Team:UCL London/Bioprocess Flowsheet Development

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UCL IGEM 2010

Bioprocess Flowsheet

A pharmaceutical available at your nearest pharmacy's shelf has been through a similar process prior to its packaging and delivery. That is why the construction of a bioprocess flowsheet is critical. A specific bioprocess flowsheet tailored to the process is a must when it comes to taking that pharmaceutical compound from the laboratory to large scale production to satisfy the needs of a population. The bioprocess flowsheet is like the recipe of a chocolate cake. If you do not weight the sugar, it will be too sweet and if you do not throw away the egg shell it will probably cost you some taste problems or a kind of side-effect, but the egg is critical for its success, so you want to keep it. In the same way, the nutrients are important to 'bake' the cells but later on, any DNA debris or toxins produced or even contaminants, like the egg shell, have to be removed prior to its final delivery to the 'patient'. Therefore, a series of steps regarding the manufacturing, recovery, purification and formulation of the biopharmaceutical is required, to ensure the product is not only in compliance with FDA regulations, but mostly that is safe and pure for consumption.

E. coli Expression

All current monoclonal antibodies on the market and most in clinical trial have been procured through mammalian cell expression systems due to the bacterial cell’s lack of post-translational modifications such as glycosylation and secretion strategies. However, for the expression of non-glycosylated antibody fragments such as Fvs, scFvs, Fabs or F(ab’)2s, Escherichia coli is the most renowned host system of choice.

For example, UCB product CIMZIA ( Crohn's disease), is a pegylated FabV fragment made using E. coli is currently in phase III trials. Of the 15 antibodies identified in phase III trials, six were single chain or Fab fragments. Genentech, a global leader in antibody fragment production, manufactures Ranibizumab as Lucentis® at a large scale producing 0.5kg/year generating sales revenues of 1.17 Billion dollars can provide the basis for the current manipulation of E. coli and manufacture of the antibody fragment.

Utilising such a copious history of experience with E. coli-based protein expression and the ease of genetic manipulation in E. coli, makes it such an astounding attractive host for expressing antibodies, with research being pioneered to produce full monoclonal forms. The interest relays the necessity of time management where conventional and labour intensive mammalian production systems require approximately four to six months as opposed to a solitary month in E. coli; with shorter processing times and increased scale of operation, cost-of-goods may be reduced.

The chief drawback to E. coli expression is the distinct lack of post translational modifications such as glycosylation; thus PEGylation (polyethylene glycol) has found favour due to the ability of PEG to effectively increase the half-life of antibody fragments by altering the solubility, immunogenicity, pharmacokinetics, aggregation and proteolytic susceptibility of therapeutic proteins. The standard protocol for production of antibody fragments require the translocation to the periplasmic space using an N-terminal signal peptide, recognised by the common secretion pathway of E. coli, encoded by the sec genes, which are responsible for the targeted export of most cellular proteins to the extracytoplasmically.

Periplasmic Expression

This secretion pathway into the periplasm becomes the ideal sub-cellular location for Fab expression due to their oxidising environments that enables formation of intra and inter-chain disulphide bonds (Humphreys., 2004a). Using such expression, the whole cell may not need to homogenised for lysis and rupture but instead ‘periplasmic extraction’ can be exploited maintaining the spheroplast.

The processing step involves the disruption of the outer membrane of the cell by the use of Tris-EDTA lyzozyme, permitting the extraction of the fragment. The product is translocated to the periplasm by an NH2 terminal PelB leader sequence where upon fermentation the addition of sucrose can provide a maximum 25 fold of increase in yield of soluble fragments. The major advantages of protein release into the medium include a higher degree of protection from cellular proteases, a lower degree of contamination with endotoxin and more importantly simplified downstream processing (Georgiou & Segatori, 2005a).

By the same set of researchers (Harvey et al, 2004), Anchored periplasmic expression (APEx) is a developed technology for the isolation of ligand-binding proteins from combinatorial libraries anchored on the periplasmic face of the inner membrane of Escherichia coli. Subsequent to disruption of the outer membrane by Tris-EDTA-lysozyme, the inner-membrane-anchored proteins readily bind fluorescently labelled ligands as large as 240 kDa.

Intracellular Expression

The intracellular accumulation of the fragment in the cytoplasm takes the form of inclusion bodies; in this environment refolding cannot be efficiently circumvented where the use mini-chaperones and oxidoreductases must be used for functional fragments (Humphreys et al 2004b). (Tsumoto et al., 1998) reported a highly efficient refolding process for immunoglobulin-folded proteins using stepwise dialysis (Figure 1). The method accentuates the critical factors for highly efficient recovery of proteins from a denatured and reduced state are prevention of aggregation by adding labilising agents and promotion of proper disulphide bond formation at the appropriate stage of refolding. Solubilized inclusion bodies could be refolded under these conditions with yields of up to 95%.

Another innovative method that could be exploited is the ability of inducing mutations that allow disulphide bonds to form in cytoplasm of E. coli (Derman et al, 1995). When the mutations are exhibited, export-defective versions of alkaline phosphatase and mouse urokinase were used to fold into their enzymatically active conformations in the cytoplasm because their disulphide bonds were formed. The mutations were mapped to the gene for thioredoxin reductase and diminish or eliminate the activity of this enzyme and thus can be used in keeping cysteines reduced in cytoplasmic proteins. Similarly, (Ohagea et al, 1999) have also resarched in overcoming the reducing enviroment of the cytoplasm, using sequence analysis into isolated immunoglobulin VL domains and ultimately a functional heterodimeric Fv fragment.