Vectors selected from adeno-associated viral display peptide libraries for leukemia cell-targeted cytotoxic gene therapy.

Stefan Michelfelder; Mi-Kyung Lee; Elisethe DeLima-Hahn; Thomas Wilmes; Felix Kaul; Oliver Müller; Jürgen A Kleinschmidt; Martin Trepel

Vectors selected from adeno-associated viral display peptide libraries for leukemia cell-targeted cytotoxic gene therapy.

Standard

Vectors selected from adeno-associated viral display peptide libraries for leukemia cell-targeted cytotoxic gene therapy. / Michelfelder, Stefan; Lee, Mi-Kyung; DeLima-Hahn, Elisethe; Wilmes, Thomas; Kaul, Felix; Müller, Oliver; Kleinschmidt, Jürgen A; Trepel, Martin.

in: EXP HEMATOL, Jahrgang 35, Nr. 12, 12, 2007, S. 1766-1776.

Publikationen: SCORING: Beitrag in Fachzeitschrift/Zeitung › SCORING: Zeitschriftenaufsatz › Forschung › Begutachtung

Harvard

Michelfelder, S, Lee, M-K, DeLima-Hahn, E, Wilmes, T, Kaul, F, Müller, O, Kleinschmidt, JA & Trepel, M 2007, 'Vectors selected from adeno-associated viral display peptide libraries for leukemia cell-targeted cytotoxic gene therapy.', EXP HEMATOL, Jg. 35, Nr. 12, 12, S. 1766-1776. <http://www.ncbi.nlm.nih.gov/pubmed/17920758?dopt=Citation>

APA

Michelfelder, S., Lee, M-K., DeLima-Hahn, E., Wilmes, T., Kaul, F., Müller, O., Kleinschmidt, J. A., & Trepel, M. (2007). Vectors selected from adeno-associated viral display peptide libraries for leukemia cell-targeted cytotoxic gene therapy. EXP HEMATOL, 35(12), 1766-1776. [12]. http://www.ncbi.nlm.nih.gov/pubmed/17920758?dopt=Citation

Vancouver

Michelfelder S, Lee M-K, DeLima-Hahn E, Wilmes T, Kaul F, Müller O et al. Vectors selected from adeno-associated viral display peptide libraries for leukemia cell-targeted cytotoxic gene therapy. EXP HEMATOL. 2007;35(12):1766-1776. 12.

Bibtex

@article{53218f359fba478ca2c56f7b65d8bd2d,

title = "Vectors selected from adeno-associated viral display peptide libraries for leukemia cell-targeted cytotoxic gene therapy.",

abstract = "OBJECTIVE: For acute myeloid leukemia (AML), gene therapy may be used to treat patients refractory to conventional chemotherapy. However, availability of vectors sufficiently and specifically transducing this cell type is very limited. METHOD: Here we report the selection of capsid-modified adeno-associated viral (AAV) vectors targeting Kasumi-1 AML cells by screening random AAV displayed peptide libraries. RESULTS: The peptide inserts of the enriched capsid mutants share a common sequence motif. The same motif was selected in an independent library screening on HL-60 AML cells. Recombinant targeted vectors displaying the selected peptides transduced the target leukemia cells they have been selected on up to 500-fold more efficiently compared to AAV vectors with control peptide inserts. One of the selected clones (NQVGSWS) also efficiently transduced all members of a panel of four other AML cell lines. Binding and blocking experiments showed that NQVGSWS binding to leukemia cells is independent of the wild-type AAV-2 receptor heparin sulfate proteoglycan. Transduction assays on a panel of hematopoietic and nonhematopoietic cell lines showed that the NQVGSWS capsid was able to overcome resistance to AAV transduction, especially in hematopoietic cancer cells, whereas normal peripheral blood mononuclear cells and CD34(+) hematopoietic progenitor cells were not transduced. CONCLUSIONS: Consequently, recombinant targeted NQVGSWS AAV vectors harboring a suicide gene conferred selective killing to Kasumi-1 cells, but not to control cells. This suggests that the AAV mutant selected here may be used as a tool to target therapeutic genes to AML cells.",

author = "Stefan Michelfelder and Mi-Kyung Lee and Elisethe DeLima-Hahn and Thomas Wilmes and Felix Kaul and Oliver M{\"u}ller and Kleinschmidt, {J{\"u}rgen A} and Martin Trepel",

year = "2007",

language = "Deutsch",

volume = "35",

pages = "1766--1776",

journal = "EXP HEMATOL",

issn = "0301-472X",

publisher = "Elsevier Inc.",

number = "12",

}

RIS

TY - JOUR

T1 - Vectors selected from adeno-associated viral display peptide libraries for leukemia cell-targeted cytotoxic gene therapy.

AU - Michelfelder, Stefan

AU - Lee, Mi-Kyung

AU - DeLima-Hahn, Elisethe

AU - Wilmes, Thomas

AU - Kaul, Felix

AU - Müller, Oliver

AU - Kleinschmidt, Jürgen A

AU - Trepel, Martin

PY - 2007

Y1 - 2007

N2 - OBJECTIVE: For acute myeloid leukemia (AML), gene therapy may be used to treat patients refractory to conventional chemotherapy. However, availability of vectors sufficiently and specifically transducing this cell type is very limited. METHOD: Here we report the selection of capsid-modified adeno-associated viral (AAV) vectors targeting Kasumi-1 AML cells by screening random AAV displayed peptide libraries. RESULTS: The peptide inserts of the enriched capsid mutants share a common sequence motif. The same motif was selected in an independent library screening on HL-60 AML cells. Recombinant targeted vectors displaying the selected peptides transduced the target leukemia cells they have been selected on up to 500-fold more efficiently compared to AAV vectors with control peptide inserts. One of the selected clones (NQVGSWS) also efficiently transduced all members of a panel of four other AML cell lines. Binding and blocking experiments showed that NQVGSWS binding to leukemia cells is independent of the wild-type AAV-2 receptor heparin sulfate proteoglycan. Transduction assays on a panel of hematopoietic and nonhematopoietic cell lines showed that the NQVGSWS capsid was able to overcome resistance to AAV transduction, especially in hematopoietic cancer cells, whereas normal peripheral blood mononuclear cells and CD34(+) hematopoietic progenitor cells were not transduced. CONCLUSIONS: Consequently, recombinant targeted NQVGSWS AAV vectors harboring a suicide gene conferred selective killing to Kasumi-1 cells, but not to control cells. This suggests that the AAV mutant selected here may be used as a tool to target therapeutic genes to AML cells.

AB - OBJECTIVE: For acute myeloid leukemia (AML), gene therapy may be used to treat patients refractory to conventional chemotherapy. However, availability of vectors sufficiently and specifically transducing this cell type is very limited. METHOD: Here we report the selection of capsid-modified adeno-associated viral (AAV) vectors targeting Kasumi-1 AML cells by screening random AAV displayed peptide libraries. RESULTS: The peptide inserts of the enriched capsid mutants share a common sequence motif. The same motif was selected in an independent library screening on HL-60 AML cells. Recombinant targeted vectors displaying the selected peptides transduced the target leukemia cells they have been selected on up to 500-fold more efficiently compared to AAV vectors with control peptide inserts. One of the selected clones (NQVGSWS) also efficiently transduced all members of a panel of four other AML cell lines. Binding and blocking experiments showed that NQVGSWS binding to leukemia cells is independent of the wild-type AAV-2 receptor heparin sulfate proteoglycan. Transduction assays on a panel of hematopoietic and nonhematopoietic cell lines showed that the NQVGSWS capsid was able to overcome resistance to AAV transduction, especially in hematopoietic cancer cells, whereas normal peripheral blood mononuclear cells and CD34(+) hematopoietic progenitor cells were not transduced. CONCLUSIONS: Consequently, recombinant targeted NQVGSWS AAV vectors harboring a suicide gene conferred selective killing to Kasumi-1 cells, but not to control cells. This suggests that the AAV mutant selected here may be used as a tool to target therapeutic genes to AML cells.

M3 - SCORING: Zeitschriftenaufsatz

VL - 35

SP - 1766

EP - 1776

JO - EXP HEMATOL

JF - EXP HEMATOL

SN - 0301-472X

IS - 12

M1 - 12

ER -