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    Unit 10 - Mutagenesis PDF

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    vuivevuive
    Site-directed mutagenesis used to make specific and intentional changes to the DNA sequence of a gene and any gene products. M13 phages can be used to make mutagenic changes to the genetic code. Phage-based mutations can Also be used to Alter the function of a protein.

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    Unit 10 - Mutagenesis PDF

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    vuivevuive
    231 views5 pages
    Site-directed mutagenesis used to make specific and intentional changes to the DNA sequence of a gene and any gene products. M13 phages can be used to make mutagenic changes to the genetic code. Phage-based mutations can Also be used to Alter the function of a protein.

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    Site-directed mutagenesis used to make specific and intentional changes to the DNA sequence of a gene and any gene products. M13 phages can be used to make mutagenic changes to the genetic code. Phage-based mutations can Also be used to Alter the function of a protein.

    Copyright:

    © All Rights Reserved
    Download as PDF, TXT or read online from Scribd
    Download as pdf or txt
    231 views5 pages

    Unit 10 - Mutagenesis PDF

    Uploaded by

    vuivevuive
    Site-directed mutagenesis used to make specific and intentional changes to the DNA sequence of a gene and any gene products. M13 phages can be used to make mutagenic changes to the genetic code. Phage-based mutations can Also be used to Alter the function of a protein.

    Copyright:

    © All Rights Reserved
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    Download as pdf or txt
    You are on page 1of 5

    30-May-16

    Uses for mutagenesis


    Unit 10
    Recombinant engineering of
    gene function: mutagenesis

    Define the role of a gene--are phenotypes


    altered by mutations?
    Determine functionally important regions of a
    gene (in vivo or in vitro)
    Improve or change the function of a gene
    product
    Investigate functions of non-genes, eg. DNA
    regions important for regulation

    Obtaining useful enzymes

    Protein engineering-Why?
    Enhance stability/function under new conditions
    temperature, pH, organic/aqueous solvent,
    Alter enzyme substrate specificity
    Enhance enzymatic rate
    Alter epitope binding properties

    From Koeller and Wang, enzymes for chemical synthesis, Nature 409, 232 - 240 (2001)

    Types of Mutagenesis
    PCR Based Methods

    Site-directed mutagenesis
    Mismatched mutagenesis
    5 add on mutagenesis
    Cassette Mutagenesis

    Insertional Mutagenesis
    Trasposon mutagenesis

    In vivo Mutagenesis
    Direct Mutagenesis

    Site-directed mutagenesis
    used to make specific and intentional changes to
    the DNA sequence of a gene and any gene
    products.
    Also called site-specific mutagenesis or
    oligonucleotide-directed mutagenesis, it is used
    for investigating the structure and biological
    activity of DNA, RNA, and protein molecules,
    and for protein engineering.

    30-May-16

    Mismatched mutagenesis
    Similar to Site-Directed Mutagenesis
    But only focuses on a single amino acid
    Important when trying to determine a
    particular missense mutation in known gene
    of a disease.
    Or when just trying to evaluate the
    contributation of the single amino acid to the
    function of the protein.

    Altering the genetic code

    The genetic code


    61 sense codons, 3 non-sense (stop) codons
    20 amino acids
    Other amino acids, some in the cell (as precursors to other
    amino acids), but very rarely have any been added to the
    genetic code in a living system
    Is it possible to add new amino acids to the code?
    Yes...sort of
    Wang et al. (2001) Expanding the genetic code Science 292, p.
    498.

    1. Mutagenesis using Using M13 phage vector

    on gene or
    cDNA c ci
    vo

    Screen for
    mutant

    In this way, a single-stranded DNA molecule is converted into a


    double-stranded molecule, where all sequences will be wild-type
    except the region containing the nucleotides. The resulting doublestranded heteroduplex DNA molecule, composed of one wild-type
    strand and one mutant strand, is introduced into competent E. coli
    cells, where the two strands segregate by DNA replication.
    Theoretically, each colony should contain both wild-type and mutant
    plasmids; in practice, however, only one sequence is often obtained
    from a colony due to mismatch repair prior to replication of the two
    strands. Generally, the frequency of mutant plasmids is lower than
    that of the wild type. This is most likely due to incomplete DNA
    replication in vitro. A number of selection or screening methods have
    been developed to enrich for plasmids with the desired mutation
    mismatch repair prior to replication of the two strands.

    30-May-16

    (Stratagene)

    Primer design for


    site-directed mutagenesis

    5
    3

    *
    *

    3
    5

    5. Mega-primer
    method

    6. Overlapextension
    method

    The amplified
    product from the
    first round of PCR is
    used as a primer in
    the second round of
    PCR.

    WRONG?

    7. Inverse PCR

    Inverse PCR

    Q5 Site-Directed Mutagenesis Kit

    30-May-16

    Inverse PCR

    Q5 Site-Directed Mutagenesis Kit

    8. The 5 add on Mutagenesis


    Involves adding on a new sequence or
    chemical group to the 5end of a PCR product
    This involves a particular way of designing the
    primers:
    3 end of the primer matches the sequence of PCR
    product.
    5 end contains the novel sequence
    Suitable restriction site
    Addition of a functional sequence (promoter sequence)
    Modified nucleotide that contains labeled group,
    biotinlyated, or fluorophore.

    9. Cassette
    Mutagenesis

    Used to introduce
    multiple mutations
    into the DNA
    sequence
    Synthesis oligo

    T4 lysozyme: a model for stability studies

    An example
    Cysteines were added to
    areas of the protein in
    close proximity--disulfide
    bridges could form
    T4 lysozyme: structure known
    Can it be made more stable by
    the addition of pairs of cysteine
    residues (allowing disulfide
    bridges to form?) without altering
    activity of the protein?

    30-May-16

    Stability can be increased - but there can be a cost in activity

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