Quantification of camelid cytokine mRNA expression in PBMCs by microfluidic qPCR technology

Rodon, Jordi; Te, Nigger; Ballester, Maria; Segalés, Joaquim; Serra Gironella, Joan; Bensaid, Albert

dc.contributor.author	Rodon, Jordi
dc.contributor.author	Te, Nigger
dc.contributor.author	Ballester, Maria
dc.contributor.author	Segalés, Joaquim
dc.contributor.author	Serra Gironella, Joan
dc.contributor.author	Bensaid, Albert
dc.contributor.other	Producció Animal	ca
dc.date.accessioned	2024-01-25T18:22:12Z
dc.date.available	2024-09-16T22:45:16Z
dc.date.issued	2023-09-17
dc.identifier.citation	Rodón, Jordi, Nigeer Te, María Ballester, Joaquím Segalés, Júlia Vergara‐Alert, and Albert Bensaïd. 2023. “Quantification of Camelid Cytokine mRNA Expression in PBMCs by Microfluidic qPCR Technology.” Developmental and Comparative Immunology 149: 105061. doi:10.1016/j.dci.2023.105061.	ca
dc.identifier.issn	0145-305X	ca
dc.identifier.uri	http://hdl.handle.net/20.500.12327/2761
dc.description.abstract	Camelids are economically and socially important in several parts of the world and might carry pathogens with epizootic or zoonotic potential. However, biological research in these species is limited due to lack of reagents. Here, we developed RT-qPCR assays to quantify a panel of camelid innate and adaptive immune response genes, which can be monitored in a single run. The assays were validated with PHA, PMA-ionomycin, and Poly I:Cstimulated PBMCs from alpaca, dromedary camel and llama, including normalization by multiple reference genes. Further, comparative gene expression analyses for the different camelid species were performed by a unique microfluidic qPCR assay. Compared to unstimulated controls, PHA and PMA-ionomycin stimulation elicited robust Th1 and Th2 responses in PBMCs from camelid species. Additional activation of type I and type III IFN signalling pathways was described exclusively in PHA-stimulated dromedary lymphocytes, in contrast to those from alpaca and llama. We also found that PolyI:C stimulation induced robust antiviral response genes in alpaca PBMCs. The proposed methodology should be useful for the measurement of immune responses to infection or vaccination in camelid species.	ca
dc.description.sponsorship	This study was performed as part of the Zoonotic Anticipation and Preparedness Initiative (ZAPI project) [Innovative Medicines initiative (IMI) grant 115760] and the Veterinary Biocontained research facility Network (VetBioNet) project (EU Grant Agreement INFRA-2016-1 Nº731014), with assistance and financial support from IMI and the European Commission and contributions from EFPIA partners. J.R. was partially supported by the VetBioNet project. IRTA is supported by CERCA Programme/Generalitat de Catalunya.	ca
dc.format.extent	44	ca
dc.language.iso	eng	ca
dc.publisher	Elsevier	ca
dc.relation.ispartof	Developmental and Comparative Immunology	ca
dc.rights	Attribution-NonCommercial-NoDerivatives 4.0 International	ca
dc.rights.uri	http://creativecommons.org/licenses/by-nc-nd/4.0/	*
dc.title	Quantification of camelid cytokine mRNA expression in PBMCs by microfluidic qPCR technology	ca
dc.type	info:eu-repo/semantics/article	ca
dc.description.version	info:eu-repo/semantics/acceptedVersion	ca
dc.rights.accessLevel	info:eu-repo/semantics/openAccess
dc.relation.projectID	EC/PF7/115760/EU/Zoonotic Anticipation and Preparedness Initiative/ZAPI	ca
dc.relation.projectID	EC/H2020/731014/EU/Veterinary Biocontained facility Network for excellence in animal infectiology research and experimentation/VetBioNet	ca
dc.subject.udc	619	ca
dc.identifier.doi	https://doi.org/10.1016/j.dci.2023.105061	ca
dc.contributor.group	Genètica i Millora Animal	ca
dc.contributor.group	Sanitat Animal	ca