Combined overexpression of four transcription factors promotes effector T cell dedifferentiation toward early phenotypes

Lijun Yan; Yusheng Ou; Shengfang Xia; Jianqing Huang; Wenfeng Zhang; Hongwei Shao; Han Shen; Huaben Bo; Changli Tao; Jinquan Wang; Fenglin Wu

doi:10.1007/s00251-021-01248-z

Combined overexpression of four transcription factors promotes effector T cell dedifferentiation toward early phenotypes

Immunogenetics. 2022 Apr;74(2):231-244. doi: 10.1007/s00251-021-01248-z. Epub 2022 Jan 10.

Authors

Lijun Yan^#^{1

2}, Yusheng Ou^#^{1

2}, Shengfang Xia^{1

2}, Jianqing Huang^{1

2}, Wenfeng Zhang^{1

2}, Hongwei Shao^{1

2}, Han Shen^{1

2}, Huaben Bo^{1

2}, Changli Tao^{1

2}, Jinquan Wang^{1

2}, Fenglin Wu^{3

4}

Affiliations

¹ Guangdong Province Key Laboratory of Biotechnology Drug Candidates, Guangdong Pharmaceutical University, Guangzhou, China.
² School of Life Sciences and Biopharmaceutics, Guangdong Pharmaceutical University, Guangzhou, China.
³ Guangdong Province Key Laboratory of Biotechnology Drug Candidates, Guangdong Pharmaceutical University, Guangzhou, China. Gdpuwfl@163.com.
⁴ School of Life Sciences and Biopharmaceutics, Guangdong Pharmaceutical University, Guangzhou, China. Gdpuwfl@163.com.

^# Contributed equally.

PMID: 35001141
DOI: 10.1007/s00251-021-01248-z

Abstract

Effector T cells, which are abundant but are short-lived after reinfusion into the body, are generally used for T-cell therapy, and antitumor immunity is typically not maintained over the long term. Genetic modification by early differentiated T cells and reinfusion has been shown to enhance antitumor immunity in vivo. This study overexpressed the characteristic transcription factors of differentiated early T cells by transfecting effector T cells with transcription factor recombinant lentivirus (S6 group: BCL6, EOMES, FOXP1, LEF1, TCF7, KLF7; S1 group: BCL6, EOMES, FOXP1, KLF7; S3 group: BCL6, EOMES, FOXP1, LEF1) to induce a sufficient number of effector T cells to dedifferentiate and optimize the transcription factor system. The results revealed that overexpression of early characteristic transcription factors in effector T cells upregulated the expression of early T cell differentiation markers (CCR7 and CD62L), with the S1 group having the highest expression level, while the rising trend of late differentiation marker (CD45RO) expression was suppressed. Moreover, the expression of early differentiation-related genes (ACTN1, CERS6, BCL2) was significantly increased, while the expression of late differentiation-related genes (KLRG-1) and effector function-related genes (GNLY, GZMB, PRF1) was significantly decreased; this difference in expression was more significant in the S1 group than in the other two experimental groups. The antiapoptotic ability of each experimental group was significantly enhanced, while the secretion ability of TNF-α and IFN-γ was weakened, with the effector cytokine secretion ability of the S1 group being the weakest. Transcriptomic analysis showed that the gene expression profile of each experimental group was significantly different from that of the control group, with differences in the gene expression pattern and number of differentially expressed genes in the S1 group compared with the other two experimental groups. The differentially expressed gene enrichment pathways were basically related to the cell cycle, cell division, and immune function. In conclusion, overexpression of early characteristic transcription factors in effector T cells induces their dedifferentiation, and induction of dedifferentiation by the S1 group may be more effective.

Keywords: Dedifferentiation; T lymphocytes; Transcription factor.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

CD8-Positive T-Lymphocytes
Cell Dedifferentiation* / genetics
Cell Differentiation / genetics
Phenotype
T-Lymphocyte Subsets
Transcription Factors* / genetics

Substances

Transcription Factors