Team:Utah State/Secretion

A small signal sequence is typically necessary for all translocation pathways. However, certain protein-coding sequences can be secreted without having an attached signal sequence due to the presence of additional targeting information within the sequence (Luiritz, 2004). Additionally, an attached signal sequence does not guarantee export of a protein, which further suggests that information in the protein sequence itself can affect secretion efficiency (Luiritz, 2004). However, the fusion of a signal sequence to a recombinant protein can lead to export of a previously non-secretable protein. There are many reported examples of recombinant protein translocation through signal sequence gene fusion. For example, fusion with the Tat-dependent signal peptide TorA allowed for export of folded GFP into the periplasm of E. coli (Palmer, 2004; Barrett, 2003; Santini, 2001; Thomas, 2001).

Two factors that affect protein export are the positive charge of the N-terminus of the signal peptide and the charge of the N-terminus of the recombinant protein (Akita 1990). Akita et. Al (1990) determined that increasing the positive charge of the signal peptide N-terminus not only enhances the interaction with SecA protein, but also reduces the requirements of SecA ATPase activity for translocation. Therefore, a higher net positive N-terminus charge improves the rate of protein translocation (Mergulhão, 2005). For the recombinant protein, the charge of the N-terminus also affects protein secretion. A net positive charge within the first five amino acids near the C-domain cleavage site of the signal sequence can reduce protein export by as much as 50-fold because the charge inhibits the protein from entering the lipid bilayer (Schatz, 1990).

Although factors like hydrophobicity and charge are known to affect protein export, there are few available guidelines for selecting a proper signal peptide for any given protein (Choi, 2004). It is advised to carry out investigation of recombinant protein secretion by trial-and-error with different host strains and signal peptides (Choi, 2004). The mechanisms of protein secretion are complicated and many obstacles can inhibit the process. Some commonly observed problems include incomplete translocation, degradation of recombinant protein by proteases, formation of inclusion bodies, and inefficiency of secretion machinery (Mergulhão, 2005; Choi, 2004). Optimization of the secretion efficiency requires balancing the promoter strength and gene copy number so as not to overwhelm the system (Mergulhão, 2005). Lastly, some proteins may simply be unsuitable for secretion due to their size or sequence (Koster, 2000).

Phasin (PhaP) is a low-molecular weight protein that plays a role in PHA granule formation by physically binding to the PHA granule surface (York, 2001). The specific purpose of phasin production is not completely understood (York 2002), although some of the affects of the phasin/PHA interaction have been studied. York et al (2001) determined that the production of phasin is dependent on PHA accumulation. Specifically, it is suggested that phasin expression requires the presence of PHA synthase (York, 2001). Maehara et al (1999) observed that the level of PHA accumulation substantially decreases and the size of PHA granules increases when phasin is either absent or regulated by a repressor, PhaR. Therefore, PHA production levels are enhanced in the presence of phasin due to an increased granule surface-to-volume ratio (York 2001; Maehara 1999).

In addition to reducing PHA granule size, other functions of phasin have been proposed. In the absence of phasin, other proteins can bind to the granule surface (Maehara, 1999). Therefore, phasins may function to inhibit attachment of other proteins to the PHA surface that could cause defects in granule formation (York 2001; Maehara, 1999). Lastly, it is suggested that phasins promote PHA synthesis through an interaction with PHA synthase (York, 2001).

Due to their physical interaction with the PHA granule, phasins can be used in recombinant protein purification (Banki, 2005), or PHA recovery as this project is investigating. For protein purification, genetic fusion of a protein product, a self-splicing element called an intein, and phasin can be used (Banki, 2005). The genetically-fused protein is produced in E. coli harboring the PHB production genes (Banki, 2005). The phasin protein binds to the surface of the PHB granule, and a cleavage-inducing buffer stimulates the release of the product protein into the soluble fraction of the solution (Banki, 2005).

For this procedure, PHB is released and proteins are recovered only after the cell lysed, which is not ideal. However, the system provides evidence that the phasin/PHA interaction may be exploited for improving production processes and that genetic fusion of other elements with phasin does not inhibit binding to PHA (Banki, 2005). The fusion of phasin with a signal peptide, which is a sequence that tags a protein for secretion, could result in a signal peptide/phasin/PHA complex that is recognized by cell for transmembrane export.

The recovery of PHA granules via secretion of a signal peptide/phasin/PHA complex may be inhibited due to the size of PHA granules. However, the binding of phasins decreases PHA molecular weight and encourages the formation of numerous, small granules (Maehara, 1999). Though the actual size of PHA granules varies, Maehara et al (1999) observed spherical granules approximately 20 – 60 nm in diameter in the presence of phasin and absence of the PhaR repressor. This indicates that enhanced production of phasin may further reduce granule size, which may make PHAs more suitable for export.

GFP is a commonly used reporter of gene regulation. It is expressed in many bioluminescent jellyfish naturally (Shimomura, 1962). Its value in the academic and biotechnology industry was recognized after successful cloning and expression in E. coli (Chalfie, 1994). Purified GFP, composed of 238 amino acids, absorbs blue light (395 nm) and emits green light (Chalfie, 1994). The detection of intracellular GFP is not limited by the availability of substrates, but requires only irradiation by near UV or blue light (Chalfie, 1994). However, to ease the process of GFP detection for many organisms, a stronger whole cell fluorescence signal is desirable. Figure 5 depicts the GFP barrel structure.