In situ and in silico modeling of the hematopoiesis-inducing effect of chelidonic acid

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Abstract

The current trend in regenerative medicine, in the context of an aging population, is the search for new ways and means to optimize tissue bioengineering. One of the convenient models for in situ studying bone marrow regeneration is the subcutaneous ectopic osteogenesis test on scaffolds that imitate the architecture of bone tissue. Chelidonic acid (CA), a small molecule, is capable of participating in various cellular processes and metabolic pathways, and it can activate the osteogenic differentiation of mesenchymal stem cells. However, the molecular mechanisms behind the regulatory effects of CA remain unknown. The aim of this study was to investigate the modulatory effect of CA on the in situ formation of hematopoietic foci, as well as to predict target genes and intracellular signalling pathways involved in the hematopoietic activity of CA. An aqueous solution of CA, isolated from an extract of the Saussurea controversa plant. Course (daily for 35 days) oral administration of CA. Ectopic osteogenesis testing in Balb/c mice. Morphometric analysis of histological sections after 45 days and in silico modelling of gene expression with statistical analysis. CA, when administered orally in a low dose (10 mg/kg), threefold increases the normalized area of bone marrow in the composition of bone tissue plates grown in situ in a test of ectopic subcutaneous osteogenesis in mice. This effect is associated essentially (a probability of CA activity Pa > 0.5 and a probability of inactivity Pi < 0.5) with enhanced expression of 358 hematopoiesis-related genes, as predicted by in silico analysis. The top list with the highest Pa value included 10 target genes, such as GATA1, CITED2, SFRP1, EP300, LGALS9, VNN1, IL10RB, RARA, CD83, and HMOX1. CA has a significant ability to enhance the reparative remodelling of hematopoietic tissue in situ. The next phase of research will be to test actual target genes and signalling pathways that mediate the regulatory effect of HC on hematopoiesis both in vitro and in vivo, as well as in clinical settings.

About the authors

T. F. Nasibov

Siberian State Medical University

Email: khlusov.ia@ssmu.ru

Laboratory Assistant, Laboratory of Cellular and Microfluidic Technologies

Russian Federation, Tomsk

A. V. Gorokhova

Siberian State Medical University

Email: khlusov.ia@ssmu.ru

Laboratory Assistant, Laboratory of Cellular and Microfluidic Technologies

Russian Federation, Tomsk

E. D. Porokhova

Siberian State Medical University

Email: khlusov.ia@ssmu.ru

Assistant Professor, Department of Morphology and General Pathology

Russian Federation, Tomsk

A. A. Starosvetskaya

Siberian State Medical University

Email: khlusov.ia@ssmu.ru

Student of the Faculty of Medicine and Biology

Russian Federation, Tomsk

U. A. Bariev

Siberian State Medical University

Email: khlusov.ia@ssmu.ru

Student of the Faculty of Medicine

Russian Federation, Tomsk

V. E. Nosov

Siberian State Medical University

Email: khlusov.ia@ssmu.ru

Laboratory Assistant, Department of Normal Physiology

Russian Federation, Tomsk

L. S. Litvinova

Immanuel Kant Baltic Federal University

Email: khlusov.ia@ssmu.ru

PhD, MD (Medicine), Director, Center for Immunology and Cellular Biotechnologies

Russian Federation, Kaliningrad

E. Yu. Avdeeva

Siberian State Medical University

Email: khlusov.ia@ssmu.ru

PhD, MD (Pharmaceutical), Research Associate, Laboratory of Cellular and Microfluidic Technologies

Russian Federation, Tomsk

Mikhail V. Belousov

Siberian State Medical University

Email: khlusov.ia@ssmu.ru

PhD, MD (Pharmaceutical), Leading Research Associate, Laboratory of Cellular and Microfluidic Technologies

Russian Federation, Tomsk

I. A. Khlusov

Siberian State Medical University

Author for correspondence.
Email: khlusov.ia@ssmu.ru

PhD, MD (Medicine), Professor, Chief, Laboratory of Cellular and Microfluidic Technologies

Russian Federation, Tomsk

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Supplementary files

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2. Figure 1. Section of ectopic bone with formed bone marrow inside (A, Control; B, CA_ig)

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3. Figure 2. Graph comparing the normalized bone marrow areas in the study groups

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Copyright (c) 2024 Nasibov T.F., Gorokhova A.V., Porokhova E.D., Starosvetskaya A.A., Bariev U.A., Nosov V.E., Litvinova L.S., Avdeeva E.Y., Белоусов M.V., Khlusov I.A.

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This work is licensed under a Creative Commons Attribution 4.0 International License.

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