Cryopreservation of human cerebral microvascular endothelial cells with glycerol

被引:7
|
作者
Mohammed, Lanah [1 ]
Marquez-Curtis, Leah A. [2 ,3 ]
Elliott, Janet A. W. [2 ,3 ,4 ]
机构
[1] Univ Alberta, Dept Cell Biol, Edmonton, AB, Canada
[2] Univ Alberta, Dept Chem & Mat Engn, Edmonton, AB, Canada
[3] Univ Alberta, Dept Lab Med & Pathol, Edmonton, AB, Canada
[4] Univ Alberta, Dept Chem & Mat Engn, Edmonton, AB T6G 1H9, Canada
关键词
Cryopreservation; Graded freezing; Human cerebral microvascular endothelial; cells; Cooling rate; Glycerol; Membrane integrity; Matrigel tube formation; ZO-1; DIMETHYL-SULFOXIDE DMSO; FREEZING-INJURY; STEM-CELLS; MEMBRANE; PERMEABILITY; MECHANISMS; VIABILITY;
D O I
10.1016/j.cryobiol.2023.104551
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
The cryopreservation of human cerebral microvascular endothelial cells (hCMEC) has facilitated their commercial availability for research studying the blood-brain barrier. The currently employed cryopreservation protocol uses 10% dimethyl sulfoxide (Me2SO) in cell medium, or 5% Me2SO in 95% fetal bovine serum (FBS) as cryoprotective agents (CPAs). However, Me2SO is toxic to cells and FBS is animal-derived and not chemically defined, so reducing the concentrations of these components is desirable. Recently, we showed that cryopreserving hCMEC in cell medium with 5% Me2SO and 6% hydroxyethyl starch (HES) results in over 90% post-thaw cell viability. This previous work was performed using an interrupted slow cooling (graded freezing) approach followed by SYTO13/GelRed staining to assay for membrane integrity. In this paper, we repeated graded freezing of hCMEC in cell medium containing 5% Me2SO and 6% HES, but this time using Calcein AM/ propidium iodide staining to ensure that the stain is an equivalent alternative to SYTO13/GelRed for assessment of cell viability, and that results are comparable to those previously published. Next, using graded freezing experiments and Calcein AM/propidium iodide staining, we examined the effectiveness of non-toxic glycerol as a CPA at different concentrations, loading times, and cooling rates. The cryobiological response of hCMEC was used to develop a protocol that optimizes both the permeating and non-permeating capabilities of glycerol. HCMEC in cell medium loaded with 10% glycerol for 1 h at room temperature, ice nucleated at-5 degrees C and held for 3 min, and then cooled at-1 degrees C/min to-30 degrees C before plunging into liquid nitrogen had post-thaw viability of 87.7% & PLUSMN; 1.8%. Matrigel tube formation assay and immunocytochemical staining of junction protein ZO-1 were carried out on post-thaw hCMEC to ensure that the cryopreserved cells were viable and functional, in addition to being membrane-intact.
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页数:12
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