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Structural Biology - Protein Expression and Engineering $9.76   Add to cart

Class notes

Structural Biology - Protein Expression and Engineering

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Lecture notes on the topic Protein Expression and Engineering, taught by Professor Bernadette Byrne at Imperial College London. Course: Bsc Biochemistry. Module: Structural Biology.

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  • February 1, 2023
  • 12
  • 2022/2023
  • Class notes
  • Byrne
  • Structural biology- protein expression and engineering
  • Unknown
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TITLE DATE
Protein Expression& Engineering

Genetic elements involved in expression of plasmid-coded protein:
controls access
to promotor
by
inducing change
in DNA
polymerase binds,
MNA shape
drives gene expression ends transcription


codon

siteribosomalbindingonstartof gene the of
end of gene
of interest




gene drives plasmid replication to synthesise
sufficient amounts of protein


PROMOTERS

e.g. LacZ promoter I operator
region



upstream Lac I
gene produce not accessible

synthesises Lac I protein


binds specifically to operator promoter region



:prevents polymerase
RNA
BINDING
from binding
a




used in bacteria binds, induces conformational
but not in labs so Lac I cannot bind to operator

Inot stable enough (

control and optimisation of expression
growth rate death rate,
=
no net ↑


Optimise by:
Optical 1.
Vary concentration of inducer
density 2. Vary temperature of growth
at600nm .
1180 vs 370C)
in
0D600-0.6 =


whencellsaremost

https://bynikkib.com

, TITLE DATE




induction -

adding 5th to the culture


Autoinduction
↳ relies on consumption of a carbon source in the media
I cell's metabolic pathway uses another method for energy production

cell C source used up, removes repression promoter
↳ as grows, on


:allows protein expression


Example:Regulation of
it polymerase expression in E. coli expression before
inducer added
1




-

expression of recombinant proteins can be toxic excess production, leaky expression)

↳ prevent by separating gene cloning from gene expression

Phage i7 promoter
>
does not bind native E.coli
T7 polymerase




plasmidw/ target gene,
controlled by PTI promoter

bacteria are specially engineered
to carry the phage it polymerase gene >bind DT7 -> add inducer
->
drives target gene expression

DNA
polymerases used for PCR
high relative processivity efficient
=




* Taq is efficient but lacks 3'-5'

proofreading ability, adds A
overhang
at3'end




rest
* makes less product (lower yield)
but more correct products
https://bynikkib.com

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