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IMPROVED METHODS FOR ENTEROVIRUS INACTIVATION, ADJUVANT ADSORPTION AND DOSE REDUCED VACCINE COMPOSITIONS OBTAINED THEREOF

20170348411 · 2017-12-07

    Inventors

    Cpc classification

    International classification

    Abstract

    The present invention is directed to improved methods of Enterovirus inactivation by formaldehyde in presence of tromethamine buffer resulting in maximum recovery of D-antigen. Subsequent adsorption of said sIPV on aluminium hydroxide provides significantly dose reduced sIPV compositions.

    Claims

    1. A method for producing a composition comprising Enteroviral particles, wherein the method comprises the steps of: a) producing a medium containing the Enteroviral particles; b) purification of the Enteroviral particles from the medium; c) stabilization of purified Enteroviral particles; d) formalin inactivation of the Enteroviral particles whereby during at least a part of the inactivation a buffer other than a phosphate buffer is present at a concentration sufficient to prevent or reduce aggregation of the Enteroviral particles thereby reducing the D-antigen losses post inactivation by 8 to 10 fold as compared to phosphate buffer; and e) adsorption of Enteroviral particles on aluminum salt adjuvant whereby percentage adsorption on alum is atleast 95%.

    2. The method according to claim 1, wherein the buffer of step (d) is selected from the group consisting of TRIS, TBS, MOPS, HEPES and bicarbonate buffers.

    3. The method according to claim 2, wherein the buffer is a TRIS buffer having a pH of about 6.8 to 7.2 and at a concentration in the range of 30 mM-70 mM, preferably 40 mM.

    4. The method according to claim 1, wherein the aluminum salt adjuvant of step (e) is selected from a group of aluminum hydroxide, or aluminum phosphate, or a mixture of both.

    5. The method according to claim 4, wherein the aluminum salt adjuvant is an aluminum hydroxide having concentration between 1.5 mg/0.5 ml dose and 2.5 mg/0.5 ml dose, preferably between 2.100 mg/0.5 ml dose and 2.4 mg/0.5 ml dose at a pH of about 6.5.

    6. The method according to claim 5, wherein total aluminum content in the trivalent vaccine is 0.8-1.2 mg, preferably 0.8 mg Al.sup.3+ per 0.5 mL dose, characterized in that atleast 0.4 mg Al.sup.3+ for Type 1, atleast 0.2 mg Al.sup.3+ for Type 2, atleast 0.2 mg Al.sup.3+ for Type 3.

    7. The method according to claim 1, wherein the composition comprising Enteroviral particles is a vaccine.

    8. The method according to claim 7, wherein the Enteroviral particles are of an Enterovirus of polioviruses.

    9. A The method according to claim 8, wherein the Enteroviral particles comprise polioviruses of the Sabin serotypes 1, 2 and 3.

    10. The method according to claim 8, wherein the Enteroviral particles comprise polioviruses of Salk serotypes IPV type 1 (Mahoney strain), IPV type 2 (MEF-1 strain); and/or IPV type 3 (Saukett strain).

    11. The method according to claim 7, wherein the vaccine is a dose reduced Inactivated Polio Vaccine (IPV).

    12. The method according to claim 11, wherein the dose reduced Inactivated Polio vaccine comprises: i) inactivated poliovirus type 1 at a dose less than 15 D-antigen units instead of standard dose of 42 DU; and/or ii) inactivated poliovirus type 2 at a dose less than 18 D-antigen units; and/or iii) inactivated poliovirus type 3 at a dose less than 15 D-antigen units instead of standard dose of 32 DU.

    13. The method according to claim 15, wherein the method for preparing the dose reduced inactivated Polio vaccine containing Salk or Sabin polioviruses comprises the steps of: a) producing a medium containing the polioviruses; b) purification of the polio viruses from the medium; c) stabilization of purified polioviruses by addition of M-199 medium containing glycine; d) inactivation of the polio viruses by using formaldehyde 0.025% at 37° C. for 5 to 13 days in presence of TRIS buffer at a concentration between 30 mM to 60 mM to prevent or reduce aggregation of the poliovirus particles thereby reducing the D-antigen losses post inactivation by 8 to 10 fold as compared to phosphate buffer; and e) adsorption of inactivated polioviruses on Alum hydroxide adjuvant having concentration between 2 to 2.5 mg/dose, whereby percentage adsorption on Alum hydroxide is greater than 95% for Type 1, Type 2 and Type 3.

    14. The method according to claim 15, wherein the method for preparing the dose reduced inactivated Polio vaccine containing Salk or Sabin polioviruses comprises the steps of: a) producing a medium containing the polioviruses; b) purification of the polio viruses from the medium; c) stabilization of purified polioviruses by addition of M-199 medium containing glycine; d) inactivation of the polio viruses by using formaldehyde 0.025% at 37° C. for 5 to 13 days in presence of TRIS buffer at a concentration between 30 mM to 60 mM to prevent or reduce aggregation of the poliovirus particles thereby reducing the D-antigen losses post inactivation by 8 to 10 fold as compared to phosphate buffer; and e) adsorption of inactivated polioviruses on Alum hydroxide adjuvant having concentration between 2 to 2.5 mg/dose, whereby percentage adsorption on Alum hydroxide is greater than 95% for Type 1 and Type 3.

    15. The method according to claim 11, wherein the dose reduced Inactivated Polio vaccine can be selected from a group of: i) Sabin single dose composition having Sabin Type 1, Type 2, Type 3 combination selected from 5-16-10; ii) Sabin two dose composition having Sabin Type 1, Type 2, Type 3 combination selected from 5-16-10; iii) Sabin single dose composition having Sabin Type 1, Type 2, Type 3 combination selected from 2.5-8-5; iv) Sabin two dose composition having Sabin Type 1, Type 2, Type 3 combination selected from 2.5-8-5; v) Sabin single dose composition having Sabin Type 1, Type 2, Type 3 combination selected from 5-8-10; vi) Sabin two dose composition having Sabin Type 1, Type 2, Type 3 combination selected from 5-8-10; vii) Salk single dose composition having Sabin Type 1, Type 2, Type 3 combination selected from 7.5-16-10; viii) Salk two dose composition having Sabin Type 1, Type 2, Type 3 combination selected from 7.5-16-10; ix) Salk single dose composition having Salk Type 1, Type 2, Type 3 combination selected from 8-2-5; x) Salk two dose composition having Salk Type 1, Type 2, Type 3 combination selected from 8-2-5; xi) Salk single dose composition having Salk Type 1, Type 2, Type 3 combination selected from 10-2-5; xii) Salk two dose composition having Salk Type 1, Type 2, Type 3 combination selected from 10-2-5; xiii) Salk single dose composition having Salk Type 1, Type 2, Type 3 combination selected from 10-2-12; xiv) Salk two dose composition having Salk Type 1, Type 2, Type 3 combination selected from 10-2-12; xv) Salk single dose composition having Salk Type 1, Type 2, Type 3 combination selected from 5-2-5; and xvi) Salk two dose composition having Salk Type 1, Type 2, Type 3 combination selected from 5-2-5.

    16. The method according to claim 15, wherein the dose reduced Salk or Sabin Inactivated Polio Vaccine does not comprise Type 2.

    17. The method according to claim 15, wherein a multivalent vaccine consisting of dose reduced IPV can comprise of one or more antigens from a pathogen selected from a list consisting of: Haemophilus influenzae b, Neisseria meningitidis type A, Neisseria Meningitidis type C, Neisseria meningitidis type W, Neisseria meningitidis type Y, Neisseria meningitidis type X, Neisseria meningitidis type B, Streptococcus pneumoniae, Streptococcus agalactiae Salmonella typhi, Hepatitis A, Hepatitis B, RSV, Hepatitis C, diphtheria toxoid, tetanus toxoid, whole cell pertussis, acellular pertussis, Staphylococcus aureus, anthrax, Vibrio cholera, Zika, Ebola, Chikungunya, dengue, malaria, measles, mumps, rubella, BCG, Japanese encephalitis, Rotavirus, smallpox, Shigella, yellow fever, typhoid, CMV, Shingles, Varicella virus, HPV, HSV, and HIV.

    Description

    DESCRIPTION OF FIGURES

    [0013] FIG. 1: Alum phosphate gel prepared in 0.9% NaCl (pH Vs Zeta potential at different concentrations of Alum phosphate gel)

    [0014] FIG. 2: Alum phosphate gel prepared in WFI (pH Vs Zeta potential at different concentrations of Alum phosphate gel)

    [0015] FIG. 3: Alum Hydroxide gel prepared in 0.9% NaCl (pH Vs Zeta potential at different concentrations of Alum hydroxide gel)

    [0016] FIG. 4: Alum Hydroxide gel prepared in WFI (pH Vs Zeta potential at different concentrations of Alum hydroxide gel)

    DETAILED DESCRIPTION

    [0017] An important aspect of the instant invention is that said improved process of formalin inactivation and adsorption on alum salt comprises of following steps: [0018] a) Adding Sabin IPV purified bulk to TRIS buffer (30 to 50 mM) having pH between 6.8 to 7.2, [0019] b) Adding M-199 medium containing glycine (5 gm/1) to mixture of (a), [0020] c) Adding 0.025% formaldehyde while mixing, [0021] d) Incubating mixture obtained in Step (c) at 37° C. from 5 to 13 days on magnetic stirrer, [0022] e) Subjecting post-incubation mixture to intermediate 0.22μ filtration on day 7 and final filtration on day 13, [0023] f) Storing bulk obtained after step (e) at 2-8° C., [0024] g) Performing D-Ag ELISA for D-Antigen unit determination, [0025] h) Taking the desired volume of autoclaved Al(OH).sub.3 to get the final concentration of Alum(Al++) between 0.8 to 1.2 mg/dose in a 50 ml Container, [0026] i) Adding sIPV bulk with adjusted D-Ag unit and making up the volume with diluent (10×M-199+0.5 Glycine %), [0027] j) Adjusting the final formulation pH and obtaining final formulation with pH between 6 and 6.5, [0028] k) Subjecting the formulation bulk to magnetic stirring overnight at 2-8° C. and wherein formalin inactivation of step (a) does not occur in presence of phosphate buffer

    [0029] A first embodiment of instant invention is that said buffer to be used during formaldehyde inactivation can be selected from the group consisting of TRIS, TBS, MOPS, HEPES, and bicarbonate buffers.

    [0030] A preferred aspect of first embodiment is that said formaldehyde inactivation can occur in presence of TRIS Buffer or TBS (TRIS Buffered saline) having concentration selected from 30 mM, 40 mM and 50 mM, preferably 40 mM and at a pH selected from 6.8, 6.9, 7, 7.1 and 7.2, preferably between 6.8 and 7.2 wherein said inactivation does not utilize any phosphate buffer.

    [0031] A second embodiment of the instant invention is that adsorption of formalin inactivated sIPV can be done on aluminium hydroxide having concentration selected from 1.5 mg/dose, 1.8 mg/dose, 2.2 mg/dose, preferably between 2 mg/dose to 2.4 mg/dose and at a pH selected from 6.2, 6.3, 6.4 and 6.5, preferably 6.5.

    [0032] A third embodiment of instant invention is that said improved process of formalin inactivation and aluminium hydroxide adsorption can result in D-Antigen recovery post-inactivation between 50% and 80% and percent adsorption of aluminium hydroxide can be between 85 and 99%.

    [0033] One aspect of third embodiment is that present invention provides an improved process of formalin inactivation and aluminium hydroxide adsorption resulting in dose reduction of atleast 8 fold for Sabin Type I, atleast 3 fold for Sabin Type III as compared to standard dose of 40 DU-8DU-32DU. Second aspect of third embodiment is that instant invention provides improved formaldehyde inactivation and aluminium hydroxide adsorption methods that result in vaccine compositions comprising of i) inactivated poliovirus type 1 at a dose of atleast 5D-antigen units, ii) inactivated poliovirus type 2 at a dose of atleast 8D-antigen units and iii) inactivated poliovirus type 3 at a dose of atleast 10D-antigen units.

    [0034] A fourth embodiment of instant invention is that said aluminium salt adjuvant is an aluminium hydroxide having concentration between 1.5 mg/0.5 ml dose and 2.5 mg/0.5 ml dose, preferably between 2.100 mg/0.5 ml dose and 2.4 mg/0.5 ml dose at a pH of about 6.5.

    [0035] One aspect of fourth embodiment is that total aluminium content in the trivalent vaccine (Type 1, 2 and 3) can be between 800-1000 μg, preferably 800 μg Al.sup.3++ per 0.5 mL dose, characterized in that atleast 400 μg Al.sup.3+ for Type 1, atleast 200 μg Al.sup.3+ for Type 2, atleast 200 μg Al.sup.3+ for Type 3.

    [0036] Another aspect of fourth embodiment is that said dose reduced polio virus vaccine composition can consist of Type 1 and Type 3 and is devoid of Type 2 wherein the dose volume can be between 0.1 and 0.4 ml.

    [0037] The dose reduced vaccine compositions prepared by instant methods can be i) “Standalone sIPV” wherein the antigens may comprise of sIPV type 1 or sIPV type 2 or sIPV type 3, or sIPV types 1 and 2, or sIPV types 1 and 3, or sIPV types 2 and 3, or sIPV types 1, 2 and 3 or ii) “Combination Vaccines containing sIPV” wherein said non-IPV antigens of combination vaccines can be selected from but not limited to diphtheria toxoid, tetanus toxoid, whole cell pertussis antigen(s), acellular pertussis antigen(s), Hepatitis B surface antigen, Haemophilus influenzae b antigen(s), Neisseria meningitidis A antigen(s), Neisseria meningitidis C antigen(s), Neisseria meningitidis W-135 antigen(s), Neisseria meningitidis Y antigen(s), Neisseria meningitidis X antigen(s), Neisseria meningitidis B bleb or purified antigen(s), Hepatitis A antigen(s), Salmonella typhi antigen(s), Streptococcus pneumoniae antigen(s).

    [0038] The non-IPV antigen(s) may be adsorbed onto an aluminium salt such as aluminium hydroxide, an aluminium salt such as aluminium phosphate or onto a mixture of both aluminium hydroxide and aluminium phosphate, or may be unadsorbed.

    [0039] Poliovirus may be grown in cell culture. The cell culture may be a VERO cell line or PMKC, which is a continuous cell line derived from monkey kidney. VERO cells can conveniently be cultured microcarriers. After growth, virions may be purified using techniques such as ultrafiltration, diafiltration, and chromatography. Prior to administration to patients, the viruses must be inactivated, and this can be achieved by treatment with formaldehyde.

    [0040] Compositions may be presented in vials, or they may be presented in ready filled syringes. The syringes may be supplied with or without needles. A syringe will include a single dose of the composition, whereas a vial may include a single dose or multiple doses (e.g. 2 doses). In one embodiment the dose is for human. In a further embodiment the dose is for an adult, adolescent, toddler, infant or less than one year old human and may be administered by injection.

    [0041] Vaccines of the invention may be packaged in unit dose form or in multiple dose form (e.g. 2 doses). The said multidose composition can be selected from a group consisting of 2 dose, 5 dose and 10 dose. For multiple dose forms, vials are preferred to pre-filled syringes. Effective dosage volumes can be routinely established, but a typical human dose of the composition for injection has a volume of 0.5 mL.

    EXAMPLES

    Example 1

    [0042] Purification of Sabin IPV (sIPV)

    [0043] 1) Tangential Flow Filtration (TFF): [0044] Clarified harvest pool was concentrated to 10× using tangential flow filtration system with 100 Kda cassettes (0.5 m.sup.2) and then diafiltered 3 times of harvest volume with phosphate buffer (40 mM, pH: 7.0)

    [0045] 2) Column Chromatography: [0046] The purification was done by Ion Exchange Chromatography (IEC). 10×TFF concentrate was passed through DEAE Sepharose fast flow (Weak-Anion exchanger) packed in column xk-26 using Akta explorer (GE Healthcare). Negatively charged impurities was found to bind to the column whereas polio virus was collected in flow through with phosphate buffer 40 mM.

    [0047] 3) TRIS Buffer Exchange: [0048] To minimize the loss of antigen in a quite cumbersome inactivation procedure (13 days), purified virus pool was buffer exchanged from phosphate buffer to TRIS buffer (40 mM, pH: 7) with TFF system (100 KDa, 0.1 m2). The purified virus pool was exchanged with three volumes of tris buffer.

    Example 2

    [0049] A) Inactivation of sIPV [0050] 10× concentrated M-199 with 0.5% glycine was added so as to achieve final concentration 1×. Inactivation agent formalin (0.025%) was added into purified virus bulk while constant mixing. Inactivation was carried out at 37° C. while continuous stirring for 13 days containing 0.22 u filtration on 7th day and 13th day.

    [0051] B) Inactivation of sIPV in TRIS Buffer and Phosphate Buffer

    [0052] 0.025% formaldehyde was used for inactivation for 13 days at 37° C.

    TABLE-US-00001 TABLE 1 D-Antigen Content, Formalin inactivation in presence of TRIS buffer and Phosphate buffer D-Antigen content (40 mM D-Antigen content (40 mM Phosphate buffer during Tris buffer during Inactivation) Inactivation) Type 1 52.70 DU/ml 408.19 DU/ml Type 2 22.63 180.20 Type 3 4.21 21.50

    [0053] When formaldehyde inactivation methods were particularly carried out in presence of phosphate buffer, significant D-antigen losses were observed for Sabin Type I. Whereas it was found that formaldehyde inactivation in presence of TRIS buffer resulted in minimum loss of D-antigen.

    TABLE-US-00002 TABLE 2 Different concentrations of TRIS Buffer used during inactivation 30 mM 40 mM 50 mM Type 1 500 DU/ml 576.80 DU/ml 585 DU/ml Type 2 140 DU/ml 165.16 DU/ml 155 DU/ml Type 3  16 DU/ml  21.17 DU/ml  19 DU/ml [0054] TRIS Buffer at a concentration of 40 mM was found to be most efficient in terms of D-Antigen content preservation for sIPV 1, 2 and 3.

    [0055] C) D-Antigen Content Determination by ELISA.

    [0056] Day 1: Plate Coating: [0057] 1. 100 ul of specific bovine anti polio was pippeted in PBS per well [0058] 2. Microtiter plate was sealed and incubated overnight at room temperature.

    [0059] Day 2: Blocking: [0060] 1. The plates were washed (Washing/dilution buffer −0.05% tween 20 in 1×PBS) 3 times. [0061] 2. 300 ul block buffer (1% BSA in PBS) was pipetted per well. [0062] 3. The plate was sealed and incubated for 45 minutes at 37±1° C.

    [0063] Sample Addition: [0064] 1. The plate was washed 3 times. [0065] 2. 100 ul of sample diluent was added in all wells except well of row A. [0066] 3. 100 ul standard was added to first two wells of column 2 and 3. [0067] 4. 100 ul sample was added to first two wells of column 4-12. [0068] 5. Prediluting sample to a suitable concentration. [0069] 6. 100 ul sample diluents was added to first two wells of column 1. [0070] 7. Serial two fold dilution were made down the column by transferring 100 ul from each well to adjacent well of the same column and discarding 100 ul from the last well. [0071] 8. Incubating at 37° C. for 2 hr. [0072] 9. Plates were kept overnight at 4° C.

    [0073] Day 3: Monoclonal Antibody Addition: [0074] 1. The plate was washed 3 times. [0075] 2. 100 ul diluted (1:240) type specific monoclonal antibodies were added. [0076] 3. The plates were sealed and incubated for 2 hours at 37° C.

    [0077] Conjugate: [0078] 1. The plate were washed 3 times [0079] 2. 100 ul diluted conjugate (Type1-1:2400, Type2-1:1500, Type3-1:4800) was added. [0080] 3. The plate was sealed and incubated for 1 hour at 37° C.

    [0081] Substrate Addition: [0082] 1. 100 ul TMB substrate was added to all wells. [0083] 2. Mixture incubated at room temperature for 10 minutes. [0084] 3. Reaction was stopped by adding 100 ul 2M H2SO4. [0085] 4. Plate was read at 450/630 nm. [0086] 5. D antigen concentration was calculated using KC4 software.

    Example 3

    [0087] Adsorption of sIPV: [0088] 1. Autoclaved 1% stock of Al(OH).sub.3 and AlPO.sub.4 was used for the preparation of formulations. [0089] 2. Desired volume of Al(OH).sub.3/AlPO.sub.4 was taken to get the required concentration of alum in a 100 ml glass bottle. [0090] 3. Inactivated polio virus bulk with known D-Ag Unit was added and volume make up was done with diluent. [0091] 4. Final formulation pH was adjusted to 6.5 with 1 N HCl/NaOH. [0092] 5. The formulation bulk was kept on magnetic stirrer overnight at 2-8° C.

    Example 4

    [0093] Preformulation Studies

    [0094] Different concentrations of Al(OH).sub.3 & AlPO.sub.4 were prepared in 0.9% saline and in WFI to check size and zeta potential with respect to change in pH.

    [0095] It was observed that zeta potential of AlPO.sub.4 decreases (negativity) with increase in pH from 5 to 7.5 in presence of WFI as well as in saline (Refer FIGS. 1 and 2).

    [0096] Whereas, zeta potential of Al(OH).sub.3 in saline remains constant, independent of pH and Al(OH).sub.3 salt concentration (Refer FIGS. 3 and 4).

    Example 5

    [0097] Adsorption Studies of sIPV on Alum Phosphate and Alum Hydroxide

    TABLE-US-00003 TABLE 3 Sabin Type 1, 2&3 (Titer 10.sup.6.0/dose) adsorption on alum (Alum phosphate and Alum Hydroxide) Virus Titer (per Particles % free in % adsorbed Sample does) (in K) SUP on gel Type 1, Control 5.45 284 NA AlOH.sub.3 Al+++ 4.15 14 4.98 95.02 125 ug/dose Al+++ 3.85 7 2.49 97.51 250 ug/dose Al+++ 3.8 6.3 2.24 97.78 500 ug/dose Type 1, Control 5.84 691 NA AlPO.sub.4 Al+++ 3.49 3 0.43 99.57 125 ug/dose Al+++ 3.09 1.2 0.17 99.83 250 ug/dose Al+++ 2.94 0.87 0.12 99.87 500 ug/dose Type 2, Control 5.49 309 NA AlOH.sub.3 Al+++ 3.59 3.89 1.25 98.75 125 ug/dose Al+++ 3.49 3.09 1 99 250 ug/dose Al+++ 3.49 3.09 1 99 500 ug/dose Type 2, Control 5.49 309 NA AlPO.sub.4 Al+++ 3.15 1.41 0.45 99.5 125 ug/dose Al+++ 3.09 1.23 0.39 99.6 250 ug/dose Al+++ 3.09 1.23 0.39 99.6 500 ug/dose Type 3, Control 5.59 389 NA AlOH.sub.3 Al+++ 4.14 13.8 3.54 96.47 125 ug/dose Al+++ 3.94 8.7 2.23 97.77 250 ug/dose Al+++ 3.54 3.4 0.87 99.13 500 ug/dose Type 3, Control 5.59 389 NA AlPO.sub.4 Al+++ 5.34 218 56.04 43.96 125 ug/dose Al+++ 5.24 173 44.47 55.53 250 ug/dose Al+++ 5.16 144 37.01 62.9 500 ug/dose

    [0098] It was found that Sabin polio virus type-3 shows only 50-60% adsorption with aluminium phosphate (AlPO.sub.4). Whereas, Sabin polio virus type-3 shows atleast 90% adsorption with Al(OH).sub.3. Thus, Alum hydroxide was found to be more efficient as compared to Alum phosphate with respect to adsorption of Sabin Type 1, 2 and 3.

    Example 6

    [0099] Immunogenicity Studies of Alum Adsorbed sIPV

    [0100] To check immune response of adjuvanted sIPV in rat (Sera Neutralisation Test) SNT test was carried out. Sera was separated and used to test the presence of neutralizing antibodies for type specific polio virus. Control sera used to validate the test. Virus back-titration was also performed to get the number of challenge virus particles added.

    [0101] Animal Model: Wistar rat (8 weeks, approx 200 gm) 50% male and 50% female per group.

    [0102] Route of Inoculation: Intra Muscular.

    [0103] Volume: 0.5 ml

    [0104] Blood withdrawal: on day 21.

    [0105] Site of bleeding: Retro-Orbital plexus.

    TABLE-US-00004 TABLE 4 Type 1 Group 1 Group 2 Group 3 Group 4 Group 5 Group 6 Group 7 Group 15 Comm. 5 DU 2.5 DU 1 DU 5 DU 2.5 DU 1 DU −ve IPV 1.15 mgOH 1.15 mgOH 1.15 mgOH 1.8 mgPO4 1.8 mgPO4 1.8 mgPO control Rat SNT Sera Sera Sera Sera Sera SNT Sera Sera Sera No +ve Titer SNT Titer SNT Titer SNT Titer SNT Titer +ve Titer SNT Titer SNT Titer 1 1 (1:2) 8 (1:256) 1 (1:2) 4  (1:16) 5 (1:32) 5 (1:32) 2 (1:4) 0 (<1:2) 2 1 (1:2) 5 (1:32)  1 (1:2) 7 .sup. (1:128) 8  (1:256) 4 (1:16) 1 (1:2) 0 (<1:2) 3 0 (<1:2)  7 (1:128) 3 (1:8) 0 (<1:2)  4 (1:16) 6 (1:64) 0 (<1:2)  0 (<1:2) 4 0 (<1:2)  11  (1:2048) 2 (1:4) 2 (1:4) 1 (1:2)  5 (1:32) 0 (<1:2)  0 (<1:2) 5 7  (1:128) 3 (1:8)  7  (1:128) 5  (1:32) 6 (1:64) 4 (1:16) 1 (1:2) 0 (<1:2) 6 4  (1:16) 7 (1:128)  7 .sup. (1:128) 1 (1:2) 5 (1:32) 6 (1:64) 3 (1:8) 0 (<1:2) 7 3 (1:8) 5 (1:32)  4 .sup. (1:16) 1 (1:2) 8  (1:256) 7 .sup. (1:128) 0 (<1:2).sup.  0 (<1:2) 8 1 (1:2) 7 (1:128) 3 (1:8) 2 (1:4) 6 (1:64) 0 (<1:2)  0 (<1:2).sup.  0 (<1:2) 9 3 (1:8) 8 (1:256)  2 (1:4) 3 (1:8) 8  (1:256) 4 (1:16) 4  (1:16) 0 (<1:2) 10 3 (1:8) 7 (1:128) 4  (1:16) 5  (1:32) 6 (1:64) 2 (1:4)  2 (1:4) 0 (<1:2)

    [0106] It was surprisingly found that Alum hydroxide adjuvanted Type 1 Sabin IPV having 5 DU/dose gave better seroconversion as compared to Salk IPV vaccine with 40 DU/dose and Alum phosphate adjuvanted Sabin IPV having 5 DU/dose.

    TABLE-US-00005 TABLE 5 Type 2 Group 1 Group 2 Group 3 Al(OH)3 Adjuvanted 4 DU( 0.6 mgOH) 8 DU( 0.6 mgOH) 16 DU 0.6 mgOH Rat Sera Sera Sera No SNT +ve Titer SNT +ve Titer SNT +ve Titer 1 3 (1:8)  4 (1:16) 7 (1:128) 2 4 (1:16) 6 (1:64) 5 (1:32)  3 0 (<1:2)  3 (1:8)  5 (1:32)  4 3 (1:8)  4 (1:16) 6 (1:64)  5 5 (1:32) 7  (1:128) 6 (1:64)  6 6 (1:64) 4 (1:16) 9 (1:512) 7 4 (1:16) 7  (1:128) 4 (1:16)  8 5 (1:32) 3 (1:8)  8 (1:256) 9 7  (1:128) 8  (1:256) 8 (1:256) 10 5 (1:32) 3 (1:8)  8 (1:256)

    [0107] Type 2 sIPV having 8 DU/dose with adjuvant gave equivalent sero conversion as compared to Salk IPV vaccine with 8 DU/dose.

    TABLE-US-00006 TABLE 6 Type 3 Group 1 Group 2 Group 3 Al(OH)3 Adjuvanted 10 DU 0.6 mgOH 5 DU 0.6 mgOH 2.5 DU 0.6 mgOH Rat Sera Sera Sera No SNT +ve Titer SNT +ve Titer SNT +ve Titer 1 3 (1:8)  2 (1:4) 0 (<1:2)  2 0 (<1:2)  5  (1:32) 1 (1:2) 3 2 (1:4)  3 (1:8) 1 (1:2) 4 4 (1:16) 2 (1:4) 0 (<1:2)  5 4 (1:16) 2 (1:4) 1 (1:2) 6 4 (1:16) 1 (1:2) 1 (1:2) 7 9  (1:512) 0 (<1:2)  2 (1:4) 8 7  (1:128) 2 (1:4) 2 (1:4) 9 1 (1:2)  0 (<1:2)  1 (1:2) 10 5 (1:32) 7  .sup. (1:128 1 (1:2)

    [0108] It was found that Type 3 sIPV having 10 DU/dose with adjuvant gave equivalent sero conversion as compared to Salk IPV vaccine with 32 DU/dose.

    TABLE-US-00007 TABLE 7 Maximum dose reduction observed for individual Sabin Type 1, 2 & 3 after studies. sIPV Standard dose *SIIL Dose Dose reduction Type 1 40 DU 5 DU ~8 Folds Type 2  8 DU 8 DU Equivalent Type 3 32 DU 10 DU  ~3 Folds

    [0109] SIIL: Serum Institute of India In House dose reduced IPV preparation.

    [0110] In view of the many possible embodiments to which the principles of the disclosed invention may be applied, it should be recognized that the illustrated embodiments are only preferred examples of the invention and should not be taken as limiting the scope of the invention. Rather, the scope of the invention is defined by the following claims. We therefore claim as our invention all that comes within the scope and spirit of these claims.