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BLOTTING TECHNIQUES

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Northern blot: Identification of a specific RNA sequence using a specific RNA probe. Western blot: Identification of a specific protein using specific antibodies. – PowerPoint PPT presentation

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Title: BLOTTING TECHNIQUES


1
BLOTTING TECHNIQUES
By
Dr. Emad AbdElhameed Morad
Lecturer of Medical Microbiology and Immunology
2
Types of blotting
  • Southern blot
  • Identification of a specific DNA sequence using
    a specific DNA probe.
  • Northern blot
  • Identification of a specific RNA sequence using
    a specific RNA probe.
  • Western blot
  • Identification of a specific protein using
    specific antibodies.

3
Southern blot
  • This method is named after its inventor (1971),
    Edmond Southern.

Whole DNA is extracted then digested by
restriction enzyme
DNA fragments
Gel electrophoresis
Blotting and transfer to membrane
Detection by probes
4
  • Restriction fragment length polymorphism
  • Extract DNA from the sample
  • Digest the extracted DNA by specific restriction
    endonuclease enzyme
  • This is followed by agarose gel electrophoresis
    of the restriction fragments
  • The pattern on the gel is called restriction
    fragment length polymorphism
  • This is used in paternity testing

5
Steps of southern blot
  • DNA is extracted from the cell.
  • Extracted DNA is digested by restriction enzyme
    into smaller fragments called restriction
    fragments.
  • These restriction fragments are then subjected
    to agarose gel electrophoresis.
  • These fragments will be separated on the gel
    according to their molecular weight. Smaller
    fragments migrate faster.

6
  1. After electrophoresis, the gel is blotted on
    nitrocellulose membrane.
  2. During blotting, the DNA fragments will be
    transferred by capillarity from the gel to the
    membrane.
  3. Special probes are then applied to the membrane
    where they will combine with the complementary
    fragments.
  4. These probes are labeled by radioactive isotope
    which could be easily detected by X-ray film as
    dark spots on the membrane.

7
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8
Northern blot
  • It is done by the same technique of Southern
    blot but replacing DNA by mRNA molecules.
  • And, labeled RNA probes are used for detection
    in stead of DNA probes.

9
Western blot
  • It consists of two steps

Western blot
1- SDS PAGE
2 steps
2- Immunoblot
10
SDS PAGE
  • First, the protein sample is subjected to
    electrophoresis on SDS polyacrylamide gel.
  • SDS sodium dodecyl sulfate unfolds the complex
    structure of the proteins and loads them with
    negative charges.
  • On the gel, the proteins will move toward the
    positive electrode and separated according to
    their molecular weight. Smaller proteins migrate
    faster.

11
Immunoblot
  • The gel is then blotted on nitrocellulose
    membrane using electrophoresis inside immunoblot
    apparatus.
  • Note that inside the immunoblot apparatus, the
    gel must be placed toward the negative electrode
    and the membrane is placed toward the positive
    electrode.
  • Inside the immunoblot apparatus, proteins on the
    gel will be transferred to the membrane.

12
  • After blotting, the membrane is blocked by
    adding serum albumin which prevents nonspecific
    absorption of antibodies that will be added to
    the membrane.
  • Then, the membrane is mixed with primary
    antibody against the protein of interest.
  • After washing the membrane, it is mixed with
    secondary antibody against the primary antibody.
    Note that secondary antibody is labeled with
    enzyme.
  • After washing the membrane, a substrate for the
    enzyme is added to the membrane.
  • The enzyme acts on the substrate producing color
    at the site of protein of interest.

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Applications of blotting techniques
  • Diagnosis of infectious diseases like
    tuberculosis.
  • Diagnosis of tumors like leukemia and lymphoma.
  • Diagnosis of genetic diseases.
  • In forensic medicine like paternity testing.

15
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