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Biotechnology and Genetic Engineering PBIO 450550

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Screening a genomic library using DNA hybridization to a (radio ... an enzyme label like alkaline phosphatase or horseradish peroxidase, but it can also be 125I ... – PowerPoint PPT presentation

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Title: Biotechnology and Genetic Engineering PBIO 450550


1
Biotechnology and Genetic EngineeringPBIO 450/550
  • Gene libraries
  • cDNA libraries
  • Library screening

2
Eukaryotic gene organization
enhancers silencers
3
Genomic library construction
4
Screening a genomic library using DNA
hybridization to a (radio-)labeled DNA probe
Note a cDNA is commonly (radio-)labeled and used
as a DNA probe to screen a genomic library
5
Production of a (radio-)labeled DNA probe by the
random primer method uses the Klenow fragment of
DNA polymerase
5
3
5
3
5
3
6
The first step in making a cDNA library
Purification of polyadenylated mRNA using
oligo(dT)-cellulose Note selection of the
proper source (organ, tissue) of the RNA is
critical here!
7
Complementary DNA or cDNA cloningcDNA library
constructionNote ds cDNAs are typically
placed in a cloning vector such as bacteriophage
lambda (l) or a plasmid
8
Bacteriophage lcloning system
9
Bacteriophage l cloning system
Cos sites at the left and right ends
Cloning site
10
There are several possible ways to screen a cDNA
library
  • Using a DNA probe with a homologous sequence
    (e.g., a homologous cDNA or gene clone from a
    related species)
  • Using an oligonucleotide probe based on a known
    amino acid sequence (requires purification of the
    protein and some peptide sequencing)
  • Using an antibody against the protein of interest
    (note this requires use of an expression vector)
  • Plus/minus or differential screening (the least
    specific way)

11
Screening a cDNA library using DNA hybridization
to a (radio-)labeled DNA probe
12
Screening a cDNA library with a labeled
oligonucleotide probe based on a known peptide
sequence
13
Using polynucleotide kinase andg-32P-labeled ATP
to radiolabel oligonucleotide probes
14
Immunological screening of an expression cDNA
library with a primary antibody and labeled
secondary antibody note the label is often an
enzyme label like alkaline phosphatase or
horseradish peroxidase, but it can also be
125INote see also MCB Chapter 9 for a related
animation http//bcs.whfreeman.com/lodish5e/pages/
bcs-main.asp?vcategorys00010n09000i09010.04
o005100061000520005300054000560005700059
00060000700007100001000020000300004000050
010000200003000040000500006000070000800009
000100001100012000130001400015000160001700
018000190002000021000220002300099000ns58
9
15
Animations for two related uses of expression
vectors
  • Expression cloning of receptor proteins-see MCB
    Chapter 9
  • http//bcs.whfreeman.com/lodish5e/pages/bcs-main.a
    sp?vcategorys00010n09000i09010.04o00510
    006100052000530005400056000570005900060000
    700007100001000020000300004000050010000200
    00300004000050000600007000080000900010000
    110001200013000140001500016000170001800019
    0002000021000220002300099000ns589
  • Looking for protein-protein interactions with the
    yeast two hybrid system-see MCB Chapter 11
  • http//bcs.whfreeman.com/lodish5e/pages/bcs-main.a
    sp?s00010n11000i11010.01vcategoryo00510
    006100052000530005400056000570005900060000
    700007100001000020000300004000050010000200
    00300004000050000600007000080000900010000
    110001200013000140001500016000170001800019
    0002000021000220002300099000ns798tuid0
    rau0

16
Plus/min (/-) or differential screening
17
A cosmid cloning systemanother possible cloning
vector which can be used for genomic library but
not for cDNA libraries
18
In summary, you have seen
  • How to make and screen gene libraries
  • How to make and screen cDNA libraries
  • Several different cloning vectors including
    plasmids, bacteriophage lambda (l), and cosmids
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