RU2130069C1 - Method of virus concentrating - Google Patents

Abstract

FIELD: applied virology. SUBSTANCE: invention relates to methods of isolation, purification and modification of viruses and viral preparations i. e. to processes associated with virus concentrating. Method involves virus binding with bioaffinity sorbent containing antibodies raised to virus and immobilized on polymer base, washing out and desorption. Polymer base of bioaffinity sorbent is cryogel of polyvinyl alcohol (pore size is 0.04-2.0 mcm). Also, bioaffinity sorbent can contain both immobilized enzymes modifying virus and antibodies. Proposed method shows the following advantages as compared with analogs and prototype: a) enhanced effectiveness of method; b) increased universality. Invention can be used both in scientific investigations and in production of vaccines and diagnostics and in medicine practice also. EFFECT: improved method of virus concentrating. 2 cl, 7 ex

Description

 The invention relates to applied virology, specifically to the processes of isolation, purification, identification, modification of viruses and viral preparations, i.e., to processes associated with the concentration of viruses. The invention can be used both in scientific research and in the production of vaccines and diagnostics, as well as in medical practice.

 Known methods for the concentration of viral particles in modern virology are multistage operations of long-term high-speed centrifugation in the density gradient of sucrose or glycerol, as well as zone electrophoresis and others [1], in addition, virus concentration is used using bioaffinity sorbents containing immobilized antibodies to the virus [2] . The latter approach is characterized by greater efficiency and technological convenience.

 Thus, a method for bioaffinity purification of measles virus is known, where a carrier is used containing monkey serum immunoglobulins, covalently sewn to the surface of modified glass beads [3]. The method includes passing a virus-containing liquid through a chromatographic column filled with a bio-affinity sorbent with immunoglobulins covalently attached to a glass carrier, followed by washing the column with 0.14 M NaCl and eluting the virus with 0.1 M glycine buffer at pH 2.3.

 The disadvantages of this method are the low biospecific capacity of the carrier used (only the surface of the glass granules works), nonspecific adsorption of impurities by the glass, and the fragility characteristic of glass carriers in general.

 There is a method of bioaffinity purification of viruses of various sizes, where silica gel with controlled pore sizes (0.05 - 1.0 μm) with grafted affinity ligands is used to purify the virus [4]. The method consists of similar chromatographic purification operations of the target product as in the previous case; only 0.1 M Na-phosphate buffer (pH 7.0) is used for washing, and 0.05 M Na-citrate buffer (pH 3.0 is used for elution) )

 The disadvantages of this method are the difficulty of obtaining an immunosorbent associated with a multi-stage scheme for the modification of an inorganic carrier, as well as the fragility characteristic of such materials. In addition, in working fluids, even with a slightly alkaline reaction of the medium (pH 7.5-8.5), silica matrices are hydrolytically unstable, which leads to dissolution of the active surface and a progressive decrease in biospecific capacity.

 The closest to the proposed technical essence is the method of purification of the marsupial disease of chickens virus selected as a prototype by its sorption concentration by passing virus-containing suspensions through a column with immunosorbent, which is an insoluble carrier - granular agarose gel (commercial name - sepharose-4B), to which after activation by bromine, immunoglobulins are covalently sewn [5]. Such a bioaffinity sorbent is used to clean not very large viruses, the size of which exceeds 0.08 μm.

 However, this method of concentrating the virus is ineffective when working with large (0.1-0.5 microns) viruses. In addition, granular agarose gels, in particular Sepharose, have a high cost and therefore cannot find large-scale application. Bromocyan used to activate this carrier is a highly toxic compound, work with it is a danger to personnel.

 The objective of the invention is the development of an effective, universal and technologically simplified method for the concentration of various viruses, including the largest viruses with a particle size of up to 0.5 microns.

 The solution to this problem is achieved by the fact that when the virus is concentrated by binding with a bio-affinity sorbent containing antibodies to the virus, immobilized on a polymer basis, washing and subsequent desorption, polyvinyl alcohol cryogel with a pore size of 0.04 - 2 is used as the polymer base of the bio-affinity sorbent. 0 microns. In addition, the bio-affinity sorbent may, according to this invention, contain, along with antibodies, immobilized virus-modifying enzymes.

 It turned out that the choice of cryogel of polyvinyl alcohol (PVA) as the polymer base of the bio-affinity sorbent provides the possibility of technological simplification of the method of concentration of the virus, increasing the efficiency of the method as a whole, its versatility, including with respect to the largest viruses with a particle size of up to 0.5 microns .

Very important properties of PVA cryogels are their biocompatibility, lack of toxicity, as well as its availability and relative cheapness. PVA cryogels are formed as a result of freezing concentrated aqueous solutions of PVA, keeping them frozen for a certain time and subsequent thawing [6]. Thus formed macroporous cryogel is stable at temperatures up to 60-65 ^o C and has a melting point of 80-100 ^o C. It has a pronounced macroporosity [6], ie meets one of the basic requirements for media designed to work with viruses. According to the invention, the use of a PVA cryogel having pores of 0.05-2.0 μm in size is provided as the polymer base of the bioaffinity sorbent. Such pores provide free penetration of even the largest viruses into the granules of the carrier, i.e., affinity ligands of the entire volume of the carrier participate in binding to viruses.

 In addition, in contrast to brittle macroporous inorganic matrices (macroporous glasses, silicas, diatomite, etc.), PVA cryogels are non-brittle viscoelastic physical bodies, little susceptible to abrasive wear even with vigorous stirring. Thus, along with macroporosity, PVA cryogels satisfy the requirement of operational stability. And finally, PVA cryogels can, if necessary, be sterilized, for example, rinsed with disinfectant solutions, irradiated or (to destroy waste material) autoclaved.

The method is as follows: the virus-containing liquid is incubated with a bio-affinity sorbent containing specific antibodies immobilized on an activated PVA cryogel matrix, unbound unbound components are washed off and the adsorbed virus is released from the complex with the bio-affinity sorbent. To modify the virus, a bio-affinity sorbent is used, containing specific immobilized specific antibodies and an enzyme (s) that can cause the modification of viral particles. A specific implementation of the invention is illustrated by the following examples:
Example 1

To concentrate the influenza virus (type A, H1N1, viral particle size 0.1 μm), a bioaffinity sorbent is used, which is a PVA cryogel with a maximum pore diameter of 1.0 μm, activated with glutaraldehyde at pH 1.0, to which specific antibodies are covalently linked obtained from the blood serum of rabbits immunized with the corresponding antigen (the capacity of the sorbent for immobilized antibodies is 0.7 - 1.2 mg / g). A weighed portion (0.5 g) of the bio-affinity sorbent is mixed with 2.0 ml of virus-containing liquid for 20 hours at +5 ^o C, then the unbound components are washed with 0.1 M PBS (control - zero absorbance at 260 nm and 280 nm, and also a negative hemagglutination reaction (RGA)), and then 0.65 NaCl virus is desorbed in 0.05 M Tris-HCl (pH 7.4) in 1.0 ml portions for three hours until the virus is completely removed. The capacity of the bioaffinity sorbent for the desorbed antigen is 1400 GAU / g of carrier. (GAE - the product of the inverse titer on the sample volume). The specificity of the obtained bioaffinity sorbent (with immobilized antibodies to influenza A, H1N1 virus) is checked using influenza A, H3N2 virus. Antigenic activity is determined by the direct hemagglutination reaction (RGA). The results show that nonspecific antigens (H3N2) are not adsorbed on this immunosorbent, i.e. only biospecific sorption (concentration) of antigens is observed.

 Example 2

To concentrate the influenza virus (type A, H1N1, viral particle size 0.1 μm), a bioaffinity sorbent is used, which is a PVA cryogel with a maximum pore diameter of 0.5 μm, activated with epichlorohydrin at pH 13, to which specific antibodies obtained from the blood serum of rabbits immunized with the corresponding antigen (the sorbent capacity for immobilized antibodies is 0.5-0.6 mg / g), and the concentrated virus is eluted in a column mode using 2.5 M MgCl ₂ in 0.05 M Tris-HCl (pH 7 ,4). The amount of desorbed virus is 800 GAU / g of carrier.

 Example 3

 To concentrate the influenza virus (type A, H3N2, viral particle size 0.12 μm), a bio-affinity sorbent is used, which is a PVA cryogel with a maximum pore diameter of 0.7 μm, activated with bromine cyanide at a pH of 11.5, to which specific antibodies are covalently attached obtained from the blood serum of rabbits immunized with the corresponding antigens (the sorbent capacity for immobilized antibodies is 1.5 mg / g), and the concentrated virus is eluted using 0.65 M NaCl in 0.5 M Tris-HCl (pH 7.4). The amount of desorbed virus is 2000 GAU / g of carrier.

 Example 4

To concentrate the parainfluenza virus GP ₆ (viral particle size 0.15 μm), a bio-affinity sorbent is used, which is a PVA cryogel with a maximum pore diameter of 1.5 μm, activated with glutaraldehyde at pH 0.5, to which specific antibodies obtained from blood serum of guinea pigs immunized with the corresponding antigen (the sorbent capacity for immobilized antibodies is 0.5 - 0.7 mg / g), and the concentrated virus is eluted with 0.65 NaCl in 0.05 M Tris-HCl (pH 7.4) . The titer of purified antigen (parainfluenza virus GP ₆ ) is determined by indirect enzyme-linked immunosorbent assay (ELISA). The capacity of the bioaffinity sorbent for this virus is 1266 units of antigenic activity per 1 g of carrier.

 Example 5

 To concentrate smallpox virus (viral particle size 0.4 x 0.2 μm), a bio-affinity sorbent is used, which is a surfactant cryogel with a maximum pore diameter of up to 2 μm, activated with glutaraldehyde at pH 1.2, to which specific antibodies obtained are covalently attached from the blood serum of rabbits immunized with the corresponding antigen (sorbent capacity for immobilized antibodies 0.8 mg / g), and the concentrated virus was eluted using 0.75 NaCl in 0.05 Tris-HCl (pH 7.8). The titer of purified antigen (smallpox virus) is determined in an indirect ELISA. The capacity of the bio-affinity sorbent for this virus is 2048 units of antigenic activity per 1 g of carrier.

 Example 6

For concentration and enzymatic modification of foot-and-mouth disease virus (viral particle size 0.02 μm), a sample (0.5 g) of bioaffinity sorbent, which is a PVA cryogel with a maximum pore diameter of up to 0.04 μm, activated with glutaraldehyde at a pH of 1.0, to which specific antibodies to foot-and-mouth disease virus are covalently sewn (obtained from the blood serum of calves immunized with the corresponding antigen) and the modifying enzyme is papain (the sorbent capacity for immobilized antibodies is 0.4 mg / g, for papain 0.2 mg / g) is mixed with 2.0 ml virusosod holding liquid for 12 hours at +5 ^o C. Similarly treated with a control bioaffinity sorbent, in which immobilized papain contains a blocked thiol group of the active center. The virus is then desorbed with 0.5 M NaCl in 0.05 M Tris-HCl (pH 7.4) in 1.0 ml portions for three hours. The capacity of the control bioaffinity sorbent for desorbed virus is 780 PFU / g of carrier (PFU - plaque forming units), the carrier with active papain is 32 PFU / g of carrier, i.e. 24.3 times less, which is the result of the action of an immobilized protease on foot and mouth disease virus, concentrated in the bioaffinity sorbent phase due to interaction with immobilized antibodies (the results of an experiment with a control bioaffinity sorbent prove the fact of such concentration), which ultimately leads to a significant decrease in virulent activity the virus.

 Example 7

For concentration and enzymatic modification of mumps virus (viral particle size 0.14 μm), a sample (0.5 g) of bioaffinity sorbent, which is a PVA cryogel with a maximum pore diameter of up to 1.4 μm, activated with glutaraldehyde at pH 1.0, to which specific antibodies to mumps virus are covalently sewn (obtained from the blood serum of hamsters immunized with the corresponding antigen) and modifying enzymes - neuraminidase and ribonuclease (the sorbent capacity for immobilized antibodies is 0.3 mg / g for neuraminidase - 0.15 mg / g, according to RNAase 0.2 mg / g), incubated with 2.0 ml of virus-containing liquid for 12 hours at +5 ^o C. Similarly treated with a control bioaffinity sorbent, which is a drug, in which only antibodies specific for mumps virus are immobilized on the carrier (the capacity of the control bioaffinity sorbent for antibodies is 0.7 mg / g of the carrier). Then unbound components of 0.1 M PBS are washed off (control — zero absorbance at 280 and 260 nm) and then desorption of the 0.5 NaCl virus in 0.05 M Tris-HCl (pH 7.4) in 1.0 ml portions for three hours. The capacity of the control bio-affinity sorbent for the desorbed virus is 650 GAU / g of carrier; for the sorbent with modifying enzymes, no virological activity was detected, which is associated with the action of immobilized neuraminidase on the mumps protein capsid of the virus and the subsequent exposure of the immobilized RNAase to virionic acid released from virionone what is the lack of virulent activity of the virus.

The proposed method of concentration of the virus has the following advantages compared to analogues and prototype:
- increased efficiency of the method, because in contrast to the analogous methods, the claimed method uses a bio-affinity sorbent based on a viscoelastic non-fragile and hydrolytically stable PVA cryogel, therefore it is possible to concentrate the virus not only in the chromatographic (column) version, but also in reactors with sorbent mixing, which significantly intensifies mass transfer processes, those. the processability is improved;
- the versatility of the method is increased, since it is possible to concentrate, along with small, even the largest viruses (0.5 μm or more), while in the prototype method the matrix of the bioaffinity carrier is able to provide diffusion into its granules of only rather small (up to 0.08 microns) viruses; in addition, the versatility of the proposed method is also due to the possibility of simultaneous concentration and enzymatic modification of the virus, when the bio-affinity sorbent along with immobilized antibodies contains an immobilized modifying enzyme (enzymes);
- bioavailable sorbents based on PVA cryogel are inert and highly specific, they can be reused without significant specific activity, the polymer used to prepare the gel base is cheap and affordable.

Literature
1. H. Frenkel-Conrat. Chemistry and biology of viruses.// M., 1972, pp. 33-37.

 2. Ya. Turkova, Affinity chromatography, // M., 1980, pp. 5-14.

 3. Purification of measles virus by affinity chromatography and by ultracentrifufation: a comparative study // Njayou M., Quash G. // J. Yirol. Meth. - 1991, v. 32, N 1, p / 67-77.

 4. Separation and purification of biopolimers by affinity chromatography on controlled-pore silica gel./Colpan M. // Ger. offen. DE 3627063, cl. B 01 D 15/08, 1988.

 5. Separation and purification of antigen for diagnosis of infectious bursa disease in chickens. Nagai Sh., Otaki Y., Ueda S., JP 63210775, cl. G 01 N 33/569, 1989.

 6. The use of polyvinyl alcohol cryogels in biotechnology. Review of literature data. // Lozinsky V.I., Vakula A.V., Zubov A.L.// Biotechnology, N 4, 1992, p. 5-14.

Claims (2)

 1. The method of concentration of the virus, including its binding by a bio-affinity sorbent containing antibodies to the virus, immobilized on a polymer basis, washing and subsequent desorption, characterized in that the polyvinyl alcohol cryogel with a pore size of 0.04 - 2 is used as the polymer base of the bio-affinity sorbent, 0 microns.  2. The method according to claim 1, characterized in that the binding of the virus is carried out using a bio-affinity sorbent containing, along with antibodies, immobilized virus-modifying enzymes.