RELATED APPLICATION

[0001] This application claims the benefit of and priority to prior filed pending Provisional Application Serial Nos. 61/848,350 and 61/848,349, both filed December 31, 2012, the disclosures of which are hereby incorporated herein by reference in their entirety.

FIELD

[0002] The present invention is directed to formulations for preserving tissue and organ function and more particularly to shelf stable formulations for preserving tissue and organ function, in particular the function of vascular conduits, prior to implantation.

BACKGROUND

[0003] Tissues and organs for implantation or transplantation in a subject are stored extracorporeal^ in liquid formulations that preserve the function of the tissues and organs until implantation. Tissue and organ preserving formulations are known. One formulation of interest is described in U.S. Patent No. 7,981,596, which is incorporated by reference in its entirety. The tissue and organ preserving formulation described in U.S. Patent No. 7,981,596 is generally referred to in the literature as the GALA formulation, referencing glutathione, ascorbic acid and L-arginine. The GALA formulation is based on Hank's balanced saline solution (HBSS), a commercially available physiological salt solution containing D-glucose 1 g/L, calcium chloride (anhydrous) 0.14 g/l, potassium chloride 0.4 g/l, potassium phosphate 0.06 g/l, magnesium chloride hexahydrate 0.1 g/l, magnesium chloride heptahydrate 0.1 g/l, sodium chloride 8 g/l, sodium bicarbonate 0.35 g/l, and sodium phosphate 0.048 g/l. As disclosed in the '596 patent, ascorbic acid (vitamin C), reduced glutathione, L-arginine, and heparin are added to the HBSS. This solution provides free radical scavengers, antioxidants, a nitric oxide (NO) substrate, a reducing agent, an energy source (glucose), an anti-coagulant, and physiological concentrations of electrolytes and buffers. [0004] The shelf life of the GALA formulation is limited due to the instability of various components of the formulation. The relatively short shelf life of the GALA formulation can limit its usefulness. Thus, there is a need to improve the GALA formulation to improve the stability of its components and thereby lengthen its shelf life.

SUMMARY

[0005] Described herein are improvements to the GALA formulation having improved stability and increased shelf life over the original formulation. Also described are methods of using the improved formulations.

[0006] The present invention is premised on the realization that the stability of tissue preservation formulations, particularly the GALA formulation, can be improved by separating the formulation into a first solution having a pH of at least 7 and a second solution having a pH of less than 7. The first solution includes components with improved stability when stored at a pH of 7.0 or above, and the second solution includes components with improved stability when stored at a pH below 7.0. The first solution includes water, a balanced salt solution, a sugar such as D-glucose, and L-arginine at a pH of at least 7.0 and preferably at a pH that ranges from pH 7.0 to about pH 8.5. The second solution includes water, an antioxidant such as ascorbic acid, and a reducing agent such as reduced glutathione at a pH of less than 7.0 and preferably from pH 6.9 to about pH 2.8. At the point of use, the first and second solutions are mixed together to form a final formulation that can be used at a physiological pH of around pH 7.4 to preserve the function of the tissue or organ.

BRIEF DESCRIPTION OF THE DRAWINGS

[0007] The accompanying drawings, which are incorporated in and constitute a part of this specification, illustrate various embodiments of the invention and, together with a general description of the invention given above and the detailed description of the embodiments given below, serve to explain the embodiments of the invention. [0008] FIG. 1 is a perspective view of a multi-chamber bag in accordance with embodiments of the invention.

[0009] FIG. 2 is a perspective view of a kit having a first container and a second container in accordance with embodiments of the invention.

DETAILED DESCRIPTION

[0010] Unless defined otherwise, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. Although any methods and materials similar or equivalent to those described herein can be used in the practice or testing of the present invention, the preferred methods and materials are described. For the purposes of the present invention, the following terms are defined below.

[0011] As used herein, "organ" includes, but is not limited to, the heart, veins, arteries, lungs, liver, pancreas, and the kidneys. Portions of organ are also contemplated.

[0012] As used herein, "sterile water" includes but is not limited to, (a) sterile water for injection, USP, (b) sterile distilled deionized water, and (c) sterile water for irrigation.

[0013] As used herein, "anitoxidant" is a substance that, when present in a mixture or structure containing an oxidizable substrate biological molecule, delays or prevents oxidation of the substrate biological molecule. For example, ascorbic acid is an antioxidant.

[0014] As used herein, "balanced salt solution" is defined as an aqueous solution that is osmotically balanced to prevent acute cell or tissue damage.

[0015] As used herein, "physiological solution" is defined as an aqueous salt solution which is compatible with normal tissue by virtue of being isotonic with normal interstitial fluid.

[0016] As used herein, "graft" is defined as tissue that is transplanted or implanted in part of the body to repair a defect. [0017] As used herein, "cardioplegia" incl udes but is not limited to, paralysis of the heart.

[0018] As used herein, "cellular reducing agent" is defined as a substance that loses electrons easily thereby causing other substance to be reduced chemically.

[0019] The present invention provides a two part tissue preservation kit which ultimately forms a GALA solution, including water, a balanced salt solution, a sugar, L-arginine, ascorbic acid and a cellular reducing agent such as reduced glutathione.

[0020] The stability of the GALA formulation can be improved by separating the formulation into a first solution having a pH of at least 7 and a second solution having a pH of less than 7. The first and second solutions are mixed together to form a final isotonic GALA formulation that can be used at a physiological pH of around pH 7.4 to preserve the function of the tissue or organ.

[0021] The first solution includes components with improved stability when stored at a pH of 7.0 or above. The first solution includes water, a balanced salt solution, a sugar such as a D-glucose, fructose or mannose and L-arginine. The balanced salt solution incl udes salts selected from the following: calcium chloride dihydrate, potassium chloride, potassium phosphate monobasic, magnesium chloride hexahydrate, magnesium sulfate heptahydrate, sodium chloride, sodium bicarbonate, sodium phosphate dibasic heptahydrate and combinations thereof. The balanced salt solution is provided at a concentration that will result in an isotonic solution when the first and second solutions are mixed together. In an exemplary embodiment, the balanced salt solution about 0.14 grams/liter calcium chloride dihydrate, about 0.4 grams/liter potassium chloride, 0.06 grams/liter potassium phosphate monobasic, about 0.1 grams/liter magnesium chloride hexahydrate, about 0.1 grams/liter magnesium sulfate heptahydrate, about 8 grams/liter sodium chloride, about 0.35 grams/liter sodium bicarbonate, and about 0.05 grams/liter sodium phosphate dibasic heptahydrate. [0022] The first solution may have a pH of at least pH 7.0 and preferably a pH that ranges from pH 7.0 to about pH 8.5. In a preferred embodiment, the first solution has a pH of at least pH 8.0 and preferably the pH is in a range from about pH 8.0 to about pH 8.5.

[0023] The second solution includes components with improved stability when stored at a pH below 7.0. The second solution consists of water, an antioxidant such as ascorbic acid, and a cellular reducing agent such as reduced glutathione. The components of the second solution are provided in relative concentrations to result in an isotonic final formulation when the first solution is mixed with the second solution. In an exemplary embodiment, the second solution includes about 0.3106 grams of reduced L-glutathione per 50 milliliters of water and about 0.09 grams of L-ascorbic acid per 50 milliliters of water. The pH of the second solution is less than 7 and preferably from about pH 6.9 to about pH 2.7. In another preferred embodiment, the pH of the second solution is less than about pH 4 and preferably from about pH 4 to about pH 2.7. In another embodiment, the pH of the second solution is in a range from about pH 3.3 to about pH 2.7 and preferably about pH 3.

[0024] In an exemplary embodiment, the volumetric ratio between the first solution and the second solution is about 19:1. In a preferred embodiment, 950 ml of the first solution is mixed with 50 ml of the second solution to result in the final formulation for preserving the function of a tissue or organ.

[0025] The first or second formulations may optionally include an anticoagulant in an amount sufficient to help prevent clotting of blood within the vasculature of a tissue or organ. Exemplary anticoagulants include heparin and hirudin, but other anticoagulants may be used. An exemplary embodiment includes heparin in concentration ranges from about 50 units/liter to about 250 units/liter.

[0026] During use, the first and second solutions are mixed together to form a final formulation that can be used at a physiological pH in a range between about pH 7.2 and about pH 7.6 and preferably about pH 7.4, to preserve the function of the tissue or organ. If the mixture of the first and second solutions does not have a physiological pH in a range between about pH 7.2 and about pH 7.6, the pH of the mixture can be adjusted with a base or acid to the physiological pH.

[0027] Embodiments of the invention may be provided in a kit wherein the first and second solutions are provided in separate compartments or containers that can be mixed at the point of use to result in the final formulation.

[0028] FIG. 1 illustrates a kit including an exemplary container 10 having a first compartment 12 separated from a second compartment 14 by a removable partition that includes a male member 16 and a female member 18. The first solution is maintained in one of the first 12 or second 14 compartments and the second solution is maintained in the other of the first 12 or second 14 compartments. The first and second solutions may be mixed by removing the removable partition, which results in the first and second compartments now forming a single compartment containing the final formulation for preserving tissue function. The mixture can then be used as needed.

[0029] FIG. 2 illustrates an alternative kit having a first container 22 and a second container 24. The first solution is provided in the first container 22 and the second solution is provided in the second container 24. During use, the second solution is transferred from the second container 24 to the first container 22 where the first and second solutions are mixed to form the final formulation for preserving the function of a tissue or organ. The kit may optionally include a preservative, such as a oxygen absorber 26, and a pouch 28 for protecting and optionally storing one or both of the first 22 and second 24 containers. The kit may also optionally include a device, such as a syringe (not shown), for transferring the contents of one of the containers to the other container.

[0030] In the embodiment shown in Figure 2, the first solution is aseptically filled in the first container 24, such as a pre-sterilized Nalgene bottle, which is then secured with a pre-sterilized HDPE screw cap. The first container may be labeled Bottle A. [0031] The second solution is aseptically filled into the second container 26, such as a pre-sterilized borosilicate, Type I, glass vial, which is secured with a pre-sterilized Stelmi septum, which is held in place with a tear-off seal. The tear-off seal is crimped to the bottle using a validated crimping process as the manufacturer's recommended crimp setting. The second container may be labeled Bottle B. Bottle B is de-gassed with Argon gas during the mixing and filling process to reduce the presence of oxygen. Bottle B is then placed in a pouch 28, such as a Mylar pouch filled with Argon gas and an oxygen absorber 28, to reduce oxygen exposure during its shelf life. The bottle and pouch are then labeled.

[0032] The first container 22 containing the first solution and the pouch 28 containing the second container containing the second solution are then placed in a package, such as a cardstock preprinted box. The package insert is also placed in the package and the box is sealed and labeled for distribution.

[0033] Exemplary embodiments of the kit will produce about 1 liter of the final formulation and will be in about 950 milliliters of the first solution and about 50 milliliters of the second solution. While it is expected that the mixture of the first and second solutions provided in the kit will result in a mixture having the desired physiological pH, the kits could optionally include a device for measuring the pH of the mixture, such as litmus paper, and a set of pH adjusting agents, i.e., a base (e.g., 84% aqueous solution of NaHC0 ₃ ) and an acid (e.g., 4N HCI), for adjusting the pH of the mixture to result in a final formulation having the desired physiological pH.

[0034] The following table provides an exemplary formulation to the first and second solutions. [0035] TABLE 1: FIRST SOLUTION (lx)

COMPONENT AMOUNT (g/L)

Calcium chloride dehydrate 0.14

Potassium chloride 0.4

Potassium phosphate, monobasic 0.06

Magnesium chloride, hexahydrate 0.10 Magnesium sulfate, heptahydrate 0.1

Sodium chloride 8.0

Sodium bicarbonate 0.35

Sodium phosphate, dibasic heptahydrate 0.050

D-Glucose 1.0

L-Arginine 0.15

PH 8.30±0.2

Color Clear

[0036] Other salts can be used to provide the active ions as long as the final formulation formed from the mixture of the first and second solutions is isotonic.

[0037] TABLE 2: SECOND SOLUTION (20x)

Color Clear

[0038] The formulations and methods described herein are not limited to use with a particular tissue, organ, or cell type. For example, embodiments of the invention may be used with harvested saphenous veins, epigastric arteries, gastroepiploic arteries, and radial arteries used in coronary bypass grafting. Embodiments of the present invention may also be used to maintain organs and tissue during transplant operations. Is it contemplated that embodiments of the invention may be used with organs and tissues that include, but are not limited to, heart, lung, kidney, brain, muscle, grafts, skin, intestine, bone, teeth, appendages, eyes, and portions thereof. Embodiments of the invention may be used as an in situ tissue or organ preservative. Embodiments of the invention may also be used to wash or bathe tissues and organs that have not been removed from a subject. For example, embodiments of the invention may be used to maintain tissues and organs during cardioplegia. Embodiments of the invention may also be used in emergency procedures where a tissue or organ needs to be bathed in the formulations to preserve its function until surgery or other medical attention can be obtained. In this regard, embodiments of the invention may be available to emergency medical personnel both in hospital settings and "in the field" (i.e., in ambulances or temporary emergency medical facilities).

[0039] EXAMPLE 1

[0040] The first and second solutions were prepared and the stability of the formulations evaluated.

[0041] The first solution was an aqueous solution that included components that are stable at a pH of 7 or higher. The first solution had a final volume of 950 milliliters and included a balanced salt solution and 1 gram per liter D-glucose, 0.15 grams per liter L-arginine and 950 milliliters of sterile water that had been saturated with argon gas. The balanced salt solution includes about 0.14 gram/liter calcium chloride dihydrate, about 0.4 grams/liter potassium chloride, 0.06 grams/liter potassium phosphate monobasic, about 0.1 grams/liter magnesium chloride hexahydrate, about 0.1 grams/liter magnesium sulfate heptahydrate, about 8 grams/liter sodium chloride, about 0.35 grams/liter sodium bicarbonate, and about 0.05 grams/liter sodium phosphate dibasic heptahydrate. The final pH of the first solution was pH 8.3 + 0.2.

[0042] The second solution was an aqueous solution that included components that are stable at a pH of less than 7. The second solution had a final volume of 50 milliliters and included 0.3106 grams of L-glutathione (reduced) and 0.09 grams L-ascorbic acid and 50 milliliters of sterile water. The final pH of the second solution was pH 3.0 + 0.2.

[0043] The first and second solutions were mixed together and the pH was adjusted with an aqueous solution of 84% NaHC0 ₃ or 4 N HCI to pH 7.4 to form 1 liter of the final formulation.

[0044] EXAMPLE 2 [0045] A second solution and the final formulation from Example 1 were analyzed to evaluate the stability of ascorbic acid and reduced glutathione over a period of time at room temperature.

[0046] The final formulation was formed by mixing together the first and second solutions and its pH was adjusted to about 7.4. A separate volume of the second solution, which had a pH of about 3.0, was prepared both according to the procedure of Example 1. The stability of ascorbic acid and the stability of reduced glutathione were determined over a period of time in both solutions. Both the final formulation and the second solution were stored at room temperature.

[0047] The chromatography method developed and employed for this study separated the ascorbic acid and glutathione reproducibly and without any mutual interference between the components or their decomposition products. Two components were detected using electrospray spectrometry in +ve selected ion monitoring mode. In addition L-Ascorbic acid, and L-glutathione were also detected by photo diode array absorbing in the 190-400nm range. The integrated chromatographic intensities of each of the component peaks was a measure of its molar quantity in solution analyzed. The pH, conductivity, and osmolalities were also measured for each sample.

[0048] The stability indicating properties of GALA were evaluated at: 40°C ± 2°C / 75% H±5% Relative Humidity (RH). A qualified stability chamber with uniform and constant temperature and relative humidity was used for storing the product containers. The chamber's thermometer and digital readout were recorded daily. Samples received for the proposed stability study were logged and tracked in a Sample Receipt and Storage Log and maintained at 2-8°C until the commencement of the study. A minimum of twenty one containers of the device from each representative batch of the first and second solutions were placed in the stability chamber maintained at 40°C±2°C / 75%RH±5% RH. This date was recorded as the zero time point. Three containers of each of the first and second solutions were pulled at 0, 5, 9, 15, 30, 50, and 80-day intervals from the stability chamber for testing.

[0049] The rate of decay of ascorbic acid in the second solution having a pH of about 3.0 was about 3 mg per day, while the rate of decay of ascorbic acid in the final formulation having a pH of about 7.4 was about 15 mg per day. The rate of decay of reduced glutathione in the second solution having a pH of about 3.0 was about 3 mg per day, while the rate of decay of reduced glutathione in the final formulation having a pH of about 7.4 was about 6 mg per day. These data demonstrate that the stabilities of both ascorbic acid and reduced glutathione are significantly increased when stored in a separate solution having a pH of about 3.0 when compared to the stability of these compounds when stored in an aqueous solution having a pH of about 7.4.

[0050] While the present invention has been illustrated by the description of specific embodiments thereof, and while the embodiments have been described in considerable detail, it is not intended to restrict or in any way limit the scope of the appended claims to such detail. The various features discussed herein may be used alone or in any combination. Additional advantages and modifications will readily appear to those skilled in the art. The invention in its broader aspects is therefore not limited to the specific details, representative apparatus and methods and illustrative examples shown and described. Accordingly, departures may be made from such details without departing from the scope or spirit of the general inventive concept.

WHAT IS CLAIMED IS: