# Unraveling resistance mechanisms to the novel nucleoside analog RX-3117 in lung cancer: insights into DNA repair, cell cycle dysregulation and targeting PKMYT1 for improved therapy

**Authors:** Mahrou Vahabi, Geng Xu, Dzjemma Sarkisjan, Btissame El Hassouni, Giulia Mantini, Valentina Donati, Bing Wang, Giulia Lencioni, Richard J. Honeywell, Dongmei Deng, Sabrina Strano, Godefridus J. Peters, Giovanni Blandino, Elisa Giovannetti

PMC · DOI: 10.1186/s13046-025-03470-z · 2025-07-24

## TL;DR

This study explores how lung cancer cells become resistant to RX-3117 and identifies PKMYT1 as a potential target to improve treatment.

## Contribution

The study is the first to identify DNA repair and cell cycle dysregulation as resistance mechanisms and highlights PKMYT1 as a novel therapeutic target.

## Key findings

- RX-3117-resistant cells showed reduced nucleotide accumulation but not due to metabolic enzyme downregulation.
- CRISPR-Cas9 screening identified DNA repair and cell cycle genes as key to RX-3117 sensitivity.
- PKMYT1 inhibition synergized with RX-3117 and showed promise in patients with high PKMYT1 expression.

## Abstract

Nucleoside analogues are crucial in treating non-small cell lung cancer (NSCLC), but resistance hampers patient outcomes. The cytidine analogue RX-3117 shows promise in gemcitabine-resistant cancers, yet mechanisms underlying acquired resistance to this drug remain unexplored. This study includes a comprehensive investigation into RX-3117 resistance mechanisms by leveraging new preclinical models and cutting-edge genomic tools, including a CRISPR-Cas9 knockout screen and transcriptomics.

NSCLC cell lines A549 and SW1573 were exposed to stepwise increasing concentrations of RX-3117 to establish stable resistant subclones, confirmed by SRB and clonogenic assays. Intracellular RX-3117 nucleotide levels were measured via LC/MS-MS, prompting the evaluation and modulation of the expression of key metabolic enzymes by Western blot and siRNA. A CRISPR-Cas9 screen identified genes whose loss increased RX-3117 sensitivity, while RNA-sequencing with differential expression analyses revealed resistance-related pathways, further investigated through cell cycle distribution, knock-out, and ELISA assays.

Resistant clones exhibited decreased accumulation of RX-3117 nucleotides, which however, was not associated to reduced expression of activation enzymes (UCK2, UMPK, CMPK, NME1/NDPK, RR1 and RR2). Instead, increased expression was observed in certain DNA repair and deactivation enzymes (NT5C3) but pharmacological inhibition and silencing of the latter did not circumvent resistance. Remarkably, a comprehensive approach with CRISPR-Cas9 screen highlighted DNA-repair and cell cycle determinants as key sensitizing genes. XL-PCR and RNA-sequencing confirmed aberrations in DNA-repair and pathways involved in cell cycle regulation. Knock-out and pharmacological inhibition validated the role of PKMYT1, a protein kinase involved in G2/M transition and genomic stability. RX-3117-resistant A549 cells showed enhanced sensitivity to the PKMYT1 inhibitor lunresertib and its synergism with RX-3117, suggesting further studies, especially in patients with high PKMYT1 expression who have significantly shorter survival rates, as observed in public databases and validated in an internal cohort of NSCLC patients.

By integrating CRISPR-Cas9 with functional assays and transcriptomics, our study established a framework for decoding resistance mechanisms and highlights potential therapeutic strategies to enhance RX-3117 efficacy in NSCLC. We demonstrated for the first time that aberrant DNA repair and cell cycle dysregulation led resistance, identifying PKMYT1 as a promising target.

The online version contains supplementary material available at 10.1186/s13046-025-03470-z.

## Linked entities

- **Genes:** UCK2 (uridine-cytidine kinase 2) [NCBI Gene 7371], UCK2 (uridine-cytidine kinase 2) [NCBI Gene 7371], CMPK1 (cytidine/uridine monophosphate kinase 1) [NCBI Gene 51727], NME1 (NME/NM23 nucleoside diphosphate kinase 1) [NCBI Gene 4830], awd (abnormal wing discs) [NCBI Gene 43739], RRM1 (ribonucleotide reductase catalytic subunit M1) [NCBI Gene 6240], RRM2 (ribonucleotide reductase regulatory subunit M2) [NCBI Gene 6241], NT5C3A (5'-nucleotidase, cytosolic IIIA) [NCBI Gene 51251], PKMYT1 (protein kinase, membrane associated tyrosine/threonine 1) [NCBI Gene 9088]
- **Proteins:** PKMYT1 (protein kinase, membrane associated tyrosine/threonine 1)
- **Chemicals:** RX-3117 (PubChem CID 3008319), lunresertib (PubChem CID 156869388)
- **Diseases:** non-small cell lung cancer (MONDO:0005233), lung cancer (MONDO:0005138)

## Full-text entities

- **Genes:** UCK2 (uridine-cytidine kinase 2) [NCBI Gene 7371] {aka TSA903, UK, UMPK}, NME1 (NME/NM23 nucleoside diphosphate kinase 1) [NCBI Gene 4830] {aka AWD, GAAD, NB, NBS, NDK1, NDKA}, CMPK1 (cytidine/uridine monophosphate kinase 1) [NCBI Gene 51727] {aka CK, CMK, CMPK, UMK, UMP-CMPK, UMPK}, RRM1 (ribonucleotide reductase catalytic subunit M1) [NCBI Gene 6240] {aka PEOB6, R1, RIR1, RR1}, RRM2 (ribonucleotide reductase regulatory subunit M2) [NCBI Gene 6241] {aka C2orf48, R2, RR2, RR2M}, NT5C3A (5'-nucleotidase, cytosolic IIIA) [NCBI Gene 51251] {aka CNSHA8, NT5C3, P5'N-1, P5N-1, PN-I, POMP}, PKMYT1 (protein kinase, membrane associated tyrosine/threonine 1) [NCBI Gene 9088] {aka MYT1, PPP1R126}
- **Diseases:** NSCLC (MESH:D002289), lung cancer (MESH:D008175), cancers (MESH:D009369)
- **Chemicals:** gemcitabine (MESH:D000093542), cytidine (MESH:D003562), RX-3117 (MESH:C000589325), RX-3117 nucleotide (-), Nucleoside (MESH:D009705)
- **Species:** Homo sapiens (human, species) [taxon 9606]
- **Cell lines:** A549 — Homo sapiens (Human), Lung adenocarcinoma, Cancer cell line (CVCL_0023), SW1573 — Homo sapiens (Human), Minimally invasive lung adenocarcinoma, Cancer cell line (CVCL_1720)

## Figures

12 figures with captions in the complete paper: https://tomesphere.com/paper/PMC12288264/full.md

---
Source: https://tomesphere.com/paper/PMC12288264