• 专利附录
  • 专利说明
  • 权利要求
  • 类似技术
  • 同族专利
  • 引用文献
  • 法律状态
  • 优先权
    • 专利摘要:
    The invention relates to a process for the preparation of the lyophilized vaccine against duck hepatitis by using the attenuated hepatitis virus TN cultivated by Asplin. According to the invention the virus deposited in the Strain Collection of the Hungarian Institute of Public Healts under No. 00220 is injected into the allantoic cavity of embryonated SPF-hen's eggs, the eggs are incubated at a temperature of about 37 DEG C., the embryos died between 24 and 96 hours are collected, homogenized with a physiological saline solution, antibiotics are added to the pure suspension, and after the addition of protective and skeleton forming agents the sterile virus material is lyophilized in a manner known per se. The lyophilized vaccine can be stored at a temperature of +4 DEG C. for one year in contradiction to the known liquid vaccine storable in freezed state at a temperature of -20 DEG C. for half a year and which has to be used within 7 days from the delivery (with a storage temperature of +4 DEG C.). The titre of the vaccine prepared according to the invention is at least tenfold of that of the known vaccine, thus much less embryonated eggs are used for the process according to the invention what means cost saving. Due to the lyophilization the vaccine can be transported to far destinations, too, what was not possible at the known liquid product stored in freezed state.
    公开号:SU1237081A3
    申请号:SU823524763
    申请日:1982-12-22
    公开日:1986-06-07
    发明作者:Хорват Эржебет;Толлаш Габор
    申请人:Филаксиа Олтоаньагтермеле Валлалат (Фирма);
    IPC主号:
    专利说明:

    one .
    The invention relates to veterinary virology, in particular, to methods of producing a lyophilized duck hepatitis vaccine using an attenuated hepatitis TN virus, which is cultured by asplin.
    The purpose of the invention is to increase the activity and stability of the vaccine.
    The Asplin cultured weakened hepatitis TN virus, stored under number 00220 in the funds of the Hungarian Agricultural Institute of Public Health (OKI), is injected into the allargtoid cavity of chicken eggs.
    Eggs are incubated at 37 ° C, the dead are collected during 24-96 hours of incubation, and the surviving embryos are destroyed, if necessary, the solid tissues are removed under sterile conditions, then they are homogenized in sterile saline sodium chloride, centrifuged the homogenate, the antibiotic is introduced into the clear suspension and the liquid is lyophilized in a known manner after the addition of protective colloids and structure-forming substances to it.
    By SPF, we mean eggs, which do not contain Avian encephalomyelitis pathogens, bird plague, EDZ, bronchitis, leukemia, AB, Gumboro, Marok, reovirus, and also Salmonella Gall, Salmonella typhinurium, Musoplasma Gall, Mycoplasma Synoviae or their antibodies.
    When homogenizing, the suspension is diluted, preferably in such a ratio that 25-35 vol.% Of the embryonic mass and 76-65% by volume of the physiological saline solution are contained.
    A combination of poly vinylpyrrolidone, gelatin, glucose and sucrose is preferably used as a protective colloid and structure-forming substance.
    When the shelves of the freeze dryer are lyophilized, the material intended for laying is cooled to O - (-6) Cj and the material found in the shelves is (-30) - (-40) C, after the sublimation is completed, the shelves are heated to 30 -40 ° C and dry the material for 4-10 hours
    370812
    Example. SPF chicken eggs are incubated for 10 days, then shine and mark the position of the air chamber and the embryo on the egg shell. Then the blunt end of the egg is disinfected. A suspension of an infected virus through the hole made above the air bladder is introduced into the allantoic cavity. Initiate the material contains in one milliliter 50,000 ElDjQ. 0.2 ml of infectious material is used per egg. Then the hole is closed with paraffin and the eggs are incubated in an incubator at 37 ° C. Eggs are translucent every day, and eggs containing dead embryos are stored until further use at 2-5 ° C. Left alive after 96 hours from incubation, the embryos are destroyed.
    The embryos remove the eggs under sterile conditions, cut off the front part of the head and crush. Then, physiological saline sodium chloride solution is added, homogenization is continued in a homogenizer. The mass is subjected to further dilution until the amount of the added saline solution is 70% of the obtained suspension. The suspension is centrifuged for 20 minutes at a speed of 3000 rpm. The transparent supernatant is filtered through four layers of sterile gauze.
    35 The resulting material is subjected to a sample for purity and is immediately subjected to antibiotic treatment (penicillium, streptomycin, neomycin, and chlorocide). The suspension is kept 40 at room temperature for one hour and then checked for sterility by plating on the nutrient medium.
     If material is not stapled. it is sterilized with gentamicin. Not later than 5-6 days after the breach of integrity, the shells are suspended and lyophilized. Until that time, suspended 50
    55
    Zia stored at 4 s. Before lyophilization, the following protective substances are added: 5% 10 vol.% Kollidonovogo solution, 5% 10 vol.% - solution of gel (Atina, 4% 50 vol.% - glucose solution and .3% 50% vol. Sucrose solution.
    Total amount of protective colloid; IDs and structure-forming substances
    is 17%. Before freezing, the suspension titer is determined to be 10 ElDjo / Mn.
    The suspension was packaged in 2 ml portions in cups. They are placed on pre-cooled to -5 ° C shelves of the device for lyophilization. When the material temperature drops to -45 ° C, ba10 turns on.
    kum After the pressure is 0.1 mbar, heating is switched on.
    shelves and is adjusted so that the temperature of the material is kept within (-30) - (-35) ° C (at 0.1 mbar, this requires a shelf temperature of about –15 ° C). At the end of sublimadia, the shelves are heated to 35 ° C and the maximum capacity of the vacuum unit is established. After drying for 8 hours, the residual amount of moisture is less than 2%. The cups are sealed with rubber stoppers with metal caps even in a vacuum vacuuming unit under vacuum. 25
    EXAMPLE 2. To obtain an infectable virus, the procedure outlined in Example 1 is repeated, with the difference that no antibiotic is added to the suspension, and the finished vaccine is not lyophilized. stored frozen in liquid nitrogen. The titer of the virus to be infected is at least 10 -10 ElDjp / ml. Before use, a diluted solution is prepared from the infected material in the ratio 1: 60-1: 200. One vaccination dose (0.2 ml) contains approximately lOOOO / ElDjj. Infected virus should not cause hemagglutinization of 40 red blood beads of chickens.
    PRI me R 3. Immunogenicity evaluated in the neutralization reaction. For the experiment, 480 tons of households are used in which, due to export supplies, livestock are not subjected to immunization. Each group consists of 20 birds.
    In the experiment with vaccination, a buffer of the following composition is used, g: 50
    an
    eight
    0.2 1.15 0.2 0.1 0.1
    Up to 1000 ml
    ten
    23708 4
    From the vaccine obtained according to the method of Example 1, diluted solutions of different concentrations are obtained using the buffer of the composition given. These 5 solutions are used both for intramuscular injections and in drinking water. For the purpose of comparison, similar experiments were carried out with a commercial liquid vaccine.
    After 12 days, samples of blood flow are taken 15 20 25
    - zo es 40
    five
    0
    five
    virus and serum, inactivate at 56 ° C for 30 minutes. Then dilution of serum in a ratio of 1:10. are brought into contact with different dilutions of the virus and kept at room temperature for one hour, and then the resulting mixture is infected with SPF eggs incubated for 1-1 days. The virus titer or neutralization index (IN) is determined after the expiration of one week by the number of dead or still living, but subjected to characteristic Pathological changes of embryos according to the Reed-Münch method.
    Comparative data on the immunogenic activity of the frozen liquid vaccine and the proposed vaccine are given in the table.
    An index greater than 2 is positive, an index greater than 3 is an excellent result.
    J From the table it can be seen that the vaccine obtained according to the proposed method has excellent protective qualities.
    Example 4. The storage capacity of the vaccine is examined by simulating actual storage as well as by the usual heat load. When modeling storage conditions, it is assumed that storage capacity at 4 ° C is prescribed in the instructions of most countries, therefore the storage capacity of the product intended for export is checked at this temperature. The vaccine stored for 12 months at 2-5 seconds loses 0.6 decimal degrees of its activity (according to the degree of EID value). This value is insignificant and does not exceed the spread of the value of EY-, two cones.
    yQ
    A sample with a thermal load provides a sufficiently quick check. If the titer stored for one week during the vaccination is satisfactory, then it is guaranteed that when stored for a year under the prescribed conditions, it is suitable, for use. The resultant cohort 5 is an excellent result.
    Control
    Frozen. liquid vaccine
    subcutaneously

    Lyophilized vaccine according to the proposed method
    1237081 .§
    During the course of one week at 37 ° C, the vaccine of the present invention loses only 0.5 decimal degrees of its activity, which
    1.6
    25
    87.5
    125
    权利要求:
    Claims (1)
    [1]
    METHOD FOR PRODUCING A LYOPHILIZED VACCINE AGAINST DECK HEPATITIS, which involves culturing duck hepatitis vaccine virus on embryos, adding antibiotics and a protective medium to the resulting virus-containing material, followed by lyophilization of the resulting suspension, characterized in that, in order to increase the vaccine's activity and the stability of the vaccine, the vaccine use strain TN No. 00220, chicken is used from embryos, after cultivation of the hepatitis virus, chicken embryos are homogenized in the presence of a physiologist an organic solution of sodium chloride with embryomass and physiological saline equal to 25-35 and 65-75 vol.%, respectively, is centrifuged, the homogenate supernatant is used as the virus-containing material, and a mixture containing 0.5% polyvinylpyrrolidone is used as a protective medium, 0.5% gelatin, 2% glucose, 1.5% sucrose from a virus-containing suspension.
    SU 1237081 AZ
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    同族专利:
    公开号 | 公开日
    GB2111829A|1983-07-13|
    NL8204915A|1983-07-18|
    US4622222A|1986-11-11|
    HU183765B|1984-05-28|
    GB2111829B|1985-09-18|
    PL133923B1|1985-07-31|
    PL239715A1|1983-07-18|
    引用文献:
    公开号 | 申请日 | 公开日 | 申请人 | 专利标题
    DE2126957B2|1971-05-29|1977-07-07|Schettler, Hermann, Dr, East Lan sing, Mich |PROCESS FOR MANUFACTURING VACCINES AGAINST GAENSEHEPATITIS|
    GB1590448A|1977-03-04|1981-06-03|Akzo Nv|Vaccine and its preparations|US5024836A|1987-05-04|1991-06-18|Merck & Co., Inc.|Stable lyophilized live herpes virus vaccine|
    US6005916A|1992-10-14|1999-12-21|Techniscan, Inc.|Apparatus and method for imaging with wavefields using inverse scattering techniques|
    EP0728195A1|1993-10-12|1996-08-28|Chiron Corporation|Methods for preserving recombinant viruses|
    US5653686A|1995-01-13|1997-08-05|Coulter Corporation|Closed vial transfer method and system|
    CA2212574C|1995-02-13|2010-02-02|Electronic Publishing Resources, Inc.|Systems and methods for secure transaction management and electronic rights protection|
    US6658568B1|1995-02-13|2003-12-02|Intertrust Technologies Corporation|Trusted infrastructure support system, methods and techniques for secure electronic commerce transaction and rights management|
    US5943422A|1996-08-12|1999-08-24|Intertrust Technologies Corp.|Steganographic techniques for securely delivering electronic digital rights management control information over insecure communication channels|
    US5892900A|1996-08-30|1999-04-06|Intertrust Technologies Corp.|Systems and methods for secure transaction management and electronic rights protection|
    GB9808922D0|1998-04-24|1998-06-24|Cantab Pharmaceuticals Res Ltd|Virus preparations|
    US8124397B2|2005-08-08|2012-02-28|Oregon Health & Science University|Inactivating pathogens with oxidizing agents for vaccine production|
    CN102772799A|2012-05-31|2012-11-14|郑州后羿制药有限公司|Duplex egg yolk antibody freeze-drying powder for duck virus hepatitis and duck plague and preparation method thereof|
    法律状态:
    优先权:
    申请号 | 申请日 | 专利标题
    HU813935A|HU183765B|1981-12-23|1981-12-23|Process for producing lyophilized vaccine against duck hepatitis|
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