Download Cloning, Sequencing and expression in Escherichia coli of

Survey
yes no Was this document useful for you?
   Thank you for your participation!

* Your assessment is very important for improving the workof artificial intelligence, which forms the content of this project

page
1
page
2
page
3
page
4
page
5
page
6
page
7
page
8
page
9
page
10
page
11
page
12
page
13
page
14
page
15
page
16
page
17
Document related concepts

Epigenetics of neurodegenerative diseases wikipedia , lookup

Gene desert wikipedia , lookup

Genome evolution wikipedia , lookup

Molecular cloning wikipedia , lookup

Expanded genetic code wikipedia , lookup

History of genetic engineering wikipedia , lookup

Gene wikipedia , lookup

Genetic engineering wikipedia , lookup

Metagenomics wikipedia , lookup

Gene therapy wikipedia , lookup

Neuronal ceroid lipofuscinosis wikipedia , lookup

Epigenetics of diabetes Type 2 wikipedia , lookup

Nutriepigenomics wikipedia , lookup

Microevolution wikipedia , lookup

Gene expression programming wikipedia , lookup

RNA-Seq wikipedia , lookup

Genomic library wikipedia , lookup

Gene expression profiling wikipedia , lookup

Polycomb Group Proteins and Cancer wikipedia , lookup

Vectors in gene therapy wikipedia , lookup

Cloning wikipedia , lookup

Gene nomenclature wikipedia , lookup

Genome editing wikipedia , lookup

Gene therapy of the human retina wikipedia , lookup

Site-specific recombinase technology wikipedia , lookup

Point mutation wikipedia , lookup

Genomics wikipedia , lookup

Designer baby wikipedia , lookup

Helitron (biology) wikipedia , lookup

NEDD9 wikipedia , lookup

Protein moonlighting wikipedia , lookup

Therapeutic gene modulation wikipedia , lookup

No-SCAR (Scarless Cas9 Assisted Recombineering) Genome Editing wikipedia , lookup

Artificial gene synthesis wikipedia , lookup

Transcript 
Cloning, Sequencing and
expression in Escherichia coli
of the Rubredoxin gene from
Clostridium pasteurianum
Mathieu, I., Meyer, J., and Moulis, J. (1992)
J. Biochem. 285, (255-262)
Background: Structure
•
•
•
•
Non-heme proteins
Composed of 45 to
54 amino acid
residues
Majority occur in
anaerobic bacterium
Molecular weight
ranging from 5000
and 6000 Daltons
Background: Structure
Ribbon structure of Rubredoxin from Clostridium pasteurianum showing
iron (orange core), and four Cystiene residues.
Background: Function
•Presumed to serve as electron carriers
•Electron-transfer chain in which they
participate has only been identified in P.
oleovorans
Purpose
Why study Rubredoxin:
•
•
ETC is important to
cellular function
Structure is known, but
not function
Goals:
•
•
Develop a method for
over-expression of
Rubredoxin
Use resultant protein
to study role in ETC
Cloning Step 1
•
•
•
Derived probes (p1) and (p2) for Rub
Digested Cpa genome with RE
Southern blotted using p1 and p2
Cloning Step 2
•
Determined that Rub
DNA appears at 3.9
kb by using gel
electrophoresis
Cloning Step 3
•
•
Digested Cpa with
RE to isolate Rub
sequence
Sequence inserted
into HindIII-BamHI
pUC18
Cloning Step 4
•
pUC18 transformed into E.coli DH5alpha cells
•
Plated on amp plates
•
•
Retested colonies by SB to ensure Rub gene
transformed
Rub gene was in fact transformed; One clone
produced pCPRD1
Sequencing
•
•
•
•
•
•
•
pCPRD1 sequenced
BgLII-SspI no remarkable
features
ORF1: compared to known
reductases
ORF2: gene product has no
function
ORF3: compared to Cpa
reductases
ORF4: Rubredoxin gene
Specific site of Rub gene
found
Sequenced fragment taken from
Cpa
Over-Expression
•
•
•
Plasmid pCPRD 1
was moved to JM109
E.coli cells
Added IPTG to
increase expression
Did not work
Over-Expression
•
•
•
Made a second clone,
pCPRD2, using specific
sites identified on
pCPRD1
Plasmid pCPRD2 was
moved to JM109 E.coli
cells
Added IPTG
•
•
Used UV spectroscopy to
identify time at which
IPTG was most effective:
• After 1hr detectable
expression
• After 4hr leveled off
• Stable for at least 24
hrs
At optimum time, proteins
were harvested
Discussion
•
•
•
•
•
Determined that Rubredoxin is generated in one piece
Rub function in Cpa still unknown
Found no direction connection between ORF1/ORF3
and Rub
Even though E.coli does not contain naturally
occurring Rub, it is efficient in expressing foreign
proteins that have elaborate iron-sulfur clusters
Method using Cpa in E.coli and IPTG produces
substantially more protein than Cpa
Discussion
•
Amino acid sequence of cloned Rub gene compared to known
sequences of Rub and found to have conserved residues.
Discussion
•
Compared UV spec
of Rub protein
(naturally occurring)
to Rub protein (in
E.coli) and found
them to be the same.
Questions?
What is ETC?
Related documents
application methods
application methods
Hand Hygiene - Western Health
Hand Hygiene - Western Health
What Is Gene cloning and How Is It Used? 1. Explain what is meant
What Is Gene cloning and How Is It Used? 1. Explain what is meant
fcs102607
fcs102607
Ch 20 Reading Guide - Dublin City Schools
Ch 20 Reading Guide - Dublin City Schools
Cloning and Gene Therapy
Cloning and Gene Therapy
Fig 5. Comparison of the genes specifically up- or
Fig 5. Comparison of the genes specifically up- or
AP Biology: Gene Regulation and Biotechnology
AP Biology: Gene Regulation and Biotechnology
Emerging Technologies
Emerging Technologies
Three Things You Can Do to Prevent Infection
Three Things You Can Do to Prevent Infection
“Who Wants To Be A Millionaire?” Inertia Style Created by Claire
“Who Wants To Be A Millionaire?” Inertia Style Created by Claire
Slide 1
Slide 1
Human Genome Project, Gene Therapy, and Cloning
Human Genome Project, Gene Therapy, and Cloning
Human Genome Project, Gene Therapy, and Cloning
Human Genome Project, Gene Therapy, and Cloning
Document
Document
Chapter 13.4
Chapter 13.4
Cloning DNA into Plasmid Vectors and Sequencing.
Cloning DNA into Plasmid Vectors and Sequencing.
E2A and pre-B cell acute lymphoblastic leukemias (ALL)
E2A and pre-B cell acute lymphoblastic leukemias (ALL)
Document 8315648
Document 8315648
Eukaryotically Encoded and Chloroplast
Eukaryotically Encoded and Chloroplast