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Dive into the research topics where Alice Ghidini is active.

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Featured researches published by Alice Ghidini.


Beilstein Journal of Organic Chemistry | 2015

Sequence-specific RNA cleavage by PNA conjugates of the metal-free artificial ribonuclease tris(2-aminobenzimidazole).

Friederike Danneberg; Alice Ghidini; Plamena Dogandzhiyski; Elisabeth Kalden; Roger Strömberg; Michael W. Göbel

Summary Tris(2-aminobenzimidazole) conjugates with antisense oligonucleotides are effective site-specific RNA cleavers. Their mechanism of action is independent of metal ions. Here we investigate conjugates with peptide nucleic acids (PNA). RNA degradation occurs with similar rates and substrate specificities as in experiments with DNA conjugates we performed earlier. Although aggregation phenomena are observed in some cases, proper substrate recognition is not compromised. While our previous synthesis of 2-aminobenzimidazoles required an HgO induced cyclization step, a mercury free variant is described herein.


Beilstein Journal of Organic Chemistry | 2014

Pyrene-modified PNAs: Stacking interactions and selective excimer emission in PNA2DNA triplexes

Alex Manicardi; Lucia Guidi; Alice Ghidini; Roberto Corradini

Summary Pyrene derivatives can be incorporated into nucleic acid analogs in order to obtain switchable probes or supramolecular architectures. In this paper, peptide nucleic acids (PNAs) containing 1 to 3 1-pyreneacetic acid units (PNA1–6) with a sequence with prevalence of pyrimidine bases, complementary to cystic fibrosis W1282X point mutation were synthesized. These compounds showed sequence-selective switch-on of pyrene excimer emission in the presence of target DNA, due to PNA2DNA triplex formation, with stability depending on the number and positioning of the pyrene units along the chain. An increase in triplex stability and a very high mismatch-selectivity, derived from combined stacking and base-pairing interactions, were found for PNA2, bearing two distant pyrene units.


Molecules | 2017

Zinc Ion-Dependent Peptide Nucleic Acid-Based Artificial Enzyme that Cleaves RNA—Bulge Size and Sequence Dependence

Merita Murtola; Alice Ghidini; Roger Strömberg

In this report, we investigate the efficiency and selectivity of a Zn2+-dependent peptide nucleic acid-based artificial ribonuclease (PNAzyme) that cleaves RNA target sequences. The target RNAs are varied to form different sizes (3 and 4 nucleotides, nt) and sequences in the bulge formed upon binding to the PNAzyme. PNAzyme-promoted cleavage of the target RNAs was observed and variation of the substrate showed a clear dependence on the sequence and size of the bulge. For targets that form 4-nt bulges, we identified systems with an improved efficacy (an estimated half-life of ca 7–8 h as compared to 11–12 h for sequences studied earlier) as well as systems with an improved site selectivity (up to over 70% cleavage at a single site as compared to 50–60% with previous targets sequences). For targets forming 3-nt bulges, the enhancement compared to previous systems was even more pronounced. Compared to a starting point of targets forming 3-nt AAA bulges (half-lives of ca 21–24 h), we could identify target sequences that were cleaved with half-lives three times lower (ca 7–8 h), i.e., at rates similar to those found for the fastest 4-nt bulge system. In addition, with the 3-nt bulge RNA target site selectivity was improved even further to reach well over 80% cleavage at a specific site.


Bioconjugate Chemistry | 2015

Studies on Tris(2-aminobenzimidazole)-PNA Based Artificial Nucleases: A Comparison of Two Analytical Techniques

Plamena Dogandzhiyski; Alice Ghidini; Friederike Danneberg; Roger Strömberg; Michael W. Göbel

A new peptide nucleic acid (PNA) construct carrying a tris(2-aminobenzimidazole) phosphodiester cleaver is presented. This non-metal-based artificial nuclease hydrolyzes RNA substrates that form a bulge upon binding to the PNA. Reaction rates depend on the bulge sequence. For conjugates of tris(2-aminobenzimidazole), substrate turnover is shown for the first time. Two methods of analysis for the kinetics are compared: IE-HPLC separation of oligonucleotide fragments and analysis of Cy5-labeled oligonucleotide fragments by denaturating PAGE on a DNA sequencer, respectively. The different methods give rates that are in the same range where, in general, the substrates for the sequencer method give slightly lower rates.


Molecules | 2014

Synthesis of PNA oligoether conjugates.

Alice Ghidini; Peter Steunenberg; Merita Murtola; Roger Strömberg

Several different approaches have been explored for conjugation of oligoethers to PNA with internally or N-terminal placed diaminopropionic acid residues. Single and double conjugation of 2-(2-(2-aminoethoxy)ethoxy)ethanol was obtained using carbonyldimidazole. Using a post PNA-assembly coupling procedure the building block 2-(2-(2-(benzoyloxy)ethoxy)ethoxy)acetic acid multiple attachment of 2-(2-(2-hydroxyethoxy)ethoxy)acetyl groups to both N-terminal and β-amino groups of inserted diaminopropionic acids residues was achieved. Use of a new oligoether functionalized amino acid allows inclusion of oligoether conjugates during on-line machine assisted synthesis which also allowed combination of methods for attachment of different oligoethers and co-conjugation of neocuproine as well as conjugation of an aminosugar.


Organic and Biomolecular Chemistry | 2016

Influence of conjugation and other structural changes on the activity of Cu2+ based PNAzymes

Alice Ghidini; Merita Murtola; Roger Strömberg


Organic and Biomolecular Chemistry | 2016

Clamping of RNA with PNA enables targeting of microRNA

Alice Ghidini; Helen Bergquist; Merita Murtola; Tanel Punga; Rula Zain; Roger Strömberg


Bioconjugate Chemistry | 2016

Enabling Multiple Conjugation to Oligonucleotides Using “Click Cycles”

Martina Jezowska; Dmytro Honcharenko; Alice Ghidini; Roger Strömberg; Malgorzata Honcharenko


Chemical Communications | 2013

An RNA modification with remarkable resistance to RNase A

Alice Ghidini; Charlotte Ander; Anna Winqvist; Roger Strömberg


Archive | 2015

Mimicking the action of ribonucleases : studies on RNase A and design of PNA based artificial enzymes

Alice Ghidini

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Michael W. Göbel

Goethe University Frankfurt

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