Team:UNIPV-Pavia/Project/motivation
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[[Image:pv_ExpressionVector.png|330px|thumb|center|Expression vector for the production of recombinant proteins]] | [[Image:pv_ExpressionVector.png|330px|thumb|center|Expression vector for the production of recombinant proteins]] | ||
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+ | ===ORIGIN OF REPLICATION AND RESISTANCE MARKER=== | ||
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In order to achieve high expression levels, heterologous proteins are often cloned in vectors replcating by the ColE1 or the p15A replicon, that replicate in a relaxed fashion and are present in the cells in medium/high copy number (from 15–20 to few hundreds copies). When co-overexpression of additional gene products is desired, derivatives of ColE1 and p15A replicons are often combined. These multiple-copy plasmids are stably replicated and maintained by the cell under selective pressure and plasmid-free daughter cells are infrequent. In the absence of selective pressure, plasmid loss frequency remains low (10-5/10-6 per generation) for medium copy number plasmids, but can increase significantly for high and very high copy number plasmids. The simplest way to exert a selective pressure is to provide the plasmid with a sequence encoding for a resistance marker. Usually an antibiotic resistance is used, such as Beta-lactamase from ''bla'' gene for Amipicillin resistance, ''cat'' gene encoding Chloramphenicol resistance. Other well known selection markers are Kanamycin and Tetracycline resistances. | In order to achieve high expression levels, heterologous proteins are often cloned in vectors replcating by the ColE1 or the p15A replicon, that replicate in a relaxed fashion and are present in the cells in medium/high copy number (from 15–20 to few hundreds copies). When co-overexpression of additional gene products is desired, derivatives of ColE1 and p15A replicons are often combined. These multiple-copy plasmids are stably replicated and maintained by the cell under selective pressure and plasmid-free daughter cells are infrequent. In the absence of selective pressure, plasmid loss frequency remains low (10-5/10-6 per generation) for medium copy number plasmids, but can increase significantly for high and very high copy number plasmids. The simplest way to exert a selective pressure is to provide the plasmid with a sequence encoding for a resistance marker. Usually an antibiotic resistance is used, such as Beta-lactamase from ''bla'' gene for Amipicillin resistance, ''cat'' gene encoding Chloramphenicol resistance. Other well known selection markers are Kanamycin and Tetracycline resistances. | ||
This approach is commonly used, but for some applications it is not desirable to add antibiotic to the culture for the following reasons: | This approach is commonly used, but for some applications it is not desirable to add antibiotic to the culture for the following reasons: | ||
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A radically different solution to the problem of plasmid loss is the direct insertion of the desired part within the chromosome of ''E. coli''. This approach was attempted with different strategies, such as using simple delivery vehicles (e.g. bacteriophage lambda) or exploiting the Tn1545 site specific recombination module to randomly integrate a gene in the host strain, obtaining a library of clones containing the gene integrated in different positions. These solution avoids instability problems: in fact, chromosomally based expression usually provide genetically stable organisms and acceptable expression levels. This strategy may be compromised if essential loci in the chromosome are disrupted. Chromosomal integration also avoids the need of supplementing culture medium with antibiotic. A different approach was proposed in literature, based on genome targeting systems that use vectors carrying a conditional-replication origin and a phage attachment (attP) site. These plasmids, named ''CRIM'' (Conditional-Replication, Integration and Modular) can be used for the construction of the desired expression systems that can be directly integrated into bacterial chromosomes in single copies. Recently, the essential elements of this system have been refactored in standard parts and improved in order to get a more robust method [Anderson JC et al., 2010]. The performance of the CRIM systems had been proved, but a standard user-friendly solution for the stable integration of the desired genes in the host genome is not yet available. | A radically different solution to the problem of plasmid loss is the direct insertion of the desired part within the chromosome of ''E. coli''. This approach was attempted with different strategies, such as using simple delivery vehicles (e.g. bacteriophage lambda) or exploiting the Tn1545 site specific recombination module to randomly integrate a gene in the host strain, obtaining a library of clones containing the gene integrated in different positions. These solution avoids instability problems: in fact, chromosomally based expression usually provide genetically stable organisms and acceptable expression levels. This strategy may be compromised if essential loci in the chromosome are disrupted. Chromosomal integration also avoids the need of supplementing culture medium with antibiotic. A different approach was proposed in literature, based on genome targeting systems that use vectors carrying a conditional-replication origin and a phage attachment (attP) site. These plasmids, named ''CRIM'' (Conditional-Replication, Integration and Modular) can be used for the construction of the desired expression systems that can be directly integrated into bacterial chromosomes in single copies. Recently, the essential elements of this system have been refactored in standard parts and improved in order to get a more robust method [Anderson JC et al., 2010]. The performance of the CRIM systems had been proved, but a standard user-friendly solution for the stable integration of the desired genes in the host genome is not yet available. | ||
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+ | ===TRANSCRIPTIONAL PROMOTERS=== | ||
Promoters are small DNA portions that allow the transcription of downstream genes. These DNA parts can be catalogued by their transcriptional strength, by their activity or by their regulation mode. | Promoters are small DNA portions that allow the transcription of downstream genes. These DNA parts can be catalogued by their transcriptional strength, by their activity or by their regulation mode. | ||
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Despite these approaches are largely used in laboratories, where a small amount of an expensive inducer is not a problem, it becomes quite expensive, when moved to the large scale of an industrial process, to obtain the desired regulation control. | Despite these approaches are largely used in laboratories, where a small amount of an expensive inducer is not a problem, it becomes quite expensive, when moved to the large scale of an industrial process, to obtain the desired regulation control. | ||
- | + | ===RECOMBINANT PROTEIN PURIFICATION=== | |
Another topic of recombinant protein production deals with the purification of products: in fact a highly purified and well-characterized form has become a major task in this field. On the other hand, the goal of a rapid and economical purification of recombinant proteins represents a persistent challenge in the field of biotechnology: in fact, generally, purification is very costly and can represent up to the 80% of the total production costs. | Another topic of recombinant protein production deals with the purification of products: in fact a highly purified and well-characterized form has become a major task in this field. On the other hand, the goal of a rapid and economical purification of recombinant proteins represents a persistent challenge in the field of biotechnology: in fact, generally, purification is very costly and can represent up to the 80% of the total production costs. |
Revision as of 22:59, 23 October 2010
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ORIGIN OF REPLICATION AND RESISTANCE MARKERIn order to achieve high expression levels, heterologous proteins are often cloned in vectors replcating by the ColE1 or the p15A replicon, that replicate in a relaxed fashion and are present in the cells in medium/high copy number (from 15–20 to few hundreds copies). When co-overexpression of additional gene products is desired, derivatives of ColE1 and p15A replicons are often combined. These multiple-copy plasmids are stably replicated and maintained by the cell under selective pressure and plasmid-free daughter cells are infrequent. In the absence of selective pressure, plasmid loss frequency remains low (10-5/10-6 per generation) for medium copy number plasmids, but can increase significantly for high and very high copy number plasmids. The simplest way to exert a selective pressure is to provide the plasmid with a sequence encoding for a resistance marker. Usually an antibiotic resistance is used, such as Beta-lactamase from bla gene for Amipicillin resistance, cat gene encoding Chloramphenicol resistance. Other well known selection markers are Kanamycin and Tetracycline resistances. This approach is commonly used, but for some applications it is not desirable to add antibiotic to the culture for the following reasons:
Many solutions to these drawbacks have been proposed, such as expression of plasmid-encoded genes that causes cell death upon plasmid loss (e.g. the Toxin-Antitoxin systems). A radically different solution to the problem of plasmid loss is the direct insertion of the desired part within the chromosome of E. coli. This approach was attempted with different strategies, such as using simple delivery vehicles (e.g. bacteriophage lambda) or exploiting the Tn1545 site specific recombination module to randomly integrate a gene in the host strain, obtaining a library of clones containing the gene integrated in different positions. These solution avoids instability problems: in fact, chromosomally based expression usually provide genetically stable organisms and acceptable expression levels. This strategy may be compromised if essential loci in the chromosome are disrupted. Chromosomal integration also avoids the need of supplementing culture medium with antibiotic. A different approach was proposed in literature, based on genome targeting systems that use vectors carrying a conditional-replication origin and a phage attachment (attP) site. These plasmids, named CRIM (Conditional-Replication, Integration and Modular) can be used for the construction of the desired expression systems that can be directly integrated into bacterial chromosomes in single copies. Recently, the essential elements of this system have been refactored in standard parts and improved in order to get a more robust method [Anderson JC et al., 2010]. The performance of the CRIM systems had been proved, but a standard user-friendly solution for the stable integration of the desired genes in the host genome is not yet available.
TRANSCRIPTIONAL PROMOTERSPromoters are small DNA portions that allow the transcription of downstream genes. These DNA parts can be catalogued by their transcriptional strength, by their activity or by their regulation mode. The transcriptional strength is a very important parameter to be evaluated, because it determines the amount of produced protein. For this reason, many efforts were performed in synthetic biology towards the definition of standard measurement techniques that can evaluate the promoter activity. The kind of regulation is another crucial element to evaluate, because it might affect the yield of the whole process of protein production:
For protein manufacturing, many expression systems are available, with several regulation mechanisms, to suite every necessity. Usually, in order to achieve high yields in the amount of produced protein, it is preferable to use inducible expression systems. The culture of cells harbouring the plasmid encoding for the desired peptide is grown undisturbed (i.e. the expression of the recombinant protein is off) until it reaches a desired culture density. When the cell population reaches the desired growth phase, the production is triggered by the inducer stimulus. This solution may be preferred to a constitutive production, because it eases the burden on the organisms, allowing the cultures to grow without metabolic stress before initiating production and prevents the lowering of growth rates if the produced peptide is toxic to the cell. In these cases, a tightly regulation is fundamental, because leakage activity can result in an early overproduction of the heterologous protein, due to a non-silent promoter. This might impair cell growth. It is therefore desirable to be able to repress the promoter during the initial cell growth phase, in order to achieve high cell densities, after which the high-rate protein production would be initiated by induction of the promoter. For these applications, promoter repressor signals are used to maintain the promoter activity off during the initial growth phase (e.g. in the DE3/pLys system where the T7 phage lysozyme, an inhibitor for T7 polymerase, reduces and almost eliminates the leaky expression of the inducible T7 promoter). As already explained, expression initiation by promoter induction can be obtained in several ways. For laboratory-scale production, the isopropyl beta-D-thiogalactopyranoside (IPTG)-inducible promoters, which are regulated by the product of the lacI gene (the lac repressor) are widely used. A disadvantage with some of these promoters is that they are not completely unactive under non-induced conditions, and thus are not suitable if the target-gene product is toxic for the host. Lactose has been shown to be an inexpensive, but somewhat weaker, alternative for induction of the lac promoter in some applications. For large-scale cultivations, either the trp promoter or heat-induced promoters are commonly used. Systems using the Plambda promoter/cI repressor, Trc promoter, Tac promoter and hybrid lac/T7 promoters are common. Self-inducible systems which trigger gene expression upon carbon- or phosphate- starvation are also used. The drawback of this kind of systems is that they are usually not titratable, the media options are limited and the protein production may be limited to a time interval in which part of the nutrients is already depleted. Despite these approaches are largely used in laboratories, where a small amount of an expensive inducer is not a problem, it becomes quite expensive, when moved to the large scale of an industrial process, to obtain the desired regulation control. RECOMBINANT PROTEIN PURIFICATIONAnother topic of recombinant protein production deals with the purification of products: in fact a highly purified and well-characterized form has become a major task in this field. On the other hand, the goal of a rapid and economical purification of recombinant proteins represents a persistent challenge in the field of biotechnology: in fact, generally, purification is very costly and can represent up to the 80% of the total production costs. A large number of commercial vectors that facilitate single step purification via the use of different fusion tags have been developed. These systems are based on the fusion of the target protein with affinity tags that allow one-step absorption purification, minimally affecting the tertiary structure and the biological activity of the protein. Some commonly used tags are, for example, Polyarginine-tag (Arg-tag), Polyhistidine-tag (His-tag) or FLAG-tag. They allow easy and specific removal to produce the native protein and can be applied to several different proteins. The removal of the tag from a protein of interest can be accomplished with a site-specific protease, and the cleavage should not affect protein activity. Several drawbacks affect this purification step: in fact, the proteases are expensive, the cleavage is not always specific, elevated temperatures are required for many proteolytic cleavage reactions and may affect protein stability or activity. Furthermore, the cleavage is sometimes inefficient, due to the inaccessibility of the cleavage site on the fusion protein or additional chromatographic steps could be required to separate the target protein from the affinity tag and the protease. Another important drawback affecting the purification process is the high cost of the affinity resins that are typically used in separations. For all these reasons, many researchers are working on novel purification methods in order to improve the process yield and lower the manufacturing overall cost.
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