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Title: Welcome to MB Class


1
Welcome to MB Class
2
Molecular Biology of the Gene, 5/E --- Watson et
al. (2004)
Part I Chemistry and Genetics Part II
Maintenance of the Genome Part III Expression
of the Genome Part IV Regulation Part V Methods
3
Part V METHODS
  • Ch 20 Techniques of
  • Molecular Biology
  • Ch 21 Model Organisms

4
  • Molecular Biology Course
  • Chapter 20
  • Techniques of
  • Molecular Biology

Preparation, analysis and manipulation of nucleic
acids and proteins
5
  • The methods depend upon, and were developed from,
    an understanding of the properties of biological
    macromolecules themselves.
  • Hybridization---the base-pairing characteristics
    of DNA and RNA
  • DNA cloning--- DNA polymerase, restriction
    endonucleases and DNA ligase
  • PCR---Thermophilic DNA polymerase

6
CHAPTER20 Techniques of Molecular Biology
  • Topic 1 Nucleic acids
  1. Separation by Electrophoresis (????)
  2. Cut by Restriction endonuclease (????????)
  3. Identification by Hybridization (????)
  4. Amplification by PCR (PCR??)
  5. DNA Cloning and gene expression (DNA???????)
  6. Genome sequence analysis (????????)

7
1. Gel electrophoresis separates DNA and RNA
molecules according to size, shape and
topological properties.
Topic 1 Nucleic acids-separation
8
DNA gel mobility (DNA???????)
  • 1.DNA and RNA molecules are negatively charged,
    thus move in the gel matrix (????) toward the
    positive pole (???).
  • 2.Linear DNA molecules are separated according to
    sizes. The large DNA molecules move slower than
    the small molecules.
  • 3.The mobility of circular DNA molecules is
    affected by their topological structures. The
    mobility of the same molecular weight DNA
    molecule with different shapes is
  • supercoiled (???)gt linear (??) gt nicked or
    relaxed (?????)

9
moderate
large
small
Fig 21-1 DNA is separated by gel electrophoresis
10
Gel matrix (????)
Gel matrix (????) is an inserted, jello-like
porous material that supports and allows
macromolecules to move through.
11
  • Agarose (???)
  • a much less resolving power than polyacrylamide,
  • but can separate DNA molecules of up to tens of kb

DNA can be visualized by staining the gel with
fluorescent dyes, such as ethidium bromide (EB
????)
12
  • Polyacrylamide (?????)
  • has high resolving capability, and can resolve
    DNA that differ from each other as little as a
    single base pair/nucleotide.
  • but can only separate DNA over a narrow size
    range (1 to a few hundred bp).

13
Pulsed-field gel electrophoresis (????)
  1. The electric field is applied in pulses that are
    oriented orthogonally (???) to each other.
  2. Separate DNA molecules according to their
    molecule weight, as well as to their shape and
    topological properties.
  3. Can effectively separate DNA molecules over 30-50
    kb and up to several Mb in length.

14
Fig. 21-2 pulsed-field gel electrophoresis
Switching between two orientations the larger
the DNA is, the longer it takes to reorient
15
Electrophoresis is also used to separate RNAs
  1. RNA have a uniform negative charge as DNA does.
  2. RNA is single-stranded and have extensive
    secondary and tertiary structure, which
    significantly influences their electrophoretic
    mobility.
  3. RNA can be treated with reagent such as glyoxal
    (???) to prevent RNA base pairing, so that its
    mobility correlates with the molecular weight

16
2. Restriction endonucleases (??????) cleave DNA
molecules at particular sites
Nucleic acids-Restriction digestion
  • Why use endonucleases?
  • --To break large DNA molecules into manageable
    fragments.

17
  • Restriction endonucleases (RE) are the nucleases
    that cleave DNA at particular sites by the
    recognition of specific sequences.
  • RE used in molecular biology typically recognize
    (??) short (4-8bp) target sequences that are
    usually palindromic (????), and cut (??) at a
    defined sequence within those sequences.
  • e.g. EcoRI

18
How to name a restriction endonuclease?
EcoRI
the 1st such enzyme found
Escherichia coli Species category
R13 strain
19
How to estimate the frequency of the RE in a DNA
molecule or genome?
  • The random occurrence of the hexameric (?????)
    sequence
  • 1/4096 (4-61/46)
  • What are the frequencies if the recognition
    sequences are four (tetrameric) and eight
    (octameric) nucleotides? homework

20
(1) Restriction enzymes differ in the recognition
specificity target sites are different.(2)
Restriction enzymes differ in the length they
recognized, and thus the frequencies differ.(3)
Restriction enzymes differ in the nature of the
DNA ends they generate blunt/flush ends (???),
sticky/staggered ends (????).(4) Restriction
enzymes differ in the cleavage activity.
21
Table 21-1 Some restriction Endonucleases and their recognition sequences Table 21-1 Some restriction Endonucleases and their recognition sequences Table 21-1 Some restriction Endonucleases and their recognition sequences
Enzyme Sequence Frequency
Sau3A1 EcoRI NotI 5-GATC-3 5-GAATTC-3 5-GCGGCCGC-3 0.25 kb 4 kb 65 kb
22
Fig 21-4 Recognition sequences and cut sites of
various endonucleases
blunt ends (???)
sticky ends (????)
23
Fig 21-5 Cleavage of an EcoRI site. The 5
protruding ends are said to be sticky because
they readily anneal through base-pairing to DNA
molecules cut with the same enzyme
24
3-1. DNA hybridization can be used to identify
specific DNA molecules
Topic 1 Nucleic acids- DNA hybridization
  • Hybridization the process of base-pairing
    between complementary ssDNA or RNA from two
    different sources.

25
Probe (??)
  • A labeled, defined sequence used to search
    mixtures of nucleic acids for molecules
    containing a complementary sequence.

The mixture being probed has typically either
been separated by size on a gel, or is
distributed as a library in different colonies
26
A probe must be labeled before applied in
hybridization (Why?)
  • It can be readily located once it has found its
    target sequence.

27
Labeling (??) of DNA or RNA probes
Radioactive labeling display and/or magnify the
signals by radioactivity. Non-radioactive
labeling display and/or magnify the signals by
antigen labeling antibody binding enzyme
binding - substrate application (signal release)
End labeling put the labels at the ends Uniform
labeling put the labels internally
28
End labeling
5-end labeling using polynucleotide kinase
(PNK) 3-end labeling using terminal transferase
29
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30
How to label one end of a DNA Labeling at both
ends by kinase, then remove one end by
restriction digestion.
---------------------G ---------------------CTTAAp
5
5pAATTC G
31
Uniformly labeling of DNA/RNA
Nick translation labeling of DNA DNase I to
introduce random nicks into template DNA ? DNA
pol I to remove dNMPs from 3 to 5 and add new
dNMP including labeled nucleotide at the 3 ends.
Hexanucleotide primered labeling of DNA Denature
DNA ? add random hexanucleotide primers and DNA
pol ? synthesis of new strand incorporating
labeled nucleotide.
32
Strand-specific RNA probes labeled by in
vitro transcription of the desired RNA sequence.
33
3-2 Hybridization probes can identify
electrophoretically-separated DNAs and RNAs
Topic 1 Nucleic acids- DNA hybridization
  • Hybridization the process of base-pairing
    between complementary ssDNA or RNA from two
    different sources.

34
Northern/Southern blot analysis
Electrophoresis
blotting
gel
membrane
Hybridization
Fig 21-6
35
Southern and Northern blotting
DNA on blot
RNA on blot
  • Genomic DNA preparation RNA
    preparation
  • Restriction digestion -
  • Denature with alkali -
  • Agarose gel electrophoresis ?
  • DNA blotting/transfer and fixation
    RNA
  • 6. Probe labeling ?
  • 6. Hybridization (temperature) ?
  • 7. Signal detection (X-ray film or antibody)
    ?

36
Comparison of Southern, Northern and Western bolt
hybridization
Blot type Target Probe Applications
Southern DNA DNA or RNA mapping genomic clonesestimating gene numbers, etc
Northern RNA DNA or RNA RNA sizes and abundance (gene expression level)
Western Protein Antibodies protein size and abundance (gene expression level)
37
4. Polymerase chain reaction (PCR) amplifies DNAs
by repeated rounds of DNA replication in vitro
Topic 1 Nucleic acids- amplification
  • PCR is to used to amplify a DNA sequence using a
    pair of primers each complementary to one end of
    the DNA target sequence.

38
The PCR cycle Three different steps proceed in
each PCR cycle.
  • Denaturation (??) The target DNA (template) is
    separated into two stands by heating to 95?
  • Primer annealing (??) The temperature is reduced
    to around 55? to allow the primers to anneal.
  • Polymerization (elongation, extension) (??) The
    temperature is increased to 72? for optimal
    polymerization step which uses up dNTPs and
    required Mg.

39
Denaturation
Primer annealing
Polymerization
Fig 21-11
40
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41
The PCR amplification
Many cycles (25-35 in common) are performed to
complete one PCR reaction, which resulted in an
exponential amplification of the target DNA if
both forward and reverse primers pair.
42
DNA template
Any source of DNA that provides one or more
target molecules can in principle be used as a
template for PCR. Whatever the source of
template DNA, PCR can only be applied if some
sequence information is known so that primers can
be designed.
43
PCR Primers
  1. Anneal on opposite strands of the target
    sequence.
  2. About 18 to 30 nt long and have similar GC
    contents so that they anneal to their
    complementary sequences at similar temperatures.
  3. Tm2(at)4(gc) determine annealing
    temperature. If the primer is 18-30 nt, annealing
    temperature can be Tm ? 5oC

44
5-ATTCCGATCGCTAATCGATGGC------- TCCTGTGCA
TTTCGCCACTAGAG-3 3-TAAGGCTAGCGATTAGCTACCG-------
AGGACACGTAAAGCGGTGATCTC-5
DNA sequence is written from 5 to the 3 end if
not stated. And only the sense strand is usually
given instead of both strands.
45
Degenerate primers (????) an oligo pool
derived from a protein sequence. E.g.
His-Phe-Pro-Phe-Met-Lys can generate a primer
5-CAY TTY CCN TTY ATG AAR Y Pyrimidine N any
base R purine
46
Enzymes and PCR Optimization
  • The most common is Taq polymerase. It has no 3
    to 5 proofreading exonuclease activity. Accuracy
    is low, not good for cloning. High-accuracy DNA
    polymerase is available commercially.
  • To optimize PCR, the annealing temperature and
    the Mg concentration are varied, or the nested
    PCR is carried out.

47
Nested PCR to increase specificity
First round primers
Gene of interest
Second round PCR
First round PCR
Second round primers
48
Reverse transcriptase (RT)-PCR
5-Cap
mRNA
AAA(A)n
(dT)1218 primer
anneal
5-Cap
3
5
AAA(A)n
Reverse transcription
dNTP, RT
5-Cap
5
Regular PCR
AAA(A)n
cDNAmRNA hybrid
49
PCR mutagenesis (??)
PCR can be used to introduce deletion and point
mutations
  1. Two separate PCR reactions are performed.
  2. One PCR amplifying the 5-portion of the insert,
    and the other amplifying the 3-portion of the
    insert.
  3. The point mutation/deletion mutations are located
    in the primers

50
Forward mutagenic primer
SP6 primer
T7 primer
Reverse mutagenic primer
First PCR
Remove primers Denature and anneal
3
3
Extend to full length by DNA polymerase
51
Second PCR
SP6 primer
T7 primer
DNA cloning
52
5. DNA cloning, analysis and gene expression
Nucleic acids- sequencing
The ability to construct recombinant DNA
molecules and maintain them in cells is called
DNA cloning.
53
  • Processes (??) of DNA cloning
  • Form the recombinant DNA molecules (??DNA) by
    inserting your interested DNA fragments into a
    proper vector (??). (Require restriction enzymes
    and ligase)
  • Transform (??) the recombinant DNA molecules into
    competent cells (?????).
  • Propagation of the cells containing the
    recombinant DNA to form a clone (??), a set of
    identical cells containing the same recombinant
    DNA.
  • Select the desired clones using the selective
    marker.

54
  1. Restriction digestion of your insert and vector
    using the same enzyme.
  2. Use ligase to join your insert and vector
    together.
  3. Transform the ligation products into E. coli.
    competent cells.
  4. Grow the cells on a plate containing tetracycline
    (???).

Fig 21-7 construction of a DNA library
55
  • Host organisms/cells where the plasmids get
    multiplied and propagated faithfully, which is
    crucial for DNA cloning.
  • ---Prokaryotic host E. coli ( most cases)
  • ---Eukaryotic host Yeast Saccharomyces
    cerevisiae (large fragments of human genome)

56
  • General features of a Vector
  • They contain an origin of replication and can
    autonomously replicating DNA independent of
    hosts genome.
  • Easily to be isolated from the host cell. Most
    are circular, some are linear (e.g. YAC vector).
  • Contains at least one selective marker, which
    allows host cells containing the vector to be
    selected amongst those which do not.
  • Contains a multiple cloning site (MCS) to be cut
    by restriction enzymes for DNA manipulation.

57
Cloning vectors (????) allowing the exogenous
DNA to be inserted, stored, and manipulated at
DNA level. E. coli cloning vector (circular)
plasmids (??) bacteriophages (l and M13)
(???) plasmid-bacteriophage l hybrids (cosmids)
(????-?????????). Yeast cloning vector yeast
artificial chromosomes (YACs,???????) (Linear)
58
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59
  • Plasmids small, extrachromosomal circular
    molecules, from 2 to 200 kb in size, which exist
    in multiple copies within the host cells.
  • Contain an origin of replication, at least one
    selective marker and multiple cloning site.
  • Example of selective marker ampr gene encoding
    the enzyme b-lactamse which degrades penicillin
    antibiotics such as ampicillin.
  • The commonly used plasmid are small in size ( 3
    kb)

60
Libraries of DNA molecules can be created by
cloning (Genomic library and cDNA library) A DNA
library (DNA??) is a population of identical
vectors that each contains a different DNA
insert. (Fig. 20-8) Genomic Library (?????) the
DNA inserts in a DNA library is derived from
restriction digestion or physical shearing of the
genomic DNA. cDNA library (cDNA??) the DNA
inserts in a DNA library is converted from the
mRNAs of a tissue, a cell type or an organism.
cDNA stands for the DNA copied from mRNA. (Fig.
20-19)
61
Different Insert fragments
Fig 21-8 construction of a DNA library
62
  • cDNA library generation
  • The mRNAs are firstly reverse transcript into
    cDNA, and these cDNA, both full length and
    partial, are cloned to make the cDNA library.

63
Fig 20-9 Construction of cDNA library
anneal
Reverse transcription
Regular PCR
64
Screening of positive clones
Colony screening
  1. Antibiotic screening (?????) only the
    recombinant plasmids grow on the
    antibiotic-containing plate.
  2. Blue-white screening (?????) DNA insertion in
    the vector shuts down the LacZ gene expression,
    and turns the colony to white.
  3. Colony hybridization screening (??????) from a
    library.

65
Antibiotic screening (?????) only intact
plasmids grow on the antibiotic-containing plate.
66
Recombinant DNA molecules
X if the vector is in the
phosphorylated state
67
Dephosphorylate the vector using alkaline
phosphate can prevent religation of vector
molecules
68
Blue white screening ---Allow the discrimination
of recombinant plasmid from the religated ones
Lac promoter
Ampr
MCS (Multiple cloning sites, ?????)
pUC18 (3 kb)
lacZ
Insertion of a DNA fragment interrupts the ORF of
lacZ gene, resulting in non-functional gene
product that can not digest its substrate x-gal.
ori
69
lacZ encode enzyme b-galactosidase
(substrate of the enzyme)
lac promoter?
X-gal
IPTG
Blue product
During the experiment, IPTG is added to the
selective growth medium. Insertion of the target
DNA fragment into the MCS will prevent the
formation of the blue colony, and white colony is
formed instead.
70
Recreated vector blue transformants Recombinant
plasmid containing inserted DNA white
transformants
Recreated vector (no insert)
Recombinant plasmid (contain insert)
71
Colony hybridization-Southern blot
Transfer to nitrocellulose or nylon membrane
Select positive from master plate
Keep master plate
Denature DNA(NaOH) Bake onto membrane
Probe with 32p-labled DNA complementary to
gene of interest
Expose to film
Screening by plaque hybridization
72
Analysis of DNA clones
Analysis of a clone
  1. Restriction mapping digestion of the plasmid
    prepared from a clone with restriction enzymes to
    investigate if the interested DNA is inserted the
    recombinant plasmid.
  2. Sequencing the cloned DNA to see if the inserted
    DNA maintains the correct sequence.

73
2 Positive clones digested with different
restriction enzymes
Empty vector
1 Kb ladder
Restriction mapping
74
Sequencing
75
Gene expression
Expression of a gene from a transformed/transfecte
d plasmid
  1. Transformation (??) introduction of plasmids
    into bacteria.
  2. Transfection (??) introduction of plasmids and
    other exogenous nucleic acids into eukaryotes
    such as mammalian cells.

76
Expression vectors allowing the exogenous DNA
to be stored and expressed in an organism. --E.
coli expression vector --Yeast expression
vector --Mammalian expression vector Features In
addition to the origin of replication, selective
marker, multiple cloning site, expression vector
has to contain a promoter and terminator for
transcription. The inserted gene has to have a
start codon and a stop codon for translation
77
T7 promoter
RBS
Start codon
MCS
Ampr
Transcription terminator
T7 expression vector
E. coli expression vector
ori
78
H4 Eukaryotic Vectors
MCS
Insert Figure 1
Yeast expression vector
79
Fusion proteins
Gene cloning and expression provides a very
powerful way to obtain a large amount of the
target protein fused with an enzyme, fluorescence
protein or a tag for identification (??) or
purification (??).
80
Examples
Lac fusions (Enzyme) fuse your target gene
with the LacZ coding sequence. His-tag fusions
(Tag) A sequence encodes His-tag was inserted
at the N- or C- termini of the target ORF,
allowing the fusion protein to be purified by
binding to Ni2 column. GFP fusions
(Fluorescence protein) insert your targeted gene
at the N- or C- termini of GFP (green
fluorescence protein, ??????), and your fusion
protein will give you green fluorescence signal.
81
6. Sequencing
Nucleic acids- sequencing
  • Two ways for sequencing
  • 1. DNA molecules (radioactively labeled at 5
    termini) are subjected to 4 regiments to be
    broken preferentially at Gs, Cs, Ts, As,
    separately. (Maxam and Gilbert chemical method,
    not widely used)
  • 2. Chain-termination method (Sangers method,
    widely used)

82
Sangers enzymic method
Maxam and Gilbert
83
Chain-termination method (????)
  • ddNTPs are chain-terminating nucleotides the
    synthesis of a DNA strand stops when a ddNTP is
    added to the 3 end

84
The absence of 3-hydroxyl lead to the
inefficiency of the nucleophilic attack on the
next incoming substrate molecule.
85
Tell from the gel the position of each G
If one ddGTP is added to 100 dGTP, DNA synthesis
aborts at a frequency of 1/100 every time the
polymerase meets a ddGTP
86
Fig 20-15 DNA sequencing gel
Four separate reactions dNTP ddGTP, dNTP
ddATP dNTP ddCTP, dNTP ddTTP Each ddNTP
carries a fluorescence group, allowing us to
Read the sequence directly from the gel.
87
Automatic sequencer
  • Fluorescence
  • Labeled ddNTP
  • 2. Polymerase catalyzed

88
Shotgun sequencing of a bacterial genome
(??????????)
  • The bacterial genome was randomly sheared into
    many random fragments with an average size of 1
    kb, and cloned intro a vector. (Prepare what you
    are going to shot)
  • Individual recombinant DNA clones are randomly
    picked to prepare DNA for sequencing on an
    automated sequencer. (shot)
  • This is called shotgun sequencing.

89
In use of shotgun sequencing strategy, multiple
sequence coverage is required to obtain all
genome sequence. For example The genome of
bacteria Hemophilus influenzae is 1.8 Mb, each
sequence read produces 600 bp of sequence. If
33,000 different clones were picked for
sequencing, a total of 600 bp x 33,000 20 Mb
sequence was produced.
Critical thinking how to design a pair of
primers to sequence the inserts of all the
recombinant plasmids in a genomic library?
90
The shotgun strategy permits a partial assembly
of large genome sequence
  • The core techniques for sequencing the large
    genomes, e.g. human, are
  • automated shotgun sequencing (obtain sequence)
  • then the subsequent use of computer to assemble
    the different sequences (analyze sequence, which
    is the rate-limiting step).

91
Flow chart of Human genome sequencing project
2. Shotgun sequencing
1. Recombinant Plasmid Library
3. Sequence Assembly
Fig 20-16
92
  • Assembly Step 1 form contigs
  • (A single contig is about 50,000 to 200,000 bp. )
  • Sophisticated computer programs have been
    developed that assemble the short sequences from
    random shotgun DNAs into larger contiguous
    sequences called contigs.

93
Assembly Step 2 The paired-end strategy permits
the assembly of larger scaffolds (1-2 Mb)
94
  • Fig 20-17. Contigs are linked by sequencing the
    ends of large DNA fragments (plasmid library
    containing larger DNA fragments).

95
Assembly flowchart
  1. Assemble the contigs from 1kb plasmid shotgun
    sequence. (50 kb-200 kb)
  2. Assemble the contigs to large scaffold by
    sequencing both ends of 5 kb plasmids. (lt500 kb)
  3. Assemble the larger scaffolds (gt1 Mb) by
    sequencing the end of the BAC library.

96
Genome-wide analysis
  • The purpose of this analysis is to predict the
    protein coding genes (???????) and other
    functional sequences (??????) in the genome.

97
  • For the genomes of bacteria and simple
    eukaryotes
  • Finding protein coding genes Identification of
    ORF (open-reading frames).
  • straightforward
  • fairly effective
  • but not all ORFreal protein coding genes
  • key challenge is in identifying the functions of
    these genes.

98
  • For animal genomes with complex exon-intron
    structures, the challenge is far greater
  • A variety of bioinformatics tools are required to
    identify genes and genetic composition of complex
    genomes.
  • The computer programs identifying potential
    protein coding genes are based on many sequence
    criteria including the occurrence of extended
    ORFs that are flanked by appropriate 5 and 3
    splice sites.

99
  • Limitations of the computer methods
  • one-fourths of genes cannot be identified by
    this way.
  • The failure to identify promoters because the
    core promoter elements are highly degenerate
    (???). Although the transcription complex is
    smart enough to identify these elements in cell,
    we are not yet smart enough to write programs to
    identify them in silico (??,??).
  • The most important method for validating
    predicted protein coding genes and identifying
    those missed by current gene finder program is
    the use of cDNA sequence data.

100
  • cDNA library sequencing and application
  • Sequence the cDNAs prepared from a cDNA library
    using shotgun method to generate EST (expressed
    sequence tag) database.
  • These ESTs are aligned onto genomic scaffolds to
    help us identify genes and to assemble larger
    scaffolds.

101
Fig 20-18 Gene finder method analysis of
protein-coding regions in Ciona intestinalis (?? )
A 20-kb genome sequence (scaffold)
Predicted by a gene finder program
102
  • The mostly commonly used genome tool BLAST
  • Finding regions of similarity between different
    protein coding genes.
  • Input a query sequence (????) a stretch of amino
    acids or the DNA sequence encoding your
    interested protein function.
  • Ask the computer to search for the homologous
    sequences in a protein or DNA database, and you
    will get all the available genes that may have
    the similar protein function.

103
Figure 20-21 Example of the BLAST search result
104
CHAPTER20 Techniques of Molecular Biology
  • Topic 2 Proteins
  1. Protein purification (?????)
  2. Affinity chromatography can facilitate more rapid
    protein purification (??????)
  3. Protein separation by PAGE gel electrophoresis
    (?????) and identification by Western analysis
  4. Protein sequencing (?????)
  5. Proteomics (?????)

105
1. Protein purification (?????)
  • The purification of individual proteins is
    critical to understanding their function.
  • Although there are thousands of proteins in a
    single cell, each protein has unique properties,
    such as size, charge (??), shape, and in many
    instance, function, that make its purification
    somewhat different from others.

106
  • Purification of a protein requires a specific
    assay to allow you to monitor your purification
    status, which include a measure of the function
    of the protein, use of the antibody of the
    protein.

107
Column chromatography is an efficient way to
purify proteins
  • In this approach, protein fractions are passed
    though glass columns filled with appropriated
    modified small acrylamide or agarose beads.

108
Ion exchange chromatography
  • The proteins are separated according to their
    surface charge.
  • The beads are modified with either
    negative-charged or positive-charged chemical
    groups.
  • Proteins bind more strongly requires more salt to
    be eluted.

109
Fig 20-22-a
110
Gel filtration chromatography
  • This technique separate the proteins on the bases
    of size and shape.
  • The beads for it have a variety of different
    sized pores throughout. Small proteins can enter
    all of the pores, and take longer to elute but
    large proteins pass quickly.

111
Fig 20-22-b
112
2. Affinity chromatography can facilitate more
rapid protein purification
  • If the target protein is known to establish a
    specific and high-affinity interaction with a
    specific protein/nucleic acids/small molecule, we
    can couple this specific partner of the target
    protein to the column and thus the target protein
    will be selectively bound to the column.
  • This method is called affinity chromatography.

113
  • Protein structure

Affinity chromatography
  • Enzyme-substrate binding
  • Receptor-ligand binding
  • Antibody-antigen binding
  • Ni2-His tag-fusion protein binding

114
Immunoaffinity chromatography(??????)
  • An antibody that is specific for the target is
    attached to the bead, and ideally only the target
    protein can bind to the column.
  • Disadvantage sometimes the binding is too tight
    to elute our target protein.

115
  • Sometimes tags (epitopes, ?????) can be added to
    the N- or C- terminal of the target protein,
    using DNA cloning method, to make the fusion
    protein.
  • This allows the modified fusion proteins to be
    purified using immunoaffinity purification and a
    heterologous antibody specific for the tag.
  • Importantly, the binding affinity can change
    according to the condition. e.g. the
    concentration of the Ca2 in the solution.

116
Immunoprecipitation (????)
  • Attach the antibody to the bead, which is then
    used to precipitate (??) a specific protein from
    a crude cell extract.
  • Its a useful method to detect what proteins or
    other molecules are associated with the target
    protein.

117
3. Protein separation by PAGE gel
electrophoresis, followed by a western analysis
  • The native proteins have neither a uniform charge
    nor a uniform secondary structure.
  • If we treat the protein with a strong detergent
    SDS, the higher structure is usually eliminated.
    And SDS confers the polypeptide chain a uniform
    negative charge.

118
  • Sometimes, mercaptoethanol (????) is need to
    break the disulphide bond.
  • Thus, the protein molecules can be resolved by
    electrophoresis in the presence of SDS according
    to the length of individual polypeptide.
  • After electrophoresis, the proteins can be
    visualized with a stain, such as Coomassie
    brilliant blue (?????).
  • Proteins from the PAGE gel can be transferred to
    a membrane, followed by a western analysis of the
    target protein by a corresponding antibody.

119
A protein gel stained by Coomassie Blue
Western analysis using two specific antibodies
--- P P P P
PTB
Beta-actin
120
4. Protein sequencing (?????)
  • Two sequence method
  • Edman degradation (Edman???)
  • Tandem mass spectrometry (MS/MS) (????).
  • Due to the vast resource of complete or nearly
    complete genome, the determination of even a
    small stretch of protein sequence is sufficient
    to identify the gene.

121
Edman degradation
  • A chemical reaction in which the amino acids
    residues are sequentially release for the
    N-terminus of a polypeptide chain.

122
  • Step 1 modify the N-terminal amino with PITC,
    which can only react with the free a-amino group.
  • Step 2 cleave off the N-terminal by acid
    treatment, but the rest of the polypeptide
    remains intact.
  • Step 3 identify the released amino acids by High
    Performance Liquid Chromatography (HPLC).
  • The whole process can be carried out in an
    automatic protein sequencer. ??

123
Fig 20-23
124
Tandem mass spectrometry
  • MS is a method in which the mass of very small
    samples of a material can be determined.

125
  • Step 1 digest your target protein into short
    peptides.
  • Step 2 subject the mixture of the peptide to MS,
    and each individual peptide will be separate.
  • Step 3 capture the individual peptide and
    fragmented into all the component peptide.
  • Step 4 determine the mass of each component
    peptide.
  • Step 5Deconvolution (??) of these data and the
    sequence will be revealed.

126
5. Proteomics (?????)
  • Proteomics is concerned with the identification
    of the full set of proteins produced by a cell or
    a tissue under a particular by a particular set
    of conditions.

127
Three principle methods
  • 1. 2-D gel electrophoresis for protein separation
    (?????).
  • 2. MS spectrometry for the precise determination
    of the molecular weight and identify of a protein
    (?????).
  • 3. Bioinformatics for assigning proteins and
    peptides to the predicted products of protein
    coding sequence in the genome (?????).

128
Fig 20-24
129
CHAPTER20 Techniques of Molecular Biology
  • Topic 3 Study the interaction between protein
    and nucleic acid
  1. Gel retardation assay
  2. Nuclease protection assay

130
Gel retardation (????)
  • A short labeled nucleic acid is mixed with a cell
    or nuclear extract expected to contain the
    binding protein. Then, samples of labeled nucleic
    acid, with and without being incubated with the
    extract, are run on a gel. The DNA-protein
    complexes are shown by the presence of slowly
    migrating bands.

131
A DNA bound with more than one protein to form a
larger complex.
DNA bound to two proteins
DNA-protein complex
Bare DNA
132
DNase I footprinting (DNase I ???)
  • Identify the actual region of sequence with
    which the protein interacts.

Sequence ladder is required to determine the
precise position
AATAAG

5
133
DNase footprinting (1)The protein protects DNA
from attack by DNase. (2)Treat the DNA-protein
complex with DNase I under mild conditions, so
that an average of only one cut occur per DNA
molecule.
Bind protein
DNase(mild),then remove protein and denature DNA
Electrophoresis, autoradiograph
134
The three lanes represent DNA that was bound to
0, 1, and 5 units of protein. The lane with no
protein shows a regular ladder of fragments. The
lane with one unit shows some protection, and
the lane with 5 units shows complete protection
in the middle.By including sequencing ladders,
we can tell exactly where the protein bound.
Protein
T C G G A G C A A C G C A A A C A A A C G T G C T
T G G
1
0
5
135
CHAPTER20 Techniques of Molecular Biology
  • Topic 4 Determining the Structure of
  • Protein and nucleic acids
  1. X-ray crystallography (X-????)
  2. NMR (????)

136
X-ray crystallography and NMR Determining the
tertiary structure
X-ray crystallography
  • Measuring the pattern of diffraction of a beam of
    X-rays as it pass through a crystal. The first
    hand data obtained is electron density map, the
    crystal structure is then deduced.
  • A very powerful tool in understanding protein
    tertiary structure
  • Many proteins have been crystallized and analyzed

137
The ribosome structure and its interaction with
mRNA and tRNA
138
NMR
  • Measuring the relaxation of protons after they
    have been excited by radio frequencies in a
    strong magnetic field.
  • Measure protein structure in liquid but not in
    crystal.
  • Protein measured are usually smaller than 30 KDa.

139
CHAPTER20 Techniques of Molecular Biology
Nucleic acids techniques Electrophoresis
Restriction digestion Hybridization (southern
northern) PCR amplification sequencing and
genome sequencing DNA cloning and gene
expression. Protein techniques Protein
purification affinity chromatography Protein
separation and identification by western blot
Protein sequencing Proteomics. Study the
interaction between protein and nucleic acid Gel
retardation Nuclease protection
assays Determining the Structure of protein and
nucleic acids X-ray crystallography, NMR
140
CHAPTER20 Techniques of Molecular Biology
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141
Welcome to join in our labs Thanks for your
incorporation for the whole class
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