Secondary structure of the standard one-piece tmRNAs The complete
E. coli tmRNA
secondary structure was elucidated by
comparative sequence analysis and
structural probing. Watson-Crick and G-U
base pairs were identified by comparing the bacterial tmRNA sequences using automated computational methods in combination with manual
alignment procedures. The accompanying figure shows the base pairing pattern of this prototypical tmRNA, which is organized into 12
phylogenetically supported helices (also called pairings P1 to P12), some divided into helical segments. A prominent feature of every tmRNA is the
conserved tRNA-like domain (TLD), composed of helices 1, 12, and 2a (analogs of the tRNA acceptor stem, T-stem and variable stem, respectively), and containing the 5' monophosphate and alanylatable 3' CCA ends. The mRNA-like region (MLR) is in standard tmRNA a large loop containing pseudoknots and a coding sequence (CDS) for the tag
peptide, marked by the resume
codon and the
stop codon. The encoded tag peptide (ANDENYALAA in
E. coli) varies among bacteria, perhaps depending on the set of proteases and adaptors available. tmRNAs typically contain four
pseudoknots, one (pk1) upstream of the tag peptide CDS, and the other three pseudoknots (pk2 to pk4) downstream of the CDS. The pseudoknot regions, although generally conserved, are evolutionarily plastic. For example, in the (one-piece) tmRNAs of
cyanobacteria, pk4 is substituted with two tandemly arranged smaller pseudoknots. This suggests that tmRNA folding outside the TLD can be important, yet the pseudoknot region lacks conserved residues and pseudoknots are among the first structures to be lost as
ssrA sequences diverge in plastid and endosymbiont lineages. Base pairing in the three-pseudoknot region of
E. coli tmRNA is disrupted during
trans-translation.
Two-piece tmRNAs Circularly permuted
ssrA has been reported in three major lineages: i) all alphaproteobacteria and the primitive mitochondria of jakobid protists, ii) two disjoint groups of
cyanobacteria (
Gloeobacter and a clade containing
Prochlorococcus and many
Synechococcus), and iii) some members of the betaproteobacteria (
Cupriavidus and some Rhodocyclales). All produce the same overall two-piece (acceptor and coding pieces) form, equivalent to the standard form nicked downstream of the reading frame. None retain more than two
pseudoknots compared to the four (or more) of standard tmRNA.
Alphaproteobacteria have two signature sequences: replacement of the typical T-loop sequence TΨCRANY with GGCRGUA, and the sequence AACAGAA in the large loop of the 3´-terminal pseudoknot. In mitochondria, the MLR has been lost, and a remarkable re-permutation of mitochondrial
ssrA results in a small one-piece product in
Jakoba libera. Depending on the bacterial species, the 3'-CCA is either encoded or added by
tRNA nucleotidyltransferase. Similar processing at internal sites of permuted precursor tmRNA explains its physical splitting into two pieces. The two-piece tmRNAs have two additional ends whose processing must be considered. For alphaproteobacteria, one 5´ end is the unprocessed start site of transcription. The far 3´ end may in some cases be the result of rho-independent termination.
Three-dimensional structures ] ] High-resolution structures of the complete tmRNA molecules are currently unavailable and may be difficult to obtain due to the inherent flexibility of the MLR. In 2007, the crystal structure of the
Thermus thermophilus TLD bound to the
SmpB protein was obtained at 3 Å resolution. This structure shows that SmpB mimics the D stem and the anticodon of a canonical tRNA whereas helical section 2a of tmRNA corresponds to the variable arm of tRNA. ==
Trans-translation==