Construction of lentiviral vectors and transfection of THP-1 cell lines to achieve stable low expression of sphingosine-1-phosphate receptor 1
10.13200/j.cnki.cjb.004343
- VernacularTitle:干扰鞘氨醇-1-磷酸受体1表达慢病毒质粒及其稳转THP-1细胞株的建立
- Author:
Jiajia TAN
1
Author Information
1. The First Affiliated Hospital of Guangxi Medical University, Nanning 530021, Guangxi Zhuang Autonomous Region, China
- Publication Type:Journal Article
- Keywords:
Sphingosine-1-phosphate receptor 1(S1PR1);
THP-1 cell lines;
Lentivirus
- From:
Chinese Journal of Biologicals
2026;39(03):270-276
- CountryChina
- Language:Chinese
-
Abstract:
ObjectiveTo construct lentiviral vectors that interferes with the expression of sphingosine-1-phosphate receptor 1(S1 PR1) and stably transfect the lentiviral vectors into THP-1 cells, in order to study the effect of S1 PR1 on macrophage function and the mechanism of S1 PR1 in tumor development at the cellular level.MethodsAccording to the sequence of S1 PR1 gene(1901) registered in NCBI database, three pairs of primers were designed for the shRNA sequence of this gene. The target gene was amplified by PCR, inserted into vector pLKO.1-puro, and the corresponding lentiviral plasmids were constructed,which were identified by enzymatic digestion electrophoresis and sequencing. The correct lentiviral vector plasmids were named pLKO.1-S1 PR1-shRNA1, pLKO.1-S1 PR1-shRNA2, and pLKO.1-S1 PR1-shRNA3, and the vector pLKO.1-puro containing stuffer sequence was used as control(named pLKO.1-S1 PR1-shNC). The lentiviral vector plasmids and lentivirus packaging plasmids were co-transfected into 293T cells for virus packaging, and the titer of virus solution was determined after concentration. The screening concentration of puromycin(0, 0. 5, 1. 0, 1. 5, 2. 0, 2. 5 μg/mL), culture time(0, 24, 48, 72 h)and MOI(10, 20, 30, 40, 50) of THP-1 cells were determined. THP-1 cells were infected with the lentivirus under the optimum conditions and screened by puromycin. The relative mRNA and protein expression of S1 PR1 in THP-1 cells of each group were detected by RT-qPCR and Western blot respectively.ResultsEnzymatic digestion electrophoresis identification and sequencing indicated that pLKO.1-S1 PR1-shRNA1, pLKO.1-S1 PR1-shRNA2, and pLKO.1-S1 PR1-shRNA3 lentiviral vectors were correctly constructed. The lentivirus titers of shNC, shRNA1, shRNA2 and shRNA3 groups were 9. 5 × 10~9, 4. 25 × 10~9,2 × 10~9 and 4. 4 × 10~9 TU/mL, respectively. THP-1 cells were infected with the lentivirus at the optimum MOI of 50 for 72 h.After screening with 1. 5 μg/mL puromycin, the relative expression levels of S1 PR1 mRNA in shRNA1, shRNA2 and shRNA3 groups were significantly lower than that in shNC group(F = 44. 916, P < 0. 001); the relative expression level of S1 PR1 protein in shRNA1 group decreased with no significant difference(t = 1. 921, P > 0. 05), while the relative expression levels of S1 PR1 protein in shRNA2 and shRNA3 groups decreased significantly(t = 8. 730 and 6. 957, respectively, each P < 0. 05).ConclusionThe lentiviral vectors interfering with S1 PR1 expression and THP-1 cell lines stably expressing the vectors were successfully constructed, which can be used for further related research.
