PBIO 427/527: Molecular Genetics Lecture 2 - Review Prokaryotic gene structure, processing &...

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PBIO 427/527: Molecular Genetics Lecture 2 - Review •Prokaryotic gene structure, processing & regulation •Eukaryotic gene structure, processing & regulation •Restriction enzymes & gel electrophoresis •DNA cloning & cloning vectors •Gene libraries & screening •cDNA libraries & screening

Transcript of PBIO 427/527: Molecular Genetics Lecture 2 - Review Prokaryotic gene structure, processing &...

Page 1: PBIO 427/527: Molecular Genetics Lecture 2 - Review Prokaryotic gene structure, processing & regulation Eukaryotic gene structure, processing & regulation.

PBIO 427/527: Molecular GeneticsLecture 2 - Review

•Prokaryotic gene structure, processing & regulation•Eukaryotic gene structure, processing & regulation

•Restriction enzymes & gel electrophoresis•DNA cloning & cloning vectors

•Gene libraries & screening•cDNA libraries & screening

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Prokaryotic gene expression

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Prokaryotic gene expression

Regulation lac Operon.mov

• Alternatively, see:• http://www.whfreema

n.com/lodish4e/con_index.htm?99anm

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In prokaryotes, RNA polymerase binds to the -10 and -35 regions of the promoter relative to

the start site of transcription (+1)

promoter operator

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Eukaryotic gene organization

enhancerssilencers

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Eukaryotic gene organization and RNA processing

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Basic Transcriptional Mechanism and mRNA Splicing Animations

• MCB Chapter 4-Basic Transcriptional Mechanism animation• http://bcs.whfreeman.com/lodish5e/pages/bcs-main.asp?v=category

&s=00010&n=04000&i=04010.01&o=|00510|00610|00520|00530|00540|00560|00570|00590|00600|00700|00710|00010|00020|00030|00040|00050|01000|02000|03000|04000|05000|06000|07000|08000|09000|10000|11000|12000|13000|14000|15000|16000|17000|18000|19000|20000|21000|22000|23000|99000|&ns=0

• MCB Chapter 12-mRNA splicing animation• http://bcs.whfreeman.com/lodish5e/pages/bcs-main.asp?

v=category&s=00010&n=12000&i=12010.02&o=|00510|00610|00520|00530|00540|00560|00570|00590|00600|00700|00710|00010|00020|00030|00040|00050|01000|02000|03000|04000|05000|06000|07000|08000|09000|10000|11000|12000|13000|14000|15000|16000|17000|18000|19000|20000|21000|22000|23000|99000|&ns=1211

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Eukaryotic gene expression

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MCB Chapter 4-Life Cycle of mRNA

• http://bcs.whfreeman.com/lodish5e/pages/bcs-main.asp?v=category&s=00010&n=04000&i=04010.02&o=|00510|00610|00520|00530|00540|00560|00570|00590|00600|00700|00710|00010|00020|00030|00040|00050|01000|02000|03000|04000|05000|06000|07000|08000|09000|10000|11000|&ns=0

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Recombinant DNA cloning procedure

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Recombinant DNA cloning procedure

• See MCB Chapter 9 – Plasmid Cloning• http://bcs.whfreeman.com/lodish5e/pages/bcs-main.asp?

v=category&s=00010&n=09000&i=09010.05&o=|00510|00610|00520|00530|00540|00560|00570|00590|00600|00700|00710|00010|00020|00030|00040|00050|01000|02000|03000|04000|05000|06000|07000|08000|09000|10000|11000|&ns=437

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Restriction enzymes & DNA methylation

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Recognition sequences of some REs

Enzyme Recognition site Type of cut end

EcoRI G ↓ A-A-T-T-C 5’ P extension

BamHI G ↓ G-A-T-C-C 5’ P extension

PstI C-T-G-C-A ↓ G 3’ P extension

Sau3A1 ↓ G-A-T-C 5’ P extension

PvuII C-A-G ↓ C-T-G Blunt end

HpaI G-T-T ↓ A-A-C Blunt end

HaeIII G-G ↓ C-C Blunt end

NotI G ↓ C-G-G-C-C-G-C

5’ P extension

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Mapping of restriction enzyme sites

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Vector system Host cell Insert capacity (kb)

Plasmid E. coli 0.1-10

Bacteriophage E. coli 10-20

Cosmid E. coli 35-45

Bacteriophage P1 E. coli 80-100

BAC (bacterial artificial chromosome)

E. coli 50-300

P1 bacteriophage-derived AC

E. coli 100-300

YAC Yeast 100-2,000

Human AC Cultured human cells

>2,000

Cloning vectors and their insert capacities

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Plasmid cloning vectors

Three important features1. Cloning site2. Ori-an origin of replication3. A selectable marker (ampr)

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pGEM-3Z

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Cloning foreign DNA into a plasmid vector

Alkaline phosphatase-removes 5’ phosphate (P) groups of DNA molecules; BAP is more stable but less active than CIP

T4 DNA ligase –joins 5’ phosphate (P) groups of DNA molecules to 3’ hydroxyl (OH) groups of DNA

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Some antibiotics commonly used as selective agents

Antibiotic Description

Ampicillin (Amp) Inhibits bacterial cell wall synthesis; inactivated by -lactamase, which cleaves the -lactam ring of amp

Hygromycin B (HygB)

Kanamycin (Kan) Binds to 30S ribosomal subunit and inhibits protein synthesis; inactivated by a phosphotransferase

Neomycin (Neo) Binds to 30S ribosomal subunit and inhibits protein synthesis; inactivated by a phosphotransferase

Streptomycin (Str)

Tetracycline (Tet) Binds to 30S ribosomal subunit and inhibits protein synthesis; tetr gene encodes a protein which prevents transport of tet into the cell

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Genomic library

construction

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Screening a genomic library using DNA hybridization to a

(radio-)labeled DNA probe

Note: a cDNA is commonly (radio-)labeled

and used as a DNA probe to screen a genomic library

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Production of a (radio-)labeled DNA probe by the random primer method [uses the Klenow fragment of DNA polymerase]

5’

5’5’

3’

3’3’

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The first step in making a cDNA library: Purification of

polyadenylated mRNA using oligo(dT)-

cellulose

Note: selection of the proper source (organ, tissue) of the RNA is

critical here!

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Complementary DNA or cDNA cloning:cDNA library construction

Note: ds cDNAs are typically placed in a cloning

vector such as bacteriophage lambda ()

or a plasmid

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There are several possible ways to screen a cDNA library

• Using a DNA probe with a homologous sequence (e.g., a homologous cDNA or gene clone from a related species)

• Using an oligonucleotide probe based on a known amino acid sequence (requires purification of the protein and some peptide sequencing)

• Using an antibody against the protein of interest (note: this requires use of an expression vector)

• Plus/minus or differential screening (the least specific way)

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Screening a cDNA library using DNA

hybridization to a (radio-)labeled

DNA probe

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Screening a cDNA library with a labeled oligonucleotide probe based on a known peptide sequence

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Using polynucleotide kinase and-32P-labeled ATP to radiolabel oligonucleotide probes

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Immunological screening of an expression cDNA library with a primary antibody and labeled secondary antibody;

note the label is often an enzyme label like alkaline

phosphatase or horseradish peroxidase, but it can also

be 125I

Note: see also MCB Chapter 9 for a related animation

http://bcs.whfreeman.com/lodish5e/pages/bcs-main.asp?

v=category&s=00010&n=09000&i=09010.04&o=|00510|00610|00520|00530|00540|00560|00570|00590|00600|00700|00710|00010|00020|00030|00040|00050|01000|02000|03000|04000|05000|06000|07000|08000|09000|10000|11000|12000|13000|14000|15000|16000|17000|18000|19000|

20000|21000|22000|23000|99000|&ns=589

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Animations for two related uses of expression vectors

• Expression cloning of receptor proteins-see MCB Chapter 9• http://bcs.whfreeman.com/lodish5e/pages/bcs-main.asp?

v=category&s=00010&n=09000&i=09010.04&o=|00510|00610|00520|00530|00540|00560|00570|00590|00600|00700|00710|00010|00020|00030|00040|00050|01000|02000|03000|04000|05000|06000|07000|08000|09000|10000|11000|12000|13000|14000|15000|16000|17000|18000|19000|20000|21000|22000|23000|99000|&ns=589

• Looking for protein-protein interactions with the yeast two hybrid system-see MCB Chapter 11

• http://bcs.whfreeman.com/lodish5e/pages/bcs-main.asp?s=00010&n=11000&i=11010.01&v=category&o=|00510|00610|00520|00530|00540|00560|00570|00590|00600|00700|00710|00010|00020|00030|00040|00050|01000|02000|03000|04000|05000|06000|07000|08000|09000|10000|11000|12000|13000|14000|15000|16000|17000|18000|19000|20000|21000|22000|23000|99000|&ns=798&t=&uid=0&rau=0

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Plus/min (+/-) or differential

screening

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A cosmid cloning system:

another possible cloning vector which can be

used for genomic library but not for cDNA

libraries

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In summary, you have seen:

• How to make and screen gene libraries

• How to make and screen cDNA libraries

• Several different cloning vectors including plasmids, bacteriophage lambda (), and cosmids