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@#[Abstract] Objective: To investigate the effects of CRISPR/Cas9 gene editing mediated PD-1 knockdown on the proliferation, phenotype, IFN-γ and IL-2 secretion of T cells in Cynomolgus monkeys. Methods: gRNA targeting PD-1 gene of Cynomolgus monkey was designed, and the corresponding plasmid was constructed and extracted. peripheral blood mononuclear cells (PBMCs) of Cynomolgus monkeys were isolated, and plasmid DNAs were added for transfection by using Lonza 4D electrorotometer. FACS analysis and fluorescence microscopy were used to detect transfection efficiency at 48 h after transfection. Genomic DNA of T cells was extracted for PCR amplification and T7E1 digestion identification. The proliferation of T cells was induced under the stimulation of human CD3 antibody and IL-2, and the cell growth curve was drawn. PI staining flow cytometry was used to detect cell cycle and the expression levels of CD4 and CD8, and ELISA was used to detect the secretion of IFN- γ and IL-2. Results: At 48 h after transfection, the cells with green fluorescent protein expression in experimental group were observed under fluorescence microscopy with a transfection efficiency of (21.6±3.2)%. T7E1 enzyme digestion results showed that the PCR product of genomic DNA of cells in experimental group showed 3 bands after digestion, including the target cleavage bands(243,197 bp). Compared with non-transfected cells, the cells in experimental group exhibited slow proliferation, delayed colony formation, with small volume and weak refraction; the number of T cells at G0/G1 phase of the experimental group was significantly increased (P<0.05), while the number of cells at G2/M phase was significantly reduced (P<0.05); and the secretion levels of IFN-γ and IL-2 in the cells of the experimental group increased significantly (both P<0.05). However, the difference in the expression levels of CD4 and CD8 was not statistically significant between the two groups (both P>0.05). Conclusion: PD-1 gene knockout can arrest T cells in Cynomolgus monkey at G0/G1 phase, thereby inhibiting its proliferation and increasing the secretion of IFN-γ and IL-2 in the meanwhile.
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Objective: To investigate the correlation of the occurrence and development of cervical cancer with the disturbance of vaginal flora and the expression of programmed cell death receptor-1 (PD-1) molecules on the surface of T cells in order to provide new direction for PD-1 immune checkpoint blocking therapy. Methods: Twenty-four female SPF Kunming mice were randomly divided into two groups: normal control group (CON) (n=12) and cervical cancer model group (CCM) (n=12). We established the mouse cervical cancer U14 cell subcutaneous transplantation tumor model. After 21 days of rearing under the same conditions, vaginal secretions and blood samples of mice were collected. 16S rRNA gene amplification and sequencing technology were used to analyze the vaginal flora in the two groups. Flow cytometry was used to detect the subsets of T lymphocytes in the peripheral blood of mice and the expression of PD-1 on its surface. Results: Beta diversity analysis showed that the vaginal flora of the CON group and the CCM group were significantly different in species composition and relative abundance of each species. The dominant bacteria in the CON group were Lactobacillus, while the figure in the CCM group converted to Pasteurella and Helicobacter. The mean expression of PD-1 on the surface of T cells in mice in the CCM group was 12.78%, which was significantly higher than that in the CON group (10.45%) (P<0.05). The mean of the total number of T cells (CD3+T cells) and the number of CD8+T cells in the CCM group were 38.78% and 11.98%, respectively, which were significantly lower than those in the CON group (51.37% and 20.08%) (P<0.05). Conclusion: Cervical cancer can cause vaginal flora disorder. There may be a certain correlation between the vaginal flora disorder and the high expression of PD-1 on the surface of T cells, suggesting that there may be a new regulatory mechanism for the immune escape in cervical cancer.
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@#Objective: To investigate the function of anti-PD-1 (scFv)/IL-15/IL-15Rα-sushi fusion protein (PD-S15) to specifically bind to PD-1 in vitro and to explore its effect on NK/T cell proliferation. Methods: The human anti-PD-1 (scFv) gene sequence and human IL-15/IL-15Rα-sushi fusion gene sequence were synthesized chemically. The recombinant expression plasmid pUC57-PD-S15 was constructed by enzyme digestion and ligation of the two target genes, and then transiently transfected into HEK293T cells by lipofectamineTM 2000. The supernatants of cell culture medium were acquired, and the expression of PD-S15 fusion protein in cell culture supernatants was detected by Wb assay. PBMCs and TILs were cultured in mediums with different proportion of PD-S15/X-VIVOTM15, respectively. Then, the capacity of PD-S15 fusion protein to bind to PD-1 in vitro and its effect on the proliferation of PBMCs and the proportion of CD3+CD8+, CD3+CD4+ and CD3-CD56+ subsets were detected by flow cytometry. The effect of PD-S15 fusion protein on the proliferation of TILs was detected by cytometry. Results: The successful construction of pUC57-PD-S15 eukaryotic expression plasmid was confirmed by double enzyme digestion and sequencing, and then successfully transfected into HEK293T cells. The relative molecular weight of the target protein was approximately 55 000, and was in line with expectations. PD-S15 fusion protein could specifically combine with PD-1 in vitro (P<0.05) and stimulate NK/T cell proliferation (P<0.05). Compared with classical TILs culture method, the efficiency of activation and amplification of T cells in vitro by PD-S15 culturemethodwasbetter (P<0.01). Conclusion: PD-S15 fusion protein can specifically target PD-1 and rapidly expand NK/T cells in vitro, which lays a foundation for the selective expansion of CD8+PD-1+ antigen-specific T lymphocytes from tumor tissues and even peripheral blood.