NO179127B - Method for pasteurizing blood plasma and mixing for its execution - Google Patents

Abstract

Composition for stabilizing blood plasma, whole or lacking cryoproteins, during pasteurization. The composition according to the invention is used for pasteurizing substantial volumes of plasma (up to several hundreds of litres). The invention also concerns a process for the pasteurization of plasma using said stabilizing composition. The pasteurized plasma obtained is for therapeutic use.

Description

The present invention relates to a method for pasteurizing blood plasma and a mixture for carrying out the method.

These and other features of the invention appear in the patent claims.

The mixture according to the invention makes it possible to stabilize blood plasma during pasteurisation. The plasma is particularly suitable in connection with substitution therapies for plasma and blood coagulation factors V, XI and XIII.

Total human plasma or human plasma without cryoproteins is still used as replacement therapy for people with severe burns and individuals who are seriously injured or who have undergone major operations, i.e. in all cases where the patients have undergone a significant fluid loss.

For this type of treatment, plasma from individual donations is generally used, from healthy individuals who have undergone tests to rule out any risk of transmission of viral diseases. However, this procedure does not make it possible to avoid the risk of viral contamination in the pre-serological stage, in particular the various hepatitis viruses and the AIDS virus.

It would thus be advantageous to develop a method for virus inactivation that does not affect the plasma's various biological functions.

It has been clearly shown that the hepatitis B virus was completely inactivated by heating at 60°C for ten hours in the presence of 0.5 M sodium citrate (Tabor et al. Thrombosis Res. 22, 1981, 233-238). However, this treatment leads to a loss of biological activity in the case of certain plasma proteins (Tabor et al. and Barrowcliffe et al. Fr. J. Haemotology 55, 1983, 37-46).

It has been possible to subject various proteins of therapeutic value purified from blood plasma to conventional pasteurization at 60°C for ten hours in the presence of various stabilizers. However, it should be noted that molecules that stabilize one biological activity may be completely without effect on other activities.

Albumin can e.g. is stabilized by means of acetyltryptophan and caprylate (Gellis et al. J. Clin. Invest. 27, 1948,

239 - 244) while these stabilizers have no effect on plasminogen. Thrombin can be stabilized by high concentrations of sugars (Seegers. Arch. Biochem. 3, 1944, 363-367), while these do not protect prothrombin. The addition of an amino acid and a sugar has given good results with factor VIII and antithrombin III (see patent document DE 29.16.711).

EPO patent 0 035 2 04 shows stabilization of oc-anti-trypsin, antithrombin III, prekallikrein, fibronectin and Factor VIII in the presence of a polyol, the only example of the latter being sucrose. However, the patent document shows that Factor IX and prekallikrein lose all their therapeutic activity under the same conditions.

These various elements in conjunction with experimental data confirm the generally accepted idea that virus inactivation of total plasma (fresh plasma, frozen fresh plasma or cryoprecipitated supernatant) cannot be achieved by pasteurization.

As there is still a medical need for total plasma, an attempt has been made to develop a mixture which ensures simultaneous protection of the biological activity of all the therapeutic factors of interest against denaturation during pasteurisation.

As it has been observed that sorbitol gave a certain degree of protection against thermal denaturation, but where the results varied from one plasma sample to another, and with low yields, a search has been made for various additives which, when mixed with sorbitol, could increase its stabilizing ability.

The mixture in accordance with the present invention consists of sorbitol, calcium chloride, heparin and lysine, the sorbitol concentration being between 500 and 800 g/l, the heparin concentration being between 100 and 1000 U/l, the calcium chloride concentration being between 3 and 5 mM, and the lysine concentration is between 1 and 10 g/l. The concentrations of the various components are the final concentration in the plasma to be pasteurized.

However, the sorbitol concentration is preferably 600 g/l, the heparin concentration is preferably 500 U/ml, the lysine concentration is preferably 4 g/l, and the CaCl2 concentration is preferably 4 mM.

The mixture according to the invention is added to fresh plasma or frozen-thawed fresh plasma, or to the cryoprecipitated protein-free plasma before the latter is subjected to pasteurization with heating at 60°C ± 1°C for ten hours.

After pasteurization, the temperature is continuously lowered to 20°C and the solution is subjected to dialysis to remove sorbitol and heparin. The dialysis buffer has a pH of 7 and contains sodium citrate in a concentration between 4 and 10 mM, 4 mM calcium chloride, 0.13 M sodium chloride and lysine in a concentration of 4 g/l. Dialysis buffers with other compositions can also be used when required. The solution is then concentrated to restore the physiological dose of the plasma proteins. The obtained solution is subjected to sterile filtration, it is distributed, after which it is frozen or freeze-dried.

The method according to the invention for pasteurizing blood plasma is characterized by the fact that sorbitol, heparin, calcium chloride and lysine are added to the plasma before the heating step, after which heparin and sorbitol are removed by dialysis.

This method is particularly advantageous because it can be applied to large quantities of plasma obtained from a number of different collections. More specifically, when pasteurizing boats of 100 - 200 1 or more, it is possible to guarantee that the batches have consistent quality after carrying out appropriate tests.

Furthermore, the plasma batches pasteurized using the method according to the invention can also serve as substitution products in patients with missing coagulation factors and where there are no purified concentrates such as Factor V, Factor XI or Factor XIII.

The pasteurized plasma solutions obtained using the method according to the invention are suitable for the treatment of deficiencies with respect to coagulation factors V, XI and XIII and for substitution therapies requiring total plasma or cryoprecipitate supernatant.

The following example describes an embodiment of the invention.

EXAMPLE

Heparin (1000 U), lysine is added to two liters of thawed plasma

(8 g) and calcium chloride (220 mg). The two latter products are added as salts in powder form. The plasma is gently stirred. 1200 g of undissolved sorbitol is then gradually poured in.

Pasteurization is carried out in a 5 liter container with heating at 60°C for ten hours using a water bath or in a thermostatically controlled tank. After pasteurization, sorbitol and heparin are removed by dialysis with an artificial kidney or an ultrafiltration system such as the Pellicon system on cassettes, using a citrate buffer containing lysine at a concentration of 4 g/l, 4 mM CaCl2 and 0.13 M NaCl. The dialysis can be followed by concentration using the same equipment to bring the ratios of coagulation factors back to about 1 U/ml as for a good quality therapeutic plasma. The product is dialysed at an osmolarity of 370 mosmol/1 and at a pH of 7. The product is then sterile filtered using e.g. a Milli-pack filter 40 (Millipore) with 0.22 µm pores. The product is then placed in plastic containers for freezing, or in bottles for freeze-drying.

Plasma stabilization thus makes it possible to obtain the following yields, in relation to (as indicated in the following by "versus") a control product containing only lysine and sorbitol:

No signs of activation of the coagulation factors in the presence of the above-mentioned amount of calcium have been observed. The ratio between bovine FVII/coagulant FVII is thus 0.95 against 1.09 for the control product. The stability tested by measuring the activity of FVIII after the product had been stored for 24 hours in a liquid state and at ambient temperature is not adversely affected by comparison with the control sample (recovery of 100% activity). This is in accordance with a PKA of < 2% for the pasteurized products and the control products.

In addition, tests on rats through intravenous injection of the thus pasteurized plasma indicated the absence of a hypertensive effect and produced no change in heart rhythm.

Claims (4)

1. Method for pasteurizing blood plasma, characterized in that sorbitol, heparin, calcium chloride and lysine are added to the plasma before the heating step, after which heparin and sorbitol are removed by dialysis. 2. Method as stated in claim 1, characterized in that the dialysis is carried out at pH 7 against a buffer solution containing sodium citrate in a concentration between 4 and 10 mM, 4 mM calcium chloride, 0.13 M sodium chloride and lysine in a concentration of 4 g/ l. 3. Method as stated in claim 1 or 2, characterized in that it can be applied to plasma volumes between one liter and several hundred litres. 4. Mixture for carrying out the method according to claim 1, characterized in that it consists of sorbitol, heparin, calcium chloride and lysine, the sorbitol concentration being between 500 and 800 g/l, the heparin concentration being between 100 and 1000 U/l, the calcium chloride concentration -tration is between 3 and 5 mM, and the lysine concentration is between 1 and 10 g/l.