Secretion
Chaperone-usher secretion is related to type V secretion. This type of secretion is often used to assemble some types of pilins on the cell surface, such as the P pilus of uropathogenic E. coli. The secretion system consists of three proteins, a β-barrel-forming protein in the outer membrane called the usher, a periplasmic protein called the chaperone, and the pilin subunit to be assembled on the cell surface. The pilin protein is transported through the inner membrane by the SecYEG channel and therefore has a cleavable signal sequence. Once in the periplasm, the pilin protein is bound by the dedicated periplasmic chaperone. However, rather than merely helping it fold like other chaperones, this chaperone actually contributes a strand to the pilus protein that completes one of the folds of the pilin protein and makes it much more stable (see Waksman and Hultgren, Suggested Reading). The complex of pilin protein and chaperone is then targeted to the usher channel in the outer membrane, where it is assembled into the growing pilus. Again, there is the problem of where the energy for pilus assembly comes from, since the assembly of the pilus occurs at the inner face of the outer membrane after the pilin protein has been transported through the inner membrane and cytoplasm. One idea is that the periplasmic chaperone holds the pilin protein in a high-energy state, and its eventual folding at the usher drives the assembly process.
TYPE VI SECRETION SYSTEMS
Type VI secretion systems (T6SS) are very large, with up to 21 proteins encoded within the gene cluster, 12 of which are highly conserved and are thought to play structural roles in the secretion apparatus. At least some of the others unique to each system may encode effectors specifically transported by that system. An intriguing observation has been made that some of the highly conserved proteins structurally resemble components of phage tails (see chapter 7). The highly conserved protein Hcp resembles gp19, the major tail protein of phage T4, and another, VgrG, resembles the syringe of the baseplate of phage T4, consisting of gp27 and gp5. This has led to speculation that T6SS are derived from phage genes and act as inverted phage tails that now eject proteins from the bacterial cell instead of injecting DNA (and sometimes proteins) into the cell.
These systems are required for the secretion of proteins involved in pathogenesis and symbiosis, but they are also found in marine and soil bacteria, where they may have roles in biofilm formation and cell-to-cell communication. There can be little doubt of the importance of these systems, since mutations in their genes can have dramatic phenotypes, but many questions remain about their structure and function.
Protein Secretion in Bacteria That Lack an Outer Membrane
So far, we have limited our discussion of protein transport to the mechanisms used by bacteria that contain an outer lipid bilayer membrane (commonly referred to as Gram-negative bacteria). However, a large group of bacteria, notably the Firmicutes and Actinobacteria, lack an outer membrane (and are often referred to as the Grampositive bacteria). Organisms in this group have evolved different types of secretion systems.
INJECTOSOMES
Pathogenic bacteria that lack the secretion systems described above require alternative mechanisms to translocate virulence effectors into eukaryotic cells. Some AB-type toxins, such as diphtheria toxin, and clostridial neurotoxins, such as botulinum toxin, are self-translocating, similar to the autotransporter systems described above. However, some bacteria, such as Streptococcus pyogenes, inject a virulence effector into the mammalian target cell by a mechanism functionally analogous to the T3SS (see Madden et al., Suggested Reading). This has been named an injectosome to distinguish it from the standard type III injectisome (note the different spellings). As shown in Figure 2.41, the function of the injectosome requires cotranslational translocation of the effector by the Sec-dependent secretion system across the bacterial membrane before it translocates the effector through the cell wall and directly across the membrane of the eukaryotic target cell.
Sortases
In bacteria that lack a bilipid outer membrane, the cell wall is available to the external surface of the cell. These bacteria take advantage of this by attaching some proteins directly to their cell wall so that the proteins will be exposed on the cell surface. Proteins destined for covalent attachment to the outer surface of the cell wall are the targets of a type of cell wall-sorting enzyme called a sortase. The general sortase, sortase A (StrA), sometimes called the housekeeping sortase, may attach as many as 40 different proteins to the cell wall. Others are more specific for certain proteins.
A sortase is able to create covalent attachments between peptides by catalyzing a transpeptidation reaction. Figure 2.42 illustrates a typical StrA pathway. Surface proteins that are StrA targets contain an N-terminal signal sequence and a 30- to 40-residue C-terminal sorting signal, which is composed of a pentapeptide cleavage site, LPXTG, and a hydrophobic domain that together constitute the cell wall-sorting signal (Cws) (Figure 2.42A). The N-terminal signal sequence of the sortase target protein directs the protein to the membrane translocase, where the signal sequence is removed (Figure 2.42B). After the protein has been translocated across the cytoplasmic membrane, the sortase cuts between the threonine (T) and glycine (G) in the pentapeptide sorting signal and then covalently links the carboxyl group of the threonine to a specific cysteine in the sortase C terminus. The sortase then attaches it to the terminal amino acid in the lipid II interlinking peptide that links two peptide crosslinks in the cell wall. When the N-acetylmuramic acid (MurNac) in this lipid II is incorporated into the cell wall, the protein becomes covalently attached to the cell wall.
Figure 2.41 Comparison of the Firmicute-type injectosome (A) and the type III injectisome (B). Modified from Tweten RK, Caparon M, in Waksman G, Caparon M, Hultgren S (ed), Structural Biology of Bacterial Pathogenesis (ASM Press, Washington, DC, 2005).
Sortase subfamilies are defined based on their taxonomic distributions and differences in the sorting signal and the peptide to which it can be attached (see Hendrickx et al., Suggested Reading). A particularly interesting example is the assembly of pili from their subunits on the cell surfaces. Pili are composed of one major subunit, often called pilin, and one or more minor subunits. In the simplest example, pili composed of pilin and only one other subunit, the minor subunit at the tip is attached to the first pilin subunit by a specialized sortase, and this first subunit is then attached to a number of other pilin subunits by the same specialized sortase. Finally, the last subunit is attached to the cell wall by the housekeeping sortase A, which attaches most other proteins to the cell wall. This makes for a very stable pilus and secures its attachment to the cell wall.
Regulation of Gene Expression
The previous sections have reviewed how a gene is expressed in the cell, from the time mRNA is transcribed from the gene until the protein product of the gene reaches its final destination in or outside the cell and has its effect. In general, genes are expressed in the cell only when the product is needed by the cell and then only as much as is required to make the amount of product needed by the cell. This saves energy and prevents the products of different genes from interfering with each other. The process by which the output of genes is changed depending on the state of the cell is called the regulation of gene expression and can occur at any stage in the expression of the gene (see chapter