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Library screening

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LIBRARY SCREENING
The identification of specific clone from a DNA library can be carried out by exploiting either (1)the sequence of the clone or (2)the structure/function of its expressed product. Former type can be applied to genomic or cDNA libraries and nucleic acid hybridization is done with the help of probes or primers. Screening the product of a clone is applied only to expression libraries where the DNA fragment is expressed to yield proteins and the product is recognized by antibody /ligand SEQUENCE DEPENDENT SCREENING Screening by hybridization Nucleic acid hybridization is the most commonly used method and it is rapid
Grunstein &hogness (1975) developed a screening procedure to detect DNA sequences in transformed colonies by hybridization with radioactive RNA probes. The variation of this method is devised By benton and davis and it is called as Plaque lift method. This method is widely used in isolating Recombinant phage particles. Thus hybridiztion has potential to isolate any sequence if probe is available. A number of alternative labeling methods are available that avoid use of radioacticity Incorporation of digoxigenin or biotin detected by specific antibody
SCREENING BY PCR The PCR is widely used to isolate specific DNA sequences from uncloned genomic DNA and now It has been a useful technique for library screening. This method is first demonstrated by takumi . And lodish in 1994 Versatile like hybridization. To isolate a specific clone the PCR is carried out with gene specific primers that flank a unique sequence in the target. Pools of clones are maintained in multiwell plates. Each well is screened by the PCR and positive wells are identified The clone in each positive well are then identified are then diluted into series in a secondary set of plates and screened again
The process is repeated until wells carrying homogeneous clones corresponding the gene of interest have been identified. EXPRESSION LIBRARIES SCREENING. If a DNA library is established using expression vectors, each individual clone can be expressed to yield a polypeptide. This type of screening is important where the DNA sequence of the target sequence is unknown.
IMMUNOLOGICAL SCREENING Developed in 1970 when plasmid vectors are used to construct genomic libraries Immunological screening involves the use of antibodies that specifically recognize antigenic determinants on the polypeptide This technique can be applied to any protein for which an antibody is available. The molecular target for recognition is generally an Epitope. It is a short sequence of amino acid that folds in a particular three dimensional conformation on the surface of the protein.
Broome and Gilbert method was widely used. Transformed cells were plated in Petri dishes and allowed to form colonies. The replica plating is done and colonies were lysed. A sheet of polyvinyl that had been coated with appropriate antibody was then applied to surface allowing antigen antibody complex formation Then sheet was then removed and exposed to 125I labeled IgG and then exposed to X-Ray film. This technique also known as sandwich technique and the protein must have atleast two determinants.
SOUTHWESTERN AND NORTH WESTERN SCREENING a plaque lift is carried out to transfer a print of the library onto nitrocellulose membrane . Here screening is carried out by incubating radio labeled double stranded DNA oligonucleotide probe containing recognition sequence for the DNA-binding protein . Combines the principles of southern and western blots. It has been particularly successful in the isolation of clones expressing cDNA sequences. A limitation of this technique is that since individual plaques contain only single cDNA clones, transcription factors that function only in the form of heterodimers or multimeric complex do not recognize DNA probe. The affinity of the polypeptide for specific DNA sequence must be high. To isolate RNA binding proteins single stranded RNA is used and this method is called as north western screening
Alternatively ligands can be used to identify polypeptides that specifically bind certain molecules. It is not widely used because of low sensitivity .
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Library screening

  • 2. The identification of specific clone from a DNA library can be carried out by exploiting either (1)the sequence of the clone or (2)the structure/function of its expressed product. Former type can be applied to genomic or cDNA libraries and nucleic acid hybridization is done with the help of probes or primers. Screening the product of a clone is applied only to expression libraries where the DNA fragment is expressed to yield proteins and the product is recognized by antibody /ligand SEQUENCE DEPENDENT SCREENING Screening by hybridization Nucleic acid hybridization is the most commonly used method and it is rapid
  • 3. Grunstein &hogness (1975) developed a screening procedure to detect DNA sequences in transformed colonies by hybridization with radioactive RNA probes. The variation of this method is devised By benton and davis and it is called as Plaque lift method. This method is widely used in isolating Recombinant phage particles. Thus hybridiztion has potential to isolate any sequence if probe is available. A number of alternative labeling methods are available that avoid use of radioacticity Incorporation of digoxigenin or biotin detected by specific antibody
  • 4. SCREENING BY PCR The PCR is widely used to isolate specific DNA sequences from uncloned genomic DNA and now It has been a useful technique for library screening. This method is first demonstrated by takumi . And lodish in 1994 Versatile like hybridization. To isolate a specific clone the PCR is carried out with gene specific primers that flank a unique sequence in the target. Pools of clones are maintained in multiwell plates. Each well is screened by the PCR and positive wells are identified The clone in each positive well are then identified are then diluted into series in a secondary set of plates and screened again
  • 5. The process is repeated until wells carrying homogeneous clones corresponding the gene of interest have been identified. EXPRESSION LIBRARIES SCREENING. If a DNA library is established using expression vectors, each individual clone can be expressed to yield a polypeptide. This type of screening is important where the DNA sequence of the target sequence is unknown.
  • 6. IMMUNOLOGICAL SCREENING Developed in 1970 when plasmid vectors are used to construct genomic libraries Immunological screening involves the use of antibodies that specifically recognize antigenic determinants on the polypeptide This technique can be applied to any protein for which an antibody is available. The molecular target for recognition is generally an Epitope. It is a short sequence of amino acid that folds in a particular three dimensional conformation on the surface of the protein.
  • 7. Broome and Gilbert method was widely used. Transformed cells were plated in Petri dishes and allowed to form colonies. The replica plating is done and colonies were lysed. A sheet of polyvinyl that had been coated with appropriate antibody was then applied to surface allowing antigen antibody complex formation Then sheet was then removed and exposed to 125I labeled IgG and then exposed to X-Ray film. This technique also known as sandwich technique and the protein must have atleast two determinants.
  • 8. SOUTHWESTERN AND NORTH WESTERN SCREENING a plaque lift is carried out to transfer a print of the library onto nitrocellulose membrane . Here screening is carried out by incubating radio labeled double stranded DNA oligonucleotide probe containing recognition sequence for the DNA-binding protein . Combines the principles of southern and western blots. It has been particularly successful in the isolation of clones expressing cDNA sequences. A limitation of this technique is that since individual plaques contain only single cDNA clones, transcription factors that function only in the form of heterodimers or multimeric complex do not recognize DNA probe. The affinity of the polypeptide for specific DNA sequence must be high. To isolate RNA binding proteins single stranded RNA is used and this method is called as north western screening
  • 9. Alternatively ligands can be used to identify polypeptides that specifically bind certain molecules. It is not widely used because of low sensitivity .