A specific anti-cyclin D1 intrabody represses breast cancer cell proliferation by interrupting the cyclin D1-CDK4 interaction

Jialiang Zhao; Yan Wu; Tong Xiao; Cheng Cheng; Tong Zhang; Ziyang Gao; Siyuan Hu; Ze Ren; Xinze Yu; Fang Yang; Guiying Li

doi:10.1007/s10549-023-06866-7

A specific anti-cyclin D1 intrabody represses breast cancer cell proliferation by interrupting the cyclin D1-CDK4 interaction

Breast Cancer Res Treat. 2023 Apr;198(3):555-568. doi: 10.1007/s10549-023-06866-7. Epub 2023 Feb 19.

Authors

Jialiang Zhao^#¹, Yan Wu^#^{1

2}, Tong Xiao¹, Cheng Cheng¹, Tong Zhang¹, Ziyang Gao¹, Siyuan Hu¹, Ze Ren¹, Xinze Yu¹, Fang Yang³, Guiying Li⁴

Affiliations

¹ Key Laboratory for Molecular Enzymology and Engineering of the Ministry of Education, School of Life Sciences, Jilin University, Changchun, 130012, China.
² Medical Research Center, Binzhou Medical University Hospital, Binzhou, 256600, China.
³ Key Laboratory for Molecular Enzymology and Engineering of the Ministry of Education, School of Life Sciences, Jilin University, Changchun, 130012, China. fangyang@jlu.edu.cn.
⁴ Key Laboratory for Molecular Enzymology and Engineering of the Ministry of Education, School of Life Sciences, Jilin University, Changchun, 130012, China. ligy@jlu.edu.cn.

^# Contributed equally.

PMID: 36808524
DOI: 10.1007/s10549-023-06866-7

Abstract

Background: Cyclin D1 overexpression may contribute to development of various cancers, including breast cancer, and thus may serve as a key cancer diagnostic marker and therapeutic target. In our previous study, we generated a cyclin D1-specific single-chain variable fragment antibody (ADκ) from a human semi-synthetic single-chain variable fragment library. ADκ specifically interacted with recombinant and endogenous cyclin D1 proteins through an unknown molecular basis to inhibit HepG2 cell growth and proliferation.

Results: Here, using phage display and in silico protein structure modeling methods combined with cyclin D1 mutational analysis, key residues that bind to ADκ were identified. Notably, residue K112 within the cyclin box was required for cyclin D1-ADκ binding. In order to elucidate the molecular mechanism underlying ADκ anti-tumor effects, a cyclin D1-specific nuclear localization signal-containing intrabody (NLS-ADκ) was constructed. When expressed within cells, NLS-ADκ interacted specifically with cyclin D1 to significantly inhibit cell proliferation, induce G1-phase arrest, and trigger apoptosis of MCF-7 and MDA-MB-231 breast cancer cells. Moreover, the NLS-ADκ-cyclin D1 interaction blocked binding of cyclin D1 to CDK4 and inhibited RB protein phosphorylation, resulting in altered expression of downstream cell proliferation-related target genes.

Conclusion: We identified amino acid residues in cyclin D1 that may play key roles in the ADκ-cyclin D1 interaction. A nuclear localization antibody against cyclin D1 (NLS-ADκ) was constructed and successfully expressed in breast cancer cells. NLS-ADκ exerted tumor suppressor effects via blocking the binding of CDK4 to cyclin D1 and inhibiting phosphorylation of RB. The results presented here demonstrate anti-tumor potential of intrabody-based cyclin D1-targeted breast cancer therapy.

Keywords: Breast cancer; Cell proliferation; Cyclin D1; Epitope; Intrabody; Single-chain variable fragment.

MeSH terms

Breast Neoplasms* / drug therapy
Breast Neoplasms* / genetics
Breast Neoplasms* / pathology
Cell Proliferation
Cyclin D1 / immunology
Cyclin-Dependent Kinase 4 / genetics
Female
G1 Phase / genetics
Humans
Phosphorylation

Substances

CDK4 protein, human
Cyclin-Dependent Kinase 4
Cyclin D1

Abstract

MeSH terms

Substances

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