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Guidelines to reach high-quality purified recombinant proteins
by
Domingues, Lucília
, Oliveira, Carla
in
Circular dichroism
/ Cloning
/ Conditioning
/ Dichroism
/ E coli
/ Gel electrophoresis
/ Guidelines
/ Light scattering
/ Protein purification
/ Proteins
/ Purification
/ Quality
/ Quality control
/ Size exclusion chromatography
/ Sodium lauryl sulfate
/ Structural analysis
2018
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Guidelines to reach high-quality purified recombinant proteins
by
Domingues, Lucília
, Oliveira, Carla
in
Circular dichroism
/ Cloning
/ Conditioning
/ Dichroism
/ E coli
/ Gel electrophoresis
/ Guidelines
/ Light scattering
/ Protein purification
/ Proteins
/ Purification
/ Quality
/ Quality control
/ Size exclusion chromatography
/ Sodium lauryl sulfate
/ Structural analysis
2018
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While trying to remove the title from your shelf something went wrong :( Kindly try again later!
Do you wish to request the book?
Guidelines to reach high-quality purified recombinant proteins
by
Domingues, Lucília
, Oliveira, Carla
in
Circular dichroism
/ Cloning
/ Conditioning
/ Dichroism
/ E coli
/ Gel electrophoresis
/ Guidelines
/ Light scattering
/ Protein purification
/ Proteins
/ Purification
/ Quality
/ Quality control
/ Size exclusion chromatography
/ Sodium lauryl sulfate
/ Structural analysis
2018
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Guidelines to reach high-quality purified recombinant proteins
Journal Article
Guidelines to reach high-quality purified recombinant proteins
2018
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Overview
The final goal in recombinant protein production is to obtain high-quality pure protein samples. Indeed, the successful downstream application of a recombinant protein depends on its quality. Besides production, which is conditioned by the host, the quality of a recombinant protein product relies mainly on the purification procedure. Thus, the purification strategy must be carefully designed from the molecular level. On the other hand, the quality control of a protein sample must be performed to ensure its purity, homogeneity and structural conformity, in order to validate the recombinant production and purification process. Therefore, this review aims at providing succinct information on the rational purification design of recombinant proteins produced in Escherichia coli, specifically the tagging purification, as well as on accessible tools for evaluating and optimizing protein quality. The classical techniques for structural protein characterization—denaturing protein gel electrophoresis (SDS-PAGE), size exclusion chromatography (SEC), dynamic light scattering (DLS) and circular dichroism (CD)—are revisited with focus on the protein and their main advantages and disadvantages. Furthermore, methods for determining protein concentration and protein storage are also presented. The guidelines compiled herein will aid preparing pure, soluble and homogeneous functional recombinant proteins from the very beginning of the molecular cloning design.
Publisher
Springer Nature B.V
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