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COVID-19 cases showed a significant decrease in the number of peripheral CD4+ and CD8+ T cells accompanied by overactivation of cells.1 HHV8-derived viral macrophage inflammatory protein vMIP-II is the only broad-spectrum chemokine receptor inhibitor that binds to three subtribes of chemokine receptors, which can significantly increase the specific cell immune response in infected organisms and have an effect of reducing plasma viral load on the viremia period.2,3,4 Here we report the effect of vMIP-II in COVID-19.
This study included 10 patients and 35 uninfected patients from Wuhan Union Medical College Hospital and Nanyang First People’s Hospital. Lung CT scans before and 1 week after vMIP-II treatment showed the ground glass lesions and white areas of the lungs were significantly alleviated, clinical symptoms were significantly reduced. The examination of convalescent blood samples showed a significant increase in the total number and proportion of lymphocytes (Supplementary Table S1 and Fig. 1a). The median time for the virus to turn negative was 16 (SD ± 2.2) days, which was significantly shorter than that in the conventional treatment group (22 days, SD ± 3.5) (Supplementary Table S2).
In order to explore the mechanism of vMIP-II on the efficacy of COVID-19, we examined the responsiveness of blood PBMCs to S protein in recovering patients. First, we perform the cloning and expression of S protein (Supplementary Fig. S1, 2, 9). S protein had antigenic characteristics to PBMCs. The classification of CD8+ T-cell subgroups based on the PBMCs of convalescent patients showed that the ratios of TCM cells in the vMIP-II treatment and asymptomatic infection groups were significantly higher than that in the symptomatic infection group, although there was no significant difference in the total number of lymphocytes (Supplementary Table S3, Supplementary Fig. S4). There were also differences in the secretion type of PBMC cytokines and the ability to stimulate the proliferation of PBMCs in different groups treated with S protein (Fig. 1b, c). There was consistency between the vMIP-II treatment group and the asymptomatic infection group.
CD8+ T lymphocyte subgroup analysis on normal PBMCs treated with S protein and vMIP-II was performed (Supplementary Table S3, Fig. 1d, e). In the three vMIP-II treatment groups, there was no significant change in the total number of the memory CD8+ T cells, but the number of CD8+ central memory (TCM) cells increased significantly with the dose. In vMIP-II group, the levels of Th1 cytokines (IFN-γ, IL-2) were significantly increased, but the levels of TNF-α and IL-4 were significantly decreased. There were no significant differences in granulysin levels among the groups (Supplementary Fig. S4).
We applied RNA-seq to detect differential CD8+ T cell gene expression in the vMIP-II treatment group (100 ng/mL S protein + 100 ng/mL vMIP-II) and the S protein group (100 ng/mL S protein) (Fig. 1f). A total of 97 significantly differentially expressed genes were screened by the standard. GO ontological analysis and KEGG pathway analysis showed that phosphorylation pathway, TCA cycle and apoptosis regulation were the most abundant GO terms for the three differentially expressed genes (Supplementary Tables S5, S6, S7 and Supplementary Fig. S5a). We selected the differentially expressed genes with fold differences > 3. Ultimately, GNAT1, PI3K, p38mapk, AKT, TSC1, PINK1, LC-3, BCL-2, FAS, CXCR4, CX3CR1, CCR5, CCR7, PK, LDH, and SIRT1 were identified as key target genes for our subsequent research. We used qRT-PCR to verify the differentially expressed genes of these 16 genes (Supplementary Fig. S5b).
The results of gene sequencing and qRT-PCR showed that vMIP-II affected the α subunit of Gi protein in effector CD8+ T cells (the expression of GNAT1 gene was decreased). In response to this, we also carried out Gi α antisense oligodeoxynucleotides assay. Compared with S protein group, the expression of Gi α in effector CD8+ T cells treated with vMIP-II was significantly inhibited (Fig. 1g). vMIP-II affects rapid intracellular calcium ion concentration and induces calcium release from intracellular calcium ion pools (Fig. 1h and Supplementary Fig. S6). In the presence of vMIP-II the phosphorylation levels of PI3K and Akt in the Giα protein-coupled phosphorylation pathway were significantly decreased and the expression level of Dnmt3a, PK protein was also decreased while the protein expression level of LDH was significantly increased (Fig. 1i, j). This suggests that the metabolic mode of ATP in cells has changed.
The effect on cell function was further observed, and the level of cell ROS was detected, the green fluorescence of CD8+ T effector cells treated with vMIP-II was stronger than that in the S protein group (Supplementary Fig. S7). It indicates that mitochondrial damage occurred. To detect the effect of vMIP-II on mitochondrial function in CD8+ T cells, we detected changes in mitochondrial membrane potential in S protein treated CD8+ T cells (Fig. 1k, l), the results showed that the mitochondrial membrane potential decreased. Because the cellular mitochondrial network is affected by the balance of mito proliferation genes and autophagy genes. We detected and found that after vMIP-II treatment, the proliferation gene SIRT1, PGC-1α of CD8+ T effector cell mitochondria were significantly inhibited and mitochondrial autophagy gene LC3-II, LC3-I, PINK1, Parkin were activated. In addition, we also detected that the mitochondrial network was broken (Fig. 1m, n, p). The role of vMIP-II in effector CD8+ T cells is to transform energy ATP metabolism from oxidative phosphorylation to glycolysis by weakening the function and network of mitochondria, which is a characteristic of cell dry transformation.
We further explore the causes of mitochondrial dysfunction. We have found that the inhibition of the phosphorylation pathway will cause the expression of PI3K, AKT to decrease, that is, affecting the PI3K-AKT-mTOR pathway. In order to verify that mitochondrial function is impaired by inhibiting the downstream target protein of mTOR, we used the phosphorylation levels of the downstream target molecules S6K, S6, and 4E-BP1 of mTORC1 as indicators. Western blot analysis found that compared with S protein group CD8+ T cells, the phosphorylation levels of S6K, S6, and 4E-BP1 of the cells treated with vMIP-II decreased significantly at 6 h, and were strongly inhibited at 12 h, which was consistent with that of rapamycin group (Fig. 1o). These results confirm that the damage of mitochondrial function caused by vMIP-II is realized by inhibiting the downstream target protein of mTOR.
In summary, we observed that vMIP-II could significantly improve the lymphocyte decrease of COVID-19. vMIP-II inhibits multiple chemokine receptors and their related phosphorylation signaling pathways. The low level of pathway PI3K-AKT-mTOR reduces the network and function of mitochondria, to change cell energy metabolism to glycolysis, and also affects the activity of methylase Dnmt3a. The reduced phosphorylation leads to the transformation of effector CD8+ T cells into stem cells, producing more CD8+ TCM. This study shows that vMIP-II can reconstruct the cellular immune function lost in acute SARS-CoV-2 infection. The elucidation of the molecular mechanism of vMIP-II increasing CD8+ TCM provides a new strategy for the treatment of COVID-19.
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Acknowledgements
This work was supported by National Natural Science Foundation of China (NSFC Nos. 82073747, 82074133), and Su Yuan biotechnology co. Ltd.
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Li, S., Liu, S., Jiang, Z. et al. Study on the promotion of lymphocytes in patients with COVID-19 by broad-spectrum chemokine receptor inhibitor vMIP-II and its Mechanism of signal transmission in vitro. Sig Transduct Target Ther 6, 104 (2021). https://doi.org/10.1038/s41392-021-00516-4
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DOI: https://doi.org/10.1038/s41392-021-00516-4
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