Use of polyethyleneoxide and hydroxyethylstarch as blood plasma substitutes in the cryopreservation of testis interstitium cells in mice

Purpose of the study: to investigate the impact of hydroxyethyl starch (HES) and polyethylene oxide (PEO) on the indicators of preservation of murine testis interstitial cells (IC) under cryopreservation. Materials and methods. To isolate IC the enzymes were used: 0.2 mg/ml collagenase and 0.1 mg/m...

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Main Authors: O. V. Pakhomov, E. R. Grabovetskaya, N. I. Filimonova, N. V. Dubinina, O. G. Geyderikh
Format: Article
Language:English
Published: Publishing House TRILIST 2020-11-01
Series:Репродуктивная эндокринология
Subjects:
Online Access:http://reproduct-endo.com/article/view/203607
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author O. V. Pakhomov
E. R. Grabovetskaya
N. I. Filimonova
N. V. Dubinina
O. G. Geyderikh
author_facet O. V. Pakhomov
E. R. Grabovetskaya
N. I. Filimonova
N. V. Dubinina
O. G. Geyderikh
author_sort O. V. Pakhomov
collection DOAJ
description Purpose of the study: to investigate the impact of hydroxyethyl starch (HES) and polyethylene oxide (PEO) on the indicators of preservation of murine testis interstitial cells (IC) under cryopreservation. Materials and methods. To isolate IC the enzymes were used: 0.2 mg/ml collagenase and 0.1 mg/ml DNase. The obtained cell suspension was cryopreserved in the solutions that contained 0; 0,7; 1,4; 2,1; 2,8 M of dimethyl sulfoxide (DMSO) and/or 10%, 20% fetal cow serum, 10 mg/ml PEO or HES. The samples (1 ml) were cooled at a rate of 1 °C/min to -80 °C then stored in liquid nitrogen (-196 °C). They were warmed at 37 °C in the water bath. Cryopreservation solution was removed. The number of cells and their preservation were assessed before and after with the assistance of Goryaev’s camera. Viability of IC, Leydig cell preservation and preservation of metabolic activity were measured with trypan blue dye, histochemical staining for 3β-hydroxysteroid dehydrogenase activity. Results. It was shown that 1,4 M DMSO without supplements favored IC preservation. Addition to the cryopreservation solution 10% and 20% of fetal cow serum or 10 mg/ml HES increased total preservation of IC by more than 10% and Leydig cell cryopreservation by an average 15%. HES 10 mg/ml may decrease DMSO concentration to 0,7 M. This combination had the best indicators of total preservation of IC, preservation of viable cells and Leydig cells: 75,8 (53,3; 93,3), 55,6 (45,1; 69,4), 57,1 (40,2;70,3) %, respectively. PEO was ineffective. Conclusion. High-molecular weight synthetic polymers such as HES can substitute protective properties of blood serum under cryopreservation and allow decreasing effective concentration of permeable cryoprotective such as DMSO.
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spelling doaj.art-2d42798222474dba962b97d26a0a8ec42022-12-21T18:21:13ZengPublishing House TRILISTРепродуктивная эндокринология2309-41172411-12952020-11-01055677110.18370/2309-4117.2020.55.67-71203607Use of polyethyleneoxide and hydroxyethylstarch as blood plasma substitutes in the cryopreservation of testis interstitium cells in miceO. V. Pakhomov0E. R. Grabovetskaya1N. I. Filimonova2N. V. Dubinina3O. G. Geyderikh4Institute for Problems of Cryobiology and Cryomedicine of the NAS of Ukraine; V.N. Karazin Kharkiv National University; Private Higher Education Institution “Kharkiv International Medical University”, KharkivV.N. Karazin Kharkiv National University, KharkivNational University of Pharmacy of the MoH of Ukraine, KharkivNational University of Pharmacy of the MoH of Ukraine, KharkivNational University of Pharmacy of the MoH of Ukraine, KharkivPurpose of the study: to investigate the impact of hydroxyethyl starch (HES) and polyethylene oxide (PEO) on the indicators of preservation of murine testis interstitial cells (IC) under cryopreservation. Materials and methods. To isolate IC the enzymes were used: 0.2 mg/ml collagenase and 0.1 mg/ml DNase. The obtained cell suspension was cryopreserved in the solutions that contained 0; 0,7; 1,4; 2,1; 2,8 M of dimethyl sulfoxide (DMSO) and/or 10%, 20% fetal cow serum, 10 mg/ml PEO or HES. The samples (1 ml) were cooled at a rate of 1 °C/min to -80 °C then stored in liquid nitrogen (-196 °C). They were warmed at 37 °C in the water bath. Cryopreservation solution was removed. The number of cells and their preservation were assessed before and after with the assistance of Goryaev’s camera. Viability of IC, Leydig cell preservation and preservation of metabolic activity were measured with trypan blue dye, histochemical staining for 3β-hydroxysteroid dehydrogenase activity. Results. It was shown that 1,4 M DMSO without supplements favored IC preservation. Addition to the cryopreservation solution 10% and 20% of fetal cow serum or 10 mg/ml HES increased total preservation of IC by more than 10% and Leydig cell cryopreservation by an average 15%. HES 10 mg/ml may decrease DMSO concentration to 0,7 M. This combination had the best indicators of total preservation of IC, preservation of viable cells and Leydig cells: 75,8 (53,3; 93,3), 55,6 (45,1; 69,4), 57,1 (40,2;70,3) %, respectively. PEO was ineffective. Conclusion. High-molecular weight synthetic polymers such as HES can substitute protective properties of blood serum under cryopreservation and allow decreasing effective concentration of permeable cryoprotective such as DMSO.http://reproduct-endo.com/article/view/203607cryopreservationleydig cellstestespolyethylene oxidehydroxyethyl starch
spellingShingle O. V. Pakhomov
E. R. Grabovetskaya
N. I. Filimonova
N. V. Dubinina
O. G. Geyderikh
Use of polyethyleneoxide and hydroxyethylstarch as blood plasma substitutes in the cryopreservation of testis interstitium cells in mice
Репродуктивная эндокринология
cryopreservation
leydig cells
testes
polyethylene oxide
hydroxyethyl starch
title Use of polyethyleneoxide and hydroxyethylstarch as blood plasma substitutes in the cryopreservation of testis interstitium cells in mice
title_full Use of polyethyleneoxide and hydroxyethylstarch as blood plasma substitutes in the cryopreservation of testis interstitium cells in mice
title_fullStr Use of polyethyleneoxide and hydroxyethylstarch as blood plasma substitutes in the cryopreservation of testis interstitium cells in mice
title_full_unstemmed Use of polyethyleneoxide and hydroxyethylstarch as blood plasma substitutes in the cryopreservation of testis interstitium cells in mice
title_short Use of polyethyleneoxide and hydroxyethylstarch as blood plasma substitutes in the cryopreservation of testis interstitium cells in mice
title_sort use of polyethyleneoxide and hydroxyethylstarch as blood plasma substitutes in the cryopreservation of testis interstitium cells in mice
topic cryopreservation
leydig cells
testes
polyethylene oxide
hydroxyethyl starch
url http://reproduct-endo.com/article/view/203607
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