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DNA Technology

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Title: DNA Technology


1
DNA Technology
  • Chapter 20

2
Plasmid Use
  • Plasmids are good tools for DNA Technology
  • Can be isolated from bacterial cells
  • Often carry resistance genes
  • Isolated genes of interest can be inserted into
    the plasmid
  • How is this insertion done?
  • Restriction endonucleases (enzymes)

3
Restriction Enzymes
  • Where were restriction enzymes first found?
  • Bacterial cells
  • They were used to protect bacteria from intruding
    phage DNA
  • Bacterial DNA is modified to protect it from its
    own restriction enzymes
  • Restriction enzymes often cut DNA leaving sticky
    ends

4
  • Restriction sites are the regions on the DNA that
    the restriction enzyme cuts.
  • Why are restriction sites palindromes?

5
How are restriction enzymes used in DNA
technology?
6
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7
Cloning Genes of Interest
  • How can a biologist make large amounts of a gene
    and thereby produce lots of protein products?
  • Clone the genes in recombinant plasmids

8
Which method of bacterial genomic alteration is
exploited in this process?
9
Genomic Libraries
10
cDNA
  • What is the problem with inserting a human gene
    into a bacterial plasmid?
  • Introns are not spliced in prokaryotes
  • How can this problem be solved?
  • Reverse Transcription of mRNA

11
Why is cDNA shorter than the original eukaryotic
DNA?
12
Probes
  • Radioactive probes can tag a specific gene
    sequence within a mass of DNA
  • Probes are single stranded compliments to known
    sections of the DNA

13
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14
Gel electrophoresis
  • How does gel electrophoresis work?
  • Uses electric charge to separate molecules based
    on their size
  • What charge does DNA have?
  • Negative
  • Which sized fragments will move furthest through
    the gel?
  • Smallest ones

15
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16
Restriction Fragment Analysis
  • Genetic markers are regions of DNA that vary from
    person to person
  • Usually located on non-coding regions of the DNA
  • Using restriction enzymes and gel
    electrophoresis, DNA of different individuals can
    be analyzed and compared
  • Extract DNA and treat it with restriction enzymes

17
How could you detect the differences between
these 2 alleles?
18
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19
Using RFLP Analysis to Detect Harmful Alleles
  • Harmful, disease causing alleles usually have
    identical RFLPs within a family
  • Once the known RFLPs for the normal and disease
    causing alleles are known family members can be
    tested using Southern Blot analysis

20
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21
Southern Blot
Load the gel with the DNA to be tested. Markers
serve as standards for determining sizes of DNA
fragments.
22
  • Separated DNAs are denatured while still in the
    agarose, by soaking the gel in a basic solution
  • Single stranded DNAs are transferred to a nylon
    membrane by blotting

23
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24
  • A Radioactively labeled probe is added to the
    nylon membrane
  • The probe is either RNA or DNA that will
    compliment a specific bp sequence on the DNA
  • After unbound probes have been washed away only
    bound probes remain on the blot

25
VNTR
  • A VNTR is variable numbered tandem repeat
  • Tandem repeats are interspersed throughout the
    genome
  • Different VNTRs can be detected using southern
    blot technique

26
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27
One VNTR is inherited from each parent
  • Southern blot analysis usually shows 2 different
    bands one inherited from each parent
  • How could an individual have one band for the
    VNTR?
  • He/She inherited the same sized VNTR from each
    parent

28
Three different alleles for this particular VNTR
What are the different genotypes for these 6
individuals?
29
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30
Frequency of VNTRs
  • Frequency of allele pattern at a single VNTR has
    been established for specific sites within the
    genome
  • What is the probability of matching a 5 locus DNA
    profile, where each locus is0.01, 0.02, 0.03,
    0.06 and 0.10?
  • One in 27.8 million people will randomly match
    this profile
  • OJs profile was of 24 different loci and he
    matched all 24!
  • The odds were 1 in 10 billion

31
Amplification of DNA
  • What enzymes would be necessary for DNA
    amplification?
  • DNA polymerase and ligase
  • What else would be necessary for the process to
    work?
  • Primers and nucleotides!
  • How was the original DNA initially uncoiled and
    unwound?
  • Heat
  • Why did the heat cause difficulty with the
    procedure?

32
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33
Mapping the Entire Genome
  • Gene linkage mapping uses recombination
    frequencies to construct linkage maps of
    chromosome
  • Chromosome walking will identify sequential
    regions of the chromosome

34
Chromo-some Walking
35
  • DNA Sequencing uses defective nucleotides to
    sequence the DNA.

36
In Situ Hybridization
  • Denatured DNA is placed on slide
  • radioactive single stranded probe is used to
    identify complementary DNA
  • Used to identify genes that different species
    have in common

37
Microassays use in situ hybridization technique
to determine which genes are actively being
expressed in the tissue sample
38
Other uses for the new technology.
39
Gene Therapy
Stem cells are the best candidates for this
therapy
40
  • Pharmaceutical Products
  • Forensics
  • Environment
  • Agriculture
  • Paleontology

41
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42
Determining PaternityWhich child cannot belong
to this set of parents?
43
Which lane represents the father?
3
44
Rape InvestigationDid the suspect commit the
crime?
45
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46
Supplemental Lab 6A
  • In this lab we will transform E. coli bacterial
    colonies with recombinant plasmid DNA
  • It will be your job to distinguish between
    bacterial colonies that have been transformed
    with the recombinant plasmids

47
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48
Procedure for the Transformation
  • Click here to find out more about the procedure

Predict results for your procedure!
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