RU2482870C1 - Agent inducing hemopoietic stem cell differentiation into thrombocytes - Google Patents

Abstract

FIELD: medicine.

SUBSTANCE: invention refers to medicine. What is declared is an agent inducing the hematopoietic stem cell differentiation into thrombocytes, representing a recombinant human cyclophilin A (rhCfA).

EFFECT: invention provides the extended range of products for specified application.

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Description

The invention relates to the field of medicine.

The use of chemotherapy in cancer patients leads to damage and death of hematopoietic cells of the bone marrow with a decrease in the number of platelets in the peripheral blood. Thrombocytopenia is a serious problem in the treatment of cancer patients (Lorusso D, Ferrandina G, Greggi S, Gadducci A, Pignata S, Tateo S, Biamonte R, Manzione L, Di Vagno G, Ferrau 'F, Scambia G. // Phase III multicenter randomized trial of amifostine as cytoprotectant in first-line chemotherapy in ovarian cancer patients. Ann. Oncology. 2003 Jul; 14 (7): 1086-93).

A limited number of agents are known to promote platelet differentiation. Closest to the claimed agent is thrombopoietin (prototype). Thrombopoietin is a hormone that induces the differentiation of a megakaryocytic germ from bone marrow stem cells and affects the proliferation, maturation and differentiation of megakaryocytes and platelet formation (Nagahisa H, Nagata Y, Ohnuki T, Osada M, Nagasawa T, Abe T, Todokoro K. // Bone marrow stromal cells produce thrombopoietin and stimulate megakaryocyte growth and maturation but suppress proplatelet formation. Blood. 1996 Feb 15; 87 (4): 1309-16).

The objective of the invention is to expand the range of agents that induce platelet differentiation. The problem is solved by the fact that a new tool is proposed that induces platelet differentiation, which is a recombinant human cyclophilin A (rhtsfA).

RFCfA is known as a protein with a molecular weight of 18 kD, present in various tissues, enhances the migration of stem cells, precursors of dendritic cells, granulocytes and lymphocytes from bone marrow to the periphery, and promotes the differentiation of dendritic cells and granulocytes (Khromykh LM, Kulikova NL, Anfalova TV et al . // Cyclophilin A produced by thymocytes regulates the migration of murine bone marrow cells. Cell Immunol. - 2007. - vol. 249 (1). - p. 46-53; Bharadwaj U, Zhang R, Yang H, Li M, Doan LX, Chen C, Yao Q. // Effects of cyclophilin A on myeloblastic cell line KG-1 derived dendritic like cells (DLC) through p38 MAP kinase activation. J Surg Res. 2005 Jul 1; 127 (1): 29- 38; RF Patent No. 2370277).

RFCfA enhances the adhesive properties of platelets (RF Patent No. 2435607). To accomplish this task, the effect of rhcfA on the differentiation of stem cells from leukapheresis concentrate and bone marrow of cancer patients after chemo-radiation therapy and healthy donors was evaluated. Platelet cell differentiation was evaluated by expression of the marker CD61, which is present at all stages of platelet formation from stem to mature cells.

Escherichia coli BL21 cells transformed with the plasmid pCyPAwt / pGEX-2TK (M. Bukrinsky Albert Einstein College of Medicine of Yeshiva University, USA) were used to obtain rhcfA. The quality of the rhcfA obtained was evaluated using Laemmli SDS-PAAG (U. K. Laemmli. Cleavage of Structural Proteins during the Assembly of the Head of Bacteriophage T4. Nature, 1970; V.227, P.680-685). The concentration of rfCfA was determined by the Bradford method (Bradford, M. M. (1976) A Rapid and Sensitive Method for the Quantitation of Microgram Quantities of Protein Utilizing the Principle of Protein-Dye Binding. Anal. Biochem. 72: 248-254). The identification of rfcPA was carried out using Wetstern-blott analysis (Gershoni JM, Palade GE. Electroblotting of proteins from polyacrylamide gels. Methods Mol Biol. 2004; 244: 345-352) using rabbit antibodies to rfcA (e-Biosciences). The purity of the obtained rhcfA was more than 98%.

For the study, leukapheresis concentrate was used, which is a fraction of peripheral blood cells with a predominance of mononuclear cells. Leukapheresis concentrate was obtained from five cancer patients after chemo-radiation therapy by separation of peripheral blood cells.

The bone marrow of three cancer patients and three healthy donors were used as samples.

In order to mobilize hematopoietic stem cells, patients were previously stimulated with hematopoiesis with granulocyte colony stimulating factor (G-CSF) in a standard dose of 5 μg / kg for 3-14 days. The number of CD34 ⁺ stem cells in aliquots of samples of lenkapheresis concentrate varied from 0.25% to 1.3%, in aliquots of bone marrow samples from 2.1% to 5.8%.

Human blood and bone marrow cells were cultured at a concentration of 1 × 10 ⁶ / ml in alpha-MEM (for blood cells, Gibco) and IMDM (for bone marrow, Gibco) nutrient medium supplemented with 20% fetal calf serum, 2-mercaptoethanol 5 × 10 ^-5 M, L-glutamine 2 mM and cytran 100 μg / ml. Cell cultivation was carried out at a temperature of 37 ° C in the presence of 5% CO ₂ in plastic 24-well plates (Corning) for 5 days. The concentration of rhcfA was 10.0 μg / ml.

Cell marker analysis was performed using a Faxcanto II flow cytometer (Beckton Dickenson) using fluorescently labeled anti-CD61Fitc antibodies (E-Bioscience). Control markers were set according to isotypic control: anti-IgG Fitc. To exclude nonspecific staining, before staining with fluorescent antibodies, human cells were incubated with donor blood serum (group IV) at a 1:10 dilution. Dead cells were excluded by gating in forward and side scatter parameters (FSC / SSC), as well as inclusion of 7-amino-actinomycin D (Calbiochem, CA). Data was analyzed using the BD FACSDiva (version 6.1.2, Beckton Dickinson) and WinMDI 2.8 (J.Trotter, http://facs.scripps.edu/) programs.

The invention is illustrated in figures 1 and 2.

Figure 1 (A-D) shows the effect of rhcfA on platelet differentiation in leukapheresis concentrate.

In Fig. 1 (A and B), the level of expression of the CD34 marker is indicated on the abscissa axis, and the level of cell granularity on the ordinate axis (SSC) is indicated. On figa presents the identification of stem cells bearing the marker CD34 ⁺ , in the control, and figb - in the presence of rftsfA (outlined region).

Figure 1 (B and D) shows the expression level of the CD61 marker along the abscissa axis, and the expression level of the CD34 marker along the ordinate axis. Figure 1B shows the number of stem cells bearing the CD61 marker in the control (24.69%), and Figure 1G shows the effect of rhCfa (65.81%).

Figure 2 (A-D) shows the effect of rhcfA on platelet differentiation in the bone marrow.

In Fig. 2 (A and B), the level of expression of the CD34 marker is indicated on the abscissa axis, and the level of cell granularity (SSC) on the ordinate axis.

On figa presents the identification of stem cells of the bone marrow in the control and figb - in the presence of rftsfA (outlined region).

Figure 2 (B and D) shows the expression level of the CD61 marker along the abscissa axis, and the expression level of the CD34 marker along the ordinate axis.

Figure 2B shows the number of stem cells bearing the CD61 marker in the control (1.11%), and Figure 2G shows the effect of rhCfa (3.83%).

Thus, it was shown that, under the influence of rccf, there is an increase in the number of stem cells expressing the CD61 marker in leukapheresis concentrate and bone marrow - 3 times relative to control values.

The technical result of the invention

The platelet differentiation inducing agent is human recombinant cyclophilin A.

Claims (1)

A tool that induces the differentiation of hematopoietic stem cells into platelets, which is a recombinant human cyclophilin A.

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