What question did this study set out to answer?

The study aims to clarify how YTHDF2 regulates PD-L1 expression in colorectal cancer and its implications for therapy.

March 25, 2026Open Access

Reduced YTHDF2 inhibits PD-L1 expression by stabilizing m6A-containing SPOP mRNA in colorectal cancer

Key Points

The study aims to clarify how YTHDF2 regulates PD-L1 expression in colorectal cancer and its implications for therapy.
Expression profiling of CRC samples and online databases
Subcutaneous mouse model to study YTHDF2 effects
Western blots and flow cytometry for protein analysis
RNA sequencing and MeRIP to confirm m6A methylation levels
Dual-luciferase reporter to verify SPOP mRNA stability
YTHDF2 was found to be upregulated in CRC tissues, correlating with worse prognosis
Knocking down YTHDF2 reduced PD-L1 expression and PD-1/PD-L1 binding
Increased stability of SPOP mRNA was observed after YTHDF2 knockdown, leading to decreased PD-L1 levels
YTHDF2 influences CRC growth through PD-L1 modulation, highlighting a potential therapeutic target

Abstract

Abstract Colorectal cancer (CRC) is one of the most frequently diagnosed malignant tumors. However, clear evidence explaining the regulatory mechanisms of programmed death ligand 1 (PD-L1) in CRC has been limited. To illustrate the function of YTH N 6 -methyladenosine (m 6 A) RNA binding protein F2 (YTHDF2), we conducted a comprehensive evaluation of expression profiling datasets from online databases and clinical samples. We used a subcutaneous immunodeficient mouse model to investigate the impact of YTHDF2 on CRC. Western blots, flow cytometry, PD-1/PD-L1 binding assay, and cell killing assay were used to assess the relationship between YTHDF2 and PD-L1. We used RNA sequencing, along with methylated RNA immunoprecipitation (MeRIP) and RNA binding protein immunoprecipitation (RIP) sequencing to analyze mRNA expression, m 6 A methylation levels, and YTHDF2 target transcripts. The m 6 A methylation locations of mRNAs were verified using sequence-based RNA adenosine methylation site predictor (SRAMP), MeRIP-qRT-PCR, RIP-qRT-PCR, and a dual-luciferase reporter system. YTHDF2 was upregulated in CRC tissues, and patients with higher YTHDF2 expression had a worse prognosis. The in vivo model showed that YTHDF2 promoted CRC growth, whereas in vitro experiments showed that inhibiting YTHDF2 expression did not affect cell proliferation, migration, or invasion. Mechanistically, interference with YTHDF2 reduced PD-L1 expression and the binding ability between PD-1 and PD-L1. The use of RNA-seq, MeRIP-seq, RIP-seq, and bioinformatics tools confirmed that the speckle type BTB/POZ protein ( SPOP ) mRNA was a YTHDF2 target and validated its m 6 A methylation sites. After YTHDF2 knockdown, SPOP mRNA stability increased, causing an increase in SPOP expression and a decrease in PD-L1 expression. This study demonstrated that YTHDF2 might upregulate PD-L1 expression by destabilizing m 6 A-containing SPOP mRNA and promote CRC development. The biological effect of the YTHDF2-SPOP-PD-L1 axis presented a promising target for CRC treatment and provided an approach to enhance the efficacy of anti-PD-1/PD-L1 therapy.

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Cite This Study

Xu et al. (Mon,) studied this question.

synapsesocial.com/papers/69c37afeb34aaaeb1a67d0e0 https://doi.org/https://doi.org/10.1038/s41419-026-08615-2

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