METHOD FOR PRESERVING CELLS

Abstract

The present disclosure relates to a method for preserving free cells, such as blood cells, by freezing in the presence of a nontoxic cryoprotectant, i.e., one that can be administered to a living human or animal organism. The present disclosure thus relates to methods, compositions and kits for freezing and storing non-adherent cells, such as red blood cells, for extended periods of time while preventing the lesions that can occur during the storage thereof and, in the case of red blood cells, while preserving deformability and increasing survival.

Claims

1. A composition comprising non-adherent cells and an isotonic aqueous solution comprising at least one non-toxic cryoprotectant at a concentration of between 4 and 50% by weight/volume (w/v) and selected from albumins.

2. The composition according to claim 1, wherein the cryoprotectant is human serum albumin.

3. The composition according to claim 1, wherein it further comprises a cryoprotective additive selected from sucrose at a concentration of between 0.5 and 5% w/v, trehalose at a concentration of between 0.5 and 5% w/v, glucose at a concentration of between 0.5 and 5% w/v and carboxymethyl cellulose at a concentration of between 0.1 and 1% w/v.

4. The composition according to claim 1, wherein the non-adherent cells are blood cells, preferably red blood cells.

5. A method for preserving non-adherent cells by freezing comprising the steps of: a) suspending said non-adherent cells in a cryopreservation medium composed of an isotonic aqueous solution with at least one non-toxic cryoprotectant at a concentration of between 4 and 50% by weight and selected from albumins; b) optionally, conditioning the mixture obtained in step a); c) directional freezing of the mixture obtained in step a); and d) preservation at a temperature between 79 C. and 197 C., preferably at approximately 80 C.

6. The method for preserving non-adherent cells by freezing according to claim 5, wherein the cryoprotectant is human serum albumin.

7. The method for preserving non-adherent cells by freezing according to claim 5, wherein the cryopreservation medium further comprises a cryoprotective additive selected from sucrose, glucose, trehalose and carboxymethyl cellulose.

8. The method for preserving non-adherent cells by freezing according to claim 5, further comprising thawing the non-adherent cells comprising the steps of: i. contacting the frozen cells with a surface heated to a temperature of between 35 and 45 C.; ii. centrifugation; and iii. suspending the cells from the centrifugation supernatant in a saline solution comprising between 1 and 10% proline.

9. A kit for preserving non-adherent cells comprising at least one sealed device for storing sterile biological fluids and an isotonic aqueous solution comprising at least one non-toxic cryoprotectant at a concentration of between 4 and 50% by weight and selected from albumins and, optionally, a cryoprotective additive such as sucrose, carboxymethyl cellulose, trehalose or glucose.

10. The composition according to claim 2, wherein it further comprises a cryoprotective additive selected from sucrose at a concentration of between 0.5 and 5% w/v, trehalose at a concentration of between 0.5 and 5% w/v, glucose at a concentration of between 0.5 and 5% w/v and carboxymethyl cellulose at a concentration of between 0.1 and 1% w/v.

11. The composition according to claim 2, wherein the non-adherent cells are blood cells, preferably red blood cells.

12. The composition according to claim 3, wherein the non-adherent cells are blood cells, preferably red blood cells.

13. The method for preserving non-adherent cells by freezing according to claim 6, wherein the cryopreservation medium further comprises a cryoprotective additive selected from sucrose, glucose, trehalose and carboxymethyl cellulose.

14. The method for preserving non-adherent cells by freezing according to claim 6, further comprising thawing the non-adherent cells comprising the steps of: i. contacting the frozen cells with a surface heated to a temperature of between 35 and 45 C.; ii. centrifugation; and iii. suspending the cells from the centrifugation supernatant in a saline solution comprising between 1 and 10% proline.

15. The method for preserving non-adherent cells by freezing according to claim 7, further comprising thawing the non-adherent cells comprising the steps of: i. contacting the frozen cells with a surface heated to a temperature of between 35 and 45 C.; ii. centrifugation; and iii. suspending the cells from the centrifugation supernatant in a saline solution comprising between 1 and 10% proline.

Description

BRIEF DESCRIPTION OF THE DRAWINGS

[0047] FIG. 1: Recovery of red blood cells (RBCs) after directional freezing with varying BSA volume fractions (BSA) (0.04, 0.14, and 0.28) at varying translation speeds. Upper panel: Image of centrifuged samples after the freezing-thawing process. The red color is due to hemoglobin released from the lysed cells. Neg, represents the negative control obtained without being frozen. Lower panel: Cell recovery after freezing and thawing.

[0048] FIG. 2: Cell recovery after directional freezing of RBCs (510.sup.9 cells.Math.mL.sup.1) at 100 m.Math.s.sup.1.Math.ns, indicates no significant difference.

[0049] FIGS. 3A-G: SEM and flow cytometry of RBCs after freezing and thawing. RBCs were stained with Calcein-AM for flow cytometry. Negative and positive controls indicate unstained and calcein-stained cells without undergoing freezing. Varying BSA volume fractions and ice front speeds were applied to the experimental groups. Scale bar, 2 m.

[0050] FIGS. 4A-B: (A) Cell size (FSC-A) of the calcein-stained red blood cells. (B) Comparison of the cell size between the positive control (fresh cell) and the cryopreserved cells. Frozen cells with BSA of 0.14 showed a significantly smaller size than fresh cells. ***, indicates P<0.01.

[0051] FIGS. 5A-B: Cell recovery (A) and flow cytometry (B) of RBCs after 106 days of freezer storage.

[0052] FIGS. 6A-B: (A) Cell size (FSC-A) of Calcein-stained RBCs after 106 days of freezer preservation at 80 C. (B) Comparison of the cell size between the positive control (fresh cell) and the cryopreserved cells. ***, indicates a significant difference at P<0.01.

[0053] FIG. 7: Efficiency of resuspension of thawed cells followed by freezing at 100 m.Math.s.sup.1. Positive control, absorbance of hemolysis in deionized H.sub.2O with the same amount of cells compared to that in the presence of BSA.

[0054] FIGS. 8, 9, 10 and 11: Post-freezing cell suspension tests, histograms show the measurement of hemoglobin in the supernatant after suspension.

DETAILED DESCRIPTION

Examples

Freezing Protocol

[0055] a. 5 mL of sheep blood in Alsever's solution (saline solution comprising 2.05% dextrose, 0.8% sodium citrate, 0.055% citric acid, and 0.42% sodium chloride) (1:1) is centrifuged at 600 g, 4 C. for 10 min; [0056] b. The supernatant is removed and a 0.9% NaCl solution is added to restore the initial volume (5 mL); [0057] c. The suspension obtained are centrifuged at 600 g, 4 C. for 10 min; [0058] d. The supernatant is removed and a 0.9% NaCl solution is added to restore the initial volume (5 mL); [0059] e. Steps c and d are repeated once more; [0060] f. The concentration of red blood cells is calculated using a hemacytometer; [0061] g. The cells necessary to obtain a concentration of 10.sup.8 or 1.5*10.sup.9 are transferred into 2 mL of BSA solution (between 4 and 50% by weight); [0062] h. Cell suspensions are frozen in 500 L CoverWell incubation chambers (Grace Bio-Labs) 22 mm40 mm0.5 mm on a thermal gradient of 50 C..Math.mm.sup.1 (passage from the thermal block at +10 C. to the thermal block at 90 C.; gap between blocks 2 mm). The translation speeds of the samples are 10, 50 and 100 m.Math.s.sup.1. [0063] i. After freezing, the chambers containing the frozen cell suspensions are kept at 80 C. (from 1 day to 106 days).

Thawing Protocol

[0064] a. The chambers containing the cells are thawed in contact with a surface at 45 C. for 10-15 s. [0065] b. 200 L of the contents of each chamber are transferred into an eppendorf, and centrifuged under the following conditions: [0066] 1. For BSA concentrations less than or equal to 20%: 3000 rpm, 20 C., 10 min [0067] 2. For BSA concentrations above 20%: 6000 rpm, 20 C., 20 min c. The supernatant is removed and the cells are suspended in a solution of 1% proline, 0.9% NaCl. [0068] d. Steps b and c are repeated twice more for FACS characterization; four more times for SEM characterization. [0069] e. The freezing-thawing efficiency is estimated from the measurement by UV-Vis absorption at 541 nm of the hemoglobin concentration in the supernatant obtained in step b.1 or b.2.

[0070] Other formulations were tested for post-thawing cell resuspension (results correspond to the measurement of hemoglobin in the supernatant after resuspension): [0071] Proline (1, 2, 4, 8, 10%). [0072] Proline (1, 2, 4, 8, 10%) then 4% BSA [0073] (see FIG. 8) [0074] 4% BSA+proline (0.1, 0.5, 1, 2, 5%) [0075] (see FIG. 9) [0076] BSA+PBS [0077] PBS [0078] 0.9% NaCl [0079] BSA+glucose [0080] BSA+glucose+trimethylglycine+proline [0081] BSA+glucose+trimethylglycine+proline+glycine+glutamine [0082] BSA+trimethylglycine+proline+glycine+glutamine [0083] (see FIGS. 10 and 11 where C1: bsa+glucose; C2: C1+betaine+proline; C3: C2+glycine+glutamine; C4: C3-glucose)

[0084] 1% Proline in 0.9% NaCl produces results similar to other proline concentrations, systematically higher than other formulations.

Results

[0085] Increasing the BSA volume fraction (BSA) resulted in improved cell recovery that was further improved by increasing the translation freezing speed implemented (FIG. 1).

[0086] For volume fractions of 0.04 to 0.28, cell recovery increased from 18% to 30% at 10 m.Math.s.sup.1 and from 38% to 95% at 100 m.Math.s.sup.1. For all volume fractions, increasing the translation speed resulted in better cell recovery, in particular for the BSA=0.28 value that allows a three-fold increase when the translation speed varies from 10 to 100 m.Math.s.sup.1. After thawing and centrifugation, unlysed red blood cells (RBCs) were clustered at the bottom of the tube and hemoglobin from the broken cells was released into the supernatant, leading to a red color. For the negative control, the fresh blood sample showed almost no cell hemolysis, as shown by the colorless supernatant. Samples treated under other conditions showed a red color, except for BSA between 0.28 and 50 at 100 m.Math.s.sup.1, confirming the positive role of highly concentrated BSA systems on recovery of RBCs.

[0087] The cell density used in these experiments (10.sup.8 cells mL.sup.1) was 50 times lower than the physiological density (510.sup.9 cells mL.sup.1) of the human body. In the literature, the cell density has a positive effect that is essential for final cryosurvival. To account for this effect, another test was performed with a cell density of 510.sup.9 cells mL.sup.1 at 100 m.Math.s.sup.1 (FIG. 2). Frozen cells with a BSA volume fraction of 0.28 showed the highest recovery (80%), further confirming the beneficial effects of highly concentrated BSA on cell survival during directional freezing. However, a relatively lower survival compared to samples containing 10.sup.8 cells mL.sup.1 was observed, that can be attributed to the increase of mechanical stresses between cells.

Quality of Red Blood Cells

[0088] While the previous experiments allowed to determine the amount of erythrocytes whose membrane integrity was preserved, it is also useful to obtain additional information on the physiological state of the recovered cells. To this end, an observation by scanning electron microscopy and flow cytometry were carried out on the cells after freezing and thawing. It is known from the literature that healthy RBCs have a biconcave shape that gives them great flexibility and a high oxygen transport capacity; FIG. 3A shows that a majority of fresh RBCs have a biconcave disk shape. Cells frozen at 100 m.Math.s.sup.1 in the presence of a low BSA volume fraction (BSA=0.04 and 0.14) showed a shape similar to that of fresh samples (FIGS. 3B-C).

[0089] For the high-volume fraction groups, a majority of thawed cells have a disk shape in the absence of the concave feature, and a small portion of cells have morphological alteration toward a slightly spherical shape (FIG. 3D). Varying the translation speed did not significantly change the shape of RBCs when BSA=0.28 (FIGS. 3E-F). Calcein-AM, a cell-permeable non-fluorescent dye that is converted to green fluorescent calcein by intracellular esterases in living cells, was used for the flow cytometry test. In FIG. 3G, the negative control (unstained fresh cells) and the positive control (stained fresh cells) have apparent distinct fluorescence intensity, which facilitates the determination of the experimental group. Regardless of the experimental conditions (BSA concentration and translation speed), more than 97% of the cells have a high calcein intensity. This indicates that, after resuspension, most of the recovered RBCs have esterase activity and are therefore alive. In other words, the slightly altered shape of RBCs does not affect their esterase activity. In flow cytometry analysis, Forward scatter gating is generally considered an index of cell size [9]. For the experimental groups, thawed RBCs showed a median cell size similar to that of the positive control, except those frozen in the presence of BSA=0.14 (at 100 m.Math.s.sup.1) whose size is slightly smaller (FIGS. 4A-B). Considering both cell recovery and quality, more than 95% of RBCs have intact membranes with metabolic activities and similar cell size compared to the control after being cryopreserved via directional freezing with BSA=0.28 at 100 m.Math.s.sup.1.

[0090] As previously described, the limited lifespan of RBCs, even in the presence of additives (<49 days), leads to a high demand for daily blood donors. Here, cryopreservation of RBCs was carried out by directional freezing, the RBCs were then stored in a freezer at 80 C. for three months (106 days). In FIG. 5A, cell recovery followed the same survival trend as that after one day of preservation. Red blood cell survival could be improved with an increase of BSA content and even more so with higher translation speed. After 106 days, samples prepared with a volume fraction of 0.28 at 100 m.Math.s.sup.1 showed 95% survival comparable to that of samples thawed after 1 day of preservation. Additional calcein staining (FIG. 5B) indicated that more than 98% of cells had esterase activity, regardless of freezing conditions. In all samples, the size of thawed cells was similar to that of the positive control, except for the group with a volume fraction of 0.14 that had a smaller size (FIG. 6). Thus, directional freezing in the presence of BSA (BSA=0.28) allows twice as long preservation in the freezer without significantly affecting cell viability and vitality as the permitted shelf life of the red blood cells (49 days).

[0091] In conventional cryopreservation of RBCs, the deglycerolization process has adverse effects on the final quality of cells. For clinical applications, the efficiency of resuspension of frozen-thawed cells must be considered in order to obtain a highly concentrated cell suspension equivalent to the physiological cell density. In FIG. 7, no hemolysis (absorbance at 541 nm less than 0.005) occurred after resuspension of thawed cells (BSA=0.28, at 100 m.Math.s.sup.1) compared to the positive control, i.e. complete hemolysis of RBCs. In other words, the cells can be cryopreserved in a relatively dilute state, but once needed, these cells could be thawed, concentrated and then mixed in specific solutions without time-consuming and harmful post-purification of the cells, or also subjected to simple centrifugation, which is a substantial advantage of the method of the disclosure.

[0092] Further analysis of esterase-based metabolic activity indicated that more than 95% of RBCs preserved after freezing and thawing are alive, regardless of the experimental conditions. Regarding viability and quality of RBCs, the 0.28 BSA volume fraction group showed good cryosurvival and resulted in a cell size similar to that of the fresh cells. The comparable recovery and viability of RBCs thawed after 1 day and 106 days of storage made it possible to extend the commonly accepted shelf life of RBCs from 49 days to 106 days. Considering the physiological cell density, the low hemolysis rate during resuspension of thawed cells provides a simple tool for enriching RBCs for transfusion.