RGD-alpha-amanitin and isoDGR-alpha-amanitin conjugates were synthesized by joining integrin ligands to alpha-amanitin via various linkers and spacers. The conjugates were evaluated for their ability to inhibit biotinylated vitronectin binding to the purified alphaV beta3 receptor, retaining good binding affinity, in the same nanomolar range as the free ligands. The antiproliferative activity of the conjugates was evaluated in three cell lines possessing different levels of alphaV bata3 integrin expression: human glioblastoma U87 (alphaV bata3 +), human lung carcinoma A549 (alphaVbeta3 -) and breast adenocarcinoma MDA-MB-468 (alphaVbeta3 -). In the U87, in the MDA-MB-468, and partly in the A549 cancer cell lines, the cyclo[DKP-isoDGR]-alpha-amanitin conjugates bearing the lysosomally cleavable Val-Ala linker were found to be slightly more potent than alpha-amanitin. Apparently, for all these alpha-amanitin conjugates there is no correlation between the cytotoxicity and the expression of alphaVbeta3 integrin. To determine whether the increased cytotoxicity of the cyclo[DKP-isoDGR]-alpha-amanitin conjugates is governed by an integrin-mediated binding and internalization process, competition experiments were carried out in which the conjugates were tested with U87 (alphaVbeta3 +, alphaVbeta5 +, alphaVbeta6 -, alpha5beta1 +) and MDA-MB-468 (alphaVbeta3 -, alphaVbeta5 +, alphaVbeta6 +, alpha5beta1 -) cells in the presence of excess cilengitide, with the aim of blocking integrins on the cell surface. Using the MDA-MB-468 cell line, a fivefold increase of the IC 50 was observed for the conjugates in the presence of excess cilengitide, which is known to strongly bind not only alphaVbeta3 , but also alphaVbeta5 , alphaVbeta6, and alpha5beta1 . These data indicate that in this case the cyclo[DKP-isoDGR]-alpha-amanitin conjugates are possibly internalized by a process mediated by integrins different from alphaVbeta3 (e.g., alphaV beta5 ).
Synthesis and biological evaluation of RGD and isoDGR peptidomimetic-alpha-amanitin conjugates for tumor-targeting
Arosio D;
2018
Abstract
RGD-alpha-amanitin and isoDGR-alpha-amanitin conjugates were synthesized by joining integrin ligands to alpha-amanitin via various linkers and spacers. The conjugates were evaluated for their ability to inhibit biotinylated vitronectin binding to the purified alphaV beta3 receptor, retaining good binding affinity, in the same nanomolar range as the free ligands. The antiproliferative activity of the conjugates was evaluated in three cell lines possessing different levels of alphaV bata3 integrin expression: human glioblastoma U87 (alphaV bata3 +), human lung carcinoma A549 (alphaVbeta3 -) and breast adenocarcinoma MDA-MB-468 (alphaVbeta3 -). In the U87, in the MDA-MB-468, and partly in the A549 cancer cell lines, the cyclo[DKP-isoDGR]-alpha-amanitin conjugates bearing the lysosomally cleavable Val-Ala linker were found to be slightly more potent than alpha-amanitin. Apparently, for all these alpha-amanitin conjugates there is no correlation between the cytotoxicity and the expression of alphaVbeta3 integrin. To determine whether the increased cytotoxicity of the cyclo[DKP-isoDGR]-alpha-amanitin conjugates is governed by an integrin-mediated binding and internalization process, competition experiments were carried out in which the conjugates were tested with U87 (alphaVbeta3 +, alphaVbeta5 +, alphaVbeta6 -, alpha5beta1 +) and MDA-MB-468 (alphaVbeta3 -, alphaVbeta5 +, alphaVbeta6 +, alpha5beta1 -) cells in the presence of excess cilengitide, with the aim of blocking integrins on the cell surface. Using the MDA-MB-468 cell line, a fivefold increase of the IC 50 was observed for the conjugates in the presence of excess cilengitide, which is known to strongly bind not only alphaVbeta3 , but also alphaVbeta5 , alphaVbeta6, and alpha5beta1 . These data indicate that in this case the cyclo[DKP-isoDGR]-alpha-amanitin conjugates are possibly internalized by a process mediated by integrins different from alphaVbeta3 (e.g., alphaV beta5 ).| File | Dimensione | Formato | |
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Descrizione: Beilstein J Org Chem-407-2018
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