by yeast expression and used to generate a panel of alpha CXCL10 monoclonal antibodies (mAbs). All mAbs were assessed for cross-inhibition and reactivity to orthologous yeast expressed CXCL10 proteins. Characterization of a panel of nine alpha PoCXCL10 mAbs identified six distinct antigenic determinants. A sensitive quantitative sandwich ELISA was developed with anti-PoCXCL10-1.6 and -1.9 mAb; reactivity was verified with both rPoCXCL10 and native PoCXCL10, detected in supernatants of peripheral blood mononuclear cells stimulated with rPoIFN gamma or PMA/Ionomycin. Immunostaining of in vitro rPoIFN gamma stimulated pig spleen and blood cells verified CXCL10 + cells as CD3-CD4-CD172+, with occasional CD3-CD4 + CD172 + subsets. Comparison studies determined that alpha PoCXCL10-1.4 mAb was the ideal mAb clone for intracellular staining, whereas with alpha PoCXCL10-1.1 and -1.2 mAbs were best for immunohistochemistry analyses. These techniques and tools will be useful for evaluating swine immune development, responses to infectious diseases and vaccines, as well as for improving utility of pigs as an important biomedical model.
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关键词
(6 max) CXCL10,Monoclonal antibodies,Porcine,Intracellular staining,Sandwich ELISA,Chemokine
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