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Immunomodulators(Suppressant & Stimulants)
SOURIN
DE
FIRST YEAR
MPHARM
Introduction
• Immunomodulators, as the name implies, are drugs that modify the actions of the immune system
(Immunostimulants & Immunosuppressants)
• Immunostimulants or immune stimulants are drugs that energize the immune system when it is
exhausted from fighting prolonged invasion or when the immune system needs help fighting a
specific pathogen or cancer cell. It is one of the classifications of drug called immunomodulators.
• Immunosuppressants are drugs which inhibit cellular/humoral or both types of immune
responses, and have their major use in organ transplantation and autoimmune diseases.
Drugs :
Immunosuppressant :
• Glucocorticoids: Corticosteroids
• Calcineurin Inhibitor: Cyclosporine, Tacrolimus
• Antimetabolic agent: sirolimus, Everolimus, Azathioprine, Thalidomicine.
Immunostimulants:
• Bacterial vaccine: TB
• Interferons: α, β, γ
• Interleukins: Aldesleukin,Oprelvekin
• Therapeutic Vaccine : Tuberculosis, AIDS , Hepatitis B
Screening Methods:
IN VITRO MEHODS
1. Inhibition of histamine release from mast cells.
2. Mitogen induced lymphocyte proliferation.
3. Inhibition of T cell proliferation.
4. Chemiluminescence in macrophages.
5. PFC (plaque forming colony) test in vitro.
1.Acute systemic anaphylaxis in rats
2.Anti-anaphylactic activity
(Schultz-Dale reaction)
3.Delayed type hypersensitivity
4.Spontaneous autoimmune diseases in animals
5.Passive cutaneous anaphylaxis
6.Arthus type immediate hypersensitivity
7.Reversed passive Arthus reaction
8.Adjuvant arthritis in rats
IN VIVO METHODS
I. IN VITRO METHODS
a) Inhibition of histamine release from mast cells:
PURPOSE AND RATIONALE:
Hypersensitivity reactions can be elicited by various factors:
 immunologically induced
 non-immunologically induced, or
 the mediation through immune responses.
Mediators responsible for hypersensitivity reactions are released from mast cells.
An important preformed mediator of allergic reactions found in these cells is histamine.
PROCEDURE:
Preparation of mast cell suspension:
 Wistar rats are decapitated and exsanguinated
 50 ml of Hank’s balanced salt solution (HBSS) are injected into the peritoneal cavity & following massage of
the body, the abdominal wall is opened
 The fluid containing peritoneal cells is collected in a centrifuge tube and centrifuged at 2000 rpm.
 The cells are re suspended in HBSS.
 Then the cell suspension is brought to a final concentration of 105 mast cells/100 μl.
Test compound administration and induction of histamine release:
 1 ml test drug is added to the mast cell suspension. incubated at 37 °C for 15 min.
 The cells are made up to a volume of 3 ml with HBSS an equal volume of calcium-ionophore(6-10g/ml)compound or
specific allergen is added.
 The suspension incubated at 37 °C for 30 min followed by centrifugation at 2500 rpm.
Determination of histamine release : The total sample is transferred to an autosampler vial and the histamine
concentration is determined by a fluorescence detector (using excitation & emission wavelength of 350 &
450nm respectively).
EVALUATION:
 Percent histamine release can be expressed by the following formula:
sample hist. rel.- spontaneous hist. rel x 100
100% hist. rel.- spontaneous hist. rel.
b) Mitogen induced lymphocyte proliferation:
PURPOSE AND RATIONALE
 Cultured lymphocytes can be stimulated to DNA synthesis by various mitogens.
 Measurement of DNA synthesis can be accomplished by tritiated thymidine which is incorporated
into the newly synthesized DNA.
 Immunmodulating properties can be detected either by pre-treatment of the animals in vivo or by
adding the test drug to the cultured lymphocytes.
PROCEDURE:
Ex Vivo: Mice or rats are used.
 Animals receive the test compound once a day for 5 days.
• They are sacrificed, spleens are removed and a single cell suspension of 5 × 10^6 cells/ml is prepared.
 Mitogens are titrated in 0.1 ml/well and add 0.1ml suspension.
 Plates are incubated at 37 °C in 5% CO2 in air for 48–60 h and for another 8 h after addition of 3H-
thymidine per well.
 Cells are harvested on glass fibre filters and after drying the degree of radioactivity is determined.
IN VITRO
 Animals are sacrificed and their spleens removed.
 A single cell suspension of 10^7 cells/ ml is prepared and 0.05 ml placed in each microtiter well.
 Then the test compound is added in 0.05 ml.
 At last 0.1 ml of the double concentrated mitogen is added. Plates are incubated for 48–60 hr and for
another 8 hr after addition of 3H-thymidine per well.
 Cells are harvested on glass fiber filters and after drying the degree of radioactivity is determined.
EVALUATION:
 Stimulation index = proliferation ratio according to positive control, either with or without mean spleen
weight.
INVIVO METHODS
a) Anti-anaphylactic activity (Schultz-Dale reaction)
PURPOSE AND RATIONALE
 Guinea pigs are sensitized against egg albumin.
 Challenge after 3 weeks causes in isolated organs release of mediators, e.g. histamine, which induce
contraction in isolated ileum.
PROCEDURE
 Guinea pigs of either sex weighing 300–350 g are sensitized with alum precipitated egg albumin.
 Alum egg albumin is prepared by dissolving egg albumin(1 mg/ml) in six percent aluminium hydroxide gel,
suspended in saline.
 The mixture is stirred and kept at room temperature.
 Each animal receives at the same time injections of 0.125 ml of this mixture in each foot pad and 0.5 ml subcutaneously.
 After 4 weeks the animals are killed and the ileum is dissected out.
 Cleaned pieces, about 2–3 cm long, are mounted in an organ bath containing Tyrode solution at 37 °C.
 The strips are allowed to equilibrate for 15 min.
 The contractility of the ileum strips is tested by adding 10^- 4 g/ml BaCl2 solution.
 To one organ bath serve as a control.
 After 3 min ovalbumin in a final concentration of 2 × 10^ -6 g/ml is added.
 The contractions are recorded with strain gauges by a polygraph
EVALUATION
 The results are expressed as presence or absence of blocking activity (percentage inhibition).
 If anti-anaphylactic activity is observed, ED50 values using different doses are calculated.
b) Delayed type hypersensitivity
PURPOSE AND RATIONALE
 Delayed type hypersensitivity is a reaction of cell mediated immunity and becomes visible only after 16–24 h.
 The same methods as for testing immediate type hypersensitivity can be used.
PROCEDURE
 Rats are sensitized in the same way by i.m. administration of 0.5 ml ovalbumin suspension 7 days prior to the
start of the experiment .
 They are challenged by injection of 0.1 ml of 0.04% solution of highly purified ovalbumin in the left hind paw.
 Footpad thickness is measured immediately and 24 h after ovalbumin administration.
Evaluation
 The amount of Evans blue extracted from passive cutaneous anaphylactic reaction is
taken as 100 percent.
 Percent inhibition of passive cutaneous anaphylactic calculated.
 The standard disodium cromoglycate at a dose of 3 mg/kg i.v. or 30 mg/kg orally results
in 80–100% inhibition.
 Using different doses, ED50 values can be calculated.
c) Acute systemic anaphylaxis in rats
PURPOSE AND RATIONALE
• Rats are immunized with ovalbumin and Bordetella pertussis suspension as adjuvant
• After 11 days the animals are challenged by intravenous injection of ovalbumin.
• The shock symptoms can by inhibited by corticosteroids and intravenous disodium cromoglycate.
• PROCEDURE
• Female Sprague-Dawley rats weighing 120 g are immunized by i.m. injection of 10 mg/kg highly
purified ovalbumin.
• Simultaneously 1 ml of Bordetella pertussis suspension (2 × 1010 organisms) is injected
intraperitoneally .
• IgE antibodies are induced and attached to the surface of mast cells and basophilic granulocytes.
 Eleven days later the animals are challenged by intravenous injection of 25 mg/kg highly purified ovalbumin.
 This results in formation of antigen-antibody-complexes on the surface of mast cells and basophilic
granulocytes in blood and in all organs with immediate release of various mediators of anaphylaxis, such as
histamine, serotonin, SRS-A, prostaglandins; in shock symptoms and 80% lethality.
 Corticosteroids, e.g. dexamethasone 1–10 mg/kg s.c. are given 18 h prior to challenge,or 30 mg/kg disodium
cromoglycate i.v. before injection of ovalbumin. Ten–20 animals are used for each group.
 EVALUATION
 The shock symptoms are scored and mortality counted.
 Results after treatment are compared with untreated controls.
 Pre treatment with corticosteroids or disodium cromoglycate can inhibit death and ameliorate shock symptoms.
 Statistical calculation is performed using the χ2-test.
d)Arthus type Immediate hypersensitivity
PURPOSE AND RATIONALE
• There is an Ag-Ab complex after the injection of antigen. But if the animal is previously
immunized with the antibody there is precipitation of allergic reaction.
• Ag-Ab induced reaction leading to an inflammatory factors that characterized by edema,
hemorrhage.
PROCEDURE:
• Seven days prior to experiment Wistar rats of 250-300 gm are sensitized by i.m.
administration of 0.5 ml of the ovalalbumin suspension + pertusis vaccine in saline slon.
mixed together to get emulsion.
• 1st group (treated group) : 1 hr prior test compound are administered and challenge with
0.1 ml of ovalalbumin in the left hind paw.
• 2nd group ( positive control) : Sensitized animal treated with solvent alone.
• 3rd group ( negative control) : Non-sensitized animals treated with solvent.
EVALUATION
• The change in footpad thickness is expressed as percent change from
the vehicle control group.
• Thickness can be measured by calipers.
REFERENCE
• Drug Screening methods by SK Gupta
• Drug discovery and evaluation by Gerhard Vogel
• Ncbi
• Science Direct
• ResearchGate
ABSTRACT
Immunosuppressant :
• over the past decade have resulted in dramatic improvements in short- and long-term outcomes in organ
transplantation as well as a decreased incidence of acute rejection. However, immunosuppressive drugs need to
be given long term, lack specificity, and are accompanied by adverse metabolic derangements, toxicities, the risk
of infection and cancer, and a myriad of other side effects. This review will outline a number of
immunosuppressive agents that are currently being explored in experimental and clinical transplantation. These
include biologic agents that have more specificity and selectivity, and are aimed at T-cell depletion, blockade of
costimulation, adhesion markers, or at novel targets.
Immunomodulators:
• Immunology is one of the most rapidly developing areas of medical biotechnology research & has great
promises with regard to the prevention & treatment of a wide range of disorders such as inflammatory disease of
skin , gut, respiratory tract.
• Immunomodulators are natural or synthetic substances that help to regulate the immune system .
• Immunomodulators correct the immune system which are not balanced. Natural immunomodulators are less
potent than prescription immunomodulators & less likely to cause side effects.
• Prescription immunomodulators such as Azathioprine 6-mercaptopurine methotrexate , etc.
• The benefits of immunomodulators stem from their ability to stimulate natural & adaptive defense mechanisms
such as cytokines which enable the body to help itself.
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SCREENING OF immuno.pptx

  • 2. Introduction • Immunomodulators, as the name implies, are drugs that modify the actions of the immune system (Immunostimulants & Immunosuppressants) • Immunostimulants or immune stimulants are drugs that energize the immune system when it is exhausted from fighting prolonged invasion or when the immune system needs help fighting a specific pathogen or cancer cell. It is one of the classifications of drug called immunomodulators. • Immunosuppressants are drugs which inhibit cellular/humoral or both types of immune responses, and have their major use in organ transplantation and autoimmune diseases.
  • 3. Drugs : Immunosuppressant : • Glucocorticoids: Corticosteroids • Calcineurin Inhibitor: Cyclosporine, Tacrolimus • Antimetabolic agent: sirolimus, Everolimus, Azathioprine, Thalidomicine. Immunostimulants: • Bacterial vaccine: TB • Interferons: α, β, γ • Interleukins: Aldesleukin,Oprelvekin • Therapeutic Vaccine : Tuberculosis, AIDS , Hepatitis B
  • 4. Screening Methods: IN VITRO MEHODS 1. Inhibition of histamine release from mast cells. 2. Mitogen induced lymphocyte proliferation. 3. Inhibition of T cell proliferation. 4. Chemiluminescence in macrophages. 5. PFC (plaque forming colony) test in vitro.
  • 5. 1.Acute systemic anaphylaxis in rats 2.Anti-anaphylactic activity (Schultz-Dale reaction) 3.Delayed type hypersensitivity 4.Spontaneous autoimmune diseases in animals 5.Passive cutaneous anaphylaxis 6.Arthus type immediate hypersensitivity 7.Reversed passive Arthus reaction 8.Adjuvant arthritis in rats IN VIVO METHODS
  • 6. I. IN VITRO METHODS a) Inhibition of histamine release from mast cells: PURPOSE AND RATIONALE: Hypersensitivity reactions can be elicited by various factors:  immunologically induced  non-immunologically induced, or  the mediation through immune responses. Mediators responsible for hypersensitivity reactions are released from mast cells. An important preformed mediator of allergic reactions found in these cells is histamine. PROCEDURE: Preparation of mast cell suspension:  Wistar rats are decapitated and exsanguinated  50 ml of Hank’s balanced salt solution (HBSS) are injected into the peritoneal cavity & following massage of the body, the abdominal wall is opened
  • 7.  The fluid containing peritoneal cells is collected in a centrifuge tube and centrifuged at 2000 rpm.  The cells are re suspended in HBSS.  Then the cell suspension is brought to a final concentration of 105 mast cells/100 μl. Test compound administration and induction of histamine release:  1 ml test drug is added to the mast cell suspension. incubated at 37 °C for 15 min.  The cells are made up to a volume of 3 ml with HBSS an equal volume of calcium-ionophore(6-10g/ml)compound or specific allergen is added.  The suspension incubated at 37 °C for 30 min followed by centrifugation at 2500 rpm.
  • 8. Determination of histamine release : The total sample is transferred to an autosampler vial and the histamine concentration is determined by a fluorescence detector (using excitation & emission wavelength of 350 & 450nm respectively). EVALUATION:  Percent histamine release can be expressed by the following formula: sample hist. rel.- spontaneous hist. rel x 100 100% hist. rel.- spontaneous hist. rel.
  • 9.
  • 10. b) Mitogen induced lymphocyte proliferation: PURPOSE AND RATIONALE  Cultured lymphocytes can be stimulated to DNA synthesis by various mitogens.  Measurement of DNA synthesis can be accomplished by tritiated thymidine which is incorporated into the newly synthesized DNA.  Immunmodulating properties can be detected either by pre-treatment of the animals in vivo or by adding the test drug to the cultured lymphocytes. PROCEDURE: Ex Vivo: Mice or rats are used.  Animals receive the test compound once a day for 5 days. • They are sacrificed, spleens are removed and a single cell suspension of 5 × 10^6 cells/ml is prepared.  Mitogens are titrated in 0.1 ml/well and add 0.1ml suspension.
  • 11.  Plates are incubated at 37 °C in 5% CO2 in air for 48–60 h and for another 8 h after addition of 3H- thymidine per well.  Cells are harvested on glass fibre filters and after drying the degree of radioactivity is determined. IN VITRO  Animals are sacrificed and their spleens removed.  A single cell suspension of 10^7 cells/ ml is prepared and 0.05 ml placed in each microtiter well.  Then the test compound is added in 0.05 ml.  At last 0.1 ml of the double concentrated mitogen is added. Plates are incubated for 48–60 hr and for another 8 hr after addition of 3H-thymidine per well.  Cells are harvested on glass fiber filters and after drying the degree of radioactivity is determined.
  • 12. EVALUATION:  Stimulation index = proliferation ratio according to positive control, either with or without mean spleen weight.
  • 13.
  • 14. INVIVO METHODS a) Anti-anaphylactic activity (Schultz-Dale reaction) PURPOSE AND RATIONALE  Guinea pigs are sensitized against egg albumin.  Challenge after 3 weeks causes in isolated organs release of mediators, e.g. histamine, which induce contraction in isolated ileum. PROCEDURE  Guinea pigs of either sex weighing 300–350 g are sensitized with alum precipitated egg albumin.  Alum egg albumin is prepared by dissolving egg albumin(1 mg/ml) in six percent aluminium hydroxide gel, suspended in saline.
  • 15.  The mixture is stirred and kept at room temperature.  Each animal receives at the same time injections of 0.125 ml of this mixture in each foot pad and 0.5 ml subcutaneously.  After 4 weeks the animals are killed and the ileum is dissected out.  Cleaned pieces, about 2–3 cm long, are mounted in an organ bath containing Tyrode solution at 37 °C.  The strips are allowed to equilibrate for 15 min.  The contractility of the ileum strips is tested by adding 10^- 4 g/ml BaCl2 solution.  To one organ bath serve as a control.  After 3 min ovalbumin in a final concentration of 2 × 10^ -6 g/ml is added.  The contractions are recorded with strain gauges by a polygraph EVALUATION  The results are expressed as presence or absence of blocking activity (percentage inhibition).  If anti-anaphylactic activity is observed, ED50 values using different doses are calculated.
  • 16. b) Delayed type hypersensitivity PURPOSE AND RATIONALE  Delayed type hypersensitivity is a reaction of cell mediated immunity and becomes visible only after 16–24 h.  The same methods as for testing immediate type hypersensitivity can be used. PROCEDURE  Rats are sensitized in the same way by i.m. administration of 0.5 ml ovalbumin suspension 7 days prior to the start of the experiment .  They are challenged by injection of 0.1 ml of 0.04% solution of highly purified ovalbumin in the left hind paw.  Footpad thickness is measured immediately and 24 h after ovalbumin administration.
  • 17. Evaluation  The amount of Evans blue extracted from passive cutaneous anaphylactic reaction is taken as 100 percent.  Percent inhibition of passive cutaneous anaphylactic calculated.  The standard disodium cromoglycate at a dose of 3 mg/kg i.v. or 30 mg/kg orally results in 80–100% inhibition.  Using different doses, ED50 values can be calculated.
  • 18. c) Acute systemic anaphylaxis in rats PURPOSE AND RATIONALE • Rats are immunized with ovalbumin and Bordetella pertussis suspension as adjuvant • After 11 days the animals are challenged by intravenous injection of ovalbumin. • The shock symptoms can by inhibited by corticosteroids and intravenous disodium cromoglycate. • PROCEDURE • Female Sprague-Dawley rats weighing 120 g are immunized by i.m. injection of 10 mg/kg highly purified ovalbumin. • Simultaneously 1 ml of Bordetella pertussis suspension (2 × 1010 organisms) is injected intraperitoneally . • IgE antibodies are induced and attached to the surface of mast cells and basophilic granulocytes.
  • 19.  Eleven days later the animals are challenged by intravenous injection of 25 mg/kg highly purified ovalbumin.  This results in formation of antigen-antibody-complexes on the surface of mast cells and basophilic granulocytes in blood and in all organs with immediate release of various mediators of anaphylaxis, such as histamine, serotonin, SRS-A, prostaglandins; in shock symptoms and 80% lethality.  Corticosteroids, e.g. dexamethasone 1–10 mg/kg s.c. are given 18 h prior to challenge,or 30 mg/kg disodium cromoglycate i.v. before injection of ovalbumin. Ten–20 animals are used for each group.  EVALUATION  The shock symptoms are scored and mortality counted.  Results after treatment are compared with untreated controls.  Pre treatment with corticosteroids or disodium cromoglycate can inhibit death and ameliorate shock symptoms.  Statistical calculation is performed using the χ2-test.
  • 20. d)Arthus type Immediate hypersensitivity PURPOSE AND RATIONALE • There is an Ag-Ab complex after the injection of antigen. But if the animal is previously immunized with the antibody there is precipitation of allergic reaction. • Ag-Ab induced reaction leading to an inflammatory factors that characterized by edema, hemorrhage. PROCEDURE: • Seven days prior to experiment Wistar rats of 250-300 gm are sensitized by i.m. administration of 0.5 ml of the ovalalbumin suspension + pertusis vaccine in saline slon. mixed together to get emulsion. • 1st group (treated group) : 1 hr prior test compound are administered and challenge with 0.1 ml of ovalalbumin in the left hind paw. • 2nd group ( positive control) : Sensitized animal treated with solvent alone. • 3rd group ( negative control) : Non-sensitized animals treated with solvent.
  • 21. EVALUATION • The change in footpad thickness is expressed as percent change from the vehicle control group. • Thickness can be measured by calipers.
  • 22. REFERENCE • Drug Screening methods by SK Gupta • Drug discovery and evaluation by Gerhard Vogel • Ncbi • Science Direct • ResearchGate
  • 23.
  • 24. ABSTRACT Immunosuppressant : • over the past decade have resulted in dramatic improvements in short- and long-term outcomes in organ transplantation as well as a decreased incidence of acute rejection. However, immunosuppressive drugs need to be given long term, lack specificity, and are accompanied by adverse metabolic derangements, toxicities, the risk of infection and cancer, and a myriad of other side effects. This review will outline a number of immunosuppressive agents that are currently being explored in experimental and clinical transplantation. These include biologic agents that have more specificity and selectivity, and are aimed at T-cell depletion, blockade of costimulation, adhesion markers, or at novel targets. Immunomodulators: • Immunology is one of the most rapidly developing areas of medical biotechnology research & has great promises with regard to the prevention & treatment of a wide range of disorders such as inflammatory disease of skin , gut, respiratory tract. • Immunomodulators are natural or synthetic substances that help to regulate the immune system . • Immunomodulators correct the immune system which are not balanced. Natural immunomodulators are less potent than prescription immunomodulators & less likely to cause side effects. • Prescription immunomodulators such as Azathioprine 6-mercaptopurine methotrexate , etc. • The benefits of immunomodulators stem from their ability to stimulate natural & adaptive defense mechanisms such as cytokines which enable the body to help itself.