23S rRNA from Escherichia coli was cleaved
at single internucleotide bonds using ribonuclease H in
the presence of appropriate chimeric oligonucleotides;
the individual cleavage sites were between residues 384
and 385, 867 and 868, 1045 and 1046, and 2510 and 2511,
with an additional fortuitous cleavage at positions 1117
and 1118. In each case, the 3′ terminus of the 5′
fragment was ligated to radioactively labeled 4-thiouridine
5′-,3′-biphosphate (“psUp”), and
the cleaved 23S rRNA carrying this label was reconstituted
into 50S subunits. The 50S subunits were able to associate
normally with 30S subunits to form 70S ribosomes. Intra-RNA
crosslinks from the 4-thiouridine residues were induced
by irradiation at 350 nm, and the crosslink sites within
the 23S rRNA were analyzed. The rRNA molecules carrying
psUp at positions 867 and 1117 showed crosslinks to nearby
positions on the opposite strand of the same double helix
where the cleavage was located, and no crosslinking was
detected from position 2510. In contrast, the rRNA carrying
psUp at position 384 showed crosslinking to nt 420 (and
sometimes also to 416 and 425) in the neighboring helix
in 23S rRNA, and the rRNA with psUp at position 1045 gave
a crosslink to residue 993. The latter crosslink demonstrates
that the long helix 41–42 of the 23S rRNA (which
carries the region associated with GTPase activity) must
double back on itself, forming a “U-turn” in
the ribosome. This result is discussed in terms of the
topography of the GTPase region in the 50S subunit, and
its relation to the locations of the 5S rRNA and the peptidyl
transferase center.
