中国农业科学2025,Vol.58Issue(11):2253-2264,12.DOI:10.3864/j.issn.0578-1752.2025.11.013
稳定表达猪源CD163蛋白PK15细胞系的构建及评价
Construction and Evaluation of a PK15 Cell Line Stably Expressing Porcine CD163 Protein
摘要
Abstract
[Background]CD163 is an important transmembrane protein that plays a key role in host immune regulation,inflammatory response,and the infection process of various pathogens.Studies have shown that CD163,as a host receptor,not only influences cell signaling pathways but also regulates host susceptibility to foreign pathogens.Since the receptor-pathogen interaction mechanisms involving CD163 are not yet fully elucidated,establishing a cell model stably expressing CD163 is of great significance for related research.Porcine reproductive and respiratory syndrome virus(PRRSV)is an important model for studying the CD163-mediated viral entry mechanism.However,the primary target cells of PRRSV—porcine alveolar macrophages(PAMs)—cannot proliferate continuously in vitro,which limits their application in pathogenetic research.Therefore,the monkey-derived cell line MARC-145 is commonly used for PRRSV in vitro culture,but its non-porcine origin may affect the biological relevance of experimental results.[Objective]This study aimed to construct a porcine cell line stably expressing porcine CD163 protein and to evaluate its susceptibility to PRRSV infection.[Method]This study was conducted at the Guangdong Provincial Laboratory of Lingnan Modern Agricultural Science and Technology from June 2022 to November 2023.The porcine CD163 gene was cloned,and two strategies were employed to express this gene in the porcine kidney cell line(PK15).Firstly,recombinant plasmid transient transfection was attempted,but due to the low transient transfection efficiency of PK15 cells,a stably expressing cell line could not be obtained.To optimize the expression strategy,lentiviral vector-mediated gene transduction was further applied,followed by screening for stable cell lines.Lentiviral packaging was performed using 293T cells,and the resulting virus was transduced into PK15 cells.Positive clones were screened using puromycin to ensure stable integration and long-term expression of the exogenous gene.CD163 mRNA and protein expression levels were detected by RT-qPCR and Western blot,and passage experiments were further conducted to evaluate the stability of CD163 expression,ensuring the long-term application potential of the cell line.[Result]A recombinant lentiviral vector carrying the CD163 gene was successfully constructed,and a stably expressing PK15 cell line,named PK15-CD163,was obtained through lentiviral transduction.RT-qPCR and Western blot results showed that the expression levels of CD163 mRNA and protein in PK15-CD163 cells were significantly higher than those in normal PK15 cells and remained stable after multiple passages.However,PRRSV infection experiments indicated that PRRSV N protein expression could not be detected by either RT-qPCR or Western blot,suggesting that PRRSV replication might be restricted in this cell line.[Conclusion]This study successfully established a PK15-CD163 cell line,providing an important experimental tool for further investigation of CD163's biological functions in host cells.Although PRRSV infection in PK15-CD163 cells did not yield significant results,this cell line could still be used to explore CD163-mediated immune regulation,receptor function,and other pathogen infection mechanisms.Additionally,it provided a potential platform for antiviral drug screening.关键词
猪繁殖与呼吸综合征病毒/CD163/慢病毒载体/PK15Key words
porcine reproductive and respiratory syndrome virus/CD163/lentiviral vector/PK15引用本文复制引用
赵清扬,张晓晓,郭春和..稳定表达猪源CD163蛋白PK15细胞系的构建及评价[J].中国农业科学,2025,58(11):2253-2264,12.基金项目
国家重点研发计划(2023YFD1801500)、广州市科技计划项目(2023B03J0947,2025D04J0072)、岭南现代农业科学与技术广东省实验室自主项目(NG2022003) (2023YFD1801500)
