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Housekeeping

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Specific piece (directed) All genomic (random) 2. Shear DNA. 3. Clone ... Amplify the piece we want to sequence. Identify the nucleotide order. What do we need? ... – PowerPoint PPT presentation

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Title: Housekeeping


1
Housekeeping
  • Homework 3 due May 5
  • Question 4 P. multocida EcoRI BamHI 1.0, 2.0,
    5.0, 6.0 kb (no 3.0 kb)
  • SKIP QUESTION 9
  • Exam III-May 9
  • Homework 4 due May 14th
  • Lab
  • Quiz 3 THIS WEEK
  • Quiz 4 next week (cumulative)

2
The perils of tuberculosis
3
Sequencing the M. tuberculosis genome
  • Create a genomic library
  • Sequence the genomic library
  • Alignment of these sequences (what sequence goes
    where?)
  • Identification of GENES

4
Create a genomic library
  • 1. Isolate genomic DNA
  • Specific piece (directed)
  • All genomic (random)
  • 2. Shear DNA
  • 3. Clone into a vector

5
Create a genomic library
  • 1. Isolate genomic DNA
  • Specific piece (directed)
  • All genomic (random)
  • 2. Shear DNA
  • 3. Clone into a vector

What do we need to do with our pieces?
6
What do we want to do with these DNA pieces?
  • Isolate them (purify them)
  • Amplify them
  • Sequence them

Clone them!
7
Whats a vector? Why do we need one?
8
Reasons for a Vector
  • Allow for transport of individual fragments
  • Can get into its host
  • Allow for replication of individual fragments
  • Can replicate in its host
  • Allow for purification of individual fragments
  • Can extract it from its host

9
Types of vectors
Vector
Vector Host
Insert size
Plasmids
Bacteria
Up to 15 kb
Bacteria virus (lambda)
Bacteria
Up to 25 kb
Bacteria
BAC (bacterial artificial chromosome)
100-500 kb
YAC (yeast artificial chromosome)
Yeast
250-1000 kb
30-45 kb
Bacteria
Cosmid
10
Create a genomic library
  • 1. Isolate genomic DNA
  • Specific piece (directed)
  • All genomic (random)
  • 2. Shear DNA
  • 3. Clone into a vector
  • a. Ligate fragments into vector
  • b. Insert vector( insert) into host
  • c. Amplify vector (amplify host)
  • d. Isolate vector

11
Ligate sheared DNA into vector
Sheared DNA
Vector
  • Have cut ends
  • Cut so ends similar to sheared DNA

12
Ligation What do we need?
Vector
DNA fragment
DNA ligase
13
Create a genomic library
  • 1. Isolate genomic DNA
  • Specific piece (directed)
  • All genomic (random)
  • 2. Shear DNA
  • 3. Clone into a vector
  • a. Ligate fragments into vector
  • b. Insert vector( insert) into host
  • c. Amplify vector (amplify host)
  • d. Isolate vector

14
What host??
DEPENDS ON VECTOR AND HOST!!
15
Vector
Vector Host
Insert size
Plasmids
Bacteria
Up to 15 kb
Bacteria virus (lambda)
Bacteria
Up to 25 kb
Bacteria
BAC (bacterial artificial chromosome)
100-500 kb
YAC (yeast artificial chromosome)
Yeast
250-1000 kb
30-45 kb
Bacteria
Cosmid
16
What host??
DEPENDS ON VECTOR AND HOST!!
VECTOR PLASMID HOST BACTERIA (E. coli)
17
Transformation
E. coli
E. coli

E. coli
E. coli
Competent!
E. coli
E. coli
18
How do we know which E. coli cell has a vector?
19
Vector Needs a marker
Ampicillin resistance gene
E. coli
E. coli
20
How do we know the vector has an insert?
21
lacZ gene Beta-galactosidase
Plasmid
Cut plasmid for ligation in lacZ region
Ligate genomic DNA
No Beta-galactosidase produced!
Amplify in X-gal and IPTG
Select white colonies
22
What would a blue colony indicate?
Why are we growing in ampicillin?
23
Create a genomic library
  • 1. Isolate genomic DNA
  • Specific piece (directed)
  • All genomic (random)
  • 2. Shear DNA
  • 3. Clone into a vector
  • a. Ligate fragments into vector
  • b. Insert vector( insert) into host
  • c. Amplify vector (amplify host)
  • d. Isolate vector

24
Amplify host
How do we grow up E. coli?
Anything important about the media?
25
Create a genomic library
  • 1. Isolate genomic DNA
  • Specific piece (directed)
  • All genomic (random)
  • 2. Shear DNA
  • 3. Clone into a vector
  • a. Ligate fragments into vector
  • b. Insert vector( insert) into host
  • c. Amplify vector (amplify host)
  • d. Isolate vector

26
Isolate vector
  • Separate plasmid from E. coli
  • Separate from cell, proteins, carbs, etc..
  • Separate from E. coli genomic DNA!

Genomic DNA (insert)
Ampicillin resistance gene
27
Create a genomic library
  • 1. Isolate genomic DNA
  • Specific piece (directed)
  • All genomic (random)
  • 2. Shear DNA
  • 3. Clone into a vector
  • a. Ligate fragments into vector
  • b. Insert vector( insert) into host
  • c. Amplify vector (amplify host)
  • d. Isolate vector

28
Sequencing the M. tuberculosis genome
  • Create a genomic library
  • Sequence the genomic library
  • Alignment of these sequences (what sequence goes
    where?)
  • Identification of GENES

29
How do we sequence?
30
How do we sequence?
  • Amplify the piece we want to sequence
  • Identify the nucleotide order

What do we need??
Genomic DNA (insert)
Ampicillin resistance gene
31
Sequencing ingredients
Ingredient
Function
Isolated Vector insert
Amplification and sequencing template
Need a way to differentiate between nucleotides
32
Alter nucleotides
  • Add some that cause termination of amplification
  • No 3 hydroxyl end
  • Also labelled!
  • Radioactive
  • Fluorscence

A
G
T
C
A
T
C
G
C
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