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    Solutions To 7.012 Problem Set 5: 5' G 3' Cleavage by Bamhi Leaves A 5' Overhang 3' Cctag 5'

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    Ankita Kandalkar
    This document contains solutions to problems from the MIT Biology Department course 7.012: Introductory Biology - Fall 2004. The problems address topics including restriction enzyme cleavage sites, construction of a genomic DNA library, confirming insertion of a target gene into a plasmid, and screening a human library to find the homolog of a mouse gene. Key steps involved digesting DNA with restriction enzymes, ligating DNA fragments, transforming bacteria, using probes to identify sequences of interest, and analyzing DNA fragments on gels.

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    Solutions To 7.012 Problem Set 5: 5' G 3' Cleavage by Bamhi Leaves A 5' Overhang 3' Cctag 5'

    Uploaded by

    Ankita Kandalkar
    172 views5 pages
    This document contains solutions to problems from the MIT Biology Department course 7.012: Introductory Biology - Fall 2004. The problems address topics including restriction enzyme cleavage sites, construction of a genomic DNA library, confirming insertion of a target gene into a plasmid, and screening a human library to find the homolog of a mouse gene. Key steps involved digesting DNA with restriction enzymes, ligating DNA fragments, transforming bacteria, using probes to identify sequences of interest, and analyzing DNA fragments on gels.

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    This document contains solutions to problems from the MIT Biology Department course 7.012: Introductory Biology - Fall 2004. The problems address topics including restriction enzyme cleavage sites, construction of a genomic DNA library, confirming insertion of a target gene into a plasmid, and screening a human library to find the homolog of a mouse gene. Key steps involved digesting DNA with restriction enzymes, ligating DNA fragments, transforming bacteria, using probes to identify sequences of interest, and analyzing DNA fragments on gels.

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    © All Rights Reserved
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    Download as pdf or txt
    172 views5 pages

    Solutions To 7.012 Problem Set 5: 5' G 3' Cleavage by Bamhi Leaves A 5' Overhang 3' Cctag 5'

    Uploaded by

    Ankita Kandalkar
    This document contains solutions to problems from the MIT Biology Department course 7.012: Introductory Biology - Fall 2004. The problems address topics including restriction enzyme cleavage sites, construction of a genomic DNA library, confirming insertion of a target gene into a plasmid, and screening a human library to find the homolog of a mouse gene. Key steps involved digesting DNA with restriction enzymes, ligating DNA fragments, transforming bacteria, using probes to identify sequences of interest, and analyzing DNA fragments on gels.

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    © All Rights Reserved
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    MIT Biology Department

    7.012: Introductory Biology - Fall 2004


    Instructors: Professor Eric Lander, Professor Robert A. Weinberg, Dr. Claudette Gardel

    Solutions to 7.012 Problem Set 5


    Question 1
    Restriction enzymes are extensively used in molecular biology. Below are the recognition sites
    of two of these enzymes, BamHI and BclI.
    a) BamHI, cleaves after the first G:
    5’ GGATCC 3’
    3’ CCTAGG 5’
    Does cleavage by BamHI result in a 5’ or 3’ overhang? What is the sequence of this overhang?

    5’ G 3’ Cleavage by BamHI leaves a 5’ overhang


    3’ CCTAG 5’

    b) BclI cleaves after the first T:


    5’ TGATCA 3’
    3’ ACTAGT 5’
    Does cleavage by BclI result in a 5’ or 3’ overhang? What is the sequence of this overhang?

    5’ T 3’ Cleavage by BclI leaves a 5’ overhang


    3’ ACTAG 5’

    c) Given the DNA shown below …

    5’ ATTGAGGATCCGTAATGTGTCCTGATCACGCTCCACG 3’
    3’ TAACTCCTAGGCATTACACAGGACTAGTGCGAGGTGC 5’
    i) If this DNA was cut with BamHI, how many DNA fragments would you expect?
    Write out the sequence of these double-stranded DNA fragments.
    2 fragments:
    A B
    5’ ATTGAG 3’ 5’ GATCCGTAATGTGTCCTGATCACGCTCCACG 3’
    3’ TAACTCCTAG 5’ 3’ GCATTACACAGGACTAGTGCGAGGTGC 5’

    7.012 Fall 2003 1


    Question 1, continued
    c) ii) If the DNA shown on the previous page in (c) was cut with BclI, how many DNA
    fragment would you expect? Write out the sequence of these double-stranded DNA
    fragments.
    2 fragments.
    C D
    5’ ATTGAGGATCCGTAATGTGTCCT 3’ 5’ GATCACGCTCCACG 3’
    3’ TAACTCCTAGGCATTACACAGGACTAG 5’ 3’ TGCGAGGTGC 5’

    d) You can ligate a restriction fragment produced in (c, i) to one produced in (c, ii). Write out
    the sequence of the resulting fragment.
    A + B 5’ ATTGAGGATCCGTAATGTGTCCTGATCCGTAATGTGTCCTGATCACGCTCCACG 3’
    3’ TAACTCCTAGGCATTACACAGGACTAGGCATTACACAGGACTAGTGCGAGGTGC 5’
    or
    A + D 5’ ATTGAGGATCACGCTCCACG 3’
    3’ TAACTCCTAGTGCGAGGTGC 5’

    or B + C or B + D

    e) Could you cut the fragment from (d) with either BamHI or BclI? Explain.

    No, the recognition sites for both BamHI and for BclI have been destroyed,.

    7.012 Fall 2003 2


    Question 2
    You wake up one morning to your roommate exclaiming about her sudden hair growth. She
    has been supplementing her diet with a strange new fungus purchased at the local farmer’s
    market. You take samples of the fungus to your lab and you find that this fungus does indeed
    make a protein (the harE protein) that stimulates hair growth. You construct a fungal genomic
    DNA library in the hope of cloning the harE gene. If you succeed you will be a billionaire! You
    obtain DNA from the fungus, digest it with a restriction enzyme, and clone it into a vector.

    = ampicillin resistance gene


    = site for unwinding by helicase
    = origin of replication
    = promoter
    = cloning site

    a) Circle the vector that has the MINIMUM features required for your library construction.

    b) You clone your digested genomic DNA into this vector. What type of E. coli (bacteria) cells
    do you need to transform to create your library?
    You need ampicillin sensitive cells.

    c) How do you distinguish bacterial cells that carry a vector from those that do not?
    Bacterial cells that carry a vector will be able to grow on ampicillin whereas untransformed cells will
    not.

    d) Circle on the following lists ALL you would need in order to construct the genomic DNA
    library. Assume you start with intact genomic DNA.
    Enzymes Reagents
    Restriction enzyme Size separation gel
    Ligase Okasaki fragments
    DNA Polymerase ATP, TTP,CTP,GTP
    RNA Polymerase ddATP, ddTTP, ddCTP,
    Transcriptase ddGTP
    Reverse Transcriptase Primers
    3' to 5' exonuclease Replication fork
    Cloning vector Human cells
    Virus

    7.012 Fall 2003 3


    Question 3
    You find a plasmid that you think carries the harE gene, but you need to confirm that indeed
    the target gene has been inserted. When you made your library, you cut your genomic DNA
    with EcoRI and cloned it into a unique EcoRI restriction site in the vector.
    a) How can you use the EcoRI restriction enzyme to tell you if the gene has been inserted?
    You can cut the plasmid with EcoRI and look for two fragments, one that represents the vector and one
    that represents the insert. You would not know for sure that the insert is the harE gene without further
    tests. To confirm that the insert is the harE gene, you would need to know some amino acid sequence of
    the harE protein. You could then make a degenerate nucleic acid probe that would be complementary
    the harE gene sequence.

    Suppose you find that the harE gene is in the plasmid, but now you want a restriction map of
    the recombinant plasmid. You take three individual samples of the plasmid and digest one
    sample with EcoRI, the second sample with HindIII, and the third sample with both EcoRI and
    HindIII. Then you run the digested DNA on a gel to see the fragments.

    b) Considering that the harE gene is smaller than the vector,


    i) Circle the fragments on the gel that contain all or part of the harE gene.
    ii) Draw the restriction map of this recombinant plasmid.

    EcoRI
    harE
    3.0 gene

    1.1

    HindIII

    0.4

    HindIII EcoRI

    2.3
    7.012 Fall 2003 4
    Question 4
    Working in mice, you discover a gene, LC1, that when mutant decreases the incidence of
    cancer in mice. This gene is normally expressed in the lymphatic tissues of mice. You know
    the sequence of this gene, and you really want to see if there is a similar gene is in humans. So,
    you set out to find the human homolog of LC1 by screening a human library.

    a) What kind of human library would you use? Explain.


    Because the LC1 gene may only be expressed in the lymphatic tissues of mice, you may choose to screen
    a genomic library. If you were to screen a cDNA library, you would need to make sure that lymphatic
    specific mRNA’s were represented.

    b) How would you screen the human library for the homolog of LC1?
    Because you know the sequence of the LC1 gene from mice, you could make a probe complementary to
    the mouse sequence. A human homolog, by definition, would have significant sequence similarity. The
    hybridization could be performed at a temperature that would allow probe binding to similar but not
    necessarily identical sequence.

    7.012 Fall 2003 5

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