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Presenters
Aneesa Maaz 13
Mahnoor Anwar 54
Kainat Ayub 60
Contents
• INTRODUCTION
• DEFINITION
• BASIC PRICIPLE OF ELISA
• HISTORY
• EQUIPMENTS
• PROCEDURE
• TYPES(direct, indirect)
• PRECAUTIONS
• ADVANTAGES AND DISADVANTAGES
• LIMITATIONS
• APPLICATIONS
procedure
*Coat 96 well plate with suitable antibody or
antisera....(2 hours or over night)
*wash the wells for three times 5,5 mints with
PBS..(phosphate buffer salline)
*bloock the wells with 10% BSA or skim milk
protien...(1 hr room temp)
*washing again
*Add sample of your taste....(1 hour ,room
temp)
• *the antibody you coated to plate will have
complimentarity to sampl so it wil get bind.
• *washing
• *secondry antibody is added conjugated with
reporter molecule with the help of
biotin...(enzyme or radioactiv molecule)
• Biotin::::>stiptividin::::::>HRPO:::::::;
• *wash to remov unbind molecule
• *now add substrate...(TMB) to the solution
which develop a colour
• *if the test sample contain the antigen the
colour will develop if not present colour will
not develop
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications
ELISA Procedure and Applications

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ELISA Procedure and Applications

  • 1.
  • 2. Presenters Aneesa Maaz 13 Mahnoor Anwar 54 Kainat Ayub 60
  • 3.
  • 4. Contents • INTRODUCTION • DEFINITION • BASIC PRICIPLE OF ELISA • HISTORY • EQUIPMENTS • PROCEDURE • TYPES(direct, indirect) • PRECAUTIONS • ADVANTAGES AND DISADVANTAGES • LIMITATIONS • APPLICATIONS
  • 5.
  • 6.
  • 7.
  • 8.
  • 9.
  • 10.
  • 11.
  • 12.
  • 13.
  • 14.
  • 15.
  • 16.
  • 17. procedure *Coat 96 well plate with suitable antibody or antisera....(2 hours or over night) *wash the wells for three times 5,5 mints with PBS..(phosphate buffer salline) *bloock the wells with 10% BSA or skim milk protien...(1 hr room temp) *washing again *Add sample of your taste....(1 hour ,room temp)
  • 18. • *the antibody you coated to plate will have complimentarity to sampl so it wil get bind. • *washing • *secondry antibody is added conjugated with reporter molecule with the help of biotin...(enzyme or radioactiv molecule) • Biotin::::>stiptividin::::::>HRPO:::::::; • *wash to remov unbind molecule
  • 19. • *now add substrate...(TMB) to the solution which develop a colour • *if the test sample contain the antigen the colour will develop if not present colour will not develop