4S-Aminoproline polypeptide 2 forms unusual β-structure in trifluoroethanol that switches to the polyproline II (PPII) form in aqueous medium, while 4R-aminoproline peptide 1 retains PPII form in both solvents. This first instance of a polyproline derivative showing a β-structure is attributed to competitive pH-dependent (4-NH(3)(+)/NH(2)) stereoelectronic effect (4R vs 4S) and the overriding importance of stereospecific intra/intermolecular H-bonding in (2,4)-cis-4S-aminoproline in contrast to (2,4)-trans-4R-aminoproline oligomers.
The antiparallel arrangement of two strands of the non-classical β-structure, formed exclusively via cis-4S-(OH) prolyl polypeptide as established by FRET, propagates into self-assembled nanofibers upon conjugation with C12/C14/C16 hydrocarbon chains.
We previously developed reporter-peptide
nucleic acid (PNA)-peptides
for sequence-specific radioimaging and fluorescence imaging of particular
mRNAs in cells and tumors. However, a direct test for PNA-peptide
hybridization with RNA in the cytoplasm would be desirable. Thiazole
orange (TO) dye at the 5′ end of a hybridization agent shows
a strong increase in fluorescence quantum yield when stacked upon
a 5′ terminal base pair, in solution and in cells. We hypothesized
that hybridization agents with an internal TO could distinguish a
single base mutation in RNA. Thus, we designed KRAS2 PNA-IGF1 tetrapeptide agents with an internal TO adjacent to the
middle base of the 12th codon, a frequent site of cancer-initiating
mutations. Our molecular dynamics calculations predicted a disordered
bulge with weaker hybridization resulting from a single RNA mismatch.
We observed that single-stranded PNA-IGF1 tetrapeptide agents with
an internal TO showed low fluorescence, but fluorescence escalated
5–6-fold upon hybridization with KRAS2 RNA.
Circular dichroism melting curves showed ∼10 °C higher Tm for fully complementary vs single base mismatch
TO-PNA-peptide agent duplexes with KRAS2 RNA. Fluorescence
measurements of treated human lung cancer cells similarly showed elevated
cytoplasmic fluorescence intensity with fully complementary vs single
base mismatch agents. Sequence-specific elevation of internal TO fluorescence
is consistent with our hypothesis of detecting cytoplasmic PNA-peptide:RNA
hybridization if a mutant agent encounters the corresponding mutant
mRNA.
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