Chemolabile cellular microarrays for screening small molecules and peptides

被引:0
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作者
Antje Hoff
Thomas André
Rainer Fischer
Söhnke Voss
Michael Hulko
Udo Marquardt
Karl-Heinz Wiesmüller
Roland Brock
机构
[1] University of Tübingen,Institute for Cell Biology
[2] EMC microcollections GmbH,Department of Protein Evolution
[3] T,Department of Chemistry, John and Edna Davenport Chemical Laboratories
[4] Max Planck Institute for Developmental Biology,undefined
[5] University of Toronto,undefined
来源
Molecular Diversity | 2004年 / 8卷
关键词
cell-penetrating peptides; chemical microarray; ester-linkage; fluorescence; hydrogel; microscopy; non-covalent peptide microarray; solid-phase peptide synthesis;
D O I
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中图分类号
学科分类号
摘要
Microarrays that mediate the uptake of small molecules into living cells are described. Tissue culture cells were seeded onto glass substrates functionalized locally with fluorescently labelled test substances. In order to enable a localized transferof substances after contact of cells with the substrate, substances were immobilized on the surface either by non-covalent interactions or chemolabile linker groups. These chemolabile linker groups were incorporated into covalently immobilized compounds. Different ester linkages were evaluated as chemolabile linker groups. As model compounds, esters of the carboxy group of a cysteine with the hydroxy groups of carboxyfluorescein-labelled serine amide and tyrosine amide residues or the thiol group of another fluorescein-labelled cysteine amide were generated. Covalent immobilization occurred on maleimide-functionalized glass cover slips. The surface functionalization and release kinetics were assessed by confocal laser scanning microscopy. The fastest release was obtained for the phenolic tyrosine ester. Alternatively, fluorescently labelled peptides were immobilized by non-covalent interactions on glass and on a hydrogel matrix. In order to increase the efficiency of cellular uptake, peptides were N-terminally extended with a cell-penetrating peptide. Uptake of these peptides into cells was confined to the functionalized spots, and was specificfor peptides extended with the cell-penetrating peptide.
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页码:311 / 320
页数:9
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